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CBS2 Day 2015 - Association CBS2
CBS2 Association assocbs2.com Table of contents Word from the CBS2 Association.................................................................. 3 Program Overview .......................................................................................... 5 Detailed Program ............................................................................................ 6 Invited Speakers ............................................................................................ 15 Short Talks : Session 1 .................................................................................. 19 Short Talks : Session 2 .................................................................................. 27 Posters : Session 1 ......................................................................................... 37 Posters : Session 2 ......................................................................................... 77 Organizing commitee .................................................................................. 119 Jury and chairs ............................................................................................ 120 Thanks.......................................................................................................... 121 CBS2 Association assocbs2.com CBS2 Association assocbs2.com Word from the CBS2 Association It is with great pleasure that we receive you for the 13th annual meeting of the PhD students from the CBS2 doctoral school: the CBS2 Day 2015. Following the last years’ evolution, the Organizing Committee decided to strengthen this occasion for all the students to meet, talk and learn from each other and other members of the scientific community. This year will be marked by two parallel short talks sessions to let you to choose the most interesting for you. Obviously, like last year, there will be two poster sessions and two renowned scientists’communications just for you! Once again, we would like to thank all the people who made it possible: Sandrine Urvoy and Michel Desarmenien, head of ourdoctoral school, supported us in our will of change, BioCampus with Audrey Verdier and Laurent Journot, who made possible the reward for the best presentations, Genopolys with Magali Kitzmann, Géraldine Pawlak, Silke Conquet and Marchel Méchali, who opened their doors to us, All the scientists who constitute the jury and chairs, The computing facility of the IGH, for their help with the visioconference, Our partners, the University of Montpellier, MRI, IMGT, Cisbio, Pôle BioSanté Rabelais, CNRS, All of you who register in such large numbers to this event! This meeting is originally organised by PhD students, for PhD students and is dedicated to the work we carry on every day in our labs. Enjoy the fact that this year more than 50 other members of the scientific community registered to the event to hear about the work done by PhD students. Make this day your own! CBS2 Association assocbs2.com CBS2 Association assocbs2.com Program Overview Genopolys/IGF 8h30-9h Welcome of the meeting attendees 9h-9h15 Meeting opening by the doctoral school director and the CBS2 association president 9h15-10h15 3 Short Talks of PhD students for each session (in parallel) Session 1A 10h15-10h45 Session 1B 11h45-12h Coffee break Conference of Michel Tibayrenc «The predominant clonal evolution (PCE) concept of microbial pathogens» Beginning of the lunch break 12h-13h30 Poster Session 1 (with meal) 13h30-13h45 End of the lunch break 13h45-14h CBS2 Association Presentation (general infos, projects, report of the survey…) 14h-15h Conference of Serge Bauin «Decide to publish in open access: what risks for my career?» 10h45-11h45 15h-16h 3 Short Talks of PhD students for each session (in parallel) Session 2A Session 2B 16h-17h30 Poster Session 2 (with coffee break) 17h30-17h45 End of coffee break 17h45-18h Report of the PhD-Company training 18h-18h15 Award ceremony 18h15-19h Cocktail CBS2 Association assocbs2.com Detailed Program 8h30-9h15 : Welcoming Words from M. Désarménien (Director of the CBS2 Doctoral School) and Vuthy Ea (president of the CBS² Association). 9h15-10h15: PhD student’s oral presentations Session 1A : Genopolys Amphi 9h15-9h35: Efficient CRISPR-Cas9-mediated genome editing of Leishmania parasites. Lauriane SOLLELIS 9h35-9h55: Implication of CD8+ T cells in the pathophysiology of amyotrophic lateral sclerosis. Emmanuelle COQUE 9h55-10h15: Autophagy Restricts HIV-1 Infection by Selectively Degrading Tat in CD4 T Lymphocytes. Coralie DAUSSY Session 1B:IGF South Seminar Room (2nd Floor) 9h15-9h35: Characterization of P.falciparum sub-populations associated to artemisinin drug resistance in Cambodia. Ankit DWIVEDI 9h35-9h55: Wfs1-/- mice: phenotyping and gene therapy against Wolfram Syndrome. Jolanta JAGODZINSKA 9h55-10h15: New self-deployable, bioresorbable and anti-adhesive medical device for the prevention of intrauterine adhesions. Salomé LEPRINCE 10h15-10h45: Coffee-break 10h45-11h45: First invited speaker «The predominant clonal evolution (PCE) concept of microbial pathogens». Michel Tibayrenc Maladies Infectieuses et Vecteurs Ecologie, Génétique, Evolution et Contrôle (MIVEGEC), Institut de Recherche pour le Développement (IRD), Montpellier, France. 12h30-14h30: Buffet and poster session 1 CBS2 Association assocbs2.com Poster 1: Quantifying the pressure thresholds for tissue injury in paraplegic patients. Marion LE GALL Poster 2: Role of SUMOylation and Reactive Oxygen Species (ROS) in Acute Myeloid Leukemia (AML) treatment. Hayeon BAIK Poster 3: Global regulation of the SUMO pathway during Acute Myeloid Leukemia treatment with chemotherapeutic drugs. Marko RISTIC Poster 4: Identification of factors involved in proteasome-mediateddegradation of antiapoptotic Bfl-1. Loic LIONNARD Poster 5: H4K20 methylation pathway, chromatin structure and tumorigenesis. Fanny IZARD Poster 6: Toxoplasma gondii AuTophaGy protein 8 has an unusual role in apicoplast division which is essential for parasite growth. Maude LEVEQUE Poster 7: An open access part toolbox to tune genetic expression in Bacillus subtilis. Sarah GUIZIOU Poster 8: Oxidative stress: key mechanism of age-related cochlear sensory hair cell loss. Nesrine BENKAFADAR Poster 9: Membrane dynamics and partitioning of CD9 and CD81 are differentially regulated by the actin network. Laurent FERNANDEZ Poster 10: High viral load in patients failing first-line ART is associated with multidrug resistance in resource limited countries. Emilande GUICHET Poster 11: Cardioprotection against ischemia-reperfusion injury by heart rate control. Viviana DELGADO BETANCOURT Poster 12: Development of a mobile application to compute food carbohydrates. Omar DIOURI Poster 13: Adrenergic receptor gene variants are associated with late-onset generalized anxiety disorder. Xiaobin ZHANG Poster 14: Role of the ribosomal protein S6 phosphorylation in the mouse brain. Anne BIEVER CBS2 Association assocbs2.com Poster 15: Characterization of a Cancer Stem cells enriched subpopulations and role of EMT Regulators in basal Breast Cancer Cell Plasticity. Mona HOUHOU Poster 16: Metabotropic glutamate receptor type 7 (mGlu7) modulation of thalamocortical activity. Benoit GIRARD Poster 17: Modeling the role of the global regulator ShvR of Burkholderia cenocepacia in virulence using zebrafish embryos. Margarida GOMES Poster 18: Ubiquitin under stress: “Going hybrid with NEDD8”.Chantal MAGHAMES Poster 19: Modulation of lateral septal neurons by oxytocin and vasopressin, neuropeptides involved in the regulation of social behavior.Amélie BORIE Poster 20: Potential role of P2X4R expressed by sensory neurons in BDNF-evoked inflammatory pain. Sarah LALISSE Poster 21: Role of RIP140 in familial colorectal cancer. Pascale PALASSIN Poster 22: Deciphering the function of the Serine/Threonine Protein Kinase CStk from Coxiella burnetii and its role during host infection. Solene BRELLE Poster 23: Characterization and role of indirectly-activated human dendritic cells by immune-complex adenovirus in vitro in immune memory response. Thi Thu Phuong TRAN Poster 24: BDNF knockdown induces defects in zebrafish posterior lateral line development. Alaa YEHYA Poster 25: Diffuse low grade gliomas: characterization and development of in vitro model for designing innovative therapeutic approaches.Safa AZAR Poster 26: Role of the chromatin associated proteins HP1 (Heterochromatin Protein 1) in liver hemostasis. Shefqet HAJDARI Poster 27: Role of PRDM9 methyltransferase activity in mouse meiotic recombination. Boubou DIAGOURAGA Poster 28: Dynamics and function of monocyte subsets in alcohol-dependent subjects. Hélène DONNADIEU-RIGOLE Poster 29: Dissecting the role of new cortical scaffolds during epithelial biology. Elodie FOREST CBS2 Association assocbs2.com Poster 30: Role of histone modifications and non-coding RNAs in the regulation of the imprinted Dlk1-Dio3 domain. Ildem SANLI Poster 31: Molecular mechanisms of Notch1-induced pericyte-like transdifferentiation of glioblastoma stem cells. Sophie GUELFI Poster 32: A synthetic tridimensional matrix to study the migration of Glioblastoma stem cells. Ali SALEH Poster 33: Initiation of meiotic recombination in mouse; search for interacting partners of PRDM9. Yukiko IMAI Poster 34: Epigenetic modulation of intestinal cancer susceptibility. Marco BRUSCHI Poster 35: Rad18 silences the UV-dependent DNA damage checkpoint in early Xenopus embryos. Chames KERMI Poster 36: Differential effect of microparticles and exosomes isolated from mesenchymal stem cells on T cell proliferation and experimental arthritis. Stella COSENZA Poster 37: Epigenetics and phenotypes modulation in HMEC cells. Amanda ABI KHALIL Poster 38: DNA methylation and pulmonary disease in CF patients. Milena MAGALHÃES 13h45-14h: CBS2 Association Presentation General informations about the association, its projects. Report of the survey about your thesis in the CBS2 doctoral school. 14h-15h: Second invited speaker «Decide to publish in open access: what risks for my career? » Serge Bauin Coordinateur des politiques d’IST - COMUE Université Sorbonne Paris Cité et Chargé de mission pour le libre accès - DIST (Direction de l'Information Scientifique et Technique) du CNRS. 15h-16h: PhD student’s oral presentations Session 2A: Genopolys Amphi CBS2 Association assocbs2.com 15h-15h20: Generation of Alzheimer's disease (AD) genetic patients’ reprogrammed stem cells (iPS) as tools for the diagnostic and therapeutic researches for AD. Laura AUBOYER 15h20-15h40: Shifts in Migration route: Insights into GABAergic Interneurons Diversity. Christelle CADILHAC 15h40-16h: Origin of the HIV-1 group O epidemic in Western Lowland Gorillas. Mirela D'ARC Session 2B: IGF South Seminar Room (2nd Floor) 15h-15h20: Molecular Mechanisms of Zebrafish Cardiac Regeneration. Girisaran GANGATHARAN 15h20-15h40: Chromatin-bound MDM2 regulates serine metabolism and redox homeostasis independently of p53. Romain RISCAL 15h40-16h: Polycomb-Mediated Inheritance. Filippo CIABRELLI Repression in Transgenerational Epigenetic 16h-17h45: Coffee and poster session 2 Poster 39: Pro-inflammatory macrophages mediated TNFa signaling is required for caudal fin regeneration in zebrafish larvae. Béryl LAPLACE-BUILHE Poster 40: Role of miRNAs in the Cystic Fibrosis pathology. Jennifer BONINI Poster 41: Evolution of meiotic recombination: variation and function of the Prdm9 gene in mice. Denis DUNOYER DE SEGONZAC Poster 42: Biophysical interaction of nanoparticles with biological fluids. Estelle RASCOL Poster 43: Allosteric modulation of metabotropic glutamate receptors by chloride ions. Amélie TORA Poster 44: Generation of a vaccine to prevent poultry from Newcastle disease and control viral shedding. Haijin LIU Poster 45: Adaptation of Staphylococcus aureus to prolonged environmental stress conditions. Christelle NGBA ESSEBE CBS2 Association assocbs2.com Poster 46: Understanding the cooperation between Notch and the polarity determinant Scribble during neoplasia. Rémi LOGEAY Poster 47: Identification of potential therapeutic targets regulated by Fra-1 and/or Fra2 in triple negative breast cancers. Claire TOLZA Poster 48: Targeting Transferin Receptor 1 (TFR1) in Pancreatic Cancer. Rana MELHEM Poster 49: Structural characterization of Plasmodium falciparum CCT and fragmentbased drug design approach for targeting phospholipid biosynthesis pathway. Ewelina GUCA Poster 50: PPM1K (protein phosphatase, Mg2+/Mn2+ dependent, 1K) Gene Association in Polycystic Ovary Syndrome for Better Understanding of the Role of Branched-Chain Aminoacids Variation in Metabolic Disorders. Sara HAYDAR Poster 51: Identification of new regulators of the Notch pathway in KRASG12Vdriven NSCLC. Alejandra DAMIAN Poster 52: Identification of kinase inhibitors as alternatives for the treatment of metastatic castration-resistant prostate cancers. Joelle AZZI Poster 53: Assembly of proteasome and epidermal differentiation: interest in psoriasis. Barbara ZIEBA Poster 54: Expression of the transcriptional coregulator RIP140 in colorectal cancer. Mouna TRIKI Poster 55: Evolutionary Plasticity of Endodermal Gene Regulatory Networks in Ciona intestinalis and Phallusia mammillata. Alicia MADGWICK Poster 56: The role of primary cilia in colon homeostasis and tumor development. Ruizhi TANG Poster 57: The effect of dichloroacetate (DCA) on tumor cell metabolism. Sana BELKAHLA Poster 58: Heterochromatin factors stimulates telomere transcription. Sophie KAN Poster 59: Common variants on XQ28 conferring risk for rheumatoid arthritis in tunisian and french populations. Olfa KHALIFA CBS2 Association assocbs2.com Poster 60: Brucella replication in human trophoblasts: role of the eukaryotic protein CD98hc. Beren GARCIA MENDEZ Poster 61: Identification and characterization of Mabs4780, a new determinant required for intracellular survival and pathogenicity of Mycobacterium abscessus. Iman HALLOUM Poster 62: Role of R2TP/HSP90 system in mouse development and colorectal carcinogenesis. Chloé MAURIZY Poster 63: Phosphoproteomics of 5-HT2A/mGlu2 heteromers: toward new insights into the mechanism of action of hallucinogens and antipsychotics. Samy MURAT Poster 64: Immunodepression and accumulation of cancerous cells: a role of everyday perturbations? Camille JACQUELINE Poster 65: E4F1 is a major regulator of pyruvate metabolism in normal skin homeostasis and skin carcinogenesis. Berfin SEYRAN Poster 66: Risks of in utero NSAIDs and paracetamol exposure on the early development and maturation of the reproductive organs. Moïra ROSSITTO Poster 67: Physiological role of APPL in Drosophila mushroom bodies’ development. Claire MARQUILLY Poster 68: Role of the transcription factor RIP140 in colon cancer. Nour SFEIR Poster 69: Characterization of host cell proteins recruited at the Moving Junction during invasion of Toxoplasma gondii. Amandine GUERIN Poster 70: MLN4924, a NEDD8 inhibitor in a p53 based cyclotherapy approach. Lara BOU MALHAB Poster 71: Ribosome: Master Regulator of Cancer Cell Fate? Laura YAZDANI Poster 72: Pattern of drug metabolism enzyme expression in the epileptic brain: a new mechanism of drug resistance. Badreddine BOUSSADIA Poster 73: Determinants for UBA1 recruitment at sites of DNA damage. Ramhari KUMBHAR CBS2 Association assocbs2.com Poster 74: The effect of microbial LPS translocation in cross-presenting dendritic cells and in the breakdown of CD8+ T cell peripheral tolerance in irradiated mice. Gabriel ESPINOSA Poster 75: A new integrated platform for drug action mode determination in C. elegans. Myriam RICHAUD Poster 76: Transient infection induces chronic inflammation. Quang Tien PHAN 17h45-18h: Report of the PhD-Company training 18h-18h15: Award ceremony To reward the best of you and win a large variety of gifts… 17h45-18h: Coktail And don’t forget the party tonight… ! CBS2 Association assocbs2.com CBS2 Association assocbs2.com Invited Speakers Michel Tibayrenc CBS2 Association assocbs2.com « The predominant clonal evolution (PCE) concept of microbial pathogens » Maladies Infectieuses et Vecteurs Ecologie, Génétique, Evolution et Contrôle (MIVEGEC), Institut de Recherche pour le Développement (IRD), Montpellier, France. We propose that predominant clonal evolution (PCE) in microbial pathogens be defined as restrained recombination on an evolutionary scale, with genetic exchange scarce enough to not break the prevalent pattern of clonal population structure. The main features of PCE are: (i) strong linkage disequilibrium (LD); (ii) the widespread occurrence of stable genetic clusters blurred by occasional bouts of genetic exchange (“near-clades”). We hypothesize that the PCE features are not mainly due to natural selection, but chiefly originate from in-built genetic properties of pathogens. We show that the PCE model obtains even in microbes that have been considered as “highly recombining”, such as Neisseriameningitidis, and that some clonality features are observed even in Plasmodium, which has been long described as panmictic. Lastly, we evidence that PCE features are also observed in viruses, taking into account their extremely fast genetic turnover. The PCE model provides a convenient population genetic framework for any kind of micropathogen. It makes it possible to describe convenient units of analysis (clones and near-clades) for all applied studies. Lastly, the PCE model opens up the possibility of revisiting the problem of species definition in these organisms, which are responsible for devastating human, animal and crop diseases. CBS2 Association assocbs2.com Serge Bauin « Decide to publish in open access: what risks for my career? » Coordinateur des politiques d’IST - COMUE Université Sorbonne Paris Cité et Chargé de mission pour le libre accès - DIST (Direction de l'Information Scientifique et Technique) du CNRS. After having founded and led the unit in charge of science policy indicators CNRS, Serge Bauin has been director of the IST at the CNRS and director of the INIST from 2010 to 2013. Today, he is coordinator of IST policies within the Sorbonne Paris Cité COMUE University and “ambassador” for open access at the CNRS. He also serves on the scientific advisory board of the Observatory of Science and Technology. Source : oam.biu-montpellier.fr CBS2 Association assocbs2.com CBS2 Association assocbs2.com Short Talks : Session 1A Genopolys Amphi CBS2 Association assocbs2.com N°1 - Lauriane SOLLELIS Efficient CRISPR-Cas9-mediated genome editing of Leishmania parasites Protozoan pathogens that cause leishmaniasis in humans are difficult to manipulate genetically. In this work we implemented the CRISPR-Cas9 system to Leishmania parasites and demonstrate its efficient use for genome editing. The Cas9 endonuclease was expressed under the control of the DHFR promoter and the single guide RNA was produced under the control of the U6snRNA promoter and terminator. As proof of concept we chose to knockout a tandemly repeated gene family, the paraflagellar rod2 (PFR) loci. We were able to obtain null mutants in a single round of transfection. In addition, we confirmed the absence of off-target editions by whole genome sequencing of two independent clones. Our work demonstrates that CRISPR-Cas9mediated gene knockout represents a major improvement in comparison with the classical method. Beyond gene knockout, this genome editing tool opens avenues for a multitude of functional studies to speed up research on leishmaniasis. Lauriane Sollelis1,2, Mehdi Ghorbal1,2, Cameron Ross MacPherson3, Rafael Miyazawa Martins3, Nada Kuk1, Lucien Crobu2, Patrick Bastien1,2,4, Artur Scherf3, Jose-Juan Lopez-Rubio1,2 and Yvon Sterkers1,2,4 1 University of Montpellier, Faculty of Medicine, Laboratory of ParasitologyMycology, 2 CNRS 5290 - IRD 224 – University of Montpellier (UMR "MiVEGEC"), 3 Institut Pasteur – INSERM U1201 - CNRS ERL9195, Biology of Host-Parasite Interactions" Unit, Paris, France, 4 CHRU (Centre Hospitalier Universitaire de Montpellier), Department of Parasitology-Mycology, Montpellier, France CBS2 Association assocbs2.com N°2 - Emmanuelle COQUE Implication of CD8+ T cells in the pathophysiology of amyotrophic lateral sclerosis Amyotrophic lateral sclerosis (ALS) is a fatal neurodegenerative disorder caused by the loss of motoneurons. ALS leads to the atrophy and paralysis of the striated muscles, which will cause death within 3 to 5 years. Approximately 10% of ALS cases are genetically linked, and among these, 20% are caused by mutations in SOD1 gene. Mice overexpressing human SOD1 mutations develop a motor syndrome with features of the human disease. A chronic inflammatory response, associated with the accumulation of blood-derived immune cells in the CNS, is a pathological feature of ALS. Firstly, CD4+ lymphocytes invade the CNS and seem to negatively regulate the inflammatory response. However, the early symptomatic phase is characterized by an increase of CD8+ T cells in the CNS. Those CD8+ T cells are effectors of adaptive and innate immunity and can promote cytotoxic effects, however, the contribution of this cell population in the neurodegenerative process has been poorly investigated. Here, we propose to explore the impact of the infiltration of CD8+ T cells on the development of the disease. Our results show that CD8+ T cells isolated from SOD1G93A, but not from wildtype mice, trigger motoneuron death, selectively. Our co-culture experiments showed that CD8+ T cells trigger motoneuron death in a contact dependent-manner. Moreover, we showed that this contact requires the recognition of the MHC-I complex exposed by motoneurons. Our results suggest that inhibition of IFNγ, and perforin/granzyme pathway, two classical mechanisms of CD8+ T cells cytotoxicity, saves motoneuron from the CD8+ T cell-mediated toxicity. Beside this in vitro analysis, one of the main objective of this project is to assess the therapeutic effect of an immunodepletion of CD8+ T cells in the SOD1G93A mice. To this aim, we developed a protocol of long term immunodepletion of CD8 cells. Coque, E. (Montpellier)1, Carrasco, G.E. (Montpellier)2, Salsac, C. (Montpellier)1, Vincent, T. (Montpellier)1,3, Hernandez, J. (Montpellier)2, Raoul, C. (Montpellier)1 1 : INSERM U1051 - Déficits sensoriels et moteurs, Montpellier, France. 2 : INSERM U844, Montpellier, France. 3 : Hopital Saint Eloi, Département d'immunologie, Montpellier, France CBS2 Association assocbs2.com N°3 - Coralie DAUSSY Autophagy Restricts HIV-1 Infection by Selectively Degrading Tat in CD4 T Lymphocytes Autophagy is a ubiquitous mechanism involved in the lysosomal-mediated degradation of cellular components when they are engulfed in vacuoles called autophagosomes. Autophagy is also recognized as an important regulator of the innate and adaptive immune responses against numerous pathogens, which have, therefore, developed strategies to block or use the autophagy machinery to their own benefit. Upon human immunodeficiency virus type 1 (HIV-1) infection, viral envelope (Env) glycoproteins induce autophagy-dependent apoptosis of uninfected bystander CD4 T lymphocytes, a mechanism likely contributing to the loss of CD4 T cells. In contrast, in productively infected CD4 T cells, HIV-1 is able to block Env-induced autophagy in order to avoid its antiviral effect. To date, nothing is known about how autophagy restricts HIV-1 infection in CD4 T lymphocytes. Here, we report that autophagy selectively degrades the HIV-1 transactivator Tat, a protein essential for viral transcription and virion production. We demonstrated that this selective autophagy-mediated degradation of Tat relies on its ubiquitinindependent interaction with the p62/SQSTM1 adaptor. Taken together, our results provide evidence that the anti-HIV effect of autophagy is specifically due to the degradation of the viral transactivator Tat but that this process is rapidly counteracted by the virus to favor its replication and spread. Coralie F. Daussy*, Sophie Sagnier*, Sophie Borel*, Véronique Robert-Hebmann*, Mathias Faure¤, Fabien P. Blanchet*,Bruno Beaumelle*, Martine BiardPiechaczyk*, Lucile Espert* * : CPBS, Université de Montpellier, UMR 5236 CNRS, Montpellier, France; ¤ : CIRI, International Center for Infectiology Research, Université de Lyon, Lyon, France; INSERM U1111, Lyon, France;Ecole Normale Supérieure de Lyon, Lyon, France;Université Lyon 1, Centre International de Recherche en Infectiologie, Lyon, France;CNRS, UMR 5308, Lyon, France CBS2 Association assocbs2.com Short Talks : Session 1B IGF South Seminar Room (2nd Floor) N°4 - Ankit DWIVEDI CBS2 Association assocbs2.com Characterization of P.falciparum sub-populations associated to artemisinin drug resistance in Cambodia Malaria is one of the most widespread parasitic infections in the world. The undergoing WHO Malaria elimination programs are threatened by emergence of the Plasmodium falciparum artemisinin resistant parasite in South-East Asia. These parasites have emerged in the western part of Cambodia, where chloroquine and pyrimethamine drug resistance emerged in the past. Based on recent reports of 1) the presence of P.falciparum sub-populations in Cambodia (Miotto O. et al., 2013) and 2) evidence that mutations in the K13 gene are supporting artemisinin resistance in Cambodian parasite population (Ariey F. et al., 2014), we characterize the metabolic properties of parasite sub-populations. We use a large dataset based on NGS genome sequences from ENA database to analyze the distribution of parasite population over the country. We describe a reliable SNP variant calling pipeline from around 200 genome sequences based on signal parameters. The parasite sub-populations were defined based on SNP set obtained using this pipeline. We provide genetic evidence that acquisition and transmission of artemisinin resistance is related to parasite population structure in Cambodia. We identify features providing functional annotation for proteins, pathways, isolates and sub-populations. Parasite populations from western Cambodia have different metabolic capacities than eastern populations. We develop a barcode approach based on LUMINEX technology to rapidly screen for the organization of the parasite population over the country. We successfully genotypes about 300 samples. We identify a new sub-population in the south that is associated to the emergence of the most common C580Y K13 mutation. Also, observed admixture parasite population is a major risk because of the metabolic capacities and ability of the parasites to cross within sub-populations and with the members of other sub-populations. These results question the origin and the persistence of the P.falciparum sub-populations in Cambodia. Ankit Dwivedi[1][2], Christelle Reynes[3], Nimol Khim[4], Didier Ménard[4], Emmanuel Cornillot[2][5] [1] Centre d’études d’agents Pathogènes et Biotechnologies pour la Santé (CPBS), Montpellier, France. [2] Institut de Biologie Computationelle (IBC), Montpellier, France. [3] Institut de Génétique Humaine (IGH), Montpellier, France. [4] Institut Pasteur du Cambodge (IPC), Cambodia. [5] Institut de Recherche en Cancérologie de Montpellier (IRCM), Montpellier, France CBS2 Association assocbs2.com N°5 - Jolanta JAGODZINSKA Wfs1-/- mice: phenotyping and gene therapy against Wolfram Syndrome The Wolfram Syndrome (WS) is an early onset genetic disease (1/200 000) featuring diabetes mellitus and progressive optic neuropathy ensuing mutations in the WFS1 gene. We investigated mice with deleted exon 8 of the gene to imitate the visual aspects of the disease. The model has been known to exhibit pancreatic β-cell atrophy but the visual function has not yet been investigated. Therefore, we focused on assessing it via in vivo and post mortem studies of Wfs1+/+ and Wfs1-/- mice at 3 and 7 months of age. We examined visual acuity via changes in the optokinetic relfex, retinal ganglion cell (RGC) function via post-scotopic treshold responce (pSTR), and eye physiology via eye fundus observation and optical coherence tomography (OCT). We also determined proportion of retinal ganglion cells (RGC) and axonal loss at the age of 7 months, with anti-Brn3a immuno-labeling of retinal sections and electron microscopy of optic nerve (ON) sections, respectively. We observed progressive loss of visual acuity accompanied by loss of axons in the ON and pallor of the optic disc. Next, we performed an intravitreal gene therapy (GT) with AAV-2/2-CMV-WFS1 at 1 month old Wfs1+/+ and Wfs1-/- mice. The assessment of the visual acuity and the RGC function at 3 and 6 months of age showed no worsening of the vision originating from GT nor the injections themselves. Importantly, the visual acuity of WFS1-/- mice after GT was improved and the deterioration of RGC function was slower with age. Furthermore, the controls injected with AAV-2/2-CMV-GFP showed even distribution of its expression in the retina. The study is ongoing for histological analysis. The presented data qualify the murine model for investigating visual aspects of WS. Additionally, the promising preliminary results of the gene therapy encourage further studies under a treatment for the Wolfram Syndrome patients. JAGODZINSKA Jolanta1, BONNET-WERSINGER Delphine1, KOKS Sulev 2, SEVENO Marie1, LENAERS Guy1, HAMEL Christian1, DELETTRE Cecile1. 1 CHU Montpellier, Institut des Neurosciences de Montpellier INSERM U1051, Montpellier, France. 2University of Tartu, University of Tartu, Tartu, Estonia CBS2 Association assocbs2.com N°6 - Salomé LEPRINCE New self-deployable, bioresorbable and anti-adhesive medical device for the prevention of intrauterine adhesions Synechiae or intrauterine adhesions result in the fibrous adherence of opposing uterine walls, which produce partial or complete obliteration in the uterine cavity and/or the cervical canal. Trauma to a gravid uterine cavity is known to be the main cause of adhesions formation. Uterine curettage in the postpartum period, cesarean section, spontaneous miscarriage, abortion or termination of pregnancy are predisposing factors of adhesions formations. This pathology can cause menstrual abnormalities, pelvic pain, infertility and recurrent pregnancy loss [1]. In order to prevent postsurgical adhesion formation across the cavity, a new antiadhesive and bioresorbable medical device was developed to maintain separated uterine walls after surgical trauma. Anti-adhesive barrier from PLA50-PEO-PLA50 (polylactic acid – polyethylene oxyde – polylactic acid) triblock copolymer has been synthesized. This copolymer presents a strong hydrophilic character to promote swelling in water and hydrolytic degradation. Moreover high molecular weights of PEO allow to obtain excellent filmogenic properties and provide anti-adhesive properties. Biocompatibility and anti-adhesive effects of triblock were evaluated using human endometrial cells. Anti-adhesive efficiency and degradation rate of triblock copolymer were studied by implantation between cecum and peritoneal wall defects of rats. Copolymer films provide an excellent candidate as a anti-adhesion barrier owing to its anti-adhesion potential, as well as its flexibility and biodegradability. In order to provide the ideal morphology of the medical device, the next step will be the production of medical device by using 3-D printing technology (fused deposition modeling). This barrier aims at providing a preventive tool to limit the formation of adhesions after an endometrial trauma and restoring normal reproductive functions. This medical device meets the clinical requirements of the gynecologic surgeons and could become a new tool for the management of female infertility. [1] D. Yu. Fertility and Sterility 2008, 89, 759. S. Leprince1*, S. Huberlant1-2, V. Letouzey1-2, I. Le Teuff1-2, C. Paniagua1, J. Coudane1, X. Garric1. 1 Institut des Biomolécules Max Mousseron, CNRS UMR 5247, Faculté de Pharmacie, Université Montpellier, France. 2 Service de Gynécologie et Obstétrique, CHU Carémeau, Nîmes, France CBS2 Association assocbs2.com Short Talks : Session 2A Genopolys Amphi N°7 - Laura AUBOYER CBS2 Association assocbs2.com Generation of Alzheimer's disease (AD) genetic patients’ reprogrammed stem cells (iPS) as tools for the diagnostic and therapeutic researches for AD Amyloid precursor protein (APP) and Tau protein are two main molecular actors of neurodegenerative affections, which are of prime importance in Human Health (Alzheimer’s disease (AD)). Intensive research is ongoing to understand these proteins’ metabolism, action and implication in the pathological mechanism of these affections. They are the target of most therapeutic approaches and are used for biological diagnosis. In the present program, our objective is to investigate neuronal APP and Tau protein processing and metabolism using biochemical tools (single and multiplex immunodetection system (ELISA, Luminex®, MSD®)), innovative detection methods (mass spectrometry (MS)) and metabolic approach (incorporation of stable isotope labelled Leucine (6C13L)) in two complementary situations: in vivo in patients, and in vitro in cell culture. The goal is to get a comprehensive proteomic view (synthesis, cleavage, interaction..) based on the parallel analysis of patient isotope labelled samples (already available following perfusion of 6C13Leu and kinetics sampling of CSF) and samples generated in neuronal differentiated human embryonic stem cell and Induced pluripotent stem cells derived from AD-patients where pharmacological tools (secretase/kinase inhibitors) can be tested. The final goal is therefore to parallel the data in patients with those generated in differentiated iPS cells and control hESC cells. This project will offer the unique opportunity to combine state-to-the-art approaches to understand how the APP fragments and peptides are generated as well as the modifications of the Tau protein in normal and pathological situation. Auboyer, L. (Montpellier)1, Radreau, F. (Montpellier)1, Monzo, C. (Montpellier)1, Gabelle, A. (Montpellier)1, Lehmann, S. (Montpellier)1, Crozet, C. (Montpellier)1 1Institut de Médecine Régénératrice et de Biothérapie (IRMB), Montpellier, France CBS2 Association assocbs2.com N°8 - Christelle CADILHAC Shifts in Migration route: Insights into GABAergic Interneurons Diversity GABAergic cell diversity is critical for proper function of neural circuitry. In the developing brain, GABAergic interneurons use stereotyped migration route and schedule to reach their specific laminar position. Whether and how their migration journey impacts their stereotyped differentiation is not known. This is quite exemplified by cerebellar Molecular Layer GABAergic Interneurons (MLGI), which are the Basket and the Stellate cells. MLGI display major morphological differences but present no discriminating genetic marker. It has been proposed that these differences are due to distinct laminar position underlying distinct environmental cues, however there is no clear evidence to support this view. In this study, we provided insights on how local control of migratory pathways may contribute to specific cell-type differentiation program by acting as a time-shifting device. By using in vivo grafts experiments of GABAergic progenitors, we identified two distinct integration paths of MLGI. We conducted a series of time-lapse experiments on acute slices and uncovered that all MLGI entered the molecular layer using radial migration while only a proportion of interneurons performed an additional step of tangential migration in the external granule cell layer. In addition, we showed that this unexpected tangential migration took place in a define window of cerebellar development along a subpopulation of pre-migratory granular cells expressing the cell-adhesion molecule TAG1. TAG1 blocking antibody disrupts the tangential migration in acute slices and important granular cell axons reorganization revealed by TAG1 gain of function in organotypic slices favors ectopic migration of MLGI. These results show the implication of granular cell axons as a physical support for this particular migratory process. Finally, we demonstrated, using hybrid organo-grafts experiments, that interneurons capable of tangential migration belong to the Stellate cell population. Together, these findings reveal how shifts in migration itinerary of neural progenitors impacted their cell fate differentiation program. Christelle Cadilhac, Fabrice Ango (IGF, UM, CNRS, INSERM) CBS2 Association assocbs2.com N°9 - Mirela D'ARC Origin of the HIV-1 group O epidemic in Western Lowland Gorillas HIV-1 and HIV-2 are the result of multiple viral cross-species transmissions from Simian Immunodeficiency Viruses (SIVs) infecting Non Human Primates (NHP) to humans. HIV-1 is the principal responsible for the global AIDS epidemic. HIV-1 is divided into four phylogenetic lineages,called groups M, N, O, and P, which resulted each from an independent cross-species transmission event of SIVs infecting African apes. Although groups M and N have been previously traced to distinct chimpanzee communities in southern Cameroon, the reservoirs of groups O and P remained unknown. Here, we present the results recently published in PNAS journal, where we screened fecal samples from western lowland (n = 2,611), eastern lowland (n = 103), and mountain (n = 218) gorillas for gorilla SIV (SIVgor) antibodies and nucleic acids. SIVgor was identified at only four sites in southern Cameroon. Amplification of partial and full-length SIVgor sequences revealed extensive genetic diversity, but all SIVgor strains were derived from a single lineage within the chimpanzee SIV (SIVcpz) radiation. Two fully sequenced gorilla viruses from southwestern Cameroon were very closely related to, and represent the source population of, HIV-1 group P. Most of the genome of a third SIVgor strain, from central Cameroon, was very closely related to HIV-1 group O, again pointing to gorillas as the immediate source. Functional analyses identified the cytidine deaminase APOBEC3G as a barrier for chimpanzee-to-gorilla, but not gorilla-to-human, virus transmission. These data indicate that HIV-1 group O, which spreads epidemically in west central Africa and is estimated to have infected around 100,000 people, originated by cross-species transmission from western lowland gorillas. Thus, both chimpanzees and gorillas harbor viruses that can that are capable of crossing the species barrier to humans and causing major disease outbreaks. Mirela D’arca,b, Ahidjo Ayoubaa, Amandine Estebana, Gerald H. Learnc, Vanina Bouéa,d, Florian Liegeoisa,d, Lucie Etiennea, Nikki Tagge, Fabian H. Leendertzf, Christophe Boeschg, Nadège F. Madindaf,g,h, Martha M. Robbinsg, Maryke Grayi, Amandine Cournila, Marcel Oomsj,k, Michael Letkoj,k, Viviana A. Simonj,k,l, Paul M. Sharpm, Beatrice H. Hahnc, Eric Delaportea, Eitel Mpoudi Ngolen, and Martine Peetersa,o aUnité Mixte Internationale 233, Institut de Recherche pour le Développement, INSERM U1175, and University of Montpellier, 34394 Montpellier, France; bLaboratory of Human Virology, Universidade Federal do Rio de Janeiro, 21949-570 Rio de Janeiro, Brazil; cDepartments of Medicine and Microbiology, Perelman School of Medicine, University of Pennsylvania, Philadelphia, PA 19104; dCentre International de Recherches Médicales, CBS2 Association assocbs2.com Franceville, Gabon; eProjet Grands Singes, Center for Research and Conservation, Royal Zoological Society of Antwerp, 2018 Antwerp, Belgium; fEpidemiology of Highly Pathogenic Microorganisms, Robert Koch Institute, 13353 Berlin, Germany; gDepartment of Primatology, Max Planck Institute for Evolutionary Anthropology, 04103 Leipzig, Germany; hInstitut de Recherche en Ecologie Tropicale, Libreville, Gabon; iInternational Gorilla Conservation Programme, Kigali, Rwanda; jDepartment of Microbiology, kGlobal Health and Emerging Pathogens Institute, andlDivision of Infectious Diseases, Department of Medicine, Icahn School of Medicine at Mount Sinai, New York, NY 10029; mInstitute of Evolutionary Biology, and Center for Immunity, Infection, and Evolution, University of Edinburgh, Edinburgh EH9 3JT, United Kingdom; nInstitut de Recherches Médicales et d’Études des Plantes Médicinales, Prévention du Sida au Cameroun, Yaoundé, Cameroon; and oComputational Biology Institute, 34095 Montpellier, France CBS2 Association assocbs2.com CBS2 Association assocbs2.com Short Talks : Session 2B IGF South Seminar Room (2nd Floor) N°10 - Girisaran GANGATHARAN CBS2 Association assocbs2.com Molecular Mechanisms of Zebrafish Cardiac Regeneration The human heart’s inability to replace ischemia-damaged myocardium with regenerated muscle results significantly in the worldwide mortality associated with coronary artery disease. Remarkably, certain vertebrate species, such as the zebrafish, achieve complete regeneration of the amputated or injured myocardium through the proliferation of cardiomyocytes. Here, we report a bHLH transcription factor as a critical regulator of the cardiomyocyte mediated heart regeneration. This gene is known to be a key regulator of erythroid cell differentiation and endocardium formation, but its role in cardiomyocytes has not been reported previously. Immunohistochemical studies reveal its presence in cardiomyocytes. Using transgenic fish, we discovered that suppression of this gene specifically in the cardiomyocyte profoundly impairs cardiac regeneration. Next, we also hypothesized that genes involved in cardiac development could be reutilized during cardiac regeneration. Using a drug inhibition approach, we have identified upto 7 genes involved in this process. Specifically, we are characterizing the role of a family of genes in scar regression during cardiac regeneration. Girisaran Gangatharan and Chris Jopling Institut de Génomique Fonctionnelle, Montpellier, France. CBS2 Association assocbs2.com N°11 - Romain RISCAL Chromatin-bound MDM2 regulates serine metabolism and redox homeostasis independently of p53 Although the Mouse Double Minute 2 (MDM2) oncoprotein is a major negative regulator of the p53 tumor suppressor growing evidence supports p53-independent functions of MDM2. Here we describe a new p53-independent function for MDM2 in cancer cell metabolism. We show that MDM2 is recruited to chromatin independently of p53 to regulate a transcriptional program implicated in amino acid metabolism and redox homeostasis. Genome-wide MDM2 ChIP-seq experiments combined with gene expression profiling identified MDM2-responsive genes and highlighted an important role for chromatin-associated MDM2 in serine/glycine and glutathione metabolism. MDM2 recruitment to its target genes required members of the ATF family of transcription factors and this event is modulated by the M2 isoform of pyruvate kinase (PKM2), a rate-limiting metabolic enzyme that controls the glycolytic flux and its branched biosynthetic pathways. Interestingly, MDM2 recruitment to chromatin increases in specific stress conditions known to impinge on PKM2 activity, including oxidative stress and serine deprivation. Moreover, chromatin-bound MDM2 controls the pool of reduced and oxidized glutathione that impacted on reactive oxygen species (ROS) levels. Interfering with MDM2 expression and exogenous serine availability decreases cell survival in vitro and tumor growth in vivo, the latter being rescued, at least partly, by the ROS scavenger N-acetyl cysteine. Our data indicate that MDM2 is a key regulator of the balance between de novo serine synthesis and serine auxotrophy and of the redox status of cancer cells independently of p53. Romain Riscal1,2,3,4, Emilie Schrepfer1,2,3,4, Giuseppe Arena1,2,3,4, Frédérique Sabourdy5,6, Charles Vincent1,2,3,4, Imade Ait-Arsa1,2,3,4, Thierry Levade5,6, Jean-Christophe Marine7,8, JeanEmmanuel Sarry6, Laurent Le Cam1,2,3,4,9* and Laetitia K. Linares1,2,3,4,9*. 1IRCM, Institut de Recherche en Cancérologie de Montpellier, Montpellier, F-34298, France. 2INSERM, U1194, Montpellier, F-34298, France. 3Université Montpellier, Montpellier, F34298, France. 4Institut régional du Cancer Montpellier, Montpellier, F-34298. 5Laboratoire de Biochimie Métabolique, IFB, CHU Purpan, Toulouse, France. 6 INSERM UMR 1037, CRCT, Université Paul Sabatier Toulouse-III, Toulouse, France. 7Laboratory for Molecular Cancer Biology, Center for the biology of disease, VIB, 3000 Leuven, Belgium. 8Laboratory for Molecular Cancer Biology, Center for human genetics, KU Leuven, 3000 Leuven, Belgium. 9Corresponding authors: [email protected] (L.L.C.) and [email protected] (L.LK) CBS2 Association assocbs2.com N°12 - Filippo CIABRELLI Polycomb-Mediated Repression in Transgenerational Epigenetic Inheritance Transgenerational epigenetic inheritance is a hotly debated phenomenon whereby a non-genetically determined phenotype can be transmitted to the next generation. So far, this mode of inheritance has been described in few cases and it was suggested that chromatin components might be involved, including Polycomb group proteins, which act as repressors of key developmental genes and coordinate cell differentiation and proliferation. The molecular mechanisms linking Polycomb-mediated silencing to transgenerational epigenetic inheritance are far from being understood. Therefore, we developed an experimental system in Drosophila melanogaster to induce stable transgenerational epigenetic inheritance, in which alternative gene expression states can be inherited in the presence of the same genetic sequence. Starting from these highly stable epilines, we could dissect some of the genetic properties of the induced epialleles, such as their quantitative inheritance and their ability to trans-communicate. Moreover, the epialleles displayed synergy in their expression and transmission. One of the molecular signatures of the epialleles is the differential presence of the Polycomb repressive complexes and their related epigenetic marks. This diverse distribution is independent of the transcriptional activity of the downstream genes, at least in an early developmental stage, and could influence the three-dimensional organization of the locus involved. Intriguingly Ago2, an RNAi pathway component, has been found to genetically interact with the epialleles and to be directly bound on their chromatin, indicating a possible role for the ncRNAs in the expression of the epialleles and possibly in their transmission. Our results make a case for strong and stable transgenerational epigenetic inheritance in metazoan and provide a model that is amenable for the molecular dissection of this phenomenon. Filippo Ciabrelli 1, Frederic Bantignies 1, Boyan Bonev 1, Simon Fellous 2, Anne Xuereb 2, Giacomo Cavalli 1. IGH, CNRS UPR 1142, 141 rue de la Cardonille, 34090 Montpellier.CBGP, Avenuedu Campus Agropolis, 34980 Montferrier-sur-Lez. CBS2 Association assocbs2.com Posters : Session 1 CBS2 Association assocbs2.com N°1 - Marion LE GALL Quantifying the pressure thresholds for tissue injury in paraplegic patients A pressure ulcer (PU) is a localized injury to the skin and/or the underlying tissue mainly affecting people who lost their mobility or with sensory impairment. It is associated with morbidities, a decrease of the patient life quality and increase of the hospital length of stay. Nowadays prevention is still the best way to prevent PU. However, no damage threshold is unanimously accepted by professionals and the patient specificities would make any average limit level irrelevant for clinical use. The main goal of this research project is to gain a thorough quantitative understanding of the relationship between interface pressures (IP), microvasularisation and tissue inflammation involved in PU genesis. The objective is to detect, for each patient, the early stage of irreversible cell damage. Interface pressures between the patient body and the air-mattress and local microvascularisation measurement are continuously recorded on paraplegics for 3 hours (corresponding to the routine frequency of pressure points mobilization). Furthermore, specific inflammation markers can be quantified from muscle biopsies and correlated with those two parameters. Depending on how long the patient is lying on the air-mattress and how high the IP intensity is, a tissue damage threshold could be identified for each patient. The results of this PhD study will gather new clinical data to improve the PU detection sensibility and the prevention efficiency. M. Le Gall M.Sc.1, A. Lacampagne Ph.D.1, L. Teot M.D. Ph.D.2, S. Matecki M.D. Ph.D.1, C. Trial M.D.2 1 French Institute of Health and Medical Research U1046, CNRS 9214, Physiology and Experimental Medicine: Heart and Muscles, F-34295 Montpellier, France. 2 Department of Wound Healing Unit, Montpellier Regional University Hospital, Montpellier, France CBS2 Association assocbs2.com N°2 - Hayeon BAIK Role of SUMOylation and Reactive Oxygen Species (ROS) in Acute Myeloid Leukemia (AML) treatment Acute myeloid leukaemias (AML) are severe haematological malignancies characterized by the accumulation of malignant immature myeloid precursors in the bone marrow. Their treatment mainly relies on chemotherapy. However, relapses are frequent, which explain the poor prognosis. We have recently shown that SUMO, a post-translational modifier of the ubiquitin family, and its regulation by Reactive Oxygen Species (ROS) plays a critical role in AML response to chemotherapeutic drugs. A first part of my thesis project aims at charactering the role of SUMO and ROS in AML chemoresistance. To this aim, I generated AML cell lines (HL-60 and U937) resistant to clinically used drugs (cytarabine and daunorubicin). We could show that the chemoresitant AML cells present large increase in ROS production, which are due to the activation of the Nox2 NADPH oxidase at the transcriptional level. Knock down of Nox2 could sensitize AML cells to chemotherapeutic drugs. In addition, these cells present higher levels of SUMO. My project now aims at continuing the characterization of the role of Nox2 and SUMO in chemoresistance, in particular through the use of patient samples and animal models. Differentiation therapies constitute a promising alternative to chemotherapy for AML treatment. However, their clinical use is currently limited to acute promyelocytic leukaemia (APL), a subtype of AML, that is successfully treated by all-trans-retinoic acid (ATRA) induced-differentiation. So far, ATRA or other differentiating agents such as Vitamin D3 have not been successful for the treatment of non-APL leukemias. The second part of my project is to study whether the inhibition of sumoylation could promote the ATRA or Vitamine D3 induced differentiation of non APL AML. To this aim, the role sumoylation in AML differentiation, in particular in the regulation of gene expression, will be investigated both by pharmacological and genetic approaches. Hayeon Baik, Tamara Salem, Yosr Hichri, Guillaume Cartron, Jean-Emmanuel Sarry, Christian Récher, Marc Piechaczyk Guillaume Bossis CBS2 Association assocbs2.com N°3 - Marko RISTIC Global regulation of the SUMO pathway during Acute Myeloid Leukemia treatment with chemotherapeutic drugs Acute Myeloid Leukemia (AML) is a severe hematological malignancy with poor prognosis, whose treatments have not significantly changed during the past 30 years. The standard induction chemotherapy relies on a combination of the nucleoside analogue cytarabine (Ara-C) with an anthracyclin, such as daunorubicin (DNR). We have recently reported that one of their early effects is the deconjugation of the ubiquitin-like protein SUMO from its targets. This desumoylation is due to Reactive Oxygen Species(ROS)-dependent inhibition of the SUMO-conjugating enzymes through the formation of a disulfide-bond between E1 and E2 catalytic cysteines. This desumoylation is involved in transcriptional activation of specific genes and participates in the induction of apoptosis. In chemoresistant AML cells, chemotherapeutic drugs do not induce this ROS/SUMO axis. However, its reactivation by pro-oxidants or inhibition of the SUMO pathway restores apoptosis in chemoresistant cell lines and patient samples. Finally, inhibition of the SUMO pathway decreases tumor growth in mice xenografted with chemoresistant AML cells. Thus, targeting the ROS/SUMO axis might constitute a novel therapeutic strategy for AML patients resistant to conventional chemotherapies. To understand, at a global scale, which proteins are changing their sumoylation upon AML chemotherapeutic drug treatment, we recently performed, in the model AML cell line HL60, a SILAC Mass spectrometry approach. We could identify around 1000 sumoylated proteins.Among them, around 100 were desumoylated upon short DNR or Ara-C treatment (2 hours). These desumoylated proteins were mostly involved in the regulation of gene expression, confirming the role of genotoxics-induced desumoylation in the control of transcription. Interestingly, a small group of proteins showed up-sumoylation upon DNR and Ara-C treatment. These proteins are mostly involved in DNA Damage Response suggesting that their up-sumoylation could be involved in DNA repair. Our ongoing work is aimed at characterizing the role of their sumoylation in AML response to chemotherapeutic drugs. Jon Otti Sigurdsson and Jesper V. Olsen - Center for protein research, Novo Nordisk Foundation, Copenhagen Marko Ristic and Guillaume Bossis - IGMM, CNRS, Montpellier CBS2 Association assocbs2.com N°4 - Loic LIONNARD Identification of factors involved in proteasomemediateddegradation of anti-apoptotic Bfl-1 Apoptosis or programmed cell death plays a crucial role in tissue homeostasis and is regulated by the Bcl-2 proteins, which control mitochondria membrane permeability and cytochrome c release, two events that precede cell demise. Anti-apoptotic Bcl-2 family members can contribute to tumorigenesis and cause resistance to anti-cancer regimens, therefore representing important targets for novel therapeutics. Bfl-1, an anti-apototic Bcl-2 protein is often overexpressed in poor prognosis lymphoma and chemoresistant melanoma. Since no inhibitor blocks efficiently Bfl-1-mediated prosurvival activity in tumor cells, alternative strategies have to be found to inhibit it. Previous studies have shown that Bfl-1 is a short-lived protein, whose expression is tightly controlled by ubiquitination. Indeed, Bfl-1 can be ubiquitinated on its Cterminal part and degraded by the proteasome. Moreover, the phosphorylation status of proximal residues 152S and/or 156T inhibits proteasome-mediated Bfl-1 degradation. Our preliminary results of in vitro phosphorylation assay identified GSK3 as a protein kinase involved in the phosphorylation of Bfl-1 C-terminal part. In addition, this work identified TRIM28 and TRIM17, two members of the TRIM protein family (one of the subfamilies of RING type E3 ubiquitin ligases), as interactors that may influence polyubiquitination and proteasomal turnover of Bfl-1. Overall, the thesis project aims at characterizing the mechanisms through which these factors control Bfl-1 stability. This work may open new avenue to promote Bfl-1 degradation and thus reactivate apoptosis in tumors that are reliant on Bfl-1 overexpression. Loïc Lionnard1, Aurélie Cornut-Thibaut2, Abdel Aouacheria2, Claude Cochet3, Solange Desagher1 and Jérôme Kucharczak1,2. 1 Institut de Génétique Moléculaire de Montpellier, IGMM UMR 5535 CNRS, 1919 route de Mende, 34293 Montpellier cedex 5, France.2 Laboratoire de Biologie Moléculaire de la Cellule, Faculté de Médecine Lyon-Sud, LBMC UMR 5239 CNRS – UCBL – ENS Lyon - HCL, 46 Allée d’Italie, F-69364 Lyon Cedex 07, France.3 CEA Grenoble, iRTSV/BCI INSERM U1036, 17 rue des Martyrs, 38054-Grenoble, France CBS2 Association assocbs2.com N°5 - Fanny IZARD H4K20 methylation pathway, chromatin structure and tumorigenesis Assembled with DNA to form nucleosomes, histone proteins are the basic building blocks of chromatin. A striking feature of histones is that they are subject to a large number of post-translational modifications, including phosphorylation, acetylation, and methylation. These histone modifications are thought to contribute to the regulation of all DNA-templated processes by mediating both alterations in chromatin structure and recruitment of non-histone proteins to specific regions of the genome. Lysine methylation is one of the most intriguing histone modifications in view of its remarkable complexity. It is detected on many histone lysines, each of which can be mono-, di-, or tri-methylated. These modifications occur at highly conserved positions and often cluster within specific regions of the genome to organize chromosomes into distinct structural and functional domains. PR-Set7 is the sole enzyme responsible for the monomethylation of histone H4 at lysine 20 (H4-K20me1), which is required for subsequent catalysis of H4-K20 di- and tri-methylation (H4-K20me2/me3) via the activity of SUV4-20h enzymes. Loss and gain-of function experiments have shown that the concerted activity of H4-K20 enzymes is essential for the regulation of chromatin structure, DNA replication and repair mechanisms, thereby establishing this chromatin-signaling pathway as central in the maintenance of genome integrity. In line with this, breast, colorectal and prostate tumors are often characterized by alterations in levels of different H4-K20me states, which are suspected to play a role in both genesis and progression of cancer cells. The main objective of my thesis is to unravel the functions of H4-K20 enzymes and their marks in the regulation of chromatin structure and determine how alterations in the activity of these enzymes contribute to tumorigenesis. Here, I will show my most promising results and the characterization of new chemical inhibitors of PR-Set7 activity. Fanny IZARD Eric JULIEN (équipe Eric JULIEN, IRCM) CBS2 Association assocbs2.com N°6 - Maude LEVEQUE Toxoplasma gondii AuTophaGy protein 8 has an unusual role in apicoplast division which is essential for parasite growth Autophagy is a self-degradative process which is conserved in most Eukaryotes. It involves a double membrane compartment, called the autophagosome, to sequester and degrade intracellular components. The protein ATG8 (LC3 in mammals) can associate with autophagosomal membranes and it occupies a central position in the autophagy process. Toxoplasma gondii is an obligate intracellular protozoan parasite that can cause congenital toxoplasmosis and a severe pathology in immunocompromised individuals. This parasite possesses an apparently reduced autophagic machinery but is nevertheless able to generate TgATG8-decorated autophagosomes upon stress conditions. Surprisingly in normal growth conditions, this protein mainly localizes to the apicoplast, a non-photosynthetic plastid which hosts essential metabolic pathways. This organelle has been acquired through secondary endosymbiosis and is thus surrounded by four membranes. Biochemical analyses, together with super resolution microscopy imaging, suggest an outer membrane localization of TgATG8 at the apicoplast. With the aim of elucidating the function of this protein, we have generated a TgATG8 conditional mutant. This cell line is severely affected in cell-growth and in the maintenance of the apicoplast. The loss of the organelle occurs rapidly upon parasite division and remaining plastids accumulate in the residual body within the parasitophorous vacuole. This phenotype seems to be a consequence of a replication and/or targeting defect that prevents proper segregation of the organelle into daughter cells during division. Taken together, these results suggest an unusual and essential role for TgATG8 in apicoplast division which is likely independent from canonical autophagy. To decipher this function, we have developed a strategy to label in situ, purify, and identify by mass spectrometry, specific TgATG8 apicoplast partners. Maude LEVEQUE1, Laurence BERRY1, Michael CIPRIANO3, Martial SEVENO2, Boris STRIEPEN3, Sébastien BESTEIRO1 1 DIMNP- UMR5235 CNRS, Université de Montpellier. 2 Plate-forme de Protéomique Fonctionnelle, IGF - UMR5203, CNRS, Université de Montpellier. 3 Center for Tropical and Emerging Global Diseases and Department of Cellular Biology, University of Georgia, Athens, USA CBS2 Association assocbs2.com N°7 - Sarah GUIZIOU An open access part toolbox to tune genetic expression in Bacillus subtilis. Bacillus subtilis is the Gram-positive model and is highly used in industry for enzyme and antibiotic production, yet tools to precisely tune gene expression levels are not widely available. Here we engineered a toolbox of regulatory components with variable strengths (e.g. promoters, RBS) for precisely tuning gene expression in B. subtilis. We first implemented a modular and standardized cassette for genetic circuit construction in B. subtilis to make part constructions and modifications easier and to standardize genetic context. We then selected several promoters found to be constitutive over 104 conditions in the Basysbio project, along with several RBS of various ranks. We then used 3 divergent sequences as templates for randomization and obtained libraries of parts with high variability of strength (range of 500 for promoters and 20 for RBS). We also characterized part activities at the single molecule level with 2-photon microscopy using the scanning number and brightness method, pushing the limits of precision measurements of standard parts activities. This open source toolbox of regulatory components will support the engineering of complex genetic circuits in B. subtilis. All constructs and data will be released in the public domain. Sarah Guiziou1, Vincent Sauveplane2, Hung-Ju Chang1, Nathalie Declerck1, Matthieu Jules2, Jerome Bonnet1. 1 Centre de Biochimie Structurale, INSERM U1054, CNRS UMR5048, University of Montpellier, France. 2 INRA, AgroParisTech, UMR1319 Micalis, Thiverval-Grignon, France. CBS2 Association assocbs2.com N°8 - Nesrine BENKAFADAR Oxidative stress: key mechanism of age-related cochlear sensory hair cell loss Background and Introduction: In our aging society, age-related hearing loss or presbycusis is increasingly important. Based on observations of temporal bones from patients with presbycusis, Schuknecht (Schuknecht and Gacek, 1993) proposed the classification into three major forms, namely sensory, neural, and strial presbycusis according to the location of damage (sensory epithelium, spiral ganglion neuron, or stria vascularis). To date, the mechanisms underlying the age-related hearing loss remain unclear. Based on our previous study (Menardo et al., 2013) showing that the premature age-related hearing loss observed in senescence-accelerated mouse prone 8 (SAMP8) mice was correlated with altered levels of anti-oxidant enzymes and decreased activity of mitochondrial functions, we hypothesis that the oxidative stress may play a key role in presbycusis. Methods: To investigate the contribution of the oxidative stress in presbycusis, we exposed the p3 mouse cochlear explants to hydrogen peroxide (H2O2) in vitro. The cochlear cell senescence or degeneration was evaluated using the specific biomarkers. In addition, the role of endogenously-produced ROS in age-related hearing loss was assessed in adult p66KO mice which have a decreased ROS production. Results: Our results provide the evidence that the oxidative stress plays a key role in age-related hearing loss and cochlear sensory hair cell apoptosis. We demonstrate that H2O2 exposure induced a premature occurrence of cochlear sensory hair cell senescence and apoptosis, illustrated by the massive increase of the cell senescence and apoptosis biomarkers such as SA-betagal, gH2AX, AnnexinV and TUNEL, mainly in the cochlear sensory hair cells, but, not in the spiral ganglion neurons. Interestingly, our in vivo results from p66 KO and wt mice provided the functional and morphological evidence that the targeting of oxidative stress by pharmacological or genetic interventions protect the cochleae against age-related sensory hair cell death and hearing loss. Conclusion: Our results suggest that oxidative stress plays crucial role in age-related cochlear sensory hair cell degeneration and hearing loss. The use of anti-oxidants may be an attractive therapy to slowdown or stop the sensory presbycusis. Nesrine Benkafadar1,2*, Florence François1,2*, Jean-Luc Puel1,2 and Jing Wang1,2 1: INSERM - UMR 1051, Institut des Neurosciences de Montpellier, 34295 Montpellier, France. 2: Université Montpellier, 34295 Montpellier, France.* : these authors contributed equally CBS2 Association assocbs2.com N°9 - Laurent FERNANDEZ Membrane dynamics and partitioning of CD9 and CD81 are differentially regulated by the actin network Tetraspanins CD9 and CD81 are transmembrane proteins forming a network of interactions at the plasma membrane of eukaryotic cells and often described as membrane organizers. This network, composed of tetraspanins and of non-tetraspanin partners, is very dynamic, e.g. most of the tetraspanin CD9 molecules can display free lateral diffusion although some are confined in tetraspanin-enriched areas. Using single molecule tracking experiments, this study shows that CD81 molecules can freely diffuse within the membrane but are more confined and less dynamic than tetraspanins CD9. Although both proteins are often co-localized and share similar partners like EWI-2 and CD9P-1, we have demonstrated that their differential behavior is mainly due to a preferential interaction of CD81 with the cytoskeleton that restricts its diffusion at the plasma membrane. This link is mediated by the C-terminal moiety of CD81 through its interaction with ezrin/moesin/radexin (ERM) proteins and also implicates EWI-2 and CD9P-1. Interestingly, our work also reveals the functional relevance of this association with the cytoskeleton in the recruitment of CD81 and CD9 during the assembly of viral Gag proteins. Laurent Fernandez1,2, Patrice Rassam1,2 , Selma Dahmane1,2, Patrice Dosset1,2, Markus Thali3,4, Eric Rubinstein5,6, and Pierre-Emmanuel Milhiet1,2 1 Inserm, Unité 1054, Montpellier, France. 2 Université de Montpellier, CNRS, UMR 5048, Centre de Biochimie Structurale, Montpellier, France.3Graduate Program in Cell and Molecular Biology, and 4Department of Microbiology and Molecular Genetics, University of Vermont, Burlington, VT 05405 USA. 5 Inserm, U602, Villejuif, France.6 Université Paris 11, Institut André Lwoff, Villejuif, France CBS2 Association assocbs2.com N°10 - Emilande GUICHET High viral load in patients failing first-line ART is associated with multidrug resistance in resource limited countries Background: Access to ART expands, emergence of HIV drug resistance is inevitable, especially in resource limited countries where biological monitoring is limited. The objective of this study was to describe drug resistance mutations in patients that where eligible for a second line treatment in the 2LADY-ANRS12269/EDCTP trial conducted in Africa. Methods: Genotypic HIVDR testing was performed on 454 patients with virological failure (i.e. two plasma HIV-RNA viral load (VL) >1000 copies/ml after adherence intervention) in Cameroon (n=304), Burkina-Faso (n=91) and Senegal (n=59). They were taking first-line ART composed by two nucleoside (3TC+AZT/d4T) and one non-nucleoside reverse transcriptase inhibitors (EFV/NVP). HIVDR was determined using the ANRS (v24.2014) algorithm. Results: Genotyping was successful for 446/454 patients and 440(97.7%) were resistant to at least one drug. The M184IV mutation causing resistance to 3TC was present in 433(97.1%) patients and a similar number was resistant to EFV/NVP. In addition, 242(54.3%) mutations associated with resistance to AZT/d4T were found. A subset of patients also accumulated mutations leading to cross-resistance to ABC (85/446 (19.1%)), DDI (32/446 (7.2%)), TDF (6/446, 1.3%)) or ETR (56/446 (12.6%). Importantly, multi-resistant strains were observed in patients with high viral loads: 95/122 (77.9%), 125/219 (57.6%) and 24/106 (22.6%) of patients with VL>5 log10, 45 log10, and 3-4 log10, respectively were resistant to the 3 drugs of their first line regimen. Median VL in the 242 multi-resistant patients was 4.7 log10 (IQR 4.3-5.2) versus 4.2 log10 (IQR 3.7-4.7) in the other 198 resistant strains. Conclusions: This study highlights the importance of early detection of treatment failure. The extensive accumulation of HIVDR may compromise second-line regimens. High viral loads in multi-resistant patients increase the probability of transmission of these strains. These data stress the need of biological monitoring and advocate for more robust first-line regimens and continuous surveillance of HIVDR in resource limited countries. E. Guichet1,2, A. Aghokeng1,2, L. Serrano1, G. Bado3, C. Toure Kane4, A. Sawadogo4, C. Tidiane Ndour5, S. Koulla-Shiro6, S. Eymard-Duvernay1, E. Delaporte1, L. Ciaffi1, M. Peeters1 and the 2LADY-study group. 1. UMI233-TransVIHMI/ INSERM U1175/ UM, IRD,, Montpellier, France. 2. IMPM/CREMER, Yaoundé, Cameroun. 3. Hôpital de jour de Bobo-Dioulasso, BoboDioulasso, Burkina-Faso. 4. Laboratoire de Bactériologie-Virologie, CHU Le Dantec, Dakar, Sénégal. 5. UCAD, Dakar, Sénégal. 6. Université Yaoundé 1, Yaoundé, Cameroun CBS2 Association assocbs2.com N°11 - Viviana DELGADO BETANCOURT Cardioprotection against ischemia-reperfusion injury by heart rate control Background: Acute myocardial infarction (AMI) is the major cause of mortality worldwide. Early reperfusion is the only treatment recommended to reduce infarct size. However, reperfusion induces also deleterious secondary effects called ischemiareperfusion (IR) injury due to irreversible apoptotic death of cardiomyocytes. Most ischemic episodes are triggered by an increase in heart rate that induces an imbalance between myocardial oxygen delivery and consumption. The BEAUTIFUL clinical trial has demonstrated that moderate heart rate reduction diminishes the frequency of AMI episodes in patients with stable coronary artery disease having increased heart rate at rest. The HCN-mediated If current and the Cav1.3-mediated L-type Ca2+ currents play important roles in the generation of automaticity and heart rate, therefore they are interesting targets for selective control of heart rate and cardioprotection during AMI. The aim of this study was to investigate if Cav1.3 channels could be a putative target to reduce infarct size. Methods: Anesthetized C57BL/6J, Cav1.3-/- and Girk4-/- mice were subjected to a surgical protocol of myocardial IR (40 min ischemia-60 min reperfusion). Heart rate was measured with a one-lead surface ECG recording, and infarct size with triphenyl tetrazolium chloride staining. Results: Selective heart rate decrease (-26%) in an in vivo mouse model of AMI is associated with reduced IR injury. Ivabradine administration before ischemia significantly reduced infarct size (-33%). Cav1.3-/- mice presented reduced infarct size (-30%) compared to WT mice. In addition, Girk4-/- mice, a genetic model of moderate tachycardia (10%) displayed increased infarct size (+30%) compared to control mice. Conclusions: These results show a direct relationship between heart rate and IR injury. Heart rate reduction by inhibition of Cav1.3 channels constitutes a promising strategy to reduce infarct size. Delgado Betancourt V1; Covinhes A1; Mesirca P1; Bidaud I1; Nargeot J1 ; Piot C1; Striessnig J2;Mangoni M.E1; Barrère-Lemaire S1. (1) Institut de Génomique Fonctionnelle, CNRS UMR 5203, Inserm U 661, Université de Montpellier, Montpellier-France, (2) Center for Molecular Biosciences, University of Innsbruck, Innsbruck-Austria CBS2 Association assocbs2.com N°12 - Omar DIOURI Development of a mobile application to compute food carbohydrates Background: Estimating correctly the right amount of carbohydrates (CHO, carb) present in the meal is important for type 1 diabetic patients. We developed an Android application (app) to help them in this task, and this paper presents a preliminary study on it. Methods: 10 patients used our application for one week, they typed each meal on the application in blind mode, and they wrote on a logbook their own decisions. Data collected concerned mainly meal compositions and CHO content, time needed for entering meals in the applications, and when possible postprandial blood glucose. Results: 187 meals were analysed, with an average CHO quantity of 74.12 ± 32.51 grams, with a mean delta of 2.773 ± 8.91 grams, and an overall underestimation of patients compared to the APP. The average CHO quantity of lunches and dinners is significantly higher than in breakfast, with a Delta-SD twice times higher. CHO estimation errors are correlated to post-prandial blood glucose (p=0.0015).In fourth of hypoglycaemias, CHO content was underestimated by more than -9 grams, and for hyperglycaemias it was overestimated by more than 13.5 grams. The mean time to enter a meal diminished between the beginning of the week and the end (p=0.0003). Conclusion: Lunches and Dinners are meals with a high CHO content, and presents a higher discrepancy estimation. Those false estimations results in out-of-range BG excursions. A long-term clinical study will be led to measure more precisely the impact of the application on patient’s health. O. Diouri , J. Place , M. Traverso , E. Renard Institut de Génomique Fonctionnelle, UMR CNRS 5203/INSERM U1191, Université de Montpellier. Département d’Endocrinologie, Diabète, Nutrition, CHRU de Montpellier, Montpellier CBS2 Association assocbs2.com N°13 - Xiaobin ZHANG Adrenergic receptor gene variants are associated with late-onset generalized anxiety disorder Background: Generalized anxiety disorder is a common chronic condition that is understudied compared to other psychiatric disorders. Evidence from family studies suggests a relatively high heritability for GAD but few candidate genes have so far been identified. An altered adrenergic function has been reported in GAD however, direct evidence for genetic susceptibility is missing. Objectives: The current study aimed to evaluate the associations of gene variants in adrenergic receptors (ADRs) with late-onset GAD. Methods: Data were obtained from 844 French community-dwelling elderly aged 65 or over. Anxiety disorders were assessed using the Mini-International Neuropsychiatry Interview, according to DSM-IV criteria. Eight single-nucleotide polymorphisms (SNPs) involved with adrenergic function were genotyped; 2 alpha(1)adrenergic receptor subtypes, alpha(1A) (ADRA1A), alpha(2A) (ADRA2A) and beta2 (ADRB2) receptor and the transcription factor TCF7L2. Multivariate regression analyses adjusted for age, sex, physical and mental health comorbidity and adverse life events. Results: Significant associations were found for five SNPs and for ADRA1A rs17426222 and rs573514, the associations remained significant after correction for multiple testing. No significant associations were found with the 2 ADRA2A variants. Gene-environment interaction was found between certain variants and stressful life events in influencing risk of GAD. All associations appeared specific to GAD; in posthoc analysis no significant associations were found between ADR variants and phobia. Conclusions: This is the first study showing that ADR variants are susceptibility factors for late-onset GAD, but not the other major anxiety disorder, especially phobia. These data support the critical role of the adrenergic nervous system in GAD and in particular in response to stressful adverse life events. Inserm U1061 CBS2 Association assocbs2.com N°14 - Anne BIEVER Role of the ribosomal protein S6 phosphorylation in the mouse brain The 40S subunit ribosomal protein S6 (rpS6) has attracted much attention over the last three decades since it is the first ribosomal protein shown to undergo inducible phosphorylation upon a wide variety of stimuli. However, despite the profound elucidation of the respective kinases and extracellular stimuli triggering phosphorpS6, little is known about the physiological role of the phosphorylation. In this study, we aimed to charactherize the functional relevance of the in vivo rpS6 phosphorylation in the brain. For this purpose, we performed a behavioral characterization of rpS6P-/- knock-in mice, in which all phosphorylatable serine residues are substituted by alanines. Interestingly, these mice display a reduced locomotor response to d-amphetamine, which markedly increases phospho-rpS6 in the striatum of wild-type mice. Moreover, they show impaired synaptic plasticity of GABAergic medium-sized spiny neurons in the nucleus accumbens. Finally, since rpS6 phosphorylation has been widely correlated with changes in protein synthesis, we performed polysome profile and puromycin incorporation analyses in rpS6P-/knock-in as well as in wild-type mice treated with d-amphetamine. Intriguingly, we found no differences in global translational rates in the striatum, hippocampus and frontal cortex. Altogether, our results indicate that neither basal nor drug-induced transient rpS6 phosphorylation correlate with changes in overall mRNA translation. Nevertheless, despite the lack of causal relationship between both events, rpS6 phosphorylation plays an important role in striatal plasticity and behavioral responses. Anne Biever1,2,3*, Emma Puighermanal1,2,3*, Oded Meyuhas9, Emmanuel Valjent1,2,3 CNRS, UMR-5203, Institut de Génomique Fonctionnelle, Montpellier, F-34094, France. 2INSERM, U661, Montpellier, F-34094, France. 3Universités de Montpellier 1 & 2, UMR-5203, Montpellier, F-34094, France .9Department of Biochemistry and Molecular Biology, The Institute for Medical Research – Israel-Canada, The Hebrew University-Hadassah Medical School, Jerusalem 91120, Israel. 1 CBS2 Association assocbs2.com N°15 - Mona HOUHOU Characterization of a Cancer Stem cells enriched subpopulations and role of EMT Regulators in basal Breast Cancer Cell Plasticity Breast cancer is not a single disease, but rather is composed of different subtypes associated with different clinical outcomes and molecular characteristics. A better understanding of the heterogeneity is the key to the development of targeted therapeutic interventions. This heterogeneity may be explained by the concept of cancer stem cells (CSC). In breast cancer, a number of markers have been proposed to isolate and characterize breast CSC. A panel of markers such as CD44/CD24/EpCAM, ALDH, and capacity of mammospheres formation is used, but the question on CSC in ER (-) breast cancer remains to be clarified and the mechanism underlying the aggressive behavior of triple negative breast cancer (TNBC) is not well understood yet. To this purpose, SUM 159, MDA-MB-436 and MDA-MB-468 cell lines are used as ER (-) models to search for the cell fractions enriched for CSC. It has been found that the CD44+/CD24- cell population is enriched in TNBC tissues and cell lines, with a higher capacity of proliferation, migration, invasion and tumorigenicity as well as adhesion ability. In addition, a high level of CD44+/CD24- and ALDH+ cells in primary breast tumors was correlated with the presence of distant metastasis. Furthermore, CD44+ positivity has been clearly associated to the acquisition of a mesenchymal phenotype, suggesting a link between EMT and stemness. All different cell populations will then be tested for mammosphere formation and differentiation in Matrigel in comparison with the “negative” fractions. In addition, RNA profiling analysis will allow us to study various factors involved in EMT in different cell fractions. The idea is to identify a signature of genes defined as "stem" that we can analyze by qPCR and in particular by recent techniques of single-cell qPCR (Fluidigm). It would indeed be interesting to test variations of expression of these genes in the different cellular fractions enriched in CSC. Keywords : Triple negative breast cancer (TNBC), Cancer stem cells (CSC), CD44+/CD24-, ALDH+, Epithelial-mesenchymal transition (EMT), dedifferentiation, regulators of EMT Mona Houhou, directeur de thèse: Charles Theillet, Equipe: Plasticité phénotypique et génétique du cancer, IRCM U1194. CBS2 Association assocbs2.com N°16 - Benoit GIRARD Metabotropic glutamate receptor type 7 (mGlu7) modulation of thalamocortical activity. Thalamocortical activity depends on the balance between glutamatergic and GABAergic activity in order to guarantee correct somatosensory computation and sleep/wake cycle. The metabotropic glutamate receptor type 7 (mGlu7) is expressed at the presynapse where it inhibits neurotransmitter release. We have previously shown that mGlu7AAA KI mice, in which the receptor intracellular signalling is lost, develop spontaneous absence-like seizures similar to the human pathology, absence epilepsy. The present study aimed at understanding the function of mGlu7 at specific thalamic synapses using in vitro patch-clamp recording on thalamocortical slices and in vivo EEG recording in both wild-type and mGlu7AAA knock-in mice. We found that mGlu7 inhibits the synaptic inputs onto thalamic reticular nucleus (TRN) neurons, coming from either the ventroposteromedial nucleus (VPM) or within the TRN itself. Specific activation of long-range thalamocortical projections was achieved by using viral-mediated stereotaxic expression of ChannelRhodopsin 2, a light-sensitive cationic channel. This approach showed mGlu7-mediated inhibition of cortical layer 4 fast-spiking interneurons, as opposed to regular spiking interneurons or pyramidal cells. Remarkably, on top of the conventional, agonist-dependent activity, the receptor showed but also a constitutive, agonist-independent activity both in vitro and in vivo. This constitutive activity was suppressed by the negative allosteric modulator (NAM), ADX71743. In vivo administration of the NAM altered thalamocortical EEG recording, with spike-and-wave discharges typical of absence seizures and a general induction of drowsiness in the animal. The results suggest a major role of the mGlu7 receptor in the tonic control of thalamocortical function. Benoit Girard1,2,3*, Valériane Tassin1,2,3* , Apolline Chotte1,2,3, Pierre Fontanaud1,2,3, Delphine Rigaud4, Julie Perroy1,2,3, Francine Acher4, Laurent Fagni1,2,3, Federica Bertaso1,2,3 1 CNRS, UMR-5203, Institut de Génomique Fonctionnelle, Montpellier, F-34094, France, 2 INSERM, U1191, Montpellier, F-34094, France, 3 Universités de Montpellier, UMR-5203, Montpellier, F-34094, France, 4 Université Paris Descartes, CNRS UMR-8601, Paris, F-75006, France. CBS2 Association assocbs2.com N°17 - Margarida GOMES Modeling the role of the global regulator ShvR of Burkholderia cenocepacia in virulence using zebrafish embryos Burkholderia cenocepacia has been demonstrated to be capable of surviving and multiplying inside cells by evading host cell defense mechanisms. In our laboratory, we have developed a zebrafish model to study virulence caused by bacteria belonging to the Burkholderia cepacia complex, and have shown that macrophages provide an intracellular niche for Bcc in vivo. The model allowed us to distinguish strains that cause an acute, rapidly fatal infection, including the B. cenocepacia ET12 lineage strains, and strains that were persistent. In this study zebrafish embryos were used to further understand a role in virulence for the LysR-type transcriptional regulator ShvR. Initially identified based on its role in colony morphology, previous infection experiments in alfalfa seedlings and rats have shown that this regulator is important for virulence, and inflammation in rat lungs. Interestingly, bacterial numbers were, paradoxically, sometimes higher in animals infected with the mutant compared to wildtype, suggesting the shvR mutant was highly persistent. Here, we show, in agreement with these earlier results, that the shvR mutant is attenuated in virulence in zebrafish embryos, with a marked reduction in proinflammatory responses and tissue inflammation. Using real time non-invasive imaging, we observed that the shvR mutant persists in macrophages and, in contrast to the wildtype, is unable to disseminate from infected host cells. This persistent phenotype is reminiscent to those we described earlier for strains including B. stabilis LMG14294 and B. vietnamiensis LMG14942. We will present our results on the host phagocyte and immune response to infection with the B. cenocepacia shvR mutant, and further describe our recent efforts to show a role for this global regulator in persistent versus virulent infections. Margarida Gomes1,2, Sujatha Subramoni3, Pamela Sokol3 and Annette Vergunst1,2 1 INSERM, U1047, UFR Médecine Site de Nîmes, 30908 Nîmes, France. 2 Université de Montpellier, U1047, UFR Médecine, 30908 Nîmes, France. 3 Department of Microbiology, Immunology, and Infectious Diseases, University of Calgary, Calgary T2N 4N1, Canada CBS2 Association assocbs2.com N°18 - Chantal MAGHAMES Ubiquitin under stress : “ Going hybrid with NEDD8”. Cells constantly respond to stress signals that damage proteins and/or DNA. Defects in repair or elimination of damage can lead to many diseases such as cancer or neurodegeneration. Ubiquitin and Ubiquitin-like molecules are implicated in the control of myriad biological processes including detection and repair of damaged proteins/DNA. This family of proteins covalently modifies proteins through the action of E1, E2 and E3 enzymes. Historically, it was believed that each pathway employ its own and unique set of enzymes to post-translationally modify their substrates. We discovered that upon proteotoxic stress including proteasome inhibition, heat shock and oxidative stress, the Ubiquitin-like molecule NEDD8, is activated by the Ubiquitin E1 enzyme Ube1. This results in a global increase in NEDDylation and the formation of ploy- NEDD8 and mixed chains between NEDD8 and Ubiquitin. The process is reversible and cell recovery is accomplished once stress is alleviated. Our goal is to identify the cellular components that participate in this stress response, the mechanisms mediating the recovery process and to understand the biological significance for this increase in protein NEDDylation. Our results show that this accumulation of NEDDylated/Ubiquitinated substrates is dependent on the heat shock proteins 70/90, on protein synthesis and is characterized by a progressive translocation of the modified substrates from the cytosol to the nucleus leading to a nuclear aggregation after a severe stress. As for the recovery process, we found that nuclear proteasomes directly interact with and eliminate these conjugates. Future steps will include the identification of substrates that aggregate upon heat shock through the formation of mixed chains and the potential biological significance of this increased NEDDylation. In addition, we aim to characterize the recovery process by proteasomal degradation. Chantal MAGHAMES and Dimitris XIRODIMAS Centre de Recherche de Biochimie Macromoléculaire - UMR 5237, CNRS, Route de Mende 34 293, Montpellier, Cedex 5, France CBS2 Association assocbs2.com N°19 - Amélie BORIE Modulation of lateral septal neurons by oxytocin and vasopressin, neuropeptides involved in the regulation of social behavior. Central oxytocin (OT) and vasopressin (VP) have almost opposite roles in mammal behavior: OT facilitates social interactions while VP promotes aggressivity and anxiety, but their mechanism of action is unknown. We study the mouse lateral septum, an exception where both OT and VP can increase social interactions and social memory. This structure expresses significant amount of OT and VP receptors but electrophysiological consequences of their activation have not been studied in detail so far. We used patch clamp recordings from acute brain slices to characterize electrophysiological responses of mouse lateral septum neurons to TGOT (specific OT receptor agonist) and vasopressin. Strikingly, the firing frequency of almost all recorded neurons was significantly modulated by at least one of these peptides. Accordingly, we classify lateral septal neurons into three populations: i) inhibited by both peptides; ii) activated by oxytocin; iii) activated by vasopressin. Because the septo-hippocampal network is involved in theta rhythm regulation, we analyzed the effect of OT and VP on spike patterning. We observed that modulation of electrical activity results from a modification of inter-burst intervals (1.5-5 s) rather than intra-burst frequency (close to the Theta rhythm, 3-5 Hz). With the aim of deciphering a local microcircuitery involving the three abovementioned neuronal categories, we studied spontaneous synaptic events and demonstrated that they are mostly GABAergic. Their frequency was increased by TGOT and VP, opening the possibility that these peptides act locally by regulating interactions between interneurons. In the lateral septum, we observe similar effects of OT and VP, consistent with their behavioral action. We will then compare electrophysiological data obtained in the lateral septum of WT mice and mice in which the OT or VP system are perturbed and which constitutes animal models of social diseases. Work supported by CNRS, INSERM and ANR. A B supported by University of Montpellier A M Borie1,2, G Guillon1,2, F Muscatelli3 and M G Desarménien1,2 1 Institut de Génomique Fonctionnelle, CNRS UMR5203, Inserm U1191, Montpellier, France. 2 Université de Montpellier, Montpellier, France. 3 INMED, Inserm U910, Marseille, France CBS2 Association assocbs2.com N°20 - Sarah LALISSE Potential role of P2X4R expressed by sensory neurons in BDNFevoked inflammatory pain P2X receptors (P2XR) are ATP-activated ion channels. Among the different P2X subunits, P2X2 and P2X3 expressed by sensory neurons are known to be involved in both physiological and pathological pain processing. In addition, it has been recently demonstrated that P2X4R expressed by macrophages and microglial cells play a crucial role in both neuropathic and inflammatory pain through the release of proinflammatory molecules or microglial BDNF release. While P2X4R mRNA is expressed in dorsal root ganglia neurons, the functional expression of these receptors and their potential role in sensory information processing is still unexplored. Here we have investigated the functional expression of P2X4 receptors in sensory ganglia and their potential involvement in pain processing. Our results show that in physiological conditions, P2X4R are functionally expressed by a subpopulation of sensory neurons, including small and intermediate nociceptive neurons, suggesting a potential role of P2X4R in pain transmission. In inflammatory condition, 24h after the injection of Complete Freund Adjuvant in the hind paw, a subset of nociceptive neurons co-express P2X4R and BDNF. We also demonstrate that P2X4R are present in central afferents suggesting a potential role of the receptor in pre-synaptic BDNF release. Indeed, our results show that following peripheral inflammation several BDNF-dependent signaling pathways are activated in the spinal cord: activation of ERK1/2, phosphorylation of NR1 subunit and downregulation of KCC2 cotransporter, while these modifications are not observed in P2X4-deficient mice. In inflammatory conditions P2X4R expressed in sensory neurons appear to shape dorsal horn spinal network excitability by triggering BDNF release by sensory afferents, thus contributing to inflammatory pain processing. Lalisse, S. (Montpellier)1, Rassendren, F. (Montpellier)1, Ulmann, L. (Montpellier)1 1 Institut de Génomique Fonctionnelle - CNRS UMR 5203 - INSERM U1191 Université de Montpellier, Montpellier, France CBS2 Association assocbs2.com N°21 - Pascale PALASSIN Role of RIP140 in familial colorectal cancer Colorectal cancer (CRC) is a common disorder with familial forms such as Lynch syndrome which exhibit microsatellite instability (MSI) due to a loss of function of DNA mismatch repair system (MMR). However, about a quarter of clinically diagnosed families do not exhibit MMR gene alterations (Lynch Like Syndrome or LLS) thus implicating new candidate genes. The team has already shown that the transcription factor RIP140 is involved in sporadic colorectal carcinogenesis. In addition, preliminary results indicate that RIP140 regulates the expression of some MMR genes. Furthermore, a mutation in the RIP140 coding sequence (RIPMSI) which generates a truncated protein has been detected in cells and tissues from MSI CRC. The aim of this thesis project is to decipher the role of RIP140 in familial colon cancer. I will study the regulation of MMR gene expression by RIP140 using different cell lines and tissues displaying a deregulated expression (overexpression or knockdown) of the RIP140 gene. I will analyze the impact of this regulation on mismatch repair activity and on the susceptibility to various cytotoxic drugs. In parallel, I will study the effects of RIPMSI on parameters previously described and I will search for this mutation at the DNA and protein levels in a cohort of MSI CRC patients. By decreasing MMR gene expression, the inactivation of RIP140 could affect DNA repair and promote colorectal tumorigenesis. The RIPMSI mutation might explain the microsatellite instability in patients where no MMR gene mutation is found and become a useful biomarker for LLS diagnosis. Keywords : Colorectal cancer, Lynch syndrome, RIP140, Mismatch repair, DNA repair. Pascale PALASSIN, Marion LAPIERRE, Carole CORSINI, Sandrine BONNET, Stéphan JALAGUIER, Audrey CASTET-NICOLAS, Vincent CAVAILLES IRCM, INSERM U1194, Montpellier CBS2 Association assocbs2.com N°22 - Solene BRELLE Deciphering the function of the Serine/Threonine Protein Kinase CStk from Coxiella burnetii and its role during host infection. Coxiella burnetii is an intracellular Gram negative bacterial pathogen. It is the causative agent of Q fever, an emerging zoonosis with severe health and economic impact. The symptoms of Q fever range from pneumonia, fatigue and hepatitis in the acute form of the disease, to severe endocarditis and encephalitis in its chronic form. After internalisation by the host cell, C. burnetii uses a Dot/Icm type IV secretion system (T4SS) to translocate effector proteins and divert the cell machinery to generate its own parasitophorous vacuole (PV). Screening of a C. burnetii transposon mutant bank indicated that expression of a unique Ser/Thr Protein Kinase (STPK), CStk (CBU_0175) is important for the intracellular development of the bacteria. Furthermore, a previous study has shown that CStk could be translocated into the host cytoplasm using Legionella pneumophila as a surrogate host. In our study, we will characterise the Ser/Thr protein kinase activity of CStk, confirm its secretion by Coxiella and identify host targets. S. Brelle(1), E. Martinez(2), F. Cantet(2), F. Letourneur(1), M. Bonazzi(2) and V. Molle(1) 1:CNRS-UMR5235-Dynamique des Interactions Membranaires Normales et Pathologiques, Université de Montpellier, France.2:CNRS/UM-UMR5236-Centre d'études d'agents Pathogènes et Biotechnologies pour la Santé, Montpellier, France. CBS2 Association assocbs2.com N°23 - Thi Thu Phuong TRAN Characterization and role of indirectly-activated human dendritic cells by immune-complex adenovirus in vitro in immune memory response Dendritic cells (DCs) are specialized antigen-presenting cells (APCs), and critical establisment of immunological memory. They also re-stimulate T and B cells and play a role in the maintenance of their function. Human adenovirus type 5 (HAd5), nonenveloped DNA viruses that primarily cause self-limiting disease, are used as a vector for vaccination, long-term gene transfer and cancer treatment. Immune complexHAd5 (IC-HAd5) induce functional maturation of human DCs which includes cytokine and chemokine secretion. Moreover, IC-HAd5 induce a pro-inflammatory cell death of DCs called pyroptosis. DCs maturation includes up-regulation of major histocompatibility complex (MHC) class II, costimulatory CD80/CD86 molecules, and production of pro-inflamatory cytokine and chemokine. Immature DCs express receptors for inflammatory molecules (eg. type I IFN) released by DCs or other cells directly activated by pathogen associated ligand. Indirectly activated DCs acquire a mature phenotype, increasing expression of MHC II and co-stimulatory molecules. Our question is what happens to immature DCs in environment created by IC-HAd5 stimilated DC? Our goal is to characterize indirectly-activated DCs and their roles in memory immune response. In addition, we want to identify influential factors in indirect DCs maturation. We use biochemistry and fluorescences test to characterize indirectly- stimulated DCs in transferwell. Our results indicated that indirectly activated DCs increased surface marker expression after 12 hours. Moreover, we found that the percentage of cell death by IC-HAd5 of the indirectly- activated DCs is less than directly activated DCs. Thi Thu Phuong Tran, Karsten Eichholz, Eric J . Kremer(1)* (1)Adenovirus Laboratory, IGMM, CNRS, Montpellier, France. CBS2 Association assocbs2.com N°24 - Alaa YEHYA BDNF knockdown induces defects in zebrafish posterior lateral line development Derived Neurotrophic Factor (BDNF) the most abundant member of the neurotrophin family in the human brain, BDNF signaling is mediated by two principal transmembrane receptors, receptor tyrosine kinase B (TrkB) and p75NTR neurotrophin receptor (p75NTR). BDNF has been studied extensively for its major roles, in neuronal differentiation, survival, plasticity, as well as in cognition. In this study we aimed to investigate further BDNF signaling actions, we used zebrafish posterior lateral line (pLL) system as a model, which is a mechanosensory system in fish and amphibians that evolved to detect local water flow and pressure. PLL development includes different physiological processes including, morphogenesis, collective migration, and neuronal development. Our results show that Knockdown of BDNF using antisense morpholino oligonucleotides resulted in abnormal primordium migration and a significant reduction in the number of deposited neuromasts. In addition, morphant embryos had a defect in PLL nerve and neuromasts hair cells regeneration compared to complete regeneration in controls. Collectively these findings indicate that BDNF signaling has an essential role in the regulation of PLL development. In addition, the phenotypes observed in response to BDNF knockdown show the utility PLL system in studying defects in BDNF signaling that might resemble some conditions in human disorders. Alaa Yehya, Michelle Silhol, Nicolas Cubedo, Jean-Michel Verdier, Mireille Rossell 1Université Montpellier, Montpellier F-34095, France; Inserm U1198, Montpellier F34095, France; EPHE, Paris F-75014, France CBS2 Association assocbs2.com N°25 - Safa AZAR Diffuse low grade gliomas: characterization and development of in vitro model for designing innovative therapeutic approaches Diffuse low-grade glioma (DLGG) are slow growing grade II tumors that develop in different functional places in the brain and affect young patients between the second and the fourth decades of life. Although, they are clinically stable over a long period of time, these tumors can ineluctably progress to a higher grade of malignancy leading to anaplasia, which then rapidly compromises patient survival. Most grade II gliomas (around 80%) have a false sense mutation (R132H) in the IDH1 gene (isocitrate dehydrogenase) combined with a 1p19q codeletion, mutations in p53 or ATRX. IDH1 mutations induce major dysregulations of DNA methylation leading to defects in cell differentiation. These tumors, classified as astrocytoma or oligodendroglioma, are probably derived from neural progenitors which remain in the adult brain. Today, one important obstacle preventing the development of new therapies for DLGG is the lack of understanding of the cellular composition of these tumors and the absence of an in vitro model due to their low proliferation rate. The first aim of our study is to characterize by immunohistochemistry the different pools of cells causing the heterogeneous profile of the tumor and to understand the different signaling pathways that are activated and/or inhibited, as well as the interactions between the cancerous cells and their environment. The second part is to use different approaches in order to enhance the cell proliferation including cell immortalization via expressing or inhibiting the different signaling pathways that are involved in the cell cycle. Safa Azar(1),Aurélie Gennetier(1), Frédérique Lorcy(2), Valérie Rigau(2), Hugues Duffau(1) (2), Bernard Rothhut (1), Jean-Philippe Hugnot(1). (1): Institut for neurosciences of Montpellier, INSERM U1051, Team "plasticity, neural stem cells and glioma. (2): Hospital Guy De Chauliac, Montpellier CBS2 Association assocbs2.com N°26 - Shefqet HAJDARI Role of the chromatin associated proteins HP1 (Heterochromatin Protein 1) in liver hemostasis DNA is wrapped in a complex structure called chromatin that is known to play essential roles in establishment and maintenance of cellular identity and to be involved in cancer development. HP1 are chromatin associated proteins that are believed to play crucial roles in chromatin dynamics. Using animal models with specific inactivation of each of the HP1, we have obtained results indicating that HP1 are important for liver homeostasis and we are now trying to uncover the mechanisms underlying these functions of HP1. Analysis of gene expression in 5 weeks old mice with liver specific inactivation of either HP1g or HP1b in an HP1aKO background (HP1agKO, abKO) show deregulation of expression of some genes involved in different pathways. Expression of genes involved in the p53/cell cycle control pathway (p53 and p27) and B-catenin pathway (Ctnnb1 and Birc5) were increased in the HP1ag mutant as compared to WT mice. Interestingly, the expression of several cancer related genes such as Tert and AR is up-regulated in HP1ag or HP1abKO mice respectively. Additionally, genes deregulated in HP1agKO mice display a strong enrichment in genes of the KRABZFP family, suggesting a loop of auto-regulation between HP1, TRIM28 and KRABZFP. By using TMA (Tissue MicroArray), we observed that the number of AFP (liver cancer marker) positive cells increased on HP1KO histological sections as compared to WT. Analysis of Ki67 positive cells as marker of proliferation shows that HP1aKO liver cells tend to proliferate more. Additionally, livers from both HP1agKO and HP1abKO mice display hyper-proliferation as compared to WT animals. Our results demonstrate that HP1 are involved early during the development of mouse liver and suggest that these early molecular and functional deregulations in liver of mice lacking HP1 may serve as a basis for cancer development through cell cycle and aberrant expression of cancer related genes. Shefqet HAJDARI, Nelly PIROT, Florence CAMMAS Team of Epigenetics, Cell Differentiation and Cancer, Institute of Cancer Research of Montpellier (IRCM – U1194) CBS2 Association assocbs2.com N°27 - Boubou DIAGOURAGA Role of PRDM9 methyltransferase activity in mouse meiotic recombination During meiosis, genetic recombination between homologous chromosomes promotes accurate chromosome segregation and generates new combinations of alleles. DNA double-strand breaks introduced by the SPO11 protein are repaired by homologous recombination. This event occurs in 1 to 2 kb-long regions, recombination hotspots. Recently, PRDM9 has been shown to specify hotspots by targeting specific DNA sequences through its zinc finger array. The PR/SET-domain of PRDM9 possesses an H3K4me3 activity, which correlates with a PRDM9-dependent enrichment of H3K4me3 at active hotspots. Using in vitro and in vivo strategies, we characterized the catalytic activity of PRDM9 and determined its role in mouse meiosis. We have characterized the structure and the activity of the PR/SET domain (Wu et al., Cell reports 2013). The crystal structure of this PR/SET domain in complex with a histone H3 peptide and the cofactor revealed a topology similar to that of canonical SET domains. To get insights into the substrate specificity of PRDM9, we performed an in vitro methylation assay on a histone Nterminus tail peptide array with various post-translational modifications. Methyltransferase activity was detected on H3K4, H3K9, and, with a lower efficiency, on H3K36. To determine the role of PRDM9 methyltransferase activity in vivo, we used the G278A mutation, inactivating the catalytic activity of PRDM9 (Hayashi et al., Nature 2005). Taking advantage of the specificity of two Prdm9 alleles (Prdm9b and Prdm9wm7), which target each a specific set of hotspots, we generated transgenic mouse strains expressing the mutant allele Prdm9wm7-G278A and the endogenous wild-type Prdm9b. We showed that H3K4me3 mark is not enriched and there is no recombination at Prdm9wm7-specific hotspots in this strain. In mice expressing solely the mutant allele, meiosis does not progress beyond early stages. Our results show that PRDM9 methyltransferase activity is required for recombination and completing meiosis. Boubou Diagouraga, Frédéric Baudat, Bernard de Massy Institute of Human Genetics, UPR 1142, CNRS, 141 rue de la Cardonille, 34396 Montpellier, France CBS2 Association assocbs2.com N°28 - Hélène DONNADIEU-RIGOLE Dynamics and function of monocyte subsets in alcohol-dependent subjects Chronic alcohol consumption has a modulating effect on immune functions that may contribute to decreased immunity and host defense. Monocytes constitute the first line of host defense against pathogens and act as key regulators of both inflammation and tissue homeostasis. Human monocytes are heterogeneous and comprise several subtypes committed to different functions. Whether and how the chronic use of alcohol impairs blood monocyte subsets in alcohol-dependent patients remains unknown. Thus, we investigated the phenotypic and functional characteristics of blood monocyte subsets in alcohol-dependent patients (AD), before and after alcohol withdrawal. Compared to healthy controls (HC), changes in the distribution of monocyte subsets was found in AD subjects before withdrawal, as well as altered functional characteristics. The classical CD14+CD16- subset was decreased whereas the non-classical CD14dimCD16+ subset was expanded (p<0,001). The frequencies of TLR2- and TLR4-expressing monocytes were reduced in AD patients compared to HC. Althought the steady state production of TNF by monocytes was comparable to HC, the percentage of TNF-producing cells was reduced following LPS challenge. Importantly, 14 days of sobriety restored the distribution of CD14dimCD16+ monocytes and the frequency of TNF-producing cells in response to LPS stimulation to levels comparable to those in HC. Our findings indicate that chronic alcohol consumption alters the distribution as well as the phenotypic and functional characteristics of blood monocyte subsets, which are restored following 2 weeks of withdrawal. Key words: monocytes, TLR, alcohol, wthdrawal, cytokines Hélène DONNADIEU-RIGOLE1,2,3, Isabelle DUROUX-RICHARD1,2, Pierre PORTALES4, Martine BOUTHIER4, Thibault MURA5, Jean-François ELIAOU4, Christian JORGENSEN6, Pascal PERNEY3, Florence APPARAILLY1,2,6 1 INSERM, U1183, IRMB, University Hospital Saint Eloi, 80 rue Augustin Fliche, 34295 Montpellier, France. 2 University of Medicine, Boulevard Henri IV, 34090 Montpellier, France. 3 Department of addiction, University Hospital Saint Eloi, 80 rue Augustin Fliche, 34295 Montpellier, France. 4 Department of immunology, University Hospital Saint Eloi, 80 rue Augustin Fliche, 34295 Montpellier, France. 5 Department of information, University hospital of Montpellier. 6 Clinical department for osteoarticular diseases, University hospital Lapeyronie, 371 Avenue Gaston Giraud, 34295 Montpellier, France. Corresponding author : Hélène Donnadieu-Rigole @mail : [email protected] : + 0033 4 67 33 70 20 CBS2 Association assocbs2.com N°29 - Elodie FOREST Dissecting the role of new cortical scaffolds during epithelial biology Epithelial cells form the most abundant cell type in the human body. They are highly polarised along an apical-basal (A/B) axis, where the apical side faces the lumen. This A/B polarity is achieved through the asymmetric segregation of highly conserved protein scaffolds, many of which containing PDZ domains. A/B polarity controls then key features of epithelial cells such as adhesion, trafficking, proliferation or signaling. The observation that polarity is always lost in the late stages of cancers of epithelial origin highlights the important tumour-suppressive role of proper A/B polarity, and hence of the protein scaffolds controlling it. Using both the fruit fly Drosophila melanogaster and human cancer cell lines, my project is to characterise two neglected multi-PDZ scaffolds: bbg / PDZD2 and the MAGI scaffolds. First, using genetics and in-vivo and in-cellulo phenotypic analysis focusing on cell architecture, proliferation and adhesion, I will determine the function of these two families of scaffolds. Second, using massive proteomic approaches, I will identify the partners of these scaffolds to identify new protein complexes controlling and/or implementing the A/B polarity program in epithelial cells. As preliminary results, we identified that, the MAGI scaffolds are implicated in the dynamics of cell junction formation and that bbg / PDZD2 are involved in cell number and cell size control. Elodie FOREST - IRCM CBS2 Association assocbs2.com N°30 - Ildem SANLI Role of histone modifications and non-coding RNAs in the regulation of the imprinted Dlk1-Dio3 domain Genomic imprinting is an epigenetic phenomenon that mediates parent-of-origin specific mono-allelic gene expression. Most known imprinted genes are organized in clusters and their expression is regulated by differentially methylated regulatory sequence elements called ‘imprinting control regions’ (ICRs). One of these imprinted clusters, Dlk1-Dio3 domain is important for development. This domain, located on mouse chromosome 12, contains three protein-coding genes, Dlk1, Rtl1 and Dio3 expressed from the paternal chromosome and several non-coding RNAs including Gtl2, C/D box snoRNAs and many microRNAs expressed from the maternal chromosome. The imprinted gene expression at this domain is controlled by a paternally methylated ICR, called the IG-DMR. In the mouse, deletion of the IG-DMR on the maternal chromosome results in loss of expression of all the maternallyexpressed ncRNAs, and de-repression of the protein-coding genes, on the maternal chromosome. Paternal deletion of the IG-DMR has no effect. This indicates that the yet-unknown mechanisms that control imprinted expression at this domain act on the maternal chromosome. Our aim is to elucidate which mechanism(s) bring about the silencing of the paternally-expressed genes of the Dlk1-Dio3 domain on the maternal chromosome. To distinguish between the parental chromosomes, I use intra-subspecific hybrid ES cells between M. m. domesticus strain C57BL/6J and M. m. molossinus strain JF1 that were previously generated in our lab. In hybrid ES cells and neural cells differentiated in vitro, I have been investigating the repressive histone modifications and the recruitment of repressive complexes at Dlk1 and Dio3 on the maternal chromosome. I am particularly interested in the role of Gtl2 ncRNA in the repression of Dlk1 and Dio3. For this purpose, I will perform studies on the recruitment and allele-specificity of the repressive complexes and the repressive modifications in Gtl2 deficient cells. Ildem Sanli, Sébastien Lalevée, Robert Feil Institute of Molecular Genetics (IGMM), CNRS UMR5535 and University of Montpellier, 1919 Route de Mende, Montpellier 34293, France CBS2 Association assocbs2.com N°31 - Sophie GUELFI Molecular mechanisms of Notch1-induced pericyte-like transdifferentiation of glioblastoma stem cells Glioblastoma Multiforme (GBM, WHO grade IV) is the most aggressive and infiltrative of primary brain tumors. Extensive vascularization is a major hallmark of GBM, and current therapeutic strategies focus on targeting tumor angiogenesis. GBM origin is still unknown but it was shown that subpopulations of multipotent stem-like cells exist within the tumor, and could be responsible for relapse. The Notch signaling pathway is central in the maintenance and proliferation of these cells within the perivascular niche, where GBM stem cells closely interact with endothelial cells. Here, we questioned whether Notch1 pathway activation in such cells could influence the extent of tumoral vascularization and dissemination, using an activated form of the Notch1 receptor (NICD). Although Notch1 receptor is activated, target transcription factors (HES5, HEY1, HEY2) are not or barely expressed in our GBM stem cell cultures. Notch1 activation in these cells alters cell morphology, reduces their growth rate and migration. This is accompanied by a transcriptional switch where OLIG2 and SOX2 expression is reduced while HEY1/2, KLF9 and SNAI2 transcription factors are upregulated. Further analyses showed that NICD induces the expression of vascular adhesion proteins (ICAM1, VCAM1), angiogenic cytokines (IL8, PLGF), and angiogenic metalloproteinase MMP9. Remarkably, NICD expression also induces the expression of pericyte markers in vitro (NG2, PDGFRβ and αSMA). When xenotransplanted, Notch1-stimulated cells resulted in poorly disseminating but highly vascularized tumors containing round and normalized vessel structures. Cells also express pericyte markers in vivo and closely associated with host endothelial cells, which confirmed a pericyte-like differentiation of GBM stem cells. Our current project focuses on deciphering the transcriptional mechanisms underlying this phenotypic switch. We are especially interested in how SNAI2 and KLF9 are involved in Notch1-induced dormancy and pericyte-like features, by using in vitro mechanistic approaches as well as studying their function in the context of GBM perivascular niches. Guelfi, S1, Guichet, P.-O.1, Teigell, M.2, Hoppe, L.1, Bakalara, N.1, Bauchet, L.1, Duffau, H.1, Lamszus, K.3, Rothhut, B.1 and Hugnot, J.-P.1 1 INSERM U1051 - INM, Montpellier, France, 2RHEM-INM, BioCampus, CNRS Montpellier, Montpellier, France, 3Laboratory for Brain Tumor Biology, Department of Neurosurgery, University Medical Center Hamburg- Eppendorf, Martinistrasse 52, Hamburg, Germany CBS2 Association assocbs2.com N°32 - Ali SALEH A synthetic tridimensional matrix to study the migration of Glioblastoma stem cells Glioblastoma Multiforme (GBM) is the most common and aggressive primary brain tumor. After decades of fundamental and clinical research, the prognostic of this disease remains dismal and this is due to the high infiltrative capacity of a subpopulation of tumor cells called Glioblastoma Stem Cells (GSC). In our laboratory, using patient-derived primary cultures of GSC, we have developed different models to study the migration of this tumor cells at the cellular and molecular levels. In vivo, this has been possible with an orthotopic xenograft of human cancerous stem cells into the brain of immunocompromised mice. In vitro, the study was developed using a new synthetic tridimensional matrix of nanofibers. At a time when different scientific publications have demonstrated the prominence of the extracellular matrix in the control of tumor progression, the bidimensional models of cell migration are becoming obsolete. Our tridimensional support aims at mimicking the cerebral microenvironment and thus constitutes a valuable model to unravel the migratory characteristics of GSC. Using this matrix, different aspects of the migration of GSC have been determined. First of all, we have identified different modes of cell migration, collective or individual imitating then the variety of tumor cells displacement in the brain. Cell-cell cohesion, anteroposterior asymmetry and hierarchical repartition of cells with the presence of leader and follower cells have been determined. We have also identified the importance of the physical organization of the matrix in the control of the directional migration of tumor cells, a phenomenon known as physical topoinduction. In fact, by producing aligned nanofibers, we have induced a cell migration in the direction of those fibers. This topology mimics the routes used by cancerous cells to invade the brain, especially the myelinated axons and the basal lamina of blood vessels. Ali Saleh, Zahra Hassani, Marisa Teigell, Soumaya Turpault, Aziz Cherifi, David Cornu et Norbert Bakalara. Institut des Neurosciences de Montpellier - Hôpital Saint Eloi - 80, rue Augustin Fliche - 34091 Montpellier. CBS2 Association assocbs2.com N°33 - Yukiko IMAI Initiation of meiotic recombination in mouse; search for interacting partners of PRDM9 Homologous recombination during meiosis is an essential event for faithful segregation of homologous chromosomes and production of genetic diversity. Meiotic recombination is initiated by the induction of programmed DNA double strand breaks (DSBs). Meiotic recombination takes place in specific regions of a genome, called hotspots, where initiation occurs preferentially. Recently, PRDM9 was reported as a protein involved in the specification of recombination hotspots in mouse and human. PRDM9 contains a PR/SET domain with histone methyltransferase activity that catalyzes the formation of H3K4me3 and a DNA binding domain. Our recent working model includes PRDM9 as a key component for the initiation of meiotic recombination: PRDM9 binds DNA via its zinc fingers and modifies chromatin structure locally. Through an unknown process, SPO11 is recruited and catalyzes DSB formation near PRDM9 binding sites. Our goal is to address the question: how does PRDM9 recruit DSB machinery to hotspots? To gain insight in this mechanism, we focused on characterization of PRDM9 interacting proteins. Here, we report potential interactors of PRDM9 identified by yeast two hybrid screens with testis cDNA libraries, as well as complex purifications followed by mass-spectrometry analysis. Yukiko IMAI and Bernard DE MASSY, Institut de Genetique Humaine CNRS UPR 1142 CBS2 Association assocbs2.com N°34 - Marco BRUSCHI Epigenetic modulation of intestinal cancer susceptibility The interplay between genetic and epigenetic lesions leading to the initiation and progression of cancer has been extensively studied, and the epigenetic alterations are nowadays considered as hallmarks of malignancies. We now aim at shedding light on the correlation between the interindividual epigenetic polymorphisms and the relative risk to develop malignancies. To investigate the molecular aspects related with tumor initiation in the intestinal epithelium we are using mice carrying a germline heterozygous mutation on the gatekeeper gene Apc (Apcd14/+). Upon the second mutational hit, these mice invariably develop intestinal adenomas during their adult life. Adult mice in our colony display an outstanding variability in terms of number of intestinal adenomas. A remarkable degree of such variability cannot be ascribed to major genetic changes, and the determinants of such genetic-independent heterogeneity are to be researched elsewhere. By mean of epigenome-wide analyses (i.e. RNA-sequencing, methylome profiling) we are therefore attempting to identify the molecular signature associated with such heterogeneity by analyzing the tumor-free tissue of bona fide syngeneic Apcd14/+ mice. To ascertain the predictive value of our results we defined an innovative strategy based on intestinal microsurgery performed on young mice to collect intestinal biopsies before cancer initiates. We are also investigating the remodeling occurring in the epigenome of intestinal cells early after the deletion of one or both the Apc alleles, whose loss represents the most common initiating event in colorectal cancer. To this aim we are taking advantage of mouse models in which the loss the Apc alleles is selectively induced in the intestinal epithelium, or specifically in the stem cell compartment. Our ultimate aims consist in defining the very early events occurring in the epigenome during malignant transformation and in identifying powerful epigenetic biomarkers, providing evidences of their value in the early prediction of cancer-associated risk within the population. Marco BRUSCHI(1), Stanislas QUESADA(1), Pierre CESSES(1), Maxime MAHE(2), Michael HELMRATH(2), Michael WEBER(3), Philippe JAY(1) 1: Institut de Génomique Fonctionnelle, Montpellier, UMR5203, INSERM U1191, UM. 2: Cincinnati Children Hospital Medical Center, Cincinnati, USA. 3: École supérieure de biotechnologie de Strasbourg, 67411 Illkirch CBS2 Association assocbs2.com N°35 - Chames KERMI Rad18 silences the UV-dependent DNA damage checkpoint in early Xenopus embryos In early embryos the DNA damage checkpoint is silent until the midblastula transition (MBT) due to maternal-limiting factors of unknown identity. Here, we identify the Rad18 ubiquitin ligase as one such factor in Xenopus. We show in vitro and in vivo, that inactivation of Rad18 function leads to DNA damage-dependent checkpoint activation, monitored by Chk1 phosphorylation. Moreover, we show that both Rad18 and PCNAmUb abundance are developmentally-regulated. Increased DNA abundance limits availability of Rad18 close to MBT thereby reducing PCNAmUb and inducing checkpoint derepression. Further, we show that this embryonic-like regulation can be reactivated in somatic mammalian cells by ectopic Rad18 expression thus conferring resistance to DNA damage. Finally, we find high Rad18 expression in cancer stem cells highly resistant to DNA damage. Altogether these data propose Rad18 as a critical embryonic checkpoint-inhibiting factor and suggest that Rad18 deregulation may have an unexpected DNA damage-dependent oncogenic potential. Chames Kermia, Susana Prietob, Siem van der Laanc, Nikolay Tsanovb, Bénédicte Recolina, Emmanuelle Uro-Costed, Bernadette Delisled and Domenico Maioranoa a Genome Surveillance and Stability laboratory, CNRS-UPR1142, Institute of Human Genetics. Montpellier. France ; b Present address: Institute of Molecular Genetics of Montpellier ; c Present address: CNRS UMR3145. Parc Euromedicine Cap Delta. Montpellier ; d Laboratoire Universitaire d'Anatomie Pathologique. Neuropathologie humaine et expérimentale. CHU Toulouse Rangueil. INSERM CRCT - Equipe 51, Toulouse.France CBS2 Association assocbs2.com N°36 - Stella COSENZA Differential effect of microparticles and exosomes isolated from mesenchymal stem cells on T cell proliferation and experimental arthritis Mesenchymal stem cells (MSC) are multipotent cells that possess immunomodulatory functions that are of high interest for cell therapy in various pathologies. MSC functions are primarily mediated by soluble mediators released in the extracellular milieu or within extracellular vesicles (EV). Even if the use of MSC is highly controlled, the safety of MSC injection in long term is still controversial. Thus, the use of EV derived from MSC could be a good alternative for therapeutic approaches. EVs consist of three main populations: exosomes, microparticles and apoptotic bodies that differ by their size, their composition and their secretion way. EVs seem to mirror the effect of parental cells but little is known about the respective role of the various subsets of EVs (exosomes and MP) secreted by a specific cell type. The aim of this project is to compare in vitro and in vivo the immunomodulatory effects of exosomes and microparticles secreted by MSCs. After purification of the two EV subsets by differential centrifugations, we characterized exosomes and microparticles on their size (less than 100nm and 400nm respectively), their structure (bilayer phospholipids) and their specific markers (endosomal markers, membrane cell markers). Then, we studied the functional effects of EVs in vitro in proliferative assays. Our analysis indicated that addition of microparticles significantly inhibited the proliferation of total splenocytes and CD4+ T cells in a dose-dependent manner whereas exosomes were not able to exert a suppressive effect. This immunomodulatory function of microparticles was also observed in vivo in the CIA model of inflammatory arthritis with a reduced incidence and reduction of clinical symptoms: paw swelling and inflammation. Our in vitro and in vivo data indicated that the immunosuppressive effect of MSCs is at least in part mediated by EVs and microparticles seemed to play a major role in T cell proliferation inhibition. Cosenza Stella1,2, Toupet Karine1,2, Luz-Crawford P1,2, Jorgensen Christian1,2,3, Noël Danièle1,2 1 Inserm U1183, Montpellier; 2Université Montpellier 1, Montpellier; CHU Montpellier, Unité Clinique d'Immuno-Rhumatologie, Montpellier, France CBS2 Association assocbs2.com N°37 - Amanda ABI KHALIL Epigenetics and phenotypes modulation in HMEC cells In tumor cells epithelial-mesenchymal transition (EMT) has been associated to increased invasiveness and stem like properties. EMT can be induced by various cytokines, as well as by ectopic expression of transcriptional regulators (EMT genes). A link between inactivation of p53 and EMT has been described and recent work has shown a significant link between EMT and epigenetics modifications. We developed a cellular model of stepwise transformation based on the sequential transduction of primary HMECs cells with defined genetic elements. The general idea was to create models representing different steps of transformation. In step 1 cells are immortalized, upon inactivation of p53 (shp53), in step 2 cells are transformed by ectopic overexpression of known oncogenes (WNT or RAS), which belong to distinct signaling pathways. Independent biological replicates were established for each genetic variant. Genetically modified cells were characterized at the phenotypic, genetic (CNC, mRNA and miRNA expression) and epigenetic (whole genome DNA methylation) to monitor changes occurring at each step of progression in our cellular model. Our data show for the first time to our knowledge that: (1) inactivation of p53 result in a drift in DNA methylation; (2) different epigenetics patterns determined by the oncogenic pathway that was activated. We isolated different shp53 cell clones that bore different phenotypes. Some kept epithelial characteristics while the others had acquired a fully mesenchymal phenotype. The aims of my project are to determine: 1) the link between DNA methylation and phenotypic changes in shp53 cells 2) if changing the methylation state of cells will revert their phenotypes 3) the impact of the oncogenes in the relation between methylation and phenotype 4) determine if EMT is essential to cell transformation. Amanda Abi khalil, thesis director: Charles theillet at "Institut de recherche en cancerologie de Montpellier U1194" CBS2 Association assocbs2.com N°38 - Milena MAGALHÃES DNA methylation and pulmonary disease in CF patients Cystic fibrosis (CF) is a multivisceral disorder caused by mutations in CFTR (Cystic Fibrosis Transmembrane Conductance Regulator), where p.Phe508del is the most frequent mutation. Morbidity and mortality in CF are mainly due to lung disease. Decrease in lung function is very variable among patients and depends on: the residual activity of the mutated CFTR protein, the genetic background (CF modifier genes) and the environmental exposure. Because environmental factors influence the phenotypes of living organisms by shaping the epigenome, we hypothesize that DNA methylation of modifier genes modulates the severity of pulmonary disease in CF patients. To provide comprehensive profiles of CF patients, we analyze DNA methylation (a) in 13 candidate modifier genes and CFTR by Bisulfite and NGS (454 Roche) and (b) genome-wide using the 450K BeadChip (Illumina). The study is carried out with METHYLCF, a multi-center prospective cohort specifically built for this epigenetic study of 50 p.Phe508del homozygous CF patients and 25 healthy volunteers. We collected patient and control nasal epithelial and whole blood cells to establish a biobank of DNA and RNA. DNA methylation analysis of candidate genes is almost achieved. By combining global methylation data in a Partial Least Square Regression, we correctly classified 74% of CF patients providing a CF-specific molecular signature. The majority of differentially methylated CpG were hypermethylated in NEC and hypomethylated in blood samples of CF patients. Also, we identified two DMR in genes involved in sodium transport and oxidative stress. DNA methylation of three genes correlated with the severity of pulmonary disease. The genome-wide DNA methylation analysis is in progress. Besides explaining the extreme phenotypes of CF patients characterized by the same mutation, this study may reveal modifier genes that were underscored by previous genetic and transcriptomic studies and highlight predictive markers of lung disease useful for CF follow-up. M. Magalhães1, R. Chiron2 , I. Rivals3, J. Varilh1,2, A. Bergougnoux1,2, E. Beyne1,2, L. Mely4, S. Leroy5, T. Ha3, D. Caimmi2, I. Vachier2, M. Claustres1,2, A. De Sario1. 1EA Université de Montpellier; 2Montpellier Hospital; 3ESPCI Paris; 4Hyères Hospital; 5Nice Hospital CBS2 Association assocbs2.com CBS2 Association assocbs2.com Posters : Session 2 CBS2 Association assocbs2.com N°39 - Béryl LAPLACE-BUILHE Pro-inflammatory macrophages mediated TNFa signaling is required for caudal fin regeneration in zebrafish larvae. Macrophages play an important role in the immune response to injury. However, a broader role in repair and regeneration has been reported. While macrophage ablation impairs epithelialisation and reduces scar formation in skin repair model in mammals, it impairs the regeneration of the limb in axolotl and of the fin in adult zebrafish. This discrepancy is likely due to the high plasticity of macrophages, which can adopt various phenotypes and functions. Here we used the zebrafish larva to study the role of pro-inflammatory, M1-like macrophages during caudal fin regeneration. Using 4D confocal microscopy and double transgenic larvae to visualise macrophages and TNFα expressing cells, we showed that initially most recruited macrophages expressed TNF-α (referred as M1-like). However TNF-α expression was transient and decreased from 24 hours post amputation, due to the recruitment of a second wave of noninflammatory macrophages (referred as M2-like) and to a local phenotypic conversion of macrophages. We demonstrated that TNF-α expressing macrophages were crucial for fin regeneration as early depletion of macrophages blocked blastema formation and regeneration process, while the depletion of late M2-like macrophages did not. We then turned our attention to the trophic control exerted by M1-like macrophages on the regeneration process and investigated the role of TNF-α signaling. Using a combination of morpholino knock down strategy and parabiosis experiments, we showed that TNFR1 played a necessary and direct role in the induction of fin regeneration by expanding blastemal cell. In summary the present data strongly suggest that TNF-a producing macrophages stimulate blastemal cell proliferation through the TNFR1 activation, revealing a new insight into the mechanism of caudal fin regeneration. 1,2* Laplace-Builhe B., 1,2*Nguyen-Chi M.,3Travnickova J., 1,2Luz-Crawford P., 1,2Tejedor G., 3Kissa K, 3Lutfalla G., 1,2Jorgensen C.,1,2Apparailly F 1,2Djouad F. 1 Inserm U 844, Montpellier, France; 2Université Montpellier 1, Montpellier, France; 3Université Montpellier 2, Montpellier, France ; *equally contributing authors CBS2 Association assocbs2.com N°40 - Jennifer BONINI Role of miRNAs in the Cystic Fibrosis pathology. Material & Methods: To identify targets in Cystic Fibrosis (CF), we assessed the miRNAs expression profile in ALI cultures from CF patients (p.Phe508del homozygous) or healthy individuals. We compared three epithelium models from nasal, polyps or bronchial biopsies (n=4 per condition).From total RNAs, a library was prepared according to the TruSeq Small RNA protocol and samples were sequenced by using a MiSeq sequencer (Illumina). Results were analysed by sRNAbench software. Then, deregulated miRNAs that act on the CFTR 3’UTR region were studied by luciferase assays. Results:We found that 9 miRNAs are deregulated in CF compared to non CF in the three ALI models. We also identified miRNAs which have been previously described in other studies to be deregulated in CF, such as miR-145, or involved in the ciliogenesis such as miR-449 family. Then, we studied miRNAs that putatively act on the CFTR 3’UTR region. Functional analysis showed that mir100 deregulated in CF have a repressive effect on CFTR stability in bronchial cells. Conclusion: Finding new regulatory players involved in CF physiopathology and/or controlling the CFTR mRNA level help us to envision new tools for Cystic Fibrosis therapy. - This work is supported by the association Vaincre la Mucoviscidose – J. Bonini (1,2), J. Varilh (3), R. Chiron (4), E. Brochiero (5), M. Claustres (1, 2, 3), M. Taulan-Cadars (1,2) 1. Université Montpellier I, France; 2. INSERM U827, ontpellier, France; 3. Service de Génétique Moléculaire, CHRU Montpellier, France; 4. Département des maladies respiratoires, CHRU Montpellier, France; 5. Département de physiologie moléculaire et intégrative, Université de Montréal. CBS2 Association assocbs2.com N°41 - Denis DUNOYER DE SEGONZAC Evolution of meiotic recombination: variation and function of the Prdm9 gene in mice In humans and mice, the genomic positions of DNA Double Strand Breaks (DSBs) initiating meiotic recombination appear tightly controlled by the DNA binding domain of PRDM9, made of a tandem array of C2H2 zinc fingers (ZnF). This domain has been shown to be extremely polymorphic; phylogenic studies suggest that Prdm9 is a fast evolving gene with residues involved in interaction with the DNA under positive selection. Prdm9 is also a major determinant of male sterility in hybrids (HS) between certain genotypes from two subspecies (musculus and domesticus) of the house mouse. We first tested the generality of the implication of Prdm9 in hybrid sterility and speciation by examining fertility of F1 males from crosses between various wild derived strains. These strains were harboring very different Prdm9 ZnF haplotypes: the size and the dissimilarity of their Prdm9 ZnF region guided us in the selection. 32 crosses involving four different M.m. musculus and four M.m. domesticus were analyzed, none of them lead to sterility. However, using the laboratory mice C57BL/6 crossed with a M.m. musculus, a phenotype of sterility was observed. The M.m. musculus Prdm9 allele is already implicated in hybrid sterility when crossed with C57BL/6 progenitor exclusively. In our case, the sterility phenotype does not depends of the direction of the crosses. We conclude that only a very specific combination of Prdm9 and/or genetic background leads to the hybrid sterility phenotype. In addition, as hybrid sterility is associated with an arrest in meiotic prophase at the stage of DSB repair, we started to monitor in detail the DSB repair activity. We are performing this by following by ChIP-SEQ the association of Dmc1, the protein involved in strand exchange during DSB repair, to single strand DNA. We aim to test whether DMC1 localization and or enrichment differs between fertile and sterile hybrids. CBS2 Association assocbs2.com N°42 - Estelle RASCOL Biophysical interaction of nanoparticles with biological fluids Mesoporous silica nanoparticle (MSN) is a promising material as drug delivery system or nanovector. This biocompatible material associated with porous, magnetic and fluorescent properties forms a multifunctional platform. The first challenge of my thesis was to study MSN biological stability and membrane cell interaction depending of different surface coatings, such as lipid bilayer or polyethylene glycol, to limit aspecific internalization. We characterized MSN in suspension with biologic media, using dynamic light scattering associated with transmission electron microscopy and zeta potential measurements. This physicochemical study shows low stability of MSN in suspension. This poor dispersibility of MSN is largely depending of ionic strenght and medium composition, such as protein content. MSN coating with lipid bilayer is a strategy to enhance MSN stability. We used cell membrane model to investigate MSN - cell membranes interaction. The model used is supported lipid bilayer on gold surface. This model membrane is simply composed of EggPC phospholipids. Interaction between MSN and cell membrane model is followed by surface plasmon resonance (SPR). This method, based on energy absorption of gold at the nanometer scale, is able to detect, with high sensitivity, little changes in refractive index at the near vicinity of gold surface. By varying MSN medium, lipid MSN coating (both influence MSN aggregation), and transmembrane potential, different responses were observed. For example, MSN coated with lipid bilayer interacts lower with membrane model than bare MSN. As a conclusion, the large choice of phospholipids, proteins and medium composition is a powerful tool to depict specific and aspecific interactions of bare, protein or lipid coated MSN with cell membrane. Premier auteur :Estelle RASCOL, Dernier auteur, Joël CHOPINEAU, Entre les deux : Jonas CROISSANT, Jeff NYALOSASO, Clarence CHARNAY, Yannick GUARI, Christophe DORANDEU,Jean-Marie DEVOISSELLE Affiliation de ces personnes : ICGM (Institut Charles Gerhardt, UMR 5253) Également :Magali GARY BOBO, Marie Maynadier, Marcel GARCIA. Affiliation de ces personnes : NanoMedSyn Et :Cédric PISANI, Odette PRAT, Jean ARMENGAUD Affiliation de ces personnes : CEA SBTN toxicologie (Marcoule) CBS2 Association assocbs2.com N°43 - Amélie TORA Allosteric modulation of metabotropic glutamate receptors by chloride ions. Metabotropic glutamate receptors (mGluRs) play key roles in the modulation of many synapses and are considered promising targets for the treatment of various CNS disorders. Chloride (Cl-) is known to directly bind and regulate the function of different actors of neuronal activity and several studies have pointed to the possible modulation of mGluRs by Cl-. Through the use of innovative biosensors and secondmessenger assays, we demonstrate herein that Cl- behaves as positive allosteric modulator of mGluRs. At mGlu4 receptors, for example, Cl- could increase glutamate potency by more than 900-fold. Cl- potency was 78.6±3.5 mM, close to the estimated resting value of extracellular Cl-. Cl- possesses a very high positive cooperativity with glutamate (Hill slope ≈ 6 on mGlu4), meaning that small variations in [Cl-] lead to large variations in glutamate action. Interestingly at mGlu3 receptors, not only Clpotentiates glutamate action but also increases basal activity of the receptors. Using molecular modeling and site-directed mutagenesis, we have identified two wellconserved Cl- binding pockets in the extracellular domain of mGluRs. Moreover, modeling of activity-dependent Cl- variations at GABAergic synapses suggests that these variations may be compatible with a dynamic modulation of the most sensitive mGluRs present in these synapses. Taken together, these data reveal a necessary role of Cl- for the glutamate activation of many mGluRs. Exploiting Cl- binding pockets may yield to the development of innovative regulators of mGluRs activity, as already exemplified by compounds like LSP4-2022 that occupy both the glutamate binding site and one of the Cl- sites. Amélie S Tora (1,2), Xavier Rovira (1,2), Ibrahima Dione (3), Hugues-Olivier Bertrand (4), Isabelle Brabet (1,2), Yves De Koninck (3), Nicolas Doyon (3), JeanPhilippe Pin (1,2), Francine Acher (5) and Cyril Goudet (1,2) (1) Institut de Génomique Fonctionnelle, CNRS UMR5203, Université de Montpellier, F-34094 Montpellier, France.(2) INSERM, U1191, F-34094 Montpellier, France.(3) Centre de recherche de l’Institut universitaire en santé mentale du Québec and UniversitéLaval, G1J 2G3 Québec, Canada.(4) BIOVIA Dassault Systèmes, 20 rue Jean Rostand, F-91898 Orsay Cedex, France.(5) Laboratoire de Chimie et Biochimie Pharmacologiques et Toxicologiques, CNRSUMR8601, Université Paris Descartes, Sorbonne Paris Cité, F-75270 Paris Cedex 6, France. CBS2 Association assocbs2.com N°44 - Haijin LIU Generation of a vaccine to prevent poultry from Newcastle disease and control viral shedding Newcastle disease (ND) is the major viral infection of poultry inducing high morbidity, mortality, and significant economic impacts on the poultry industry. ND is caused by virulent strains of avian paramyxovirus serotype 1 (aPMV-1) which have the capacity to spread over long distances. All strains of aPMV-1 belong to a single serotype and current vaccines have demonstrated their efficacy in terms of clinical protection. However, recent studies have shown that the virus has undergone significant evolution, which has led to the progressive emergence of new genotypes with potential antigenic drifts. The recently described genotype XI in Madagascar (Maminiaina et al, 2010) contains original amino acid substitutions on F and HN proteins, some of those clustered in the head of the proteins, presumably exposed to the host immune system, suggesting that these substitutions may account for antigenic drifts. Indeed, we showed in vivo, under controlled conditions, that current vaccines (genotypes II and III) induced equal clinical protection against genotypes II and XI, but were unable to prevent viral shedding of genotype XI comparing genotype II. In order to generate a vaccine preventing chicken from viral shedding and to try to understand the forces that trigger aPMV-1 evolution and correlate with protection, reverse genetics has been applied. NDV minigenomes expressing eGFP under two promoters (T7 and CMV) have been constructed and compared in vitro. Subsequently, full genomes of the genotype XI and II (NDV MG-725 and NDV LaSota) strains, have been assembled under CMV promoter. In addition, the F and HN genes of a live attenuated old-genotype virus (the genotype II Lasota strain) have been replaced by the corresponding genes of the recent Madagascar genotype XI. These viruses including the chimeric genotype XI-II will be characterized in vitro and finally evaluated in immunization/challenge trials. Haijin Liu(1,2), Renata S D Almeida(1,2), Patricia Gil(1,2), Minet Cécile(1,2), Emmanuel Albina(1,3) 1. CIRAD, UMR CMAEE, F-34398 Montpellier,France; 2. INRA, UMR 1309 CMAEE, F-34398 Montpellier, France; 3. CIRAD, UMR CMAEE, F-97170 PetitBourg, Guadeloupe, France. CBS2 Association assocbs2.com N°45 - Christelle NGBA ESSEBE Adaptation of Staphylococcus aureus to prolonged environmental stress conditions Objectives: Staphylococcus aureus (SA) is the most prevalent pathogen isolated in diabetic foot ulcers (DFU). Two SA populations are distinguished in DFU: one with low virulence present in colonizing ulcers and one with much higher virulence isolated in infecting ulcers. The difference between these two strains is the presence in the colonizing strain of a phage (Rosa-like), which alters the metabolism of the strain and induces a low virulence. Moreover the deletion of the phage restored the virulence of the strain. The purpose of this study is to determine the adaptation of the colonizing strain under different prolonged environmental stress conditions encountered during DFU and the potential of phage excision in these environments. Methodology: During 16 weeks, the colonizing SA strain NSA1385 were grown in different conditions: glucose 10%, antibiotics at 0,75x MICs (linezolid, vancomycin), anaerobia, associations between sugars and antibiotics (glucose + linezolid, glucose + vancomycin). Excision of the ROSA-like phage was evaluated by a multiplex PCR. The expression of the two main virulence genes (hla, spa) and the virulence regulatory genes (agr, rot, sae, sarA) were evaluated by qRT-PCR. Results: Our results showed that the ROSA-like phage is stable in the colonizing strain and cannot be excised whatever the stress condition tested after 16 weeks. Concerning the adaptation of NSA1385 during stress conditions, we observed that vancomycin increased the expression of hla after 16 weeks. Linezolid caused overexpression of agr and rot. Anaerobia downregulated agr and saeP. Glucose downregulated all genes except sarA and spa. These effects are almost entirely offset by the addition of antibiotics. Discussion: This study demonstrates the stability of the phage inserted in the colonizing strain. It also showed the adaptation of the strain to prolonged stress environmental conditions. All these results allow a best comprehension of the SA virulence in chronic wound conditions. Key words: Staphylococcus aureus, sugar, antibiotic, stress, expression, adaptation CBS2 Association assocbs2.com N°46 - Rémi LOGEAY Understanding the cooperation between Notch and the polarity determinant Scribble during neoplasia One classic model of solid tumour development is a progressive model. A first set of mutations triggers hyperplastic growth of the epithelial cells: cells remain polarised, become hyperproliferative, but the tissue is not capable of invasion. A second set of mutations later transforms this hyperplasia in neoplasia: cell polarity is lost and cells become invasive. In the wing imaginal discs of Drosophila melanogaster, this progression can be mimicked by constitutive activation of the Notch pathway to trigger hyperplasia and then by removing the epithelial polarity to trigger neoplasia. The Notch pathway is implicated in development and homeostasis of many proliferating epithelia. Upon activation, the receptor Notch is cleaved to release its intra-cellular domain which then enters the nucleus and binds the transcription factor Suppressor of Hairless to activate the transcription of the Notch pathway direct targets. The loss of polarity can be accomplished by mutating Scribble, a key component of the cortical complexes that establish and maintain epithelial polarity. However scribble mutation alone does not lead to hyperproliferation or invasion. It is actually the cooperation between Notch activation and loss of polarity that leads to an invasive neoplasia. The aim of my project is to dissect this cooperation including finding out if there is addition or synergy between the two processes. By comparing RNAseq and ChIP analysis for the transcription factor Suppressor of Hairless we will be able to identify the Notch direct targets in the different conditions: wild type, hyperplasia and neoplasia. We will then be able to determine if neoplasia and invasion are due to an additive effect (the loss of polarity adds its effects to the proliferation induced in the hyperplasia) or a synergic effect (the loss of polarity redirects the Notch pathway to new targets responsible of the invasion). Rémi Logeay, Alexandre Djiane Institut de Recherche en Cancérologie de Montpellier (IRCM U1194) CBS2 Association assocbs2.com N°47 - Claire TOLZA Identification of potential therapeutic targets regulated by Fra-1 and/or Fra-2 in triple negative breast cancers Triple negative breast cancers (TNBC) are of poor prognosis and there is currently no available targeted therapy. Fra-1 and Fra-2, two members of the Fos family involved in the formation of the AP-1 transcriptional complex, are frequently overexpressed in aggressive TNBC where they contribute to the tumorigenic phenotype. However, the panel of genes under the control of Fra-1 and/or Fra-2 in TNBC is still not clearly identified and the molecular mechanisms through which Fra-1 and Fra-2 control their expression are mostly unknown. Our aim is to identify and characterize the network of genes controlled by Fra-1 and/or Fra-2 in TNBC for a better understanding of the biology of these cancers and to identify and study potential druggable therapeutic targets. To identify the panel of genes regulated by Fra-1 and/or Fra-2, I carried out transcriptomic analysis in MDA-MB231 cells in presence or in absence of Fra-1 and/or Fra-2 by RNAi approach. The data were then crossed with our ChIP-seq data obtained for Fra-1 and Fra-2 in the same cell line, to select putative direct target genes. I am currently crossing this data with breast cancer data banks (CIT and TCGA) to select genes whose expression is also correlated to that of Fra-1 and/or Fra-2 in human tumors. Functional analysis of the selected genes will be carried out using RNAi approach. The attenuation of various properties promoting tumor aggressiveness (proliferation, cell viability, cell cycle, apoptosis, migration, invasion) will be studied. The observations will be extented to other TNBC cell lines. If inhibitors for the protein product of the studied genes are avalaible, they will be included in our tests. As Fra-1 and Fra-2 are also overexpressed in many epithelial aggressive carcinomas, our observations may have repercussion beyond breast cancer. Claire TOLZA, Marc Piechaczyk and Isabelle Jariel-Encontre. IIGMM, UMR 5535 CNRS, Montpellier, France. CBS2 Association assocbs2.com N°48 - Rana MELHEM Targeting Transferin Receptor 1 (TFR1) in Pancreatic Cancer Pancreatic cancer is a highly aggressive disease associated with poor diagnosis and high mortality. It is therefore necessary to search for new therapeutic targets or treatments. One of the interesting options would be targeting iron metabolism. Indeed, cell transformation is generally accompanied with increased needs for iron together with increased expression of the transferin receptor 1, TfR1, the major receptor involved in cellular iron supply via the internalisation of plasma transferin loaded with iron. We have generated a fully human anti-transferin receptor antibody, namely 3GH7, capable of blocking the entrance of iron bound transferin to cells thus exhibiting inhibitory effects on various pancreatic cancer cell lines. On the BxPC3 pancreatic cancer cell line, we show that the antibody decreases cellular viability, inhibits proliferation, and induces apoptosis. These effects are likely due to a drastic decrease in the labile iron pool which is a consequence of the blockage of transferin uptake. At the protein level, the antibody upregulates surface transferin receptor 1 and induces the expression of the metastasis suppressor NDRG1 as well as its phosphorylated form (Ser330, Thr346). NDRG1 has a widely reported anti-tumor function and is considered as a promising therapeutic target against pancreatic cancer.These results are to be completed with in vivo studies to further elucidate the possibility of using the anti-transferin receptor antibody as a therapeutic target in pancreatic cancer. Rana Melhem, Marie-Alix Poul, Thiery Chardes, Andre Pelegrin IRCM, INSERM U1194, ICM, Universite de Montpellier 1 CBS2 Association assocbs2.com N°49 - Ewelina GUCA Structural characterization of Plasmodium falciparum CCT and fragment-based drug design approach for targeting phospholipid biosynthesis pathway. Phospholipid synthesis metabolic pathways in Plasmodium falciparum are validated drug targets for new type of antimalarials. In the de novo Kennedy pathway of phosphatidylcholine biosynthesis, the second step catalyzed by CTP:phosphocholine cytidylytransferase [EC 2.7.7.15] is rate limiting. We are focused on the structural characterization of this enzyme, the identification of effectors by fragment-based drug design approach (FBDD) and then their optimization to eventually design a lead. We solved the X-ray crystal structure of the catalytic domain of the enzyme target (PfCCT) at resolution 2.2 Å and of the complexes with substrates and product. These data allows us to give detailed images of the binding pocket, to reveal conformational changes between apo- and holo-protein forms and to provide information about the mechanism of the catalytic reaction at atomic level. The FBDD method uses a library of small molecules (fragments) with molecular weight that does not exceed 300 Da to explore target binding sites. Screenings of a fragment library (300 molecules) has been performed by fluorescence-based thermal shift assay and Nuclear Magnetic Resonance Saturation Transfer Difference (NMR STD). This combination of techniques identified so far 4 fragment hits that are currently evaluated for their binding modes and affinities. Co-crystallization of the protein-fragments complexes is carrying out to provide accurate information on the molecular interactions. Topology of these interactions will be used to rationally monitor every iterative round of the optimization process allowing subsequent rational design. Ewelina Guca1, Francois Hoh2, Jean-Francois Guichou2, Christian Roumestand2, Henri Vial1, Rachel Cerdan1 1 - DIMNP UMR 5235, Université de Montpellier. 2 - CBS CNRS UMR 5048 CBS2 Association assocbs2.com N°50 - Sara HAYDAR PPM1K (protein phosphatase, Mg2+/Mn2+ dependent, 1K) Gene Association in Polycystic Ovary Syndrome for Better Understanding of the Role of Branched-Chain Aminoacids Variation in Metabolic Disorders Polycystic ovary syndrome (PCOS), an endocrine disorder characterized by abnormalities in reproduction and metabolic disorders has been recently associated with plasma variations of branched-chain aminoacids (BCAA). Moreover, BCAA catabolism pattern has been related to insulin resistance and susceptibility to type 2 diabetes (T2D) and BCAA plasma levels were reported as different in PCOS. Many genes, as PPM1K (protein phosphatase, Mg2+/Mn2+ dependent, 1K) are implied in the catabolism of BCAA and are then candidates for the association to PCOS and its components. In this context, we carried-out a case-control study in a population from Central Europe focusing on the association of PPM1K in PCOS, using as marker the SNP (single nucleotide polymorphism) rs1440581 C/T, previously reported as leader in association with insulin resistance. At first we assessed the linkage disequilibrium (LD) pattern on the genomic region by screening, 48 SNPs surrounding the leader SNP rs1441581 in 55 cases and 48 controls, using Affymetrix technology, and continued the genotyping of rs1440581 by KASPar in the rest of the population (reaching 401 cases and 143 controls). LD pattern, haplotype reconstruction and cladograms determination were obtained by HAPLOVIEW 4.2, PHASE 2.1 and ARLEQUIN 2.000 softwares, respectively. Gene association and genotype-phenotype correlation were calculated by logistic regression and ANOVA using STATVIEW 5.0 and Abacus. We observed LD block involving 6 SNPs and rs1440581, and reconstructed 9 haplotypes among which H4 (TCTACTT), H6 (TTCATTC), H9 (CTCACCT), H3 (TCTACTC) and H2 (TCCGCTC) are more frequent (38.3, 35.9, 8.7, 8.3 and 5.3%, respectively). Trend of association of rs1440581 C allele with metabolic syndrome (MetS) in PCOS was found (P = 0.07, OR 1.97 95%CI [0.94 – 4.09]) which is concordant with the literature. This allele is the ancestral one in the cladogram. The present pilot study is in progress and further data are expected. Sara Haydar(1), Redha Attaoua(1), Mihai Coculescu(2), Madalina Vintila(2), Nicoletta Baculescu(2), Christophe Normand(1) and Florin Grigorescu(1) 1) IURC, Molecular Endocrinology Laboratory, Nutrition & Genomes, UMR-204 NUTRIPASS, Montpellier, France. 2) Departement of Endocrinology, University of Medicine and Pharmacy "Carol Davila", Bucharest, Romania CBS2 Association assocbs2.com N°51 - Alejandra DAMIAN Identification of new regulators of the Notch pathway in KRASG12V-driven NSCLC Previously, it has been shown that oncogenic mutated KRAS activates the Notch pathway in Non-small Cell Lung Cancer (NSCLC) cells and that Notch is critical for both the generation and the maintenance of NSCLC (Maraver et al., 2012; Maraver and Serrano, 2012). The aim of this study is to determine the mechanisms involved in how oncogenic KRAS activates the Notch pathway in NSCLC and to identify which are the genes mediating Notch activation only in the oncogenic setting. In order to achieve this objective, we will perform four consecutive screenings using different biological systems. First, we will use NSCLC cell lines derived from mutant KrasG12V-driven adenocarcinoma from mouse (Ambrogio et al., 2014a) to perform high-throughput screening using the NKI 15000 library of shRNAs. As a reporter, we will use the pGreenfire-Notch lentiviral plasmid that co-express destabilized GFP and luciferase under the control of Notch response elements (System Biosciences). Then, we will perform a second in vitro screen with 200 genes candidates in the human cell lines BEAS-2B transformed with KRASG12V and in the non-transformed parental one, to find those new key players that inhibit Notch pathway in KRASG12V transformed cells. To be sure that the genes that we may find in the cultured cells play a decisive role in a 3D in vivo setting, we will perform a genetic in vivo screen using Drosophila as model. Finally, those putative new regulators that are consistent among all the screens, conserved from flies to human cells, will be tested in KrasG12V-driven NSCLC in mice models. These key genes acting downstream of oncogenic KRAS to activate Notch would represent very relevant targets for the development of new anti-cancer drugs. More importantly, these genes would be selective for cancer cells not affecting the healthy ones and avoiding the side-effects of Notch inhibition. CBS2 Association assocbs2.com N°52 - Joelle AZZI Identification of kinase inhibitors as alternatives for the treatment of metastatic castration-resistant prostate cancers Prostate cancer is the most common cancer among men with an increasing incidence with age. Localized tumors are treated with surgery or radiotherapy while the most advanced forms are treated by androgen deprivation. However, most of these patients become resistant to castration and are treated with taxane-based chemotherapy (docetaxel or cabazitaxel) or second generation hormonal treatments (abiraterone acetate or enzalutamide) with limited effectiveness. Other anticancer agents have been tested without significant improvement of overall survival. Moreover, these studies do not necessarily take into account the genetic characteristics of this type of tumor. With the emergence of new sequencing techniques, it is possible to have a better idea of specifically deregulated or mutated genes in these cancers. The aim of my thesis is to identify new potential treatments that can be used as an alternative to taxanes based on the specificity of mCRPC (metastatic castration-resistant prostate cancer) tumors, in particular gene expression profiles. Using the NCI60 databases, we looked for correlations between the expression levels of 96 genes characterizing the evolution of prostate cancer evolution towards castration resistance and the sensitivity to kinase inhibitors, with the goal of identifying derivatives that may have better efficacy than taxanes. We identified several genes, the expressions of which are significantly correlated with cell sensitivity to two inhibitors of the MAPK pathway: vemurafenib (targeting RAF) and selumetinib (targeting MEK). We are currently in the process of validating these correlations at the functional level by investigating whether the modulation of their expression could indeed alter the sensitivity of prostate cancer cells to those two kinase inhibitors. In longer terms, the signatures of expression that will be validated by our approach could be used to identify patients most likely to respond to vemurafenib or selumetinib, an essential step in the development of prospective clinical trials. Joelle AZZI, Hanane AGHERBI, Philippe POURQUIER, Nadine HOUEDE INSERM U1194 Institut de Recherche en Cancérologie de Montpellier & CHU de Nîmes CBS2 Association assocbs2.com N°53 - Barbara ZIEBA Assembly of proteasome and epidermal differentiation: interest in psoriasis Proteasomes play a critical role in cell homeostasis through the regulated degradation of most intracellular proteins. Previous work in our lab has shown that it is overexpressed in the epidermis upon psoriasis, which is the most common, relapsing skin pathology characterized by inflammation, hyperprofileration of keratinocytes and impaired epidermal differentiation [ED]. This increase is likely to be caused by enhanced assembly of the proteasome since no change in the transcription levels of various subunits can be detected. Indeed one of the proteasome assembly chaperones POMP - seems to play important role in ED. It was shown that a point mutation that silences expression of this protein is directly linked to KLICK syndrome - a rare pathology of ED. We observed increased expression of POMP in psoriatic lesions compared to healthy epidermis. Therefore we hypothesize that balanced proteasome assembly plays an important role in proper keratinocyte differentiation. To test this hypothesis we established an in vitro model of ED using immortalized keratinocytes, HaCaT cells. We observed a peak (≈50% increase) in POMP expression 24h after [Ca2+]-induced differentiation. In order to then investigate deeper the role of POMP in ED we are presently creating HaCaT cell lines stably expressing POMP and we will perform POMP silencing experiments in parallel. In a different approach, we analyzed the proteasome content of HaCaT cells during differentiation and showed by native PAGE that the proteasome disassembles during differentiation, while expression of its subunits remains unchanged. We believe that this disassembly is linked to oxidative stress that is reported to participate in ED and we are planning to study the possible causal relationship between these two phenomena. CBS2 Association assocbs2.com N°54 - Mouna TRIKI Expression of the transcriptional coregulator RIP140 in colorectal cancer Receptor Interacting Protein 140 (RIP140) is a transcriptional coregulator essential for female fertility which is involved in inflammation, lipid metabolism and cognition. Recently, it has been shown that RIP140 is also implicated in intestinal homeostasis and colon cancer. Moreover, LCoR (ligand-dependent corepressor) was found to be a partner and a transcriptional target gene of RIP140. The aim of this study is to better characterize the expression of RIP140 and LCoR in colorectal tumors by immunohistochemistry. We have initiated the study of the two proteinsin 161 colorectal carcinoma (CRC) specimensf rom Tunisian patients in order to evaluate their correlation with different clinicopathological parameters.In this cohort, the male/female ratio was 1.01 and the patient ages ranged from 17 to 92 years (mean age: 63 years). Our preliminary results showed that RIP140 and LCoR expression was positive in 57.8% (93 out of 161 cases) and 67.7% (109 out of 161) respectively. Significant association of LCoR expression and tumor site was found. Indeed, 74.4% of tumors in rectum were positive for LCoR while only 51.3% of colon tumors expressed this protein (p=0.009). When we consider the expression of both proteins, we found that 56% and 38.5% of specimens were respectively positive and negative for both LCoR and RIP140. The association between RIP140 and LCoR staining and clinicopathological parameters (tumor grade, lymph node invasion, patient survival…) is under investigation. The correlation with the expression of different actors of the Wnt pathway will also be investigated.In parallel, we will analyze the methylation status of the RIP140 promoter in tumor tissues. In preliminary experiments, the unmethylated pattern of RIP140 promoter was found in 70% of cases, nevertheless, it needs to be confirmed on larger sample size. Keywords:Receptor Interacting Protein 140 (RIP140), colorectal cancer, Wnt, DNA methylation. Mouna TRIKI1,2, Lobna AYADI3, Abdelmajid KHABIR3, Vincent CAVAILLES1, Raja GARGOURI2 1 IRCM, Institut de Recherche en Cancérologie de Montpellier, INSERM U1194, Université Montpellier, Montpellier, France.2Laboratory of Cancer Genetics and Production of Therapeutic Proteins, Center of Biotechnology, Sfax, Tunisia.3 Department of Pathology, Habib Bourguiba Hospital,Sfax, Tunisia. CBS2 Association assocbs2.com N°55 - Alicia MADGWICK Evolutionary Plasticity of Endodermal Gene Regulatory Networks in Ciona intestinalis and Phallusia mammillata Regulatory evolution of developmental genes is an important source of morphogenic diversity. This phenomenon has been suggested to be invovled in many organisms such as for the vulva of C. elegans, colour patterning in Heliconius wings and even the beak shape of Darwin’s finches. However, regulatory evolution could also be a source of morphogenic conservation. Ascidians Ciona intestinalis and Phallusia mammillata diverged over 300 million years ago yet they have conserved an almost identical morphology throughout embryogenesis. Their genomes have greatly diverged which suggests that the gene regulatory networks (GRNs) regulating embryogenesis must have also undergone modifications. Ascidians are sessile marine invertebrates that belong to the subphylum Tunicata and the phylum Chordata. Their small genome and their simple, invariant early development make ascidians an invaluable tool for studying both evolution and developmental biology. These simple organisms are ideal to study GRNs at a cellular level and to observe inter-species regulatory evolution. Ciona embroygenesis is well documented; much of this data has been detailed on the ANISEED website including expression data from wild type and knockdown experiments. In contrast, Phallusia has not been studied as extensively; therefore, I am initially investigating the spatial and temporal expression of the homologous Phallusia genes known to be involved in Ciona early endoderm development by in situ hybridisation. It will therefore be possible to determine to what extent gene expression has diverged in these two species before investigating what interactions have evolved within the endodermal GRNs to accommodate these divergences. The endoderm is an interesting tissue when studying morphology as it drives gastrulation during which time the endodermal cells do not undergo division in ascidians. Once the GRNs of both organisms have been built and compared, we will then be able to evaluate the mechanisms that have allowed evolution of the regulation of these ascidians. CBS2 Association assocbs2.com N°56 - Ruizhi TANG The role of primary cilia in colon homeostasis and tumor development The primary cilium is a sensory organelle expressed on nearly all eukaryotic cells. Primary cilia are assembled on the basis of a microtubule component, the axoneme. The functions of primary cilia are modulation of signaling pathways including WNT and Hedgehog (HH), which are essential in the regulation of intestinal homeostasis. We have recently described that glycylation, a posttranslational modification of microtubules, is crucial in the maintenance of primary cilia. We observed a decreased number of primary cilia and increased cell proliferation in the colon in mice deficient for the glycylase TTLL3, which is the only glycyclase expressed in the colon. Despite this overproliferation, TTLL3-deficient mice display a normal tissue architecture of the colon. However, loss of glycylase activity promotes induced colon carcinogenesis. In my PhD project we will focus on the consequences of a complete loss of primary cilia in intestinal epithelial cells and intestinal myofibroblasts respectively. For this, we will use villin-cre-mediated recombination to generate mice in which components of the ciliary transport machinery (Kif3A or Ift88) are knocked out specifically in the intestine. Mice will be analyzed for altered colon homeostasis and altered susceptibility for induced colon carcinogenesis. In addition, we will investigate altered WNT and HH signaling by the analysis of respective target genes in colon and the use of WNT and HH reporter constructs in isolated colonic epithelial cells or intestinal organoid cell cultures. My work should provide direct proof that the primary cilia regulate proliferation of colon epithelium. Ruizhi Tang1,2, Laura Papon1,2, Cecilia Rocha1,2,3,4,5,6, Carsten Janke3,4,5,6, Michael Hahne1,2,7 1 IGMM CNRS UMR5535, Montpellier, France, 2 Université Montpellier Sud de France, Montpellier, France, 3 Institut Curie, Orsay, France, 4 PSL Research University, Paris, France, 5 CNRS UMR3306, Orsay, France, 6 INSERM U1005, Orsay, France, 7 Academic Medical Center, Amsterdam, The Netherlands CBS2 Association assocbs2.com N°57 - Sana BELKAHLA The effect of dichloroacetate(DCA) on tumor cell metabolism Several clinical studies have shown the efficacy of DCA in the treatment of several metabolic diseases and is currently in clinical trials for the treatment of cancers. DCA reverses cancer metabolism, causes cancer cell apoptosis in some cancer cells and works synergistically with other cancer therapies, such as radiation, gene therapy, and viral therapy or with chemotherapy. AMPK, is an important sensor of intracellular energy levels, targets ACC, FASN, mTORC1 and p53, thereby inducing oxidative metabolism, propelling fatty acid oxidation and inhibiting ATP-consuming anabolism. Indeed, metformin, which activates AMPK, also shows anti-cancer effect. Moreover, the mitochondrial membrane potential modulates the mitochondrial apoptotic pathway, e.g.cytochrome c redox state regulates apoptosis. An important partner of AMPK is the tumor suppressor p53, which is emerging as an important regulator of metabolic homeostasis. Therefore, a clearer understanding of the signals and mechanisms by which DCA sensitizes cancer cells to chemotherapy is needed to understand its mode of action. In addition, identification of this mechanism will help to elucidate metabolic pathways involved in cancer cell survival. During our studies, we observed a link between DCA sensitivity and p53 status. However, it is of great interest to identify the mechanism underlying DCA-induced leukemic cell elimination because this should help to select blood-borne cancer patients who could effectively benefit from this treatment. Sana Belkahla1, Ewelina Krzywinska1, Abrar Ul Haq Khan1 , Nerea Allende-Vega1 , Dang-Nghiem Vo1, Martin Villalba1,2. 1/ INSERM, U1183; Université de Montpellier 1, UFR Medecine, 80, av. Augustin Fliche. 34295 Montpellier Cedex 5, France.2/ Institut de Regenerative Medicine et Biothérapie (IRMB), CHU Montpellier, Montpellier, 34295, France. CBS2 Association assocbs2.com N°58 - Sophie KAN Heterochromatin factors stimulates telomere transcription Telomeres are critical regions that protect chromosome ends from degradation or aberrant repair. These regions are assembled into heterochromatin. Here, we investigate the function of Histone H3 lysine 9 trimethylation at the telomeres in mouse embryonic stem cells. Heterochromatin is typically believed to repress gene expression but we found that at telomeres, the H3K9me3 mark instructs transcriptional elongation and/or inhibit transcriptional termination of telomeres into the non-coding RNA TERRA. Using the quantitative PICh method, we further show that this mark controls the recruitment of histone chaperones that are necessary to maintain RNA polymerase II processivity on telomeres. We propose that it occurs genome-wide, and is broadly involved in the general transcriptional response to stressful conditions in mammals. Sophie Kan, Nehmé Saksouk and Jérôme Déjardin, Institut de Génétique Humaine, CNRS, France CBS2 Association assocbs2.com N°59 - Olfa KHALIFA Common variants on XQ28 conferring risk for rheumatoid arthritis in tunisian and french populations Background and Objectives: Rheumatoid arthritis (RA) is a systemic autoimmune disease characterized by a chronic destructive inflammation in synovial joints that is about three times more common in women than in men. Investigations into RA genetics have identified several susceptibility loci. Among these, multiple singlenucleotide polymorphisms (SNPs) at an X chromosome locus harbouring IRAK1 and TMEM187 have previously been shown to be associated with susceptibility to RA in Greek, Chinese, and Korean populations. The present study aimed at investigating the association between critical polymorphisms in Xq28, from rs1059702 (C/T) and rs1059703 (C/T) in IRAK1 through rs13397 (A/G) in TMEM187 with risk for RA in two novel populations: Tunisian and French. In addition, the present study aimed at comparing the differences in genotypic distribution in both populations. Material and methods: A case–control study of 493 RA patients and 507 healthy controls age and sex matched was conducted in both Tunisian and French. All RA patients were ACPA positive. DNA was isolated from total blood using standard phenol chloroform method. All subjects were genotyped for the three polymorphisms using a direct sequencing with the BigDye Terminator v3.1 Cycle Sequencing Kit (Applied Biosystems). The genotype distribution, haplotype analysis, and the linkage disequilibrium (LD) were analysed using the Bayesian method, and PLINK 1.07 and Haploview 4.2 softwares, respectively. Results: The three polymorphisms respected Hardy-Weinberg equilibrium, both in Tunisian and French populations. The associations between both IRAK1 rs1059703 and TMEM187 rs13397 polymorphisms and RA susceptibility were found (p<0.001 and p=0.004, respectively) in women, but not in men. The genotype CC of rs1059703 represented a protective factor for RA (OR= 0.29, 95% CI=0.17-0.50). Linkage disequilibrium between the 3 SNPs was weak (D=8-16). There were 5 haplotypes with a frequency higher than 5%, constructed from the Xq28 polymorphisms. Haplotype GTC was associated with decreased risk for RA (p=0.00075), whereas the haplotype ACC was significantly associated with increased risk for RA (p<0.001). Correlation analyses with clinical and biological parameters are in progress. Conclusion: Our case-control study replicated for the first time the association of the Xq28 chromosomal region with RA risk in Tunisian and French populations, and suggested that RA susceptibility is associated with rs1059703 polymorphism in IRAK1 and rs13397 polymorphism in TMEM187 only for female patients. These data further support the involvement of X chromosome in RA susceptibility. CBS2 Association assocbs2.com N°60 - Beren GARCIA MENDEZ Brucella replication in human trophoblasts: role of the eukaryotic protein CD98hc Brucellosis is one of the most important bacterial zoonosis worldwide, causing huge economic losses and long lasting health problems in many countries, mainly around the Mediterranean basin. This disease is caused by the pathogenic bacteria Brucella. In female animals, the main consequence of Brucella infection is abortion, but it is still unclear if it can also cause abortion in Humans. Recently, it has been shown that several species of Brucella can replicate within human placental cells (trophoblasts) (Salcedo et al., JID, 2013). This observation raised the question about a link with the ability of these bacteria to cause abortion. The aim of this PhD project is to identify some of the factors required for Brucella replication in human trophoblasts, from both the pathogen and the host side. We have examined the replication profile in trophoblasts of a panel of Brucella strains (representing different species, host or associated symptoms), including two strains that caused abortion in non-human primates. Our data shown that there is no clear correlation between the ability of Brucella to replicate within trophoblasts in vitro and whether they caused abortion or not. From the host side, we will focus on the eukaryotic protein CD98hc, which has important functions in placental cells and that was found to be essential for Brucella replication in other cellular models (Keriel et al., JID, 2014). We first checked whether Brucella infection would alter either CD98hc expression or its cellular sub-localization in trophoblasts. We found that none were affected by Brucella infection. We are now knocking-down CD98hc expression in trophoblasts to see if Brucella require this protein for intracellular replication in trophoblasts. With this project we hope to have a better comprehension of how some Brucella species can replicate in placental cells and might allow explaining why this bacteria can cause abortion. Karellen Beren GARCIA MENDEZ1,2; Jean-Pierre GORVEL3,4 ; David O’CALLAGHAN1,2 ; Anne KERIEL1,2. 1 INSERM, U1047, Nîmes, France. 2 Université Montpellier, U1047, Nîmes, France. 3 Centre d'Immunologie de Marseille-Luminy (CIML), Marseille , France. 4AixMarseille University , Marseille , France CBS2 Association assocbs2.com N°61 - Iman HALLOUM Identification and characterization of Mabs4780, a new determinant required for intracellular survival and pathogenicity of Mycobacterium abscessus Background: Mycobacterium abscessus (Mabs) is an emerging rapid-growing mycobacteria causing severe lung infections, particularly in CF patients. Unlike the smooth (S) variant, the rough (R) variant is characterized by the loss of surface glycopeptidolipids. Despite the involvement of Mabs R in severe clinical forms, the underlying physiopathological mechanisms remain obscure. Aims. Herein, we aimed to decipher the contribution of MABS4780 in Mabs virulence and investigate the molecular paradigm for its involvement in intracellular survival in various cellular and animal models. Methods: A MABS4780 deletion mutant was constructed and permeability of its cell wall and susceptibility to several antibiotics were assessed. The intracellular fate and virulence of the mutant were investigated in murine macrophages, Acanthamoeba castellanii and in zebrafish embryos. Results: The mutant exhibited a higher susceptibility to thiacetazone, compared to the parental strain and increased sensitivity to detergents, presumably due to alterations of cell envelope composition. Concurrently, the crystal structure of the M. smegmatis orthologue unraveled hotdog domains, characterizing dehydratases, thus potentially linking MABS4780 to lipid metabolism. The mutant failed to replicate in macrophages and in A. castellanii, thought to be the Mabs environmental reservoir, and was highly attenuated in zebrafish embryos. Conclusion: This demonstrates the unanticipated role of MABS4780 in Mabs R virulence and persistence in environmental amoeba. Future work will address the mechanism of attenuation of the mutant. Our results also emphasize the potential of this dehydratase as an attractive drug target. CBS2 Association assocbs2.com N°62 - Chloé MAURIZY Role of R2TP/HSP90 system in mouse development and colorectal carcinogenesis The Heat Shock Protein 90 folds the protein substrates neo-synthesized into an active state. HSP90 inhibition results in degradation or aggregation of the substrates. Many clients are involved in signal transduction pathways and related to tumor progression. We know that the inhibition of HSP90 destabilizes HSP90 clients and could lead anti tumoral effects. Until now, it was believed that this effect was due to the inhibition of receptors and kinases. A new HSP90 co-chaperon has been described: R2TP complex. It formed by four proteins: Rvb1, Rvb2, Spaghetti/RPAP3 and Pih1D1. HSP90/R2TP system is involved in the assembly of snoRNP, telomerase RNP, the nuclear RNA polymerases and PIKKs, which all play some key functions in cellular proliferation. On the one hand, HSP90 is involved in cancer so that more than 12 drugs inhibiting its activity, have been tested in clinical trials. On the other hand, three components of R2TP, Rvb1, Rvb2 and Spaghetti are overexpressed in hepatocellular and colorectal carcinoma (our unpublished results). We hypothesize that the co-chaperon R2TP is necessary to sustain, at least in part, the transforming activity of HSP90. To study the role of R2TP in animal development and carcinogenesis, we generated animals deficient for SPAGHETTI (SPAG) protein. We have generated mouse lines harboring two different alleles: a Floxed one and one encoding a truncated protein. We chose this subunit because (i) it interacts directly with HSP90, (ii) it overexpressed in colorectal and hepatocellular cancer and (iii) it is not essential in yeast. Our preliminary data show that SPAG is expressed in all tested adult tissues. Moreover, preliminary results suggest that SPAG is necessary for mouse embryonic development. This correlates with the function of Spaghetti in Drosophila Melanogaster. One fundamental interest of this work is that very few HSP90 cochaperone have been characterized in mouse model so far. Chloé Maurizy : Institut de Génétique Moléculaire de Montpellier, université de Montpellier, Bérengère Pradet-Balade : Centre de Recherche de Biochimie Macromoléculaire, Edouard Bertrand : Institut de Génétique Moléculaire de Montpellier CBS2 Association assocbs2.com N°63 –Samy MURAT Phosphoproteomics of 5-HT2A/mGlu2 heteromers: toward new insights into the mechanism of action of hallucinogens and antipsychotics The serotonin 5-HT2A receptor is the primary target of psychedelic hallucinogens such as LSD, mescaline and psilocybin (agonists), which reproduce some of the core symptoms of schizophrenia and of second-generation antipsychotics such as clozapine, olanzapine and risperidone (antagonists or inverse agonists). Recent findings demonstrate that 5-HT2A receptors form heteromers with metabotropic glutamate mGlu2 receptors, another target of last-generation antipsychotics (agonists or positive allosteric modulators). The association of both receptors has profound consequences on their pharmacology and signal transduction properties as well as on the behavioural effects of drugs that bind to either 5-HT2A receptors or mGlu2 receptors. For instance, 5-HT2A receptor/mGlu2 heteromer formation is essential for the expression of psychotropic-like effects of hallucinogens and imbalanced activity and coupling properties of 5-HT2A and mGlu2 receptors within the heterocomplex might be one of the molecular substrates for a susceptibility to schizophrenia. To get further insight into the mechanism of action of drugs acting at 5-HT2A/mGlu2 heteromers, we explored their impact upon the phosphorylation pattern of each receptor by high-resolution mass spectrometry. We show that hallucinogenic 5-HT2A receptor agonists (LSD, DOI) but not non-hallucinogenic 5HT2A receptor agonists promote 5-HT2A receptor phosphorylation at Ser280 located in the i3 loop, a region important for receptor desensitization, both in HEK-293 cells and in mice prefrontal cortex. Correspondingly, Ser280 phosphorylation was responsible for the lower capacity of hallucinogens to promote receptor desensitization and internalization, compared with non-hallucinogenic agonists. Conversely, several phosphorylated residues were identified in the C-terminal domain of mGlu2 receptors co-expressed with 5-HT2A receptors in HEK-293 cells. Glutamate treatment increased the phosphorylation state of some of these residues, an effect prevented by the coapplication of the synthetic hallucinogen DOI, which alone did not affect mGlu2 phosphorylation. Collectively, these findings reveal novel molecular substrates that might underlie the behavioural effects of drugs acting at each subunit of 5HT2A/mGlu2 heteromers. Samy Murat(1-4), Samah Karaki(1-4), Carine Becamel(1-4), Clotilde Mannoury la Cour(5), Mark J. Millan(5), Laurent Prézeau(1-4), Joël Bockaert(1-4), Philippe Rondard (1-4), Philippe Marin(1-4*), Franck Vandermoere(1-4*) (1) CNRS, UMR-5203, Institut de Génomique Fonctionnelle, Montpellier; (2) INSERM, U661, Montpellier; (3) Université Montpellier 1,Montpellier; (4) Université Montpellier 2, F-34094 Montpellier, France ; (5) Institut de Recherches Servier, Croissysur-Seine, France. (*) These authors equally contributed to the study CBS2 Association assocbs2.com N°64 - Camille JACQUELINE Immunodepression and accumulation of cancerous cells: a role of everyday perturbations? Immune cells are a key component against cancerous cells proliferation through their ability to detect and to destroy them. However, immune system experiences temporary immunodepression periods combined with long-term immunosenescence process. Thanks to a theoretical model, we wanted to show how these immunodepression periods, by their frequency and their duration, may impact cancerous cells proliferation. Our results suggested that long immunodepression period can have a significant impact on cancerous cells accumulation, with a stronger effect if such immunodepression occurs early in life. Nevertheless, for a given total duration of immunodepression, we highlight that numerous shorts episodes have a stronger influence on cancerous cells accumulation than a long one. Our results suggest new approaches where immunodepression factors should be treated to prevent threatening accumulation of cancerous cells. We can also speculate about a potential novel indirect role of infectious diseases on cancer incidence by diverting the immune reaction against cancerous cells. CBS2 Association assocbs2.com N°65 - Berfin SEYRAN E4F1 is a major regulator of pyruvate metabolism in normal skin homeostasis and skin carcinogenesis The multifunctional protein E4F1 is an essential regulator of normal skin homeostasis. E4F1 inactivation in embryonic or adult skin results in stem cell autonomous defects causing exhaustion of the epidermal stem cell (ESC) pool from their niche. At the molecular level, we have recently shown that E4F1 controls ESC maintenance through the transcriptional regulation of components or major regulators of the pyruvate dehydrogenase (PDH) macro complex, which metabolizes pyruvate into acetyl-coA in order to link glycolysis to the Krebs cycle. Our data demonstrates that defective PDH activity in E4F1KO keratinocytes results in the redirection of glycolytic flux towards lactate secretion both in vivo and in vitro. This metabolic reprogramming correlates with alterations of the microenvironment and affects ESC adhesion in their niche. Thus, our data highlights for the first time how cellular metabolism impacts on ESC maintenance and skin homeostasis. Based on these results and on growing evidences linking pyruvate metabolism to cancer development, I now wish to investigate the functions of E4F1 during skin carcinogenesis, more specifically in melanoma, which is the most aggressive type of skin cancer. Melanoma, through a multistep process, arises from melanocytes and is driven by mutations in the Ras/ Raf signaling pathway. In the early steps of melanogenesis, nevi which are benign tumors also harboring Ras/Raf genetic alterations, melanocytes display senescent features, which have been described as a barrier against malignancy. Interestingly, it has been shown that PDH is a crucial mediator of this Braf-induced senescence. Moreover, recent results from the lab point out the importance of E4F1 in regulating senescence also through PDH modulation. Taken altogether, these data led me to characterize a potential E4F1 and Ras/Raf cascade interplay, its influence on PDH regulation and how it impacts melanomagenesis. Berfin Seyran, Perrine Goguet, Laurie Gayte, Florence Bernex, Hélène Delpech, Charles Vincent, Nelly Pirot, Claude Sardet, Matthieu Lacroix and Laurent Le Cam. IRCM, Institut de Recherche en Cancérologie de Montpellier, INSERM U1194 CBS2 Association assocbs2.com N°66 - Moïra ROSSITTO Risks of in utero NSAIDs and paracetamol exposure on the early development and maturation of the reproductive organs The non-steroidal anti-inflammatory drugs (NSAIDs) and acetaminophen (ACE, paracetamol) are used worldwide to reduce mild to moderate pain, fever... Some medications are available over the counter without a prescription and are often used in self-medication. In Europe and the United States, more than 50% of pregnant women take analgesic drugs (Rebordosa et al., 2008; Werler et al., 2005). These medications are not recommended only after 5 months of pregnancy. Very few studies have focused on the putative effects of these drugs on the formation of embryonic gonads, knowing that the gonads develop in humans in the first trimester of pregnancy (between 6 and 8 weeks). The targets of NSAIDs and ACE are the cyclooxygenases (COX), the key enzymes in the synthesis of prostaglandins from arachidonic acid. My team found that prostaglandin D2 (PGD2) was involved in various stages of development and maturation of embryonic testis at the somatic and germinal levels (Malki et al., 2005; Moniot et al., 2014; Rossitto et al., 2015). The purpose of this project is to evaluate the impact of in utero exposure to ACE and NSAIDs on development and maturation of the reproductive organs in the mouse embryo. Moïra Rossitto*, Pascal Philibert*°, Candice Marchive*, Francis Poulat & Brigitte Boizet-Bonhoure* * Genetic and Development department, Institute of Human Genetics, CNRS UPR1142, Montpellier, France. ° Hormonology department, Lapeyronie Hospital, CHU Montpellier and Montpellier University, Montpellier, France CBS2 Association assocbs2.com N°67 - Claire MARQUILLY Physiological role of APPL in Drosophila mushroom bodies’ development The protein APPL (Amyloid Precursor Protein-Like) is the Drosophila homologue of human APP, known to be involved in Alzheimer’s disease (AD). Despite its implication in AD, the functional role of APP is still poorly known. Here, we investigate the role of APPL during brain development. The mushroom bodies (MBs) are the Drosophila center for learning and memory. APPL is highly expressed in the MBs. This brain structure is, therefore, particularly relevant for this study. Recently, APPL was described as a novel neuronal-specific modulator of the PCP pathway required for the robustness of axonal outgrowth of the MB during development (Soldano et al. PlosBiol 2013). It was shown that this protein facilitates the PCPspecific phosphorylation of the Wnt adaptor protein DSH/DVL (dishevelled) by the Abelson kinase (Abl). We show here that APPL also interacts with ARM (armadillo) protein, the Drosophila homologue of β-catenin, for the development of MB neurons. This interaction seems to involve the function in adherens junction of ARM rather than its function in the Wnt signaling pathway. Moreover, a previous study showed that Abl regulates the planar polarized junctional dynamics through tyrosine phosphorylation of ARM. Consequently, ABL could be a link between APPL and ARM for the axonal outgrowth in the MBs. Only one mutant allele for the Appl gene does exist which results from some very complex chromosomal rearrangements that renders its analysis very difficult. In order to circumvent this problem we are creating a molecularly defined complete deletion of the gene via the recent CRIPSR-Cas9 technic. Claire MARQUILLY , Lee G. FRADKIN , Jean-Maurice DURA CBS2 Association assocbs2.com N°68 - Nour SFEIR Role of the transcription factor RIP140 in colon cancer The RIP140 protein is a transcriptional co-regulator involved in various physiological processes. RIP140 represses the transcriptional activity of many transcription factors such as nuclear receptors and E2F1 factor. Our recent results based on approaches that combined the use of mouse models with molecular and cellular biology experiments, have shown that RIP140 controls intestinal homeostasis and suggest that this gene plays a tumor suppressor role in colorectal cancer. Indeed, in the intestinal epithelium, RIP140 regulates cell proliferation and differentiation by inhibiting the Wnt signaling pathway via the transcriptional regulation of the APC gene expression. In addition, analysis of human biopsies showed that RIP140 mRNA levels are decreased in colon cancer compared to healthy tissue (Lapierre et al, Journal of Clinical Investigation, 2014). The proposed thesis research program aims to further characterize the role of RIP140 in intestinal tumorigenesis according to the following objectives. My first goal will be to decipher the molecular interrelationships between RIP140 and the Wnt signaling pathway. In addition, knowing that a crosstalk exists between the Wnt and the Notch signaling pathways, I will study the molecular interrelationships between RIP140 and the Notch signaling pathway and the role of the transcription factor KLF4 in these crosstalks. Finally, I will analyze the role of RIP140 in vivo in colon cancer (generation and use of conditional transgenic mouse models). This project will clarify the mechanisms by which RIP140 controls colon tumorigenesis and may highlight a new biomarker for use in the diagnosis and / or treatment of this disease. Keywords: RIP140, Wnt and Notch signalling, colon cancer, transgenic mouse models. Nour SFEIR, Sandrine BONNET, Marion LAPIERRE, Vincent CAVAILLES IRCM, INSERM U1194, Montpellier Cédex 5 CBS2 Association assocbs2.com N°69 - Amandine GUERIN Characterization of host cell proteins recruited at the Moving Junction during invasion of Toxoplasma gondii Toxoplasma gondii is an obligate intracellular parasite which belongs to the Apicomplexa phylum, including Plasmodium species which are responsible for malaria. The invasion mechanism is unique among this phylum. It involves the formation of a tight connection between the parasite and the host cell plasma membranes called moving junction (MJ). During invasion, a complex formed of the parasite rhoptry neck proteins RON2/4/5/8 is injected into the host cell and localized to the MJ. RON2 spans the host plasma membrane and functions as a receptor for the microneme protein AMA1 exposed on the parasite surface, resulting in close and irreversible contact between the parasite and the host cell. The proteins RON4/5/8 localize to the cytosolic face of the host cell and are believed to provide a stable anchoring point for host penetration. Apart from being located at the MJ, the precise role of the RON4/5/8 proteins during invasion remains elusive. These proteins are ideally positioned to carry out anchoring roles for the parasite through a connection with host cytoskeleton proteins. Here, we present the specific recruitment of several host cell proteins at the MJ by the RON complex. Amandine Guérin1, Mauld H. Lamarque1, Michelle L. Tonkin2, Martin J. Boulanger2 and Maryse Lebrun1 1 UMR 5235 CNRS, Université de Montpellier 2, 34095 Montpellier, France. 2 Department of Biochemstry and Microbiology, University of Victoria, Victoria, British Columbia, Canada V8W 3P6 CBS2 Association assocbs2.com N°70 - Lara BOU MALHAB MLN4924, a NEDD8 inhibitor in a p53 based cyclotherapy approach TP53 gene also called the guardian of the genome helps maintaining our genome integrity. Under normal conditions, p53 is kept at low expression levels by its two negative regulators Mdm2 and Mdmx. Under stress conditions, different pathways will be activated to induce p53 stabilisation. According to the stress level, p53 will induce different p53-dependent genes expression involved in cell cycle arrest, DNA damage repair or apoptosis. In 50% of cancer cases, p53 gene is found mutant. In others, defects of its upstream regulators or downstream effectors are detected. MLN4924, a specific inhibitor of the NEDD8 pathway (ubiquitin-like) is now in phase I clinical trials. In order to target cancer cells specifically using MLN4924 as chemo agent and to protect normal cells against the potential toxic effects of MLN4924, a p53-based cyclotherapy was tested. Our results show that low activation of wild type p53 by Actinomycin D protects normal cells to MLN4924 treatment leaving cancerous cells with mutant p53 or no p53 to selectively commit to apoptosis upon MLN4924 treatment. Our results provide a possible combination therapy for MLN4924 based on the p53 status. We are actually validating our findings in vivo, more specifically in zebrafish model system. Lara BOU MALHAB and Dimitris XIRODIMAS. Centre de Recherche de Biochimie Macromoléculaire - UMR 5237, CNRS, Route de Mende 34 293, Montpellier, Cedex 5, France. CBS2 Association assocbs2.com N°71 –Laura YAZDANI Ribosome: Master Regulator of Cancer Cell Fate? It is well established that the ribosome acts as a master regulator of gene expression by regulating protein synthesis both quantitatively and qualitatively. An emerging concept suggests that ribosome is heterogeneous and can be "reprogrammed". These "specialized ribosomes" would preferentially engage certain mRNA at the expense of others and therefore drive cell phenotype and favor cell adaptation. From a more pathological standpoint, many studies have correlated deregulation of both translation machinery composition and activity with cancer initiation and evolution. Our goal is to demonstrate that protein synthesis is differentially regulated depending on cancer cell subpopulation and determine whether ribosomal heterogeneity could impact tumoral evolution and plasticity. Laura Yazdani1, Françoise Macari1, Oualid Ayad1, Damien Paulet2, Julie Pannequin1, Armelle Choquet1 and Alexandre David1 1Institut de Génomique Fonctionnelle (IGF), INSERM U651 - CNRS UMR5203, Montpellier. 2Laboratoire d'Informatique, de Robotique et de Microélectronique (LIRMM), Montpellier CBS2 Association assocbs2.com N°72 - Badreddine BOUSSADIA Pattern of drug metabolism enzyme expression in the epileptic brain: a new mechanism of drug resistance P450 metabolic enzymes are expressed in the human and rodent brain. Recent data support their involvement in the pathophysiology of epilepsy. However, the determinants of metabolic enzyme expression in the epileptic brain are unclear. We tested the hypothesis that status epilepticus (SE) or exposure to phenytoin or phenobarbital affects brain expression of the metabolic enzyme CYP2E1. SE was induced in C57BL/6J mice by systemic kainic acid. Brain CYP2E1 expression was evaluated 18–24 h after severe SE by immunohistochemistry. Co-localization with neuronal nuclei (NEUN), glial fibrillary acidic protein (GFAP) and CD31 was determined by confocal microscopy. The effect of phenytoin, carbamazepine and phenobarbital on CYP2E1 expression was evaluated in vivo or by using organotypic hippocampal cultures in vitro. CYP2E1 expression was investigated in brain resections from a cohort of drug-resistant epileptic brain resections and human endothelial cultures (EPI-EC). Immunohistochemistry showed an increase of CYP2E1 expression limited to hippocampal CA2/3 and hilar neurons after severe SE in mice. CYP2E1 expression was also observed at the astrocyte-vascular interface. Analysis of human brain specimens revealed CYP2E1 expression in neurons and vascular endothelial cells (EC). CYP2E1 was expressed in cultured human EC and overexpressed by EPI-EC. When analyzing the effect of drug exposure on CYP2E1 expression we found that, in vivo or in vitro, ethanol increased CYP2E1 levels in the brain and liver. Treatment with phenytoin induced localized CYP2E1 expression in the brain whereas no significant effects were exerted by carbamazepine or phenobarbital. Our data indicate that the effect of acute SE on brain CYP2E1 expression is localized and cell specific. Exposure to selected anti-epileptic drugs could play a role in determining CYP2E1 brain expression. Additional investigation is required to fully reproduce the culprits of P450 enzyme expression as observed in the human epileptic brain. Key words : CYP2E1; status epilepticus; drug exposure; biotransformation Boussadia B1, Ghosh C2, Plaud C1, Pascussi JM3, De Bock F1, Rousset MC1, JanigroD2, Marchi N1. 1 Laboratory of Cerebrovascular Mechanisms of Brain Disorders, Department of Neuroscience, Institute of Functional Genomics, CNRS, Montpellier, France. 2 Cerebrovascular Research Center, Department of Biomedical Engineering and Molecular Medicine, Cleveland Clinic, USA. 3Laboratory of Signaling, Plasticity and Cancer, Department of Cancer Biology, Institute of Functional Genomics, Centre National Recherche Scientifique (CNRS), Montpellier, France. CBS2 Association assocbs2.com N°73 - Ramhari KUMBHAR Determinants for UBA1 recruitment at sites of DNA damage Ubiquitylation is an important posttranslational modification that is necessary for protein degradation as well as for the regulation and the localization of many cellular factors. A number of proteins implicated in DNA replication and DNA damage response are ubiquitylated. Ubiquitylation during the DNA damage response is selectively dependent on the ubiquitin-activating enzyme UBA1, which functions at the apex of the ubiquitylation cascade. Our objective is to elucidate whether and how UBA1 is recruited at damaged sites and to uncover the role of ubiquitylation in ATR signaling. Using a cell free system developed in the lab that recapitulates ATR kinase-signaling pathway, we found that UBA1 is recruited to linear DNA substrates and mediates ubiquitylation of DNA-bound proteins. ATR-mediated Chk1 phosphorylation in cellfree extracts was dependent on UBA1 activity. Intriguingly, upon UBA1 inhibition, Chk1 accumulated on biotinylated DNA coupled to streptavidin beads. We found that protein ubiquitylation and the recruitment of UBA1 to DNA in cell-free extracts was dependent on the kinase DNA-PKcs and on the poly ADP-ribose polymerase PARP1, two sensors of DNA lesions. UBA1 exhibited affinity for PARP1 and for poly ADPribose (PAR) chains in vitro. Consistent with this, PARP1 promoted UBA1 recruitment at an inducible DNA double-strand break in living cell, as revealed by chromatin immunoprecipitation. These results indicate that UBA1 is recruited to DNA damaged sites in a DNA-PKcs and PARP1 dependent-manner and that protein ubiquitylation is necessary for the assembly of a productive ATR signaling complex. Thus, UBA1 inhibitors could be used to target ATR signaling in cancer cells. Ramhari Kumbhar1, Sophie Vidal-Eychenie1, Alkmini Kalousi2, Evi Soutoglou2, Cyril Ribeyre1 and Angelos Constantinou1 1 Institute of Human Genetics (IGH), CNRS UPR-1142, Montpellier France. 2 Institute of Genetics and Molecular and Cellular Biology (IGBMC), Strasbourg France CBS2 Association assocbs2.com N°74 - Gabriel ESPINOSA The effect of microbial LPS translocation in cross-presenting dendritic cells and in the breakdown of CD8+ T cell peripheral tolerance in irradiated mice We have utilized transgenic mice that express a well-characterized model antigen, influenza HA, in the beta cells of the pancreas. These mice are profoundly tolerant of the HA antigen in both the CD8+ and the CD4+ T cell compartments. Lymphodepletion is currently used as adjuvant for adoptive cytotoxic T cell immunotherapy in cancer. In fact mild irradiation enhance CD8+ T cell anti-self responses and promotes the breakdown of T cell tolerance and the onset of autoimmune diabetes. One of the effects of irradiation is the systemic translocation of LPS from commensal bacteria. To assess whether bacterial LPS is responsible for the breakdown of tolerance observed we have treated mice with a cocktail of antibiotics in the drinking water in order to prevent translocation. Our results demonstrated that antibiotic treatment can efficiently prevent the systemic translocation of LPS induced by irradiation. Surprisingly, Beta cell-specifc CD8+ T cells proliferated extensively in response to self-antigen cross-presentation in the draining lymph nodes of the pancreas, differentiated into effector cells and infiltrated the islets of Langerhans inducing disease in both antibiotic treated mice and controls. Analyses of the CD11c+ antigen presenting cells demonstrated that irradiation induces their activation as measured by the enhanced expression of CD80, CD86, CD40 and MHC II. Although antibiotic treatment partially prevent the activation of most of cross-presenting dendritic cells subsets, our results indicate that commensal bacteria LPS translocation blockade is not sufficient to prevent the breakdown of CD8+ T cell peripheral tolerance and the onset of autoimmune diabetes. Gabriel Espinosa-Carrasco12, Marine Villard12, Pascale Louis-Plence12 and Javier Hernandez12* 1 Inserm U1183, Institute for Regenerative Medicine and Biotherapy, Montpellier, F34295 France. 2 Université Montpellier, UFR de Médecine, Montpellier, F-34000 France CBS2 Association assocbs2.com N°75 - Myriam RICHAUD A new integrated platform for drug action mode determination in C. elegans We used the Caenorhabditis elegans model to decipher new molecular regulations of aging that spread out or emerge from the main pathway regulating life span: the Insulin/IGF-1/daf-2 pathway. This pathway can control many features of aging determination process including stress resistance, metabolic control as well as hormetic mechanisms. Growing evidence retrieved in model organisms indicates that molecular networks regulating aging can be now extrapolated to humans. We have developed an original set of molecular tools (Araiz et al., 2008a) as well as innovative technical sets that allow our team to look experimentally at aging determination and plasticity by molecular genetic, physiology (HTS-HCS screenings robots Cellomics array-scan), imagery, transgenesis (gene gun BioRad). We have developed new molecular and genetic toll that allow us to look at the aging process control in relation with various treatments in order to find unidentified targets. As for example, Chicoric acid can act on muscle mitochondria homeostasis as well as on metabolism linked with type 2 diabetes. We have started to analyse C. elegans aging impact of Chicoric acid and found an unexpected positive effect even at very low (micromolar) concentrations. We are now testing by gene knockout and gene knockdown (RNAi) the molecular pathways involved in Chicoric acid action. Our quantitative C.elegans technology can include either soluble or insoluble drug screenings on identified or unidentified molecular targets (or pathways) as well as monitoring of mitochondrial, metabolism or aging impact as well. Myriam Richaud, Pierre Cuq and Simon Galas Laboratoire de Toxicologie, Faculté de Pharmacie, 15 Av Charles Flahault, BP 14 491, 34093 Montpellier Cedex 5 CBS2 Association assocbs2.com N°76 - Quang Tien PHAN Transient infection induces chronic inflammation Zebrafish notochord has been used as an emerging model for the study of bone and cartilage inflammatory diseases. We have recently shown that infection of zebrafish embryo notochord by non-pathogenic E.coli could induce a chronic inflammation episode, which subsequently led to severe defects of the notochord and malformation of the vertebrae. In the present study we further identify the molecular mechanisms that promote and sustain the inflammation after the bacterial clearance. We also reveal the cellular interactions between bacteria, notochordal cells and the leukocytes of innate immune system. CBS2 Association assocbs2.com N°77 - Marianne EL BAROUK Endogenous retrovirus and mobility Les rétrovirus appartiennent à la grande famille des rétroéléments exogènes et endogènes qui ont en commun un mécanisme de réplication par transcription inverse de leurs ARN génomiques. Plus précisément, la forme provirale des rétrovirus exogènes partage avec le groupe des rétroéléments à LTR (LTR-retroelements) une structure génomique canonique : les gènes gag ou gag-like, pol, et parfois env encadrés par deux séquences répétées terminales (LTR : Long Terminal Repeat) contenant les séquences cis-régulatrices nécessaires à la transcription. Les rétrovirus endogènes représentent une composante plus ou moins importante des génomes eucaryotes selon les espèces considérées et l’étude de ces éléments soulève de nombreuses questions. Quelles sont les protéines impliquées dans l’endocytose et l’exocytose de ces rétrovirus endogènes? Quel est l’impact de ces séquences sur l’intégrité et le fonctionnement de leurs génomes hôtes? Connaît-on tous les mécanismes de régulations des rétrovirus endogènes? Au laboratoire, nous étudions un rétrovirus endogène de drosophile, gypsy ( Marlor et al., 1986). Ce rétrovirus est exprimé dans les cellules dans les cellules folliculaires de l’ovaire de drosophile et rétrotranspose dans l’ovocyte. Ceci se traduit par la présence de nouvelles copies provirales de gypsy dans la descendance des femelles. Le projet a pour but de déterminer les protéines impliquées dans le transfert de gypsy du soma au germen. Un début de réponse a été apporté pour un autre virus endogène de D. melanogaster nommé ZAM dont le cycle de réplication est très similaire à celui de gypsy (Leblanc et al., 2000). Des données expérimentales suggèrent que les particules de ZAM sont transférées aux ovocytes grâce à un «piratage» des voies d’exocytoses et d’endocytose utilisées par vitellogénine (Brasset et al., 2006). Est-ce un cas particulier, y a-t-il d’autres protéines impliquées ? Si la mobilité des rétrovirus endogènes peut s’avérer parfois bénéfique pour l’hôte, elle lui est fatale dans la plupart des cas. Des mécanismes maintenant la transposition à des taux compatibles avec la survie des espèces ont été sélectionnés au cours de l’évolution. Ces mécanismes de répression font intervenir des protéines de la famille Argonaute et des petits ARN non codants, les piRNA (Piwi-interacting RNA) (revue Senti and Brennecke 2010). À cause de cette répression, nous n’avons actuellement que peu de données concernant le passage de ces rétrovirus d’une cellule à l’autre. En utilisant la génétique de la drosophile, le laboratoire a développé un outil permettant d’augmenter la fréquence de ce passage en inactivant la voie de régulation par les piRNA. Cette approche génétique, couplée avec des approches de séquençage à haut débit, permettra de déterminer les protéines de l’hôte impliquées dans la mobilité et le passage de cellule à cellule, et aussi d’étudier d’éventuels modes de régulation indépendants de la voie des piRNA. CBS2 Association assocbs2.com N°78 - A. Mahdi LAAREF Contribution of the splicing machinery to the control of pluripotency maintenance and early embryonic development The therapeutic potential of understanding the molecular basis of pluripotency and differentiation has led to many studies comparing transcriptional profiles in different human Embryonic Stem Cell (hESC) lines and the study of expression changes during differentiation. Alternative pathways for processing the primary transcript can profoundly affect the diversity and function of the protein products that are generated from a single gene to set complex programs involved in pluripotency and/or differentiation of hECS. While our knowledge about transcriptional networks regulating pluripotency and differentiation has been intensively studied, however the role of alternative splicing in this process is not yet understood and clear examples of concerted switching of multiple genes from one isoform to another have not been demonstrated. The main objective of this project is to discover splicing factors involved in the control of pluripotency maintenance and the early differentiation potency in the three germ layers, and to explore their role in these processes. For this purpose, we will use the iPSC and high-throughput technologies that we developed in the laboratory to determine the splicing profiles that are affected by RNAi knockdown of known constitutive component of the different spliceosomal complexes. The project constitutes a fundamental investigation into the function and mechanism of alternative splicing in stem cells that might have a major impact in regenerative medicine. This investigation will capitalize on exciting discoveries made recently during analysis of high throughput data in our lab to concentrate on the growing consensus that alternative splicing is a crucial determinant of cellular morphology. A Mahdi LAAREF, Yacine BARECHE, Jamal TAZI and Laure LAPASSET Institue of Molecular Genetics of Montpellier CBS2 Association assocbs2.com CBS2 Association assocbs2.com Organizing commitee The CBS2 Day 2015 is the thirteenth edition of CBS2 days. This event was organized by the CBS2 association, with the support of the CBS2 Doctoral School and BioCampus Montpellier. Vuthy Ea (IGMM) Tania Louis (IGH) Selma Damhane (CBS) Marco Bruschi (IGF) Laurent Fernandez (CBS) Ramhari Kumbhar (IGH) Emilie Aponte (CRBM) Laura Auboyer (IRBM) Coralie Berthoux (IGF) Amélie Borie (IGF) Miriam Candelas (IGF) Romain Davaze (IGH) Benoît Girard (IGF) Sarah Guiziou (CBS) Camille Jacqueline (IRD) Pierre Lesport (IGF) Samy Murat (IGF) Ruba Nasri (IBMM) Matthias Ollivier (IGF) Naresh Yandrapalli (CPBS) Elise Goyet (IGF) Ankit Dwivedi (CBPS/IBC) Bouasse Malik (IGF) Sandrine Urvoy Secrétariat ED CBS² Michel Desarménien Directeur ED CBS² Audrey Verdier BioCampus Montpellier Laurent Journot BioCampus Montpellier Jury and chairs The organizing board wants to thank particularly the researchers who accepted to be the jury and chairs of this CBS2 Day 2015 : Dr. Bonnet Jerome (CBS : Centre de Biochimie Strcuturale) Dr. Talarek Nicolas (IGMM : Institut de Génétique Moléculaire de Montpellier) Dr. Hached Khaled (CRBM : Centre de Recherche de Biochimie Macromoléculaire) Dr. Claeysen Sylvie (IGF : Institut de Génomique Fonctionnelle) Dr. Bertaso Federica (IGF : Institut de Génomique Fonctionnelle) Dr. Basavarajaih Poornima (IGH : Institut de Génétique Humaine) Dr. Gerbe François (IGF : Institut de Génomique Fonctionnelle) Dr. Bouschet Tristan (IGF : Institut de Génomique Fonctionnelle) Dr. Lamb Ned (IGH : Institut de Génétique Humaine) Dr. Quesada Stanislas (Université de Montpellier) Louis Tania (IGH : Institut de Génétique Humaine) Yahia Yousra (IGMM : Institut de Génétique Moléculaire de Montpellier) Roussel Morgane (IGF : Institut de Génomique Fonctionnelle) Voisin Tiphaine (IGF : Institut de Génomique Fonctionnelle) Thanks In addition to the CBS² doctoral school and BioCampus Montpellier, the CBS² association is grateful to the following organizations for financial and logistical support:
