Disc1 Mutant Mice Subjected to Chronic Social Defeat Stress as a Model of Gene-Environment Interaction in Schizophrenia and Depression

Haque, F. Nipa

25 January 2010

Human genetic data suggests DISC1 (Disrupted-in-schizophrenia 1) is a susceptibility gene for schizophrenia and depression. Disc1 Q31L-/- mutants show depression-like behaviour and Disc1 L100P-/- mutants schizophrenia-like behaviour. Heterozygous mutants show an intermediate phenotype. In a gene-environment interaction study, we exposed heterozygotes to chronic social defeat (CSD) stress and phenotyped behaviour. Disc1, Bdnf(III) and Pde4b mRNA levels were also measured. Moreover, as epigenetic mechanisms may mediate some effects of CSD, we also exposed wildtype mice to CSD concurrently with the histone deacetylase inhibitor valproate. We found that CSD increased anxiety in L100P-/+ mutants, and that levels of Disc1, Bdnf(III) and Pde4b mRNA were higher in this mutant. Valproate treatment did not correct CSD-induced behavioural changes. In conclusion, we have demonstrated an interaction between a strong susceptibility gene for psychiatric disease and an environmental manipulation similar to stressors known to affect mental illness.

gene-environment interaction

social defeat

Disc1 mutant mice

schizophrenia

depression

animal model

disrupted-in-schizophrenia 1 (Disc1)

brain-derived neurotrophic factor (Bdnf)

phosphodiesterase 4b (Pde4b)

valproate

histone deacetylase (HDAC)

epigenetics

Q31L

L100P

0317

0384

0347

Characterization of Histone H3 Lysine 18 deacetylation during infection with Listeria monocytogenes

Eskandarian, Haig Alexander

05 June 2013

Bacterial pathogens dramatically affect host cell transcription programs for their own profit, however the underlying mechanism in most cases remain elusive. While investigating the effects of listeria monocytogenes on histone modifications, we discovered a new transcription regulatory machanism by which the expression of genes is repressed, during infection. Upon infection by L. monocytogenes, the secret virulence factor, InlB, binds the c-Met receptor and activates signaling through PI3K/Akt. This signaling platform is necessary for causing the relocalization of the histone deacetylase, SIRT2, to the nucleus and associating to chromatin.In characterizing the mechanism governing SIRT2 nuclear relocazing during infection, our results have demonstrated that SIRT2 undergoes a post-translational modification. SIRT2 undergoes dephosphorylation at a novel N-terminal phospho-site. SIRT2 is recruiter to the transcription star sites of genes repressed during inection leading to H3K18 deacetylation and transcriptional repression.finnaly, my results demonstrate that SIRT2 is hijacked by L monocytogenes and promotes an increase in intracellular bacteria. Together, these data uncover a key role for SIRT2 mediated H3K18 deacetylation during infection and characterize a novel mechanisme imposed by a pathogenic bacteriomto reprogram the host cell.

Host-Pathogen Interactions

Listeria monocytogenes

Infection

Histone modifications

Histone H3

Histone H3 K18

Acetylation

Deacetylation

Histone Deacetylase

Sirtuin

SIRT2

Met

PI3K

Akt

Signalling

Epigenetics

Transcriptional Control

Regulation and Characterization of Transcription Factor Activator Protein-2 Alpha (AP-2α)

Nama, Srikanth

January 2009

Introduction AP2α is a 52 kDa retinoic acid inducible and developmentally regulated activator of transcription, which binds to the DNA in a sequence-specific manner. Transcription factor AP-2α was isolated from HeLa cells by affinity chromatography using specific binding sites with in SV40 and human metallothionein promoters. Further screening of HeLa cDNA library with oligonucleotide probes predicted partial peptide sequence which led to the isolation of AP-2α cDNA and subsequently it was mapped to chromosome 6 near HLA locus. A differentially spliced version of AP-2α, which lacks most of the C-terminus, encodes a dominant negative protein (AP-2B). Subsequent studies led to the identification of four more isoforms: AP-2β, AP-2γ, AP-2δ and AP-2ε. AP-2 family members can form homo or hetero dimers among themselves through the unique C-terminal helix span helix motif and bind DNA through basic domain lies N-terminus of DNA binding domain. Several evidences suggest that AP-2α can act as a tumor suppressor gene. It has been shown that AP-2α can activate growth suppressor genes like p21WAF1/CIP1. Transforming viral oncogenes like adenovirus E1A and SV40 large T antigen have been shown to alter AP-2α function. In addition, reduced expression of AP-2α has been reported in human breast, ovary, colon, skin, brain and prostate cancers. Further, supporting evidences suggest that more invasiveness and tumorogenicity was observed when dominant negative mutant of AP-2α was expressed in melanoma cells. In this work, we have carried out a systematic study to find the various signal transduction pathways which regulate AP-2 activity as well as we attempted to demonstrate the importance of DNA binding domain in the growth inhibitory functions of AP-2α. HDAC inhibitors (HDIs) activate AP-2 activity through spleen tyrosine kinase (Syk) In the literature, ample evidences are available that genotoxic drugs such as adriamycin, induce tumor suppressors like p53 and p73. In this study, we have screened pharmacological drugs which damage DNA and specific inhibitors of various signal transduction pathways for their ability to activate AP-2 activity. AP-2 specific reporter, 3Χ-AP2-CAT was used in this study to measure the AP-2 activity. Of all the compounds studied, we found that Histone Deacetylase Inhibitors (HDIs) efficiently activated AP-2 activity and was found to be specific as they failed to activate 3X-AP2 mut CAT, which contains mutated AP-2 binding sites as well as pGL tk Luc, which contains thymidine kinase minimal promoter and no AP-2 binding sites. To understand the mechanism of HDI-mediated of AP-2 activation, AP-2 isoforms and its coactivators transcript and protein levels were analyzed. We found significant change in transcript levels of the some of the molecules tested. While the endogenous protein levels of various AP-2 isoforms were undetectable, we found stabilization of AP-2α protein expressed from exogenous source in cells treated with HDIs. HDI stabilized AP-2α was found to be functionally active as it showed increased sequence-specific DNA-binding as well as increased apoptosis. While HDIs known for their ability to modulate the gene activities by chromatin remodeling, it is also known that they alter various signal transduction pathways. In an effort to find pathway(s) by which HDIs activate AP-2 activity, we found that HDIs failed to activate AP-2 reporter in the presence of staurosporine suggesting the involvement a staurosporine sensitive pathway(s) in this process. Stauosporine is a non-specific kinase inhibitor of different signaling pathways. Further studies using different pathway specific inhibitors identified that spleen tyrosine kinase (Syk) is essential for HDIs mediated activation of AP-2 activity. Syk is a non receptor tyrosine kinase which is known to be activated in stress conditions. Syk is considered to be a tumor suppressor since Syk over expression leads to growth suppression of breast cancer cells and is also inactivated in a subset of breast cancers. These results suggest that HDI mediated activation of AP-2 involves AP-2α stabilization through Syk pathway. Regulation of AP-2 by MAP kinase pathway Cell growth, differentiation, and apoptosis are mediated by the activation of mitogenactivated protein kinase (MAPK) pathways. These kinases constitute MAP kinase cascades mainly regulated through phosphorylation status. In mammalian cells, at least four MAPKs, namely, extracellular signal-regulated kinases (ERKs), c-Jun N-terminal kinase/stress-activated protein kinases (JNK/SAPKs), p38 and ERK5/big MAP kinase have been identified. The ERKs are usually activated by mitogenic stimuli which in turn increase the proliferation and survival. Over expression of any activator of this signaling cascade lead to the unregulated proliferation of cells. In many cancers, ERK pathways are known to be up regulated. In this study, we found that MEK (MEK is the immediate upstream regulator of ERK) inhibitors - PD98059 and U0126 activate 3X-AP2-CAT suggesting that AP-2 activity is repressed by activated MAP kinase pathway. MEK inhibitor mediated activation was found to be specific because they failed to activate transcription from pGL tk Luc which contains thymidine kinase minimal promoter and no AP-2 binding sites. To understand the mechanism of MEK inhibitor-mediated of AP-2 activation, AP-2 isoforms and its coactivators transcript and protein levels were analyzed. We found significant change in transcript levels of the some of the molecules tested. The endogenous protein levels of various AP-2 isoforms were undetectable. When AP-2α was exogenously expressed, while no change in protein levels and DNA-binding ability was seen, we found evidence for appearance of post-ranslationally modified AP-2α protein in U0126 treated cells. We also found CITED2 (CBP/p300-interacting transactivator 2, co-activator of AP-2α) transcript levels were up regulated in UO126 treated cells. Post translational modifications of AP-2α and increased and increased CITED2 levels may be responsible for MEK inhibitor mediated AP-2 activation. Thus we conclude that ERK pathway, which is an oncogenic MAP kinase pathway, inhibits AP-2 activity thereby suggesting the importance of down regulation of AP-2 activity during transformation. Essential role of DNA-binding domain of AP-2α for its growth inhibitory functions Transcription factor AP-2α has three distinct domains, N-terminal transactivation domain (52-108 aa), C-terminal DNA binding domain (204-408 aa) and dimerization domain (277-395 aa) which lies within the DNA binding domain. AP-2α exerts its effects through binding to specific DNA sequence in the promoter of its target genes leading to either repression or activation. Recent evidences suggest that AP-2α represses many genes through its competitive binding to overlapping AP-2 and other transcription factor binding sites. This suggests an important role exclusively for the DNA binding domain in AP-2α mediated functions. To address the importance of DNA binding domain for AP-2α mediated apoptosis, we have tested the ability different deletion/point mutants of AP-2α with varying DNA binding and transactivation capability to perform growth suppressor function and ability to induce apoptosis. Replication-deficient recombinant adenoviruses expressing different mutants were used in this study. We found that an intact DNA-binding domain alone even in the absence of activation domain is sufficient for AP-2α to inhibit colony formation and to induce significant levels of apoptosis. These results suggest an important role for DNA binding domain growth inhibitory functions of AP-2α and thereby implying the importance of transcriptional repression in AP-2α functions.

Protein Transcription

Activator Protein-2 alpha (AP-2α)

Protein Binding

Histone Deacetylase Inhibitors (HDIs)

Mitogen Activated Protein Kinase (MAPK)

AP-2 alpha

AP-2 Transcription

MAP Kinase Pathway

AP-2 - Growth Inhibition

AP2α

HDAC Inhibitors

Biochemistry

Etude de la réactivation de l'expression des provirus HIV-1 latents par la prostratine en synergie avec des inhibiteurs de désacétylases: mécanismes moléculaires impliqués et potentiel thérapeutique

Reuse, Sophie

17 December 2009

L’infection par HIV-1 représente un des problèmes de santé publique majeurs de notre société actuelle. Le traitement HAART (Highly Active AntiRetroviral Therapy) inhibe le cycle réplicatif viral mais ne permet pas l’éradication du HIV-1. La principale cause de cet échec thérapeutique est la persistance de réservoirs cellulaires infectés de manière latente par HIV-1, qui, lors de l’arrêt du traitement HAART, sont à l’origine d’un rebond de la charge plasmatique virale. Le défi actuel est donc de découvrir de nouvelles méthodes d’élimination des cellules réservoirs. Une des stratégies envisagées est de forcer l’expression virale dans les cellules infectées de manière latente afin d’entraîner leur destruction suite à leur détection par le système immunitaire ou suite aux effets cytopathiques viraux. Parallèlement, le traitement HAART serait maintenu afin de limiter la propagation des virions néo-synthétisés. Plusieurs éléments sont impliqués dans la répression transcriptionnelle associée à la latence post-intégrationnelle du virus HIV-1 :la nature du site d’intégration ;l’absence de facteurs cellulaires inductibles tels que NF-κB ;la structure chromatinienne du provirus et les modifications post-traductionnelles des histones ;l’absence de niveaux suffisants de la protéine trans-activatrice Tat. De plus, notre laboratoire a précédemment mis en évidence un lien entre deux de ces éléments, en démontrant, dans une lignée modèle de latence post-intégrationnelle, que la cytokine pro-inflammatoire TNFα, un activateur de la voie de signalisation NF-κB, permet une réactivation synergique de l’expression virale combinée à l’inhibiteur d’histone-désacétylases (HDACI) TSA. Cependant, l’utilisation thérapeutique du TNFα et de la TSA est inenvisageable en raison de leurs toxicités.<p>\ / Doctorat en Sciences / info:eu-repo/semantics/nonPublished

Sciences exactes et naturelles

Biologie

HIV (Viruses)

Viruses -- Reproduction

Latent virus diseases

Histone deacetylase -- Inhibitors

Virus de l'immunodéficience humaine

Virus -- Reproduction

Infections latentes

Histone désacétylase -- Inhibiteurs

HIV-1

latence

prostratine

inhibiteurs de HDACs

Characterization of Histone H3 Lysine 18 deacetylation during infection with Listeria monocytogenes / Caractérisation de l'histone H3 lysine désacétylation au cours de l'infection par Listeria monocytogenes

Eskandarian, Haig Alexander

05 June 2013

De nombreuses bacteries pathogènes sont capables d'affecter les programmes transcriptionnels de la cellule hôte pendant l'infection. Cependant, les mécanismes contrôlant ce processus restent largement méconnus. En investigant les effets de la Listerai monocytogenes sur les modifications des histones de l'hôte, nous avons mis en évidence un nouveau mecanisme de régulation de transcription nécessaire pour la répression de certains gènes, pendant l'infection. Lors de l'infection par L. monocytogenes, le facteur de virulence sécrété, InlB, se lie au récepteur c-Met et active la signalisation par les intermédiaires PI3K et Akt. cette plateforme de signalisation est nécessaire pour la relocalisation de la deacetylase d'histone, SIRT2, au noyau et l'association à la chromatine.En caractérisant me mécanisme gouvernant la relocalisation nucléaire de SIRT2 lors de l'infection, nous avons démontrés que SIRT2 subit une modification post-traductionnelle. SIRT2 est déphosphorylée à un nouveau site de phosphorylation localisé à la partie terminale de la protéine. SIRT2 est recrutée au site de démarrage de la transcription des gènes réprimés lors de l'infection menant à la deacetylation de H3K18 et la répression transcriptionnelle. Nous avons mis en évidence que SIRT2 est détournée par L. monocytogenes et provoque une croissance des bactéries intracellulaires. Ces résultats démontrent un clef de SIRT2 en provoquant la deacetylation de H3K18 mors de l'infection et dévoilent un nouveau mécanisme imposée par les bactéries pathogènes dans le but de reprogrammer la cellule hôte. / Bacterial pathogens dramatically affect host cell transcription programs for their own profit, however the underlying mechanism in most cases remain elusive. While investigating the effects of listeria monocytogenes on histone modifications, we discovered a new transcription regulatory machanism by which the expression of genes is repressed, during infection. Upon infection by L. monocytogenes, the secret virulence factor, InlB, binds the c-Met receptor and activates signaling through PI3K/Akt. This signaling platform is necessary for causing the relocalization of the histone deacetylase, SIRT2, to the nucleus and associating to chromatin.In characterizing the mechanism governing SIRT2 nuclear relocazing during infection, our results have demonstrated that SIRT2 undergoes a post-translational modification. SIRT2 undergoes dephosphorylation at a novel N-terminal phospho-site. SIRT2 is recruiter to the transcription star sites of genes repressed during inection leading to H3K18 deacetylation and transcriptional repression.finnaly, my results demonstrate that SIRT2 is hijacked by L monocytogenes and promotes an increase in intracellular bacteria. Together, these data uncover a key role for SIRT2 mediated H3K18 deacetylation during infection and characterize a novel mechanisme imposed by a pathogenic bacteriomto reprogram the host cell.

Interactions hôte-pathogène

Listeria monocytogenes

Infection

Host-Pathogen Interactions

Listeria monocytogenes

Infection

Histone modifications

Histone H3

Histone H3 K18

Acetylation

Deacetylation

Histone Deacetylase

Sirtuin

SIRT2

Met

PI3K

Akt

Signalling

Epigenetics

Transcriptional Control

Studium mechanismu účinku protinádorových léčiv na neuroblastomy / Study of the mechanism of anticancer drug action on neuroblastomas

Černá, Tereza

January 2018

Despite advances in cancer diagnosis and therapy, cancer is the second leading cause of death globally. The improvements of cancer treatment are the major challenge in this research. The aim of the thesis was studying of effects of two anticancer drugs ellipticine (Elli) and doxorubicin (DOX) on some cancer and healthy cell lines. Specific consideration was given to expand current knowledge about the metabolism and cytostatic effects of Elli in neuroblastoma cell lines. Another part of this study was focused on mechanisms contributing to the development of ellipticine-resistance in cancer cells and influence of histone deacetylase inhibitors on anticancer therapy was investigated. Moreover, the aim was to develop apoferritin (Apo) nanocarrier suitable for the active transport of cytostatics to cancer cells. Several essential data were found in this doctoral thesis. Anticancer efficiency of Elli depends on the CYP3A4-mediated metabolism in cancer. The CYP3A4 enzyme encapsulated into two nanoparticle forms, liposomes and SupersomesTM , was tested to activate ellipticine to its reactive species forming covalent DNA adducts. The formation of adducts seems to be dependent on concentrations of CYP3A4 in nanoparticle systems. A higher effectiveness of CYP3A4 in SupersomesTM than in liposomes to form...

Histone Deacetylase 3 Coordinates Heart Development Through Stage-Specific Roles in Cardiac Progenitor Cells

Lewandowski, Sara L.

21 December 2016

Disruptions in cardiac development cause congenital heart disease, the most prevalent and deadly congenital malformation. Genetic and environmental factors are thought to contribute to these defects, however molecular mechanisms remain largely undefined. Recent work highlighted potential roles of chromatin- modifying enzymes in congenital heart disease pathogenesis. Histone deacetylases, a class of chromatin-modifying enzymes, have developmental importance and recognized roles in the mature heart. This thesis aimed to characterize functions of Hdac3 in cardiac development. We found loss of Hdac3 in the primary heart field causes precocious progenitor cell differentiation, resulting in hypoplastic ventricular walls, ventricular septal defect, and mid- gestational lethality. In primary heart field progenitors, Hdac3 interacts with, deacetylates, and functionally suppresses transcription factor Tbx5. Furthermore, a disease-associated Tbx5 mutation disrupts this interaction, rendering Tbx5 hyperacetylated and hyperactive. By contrast, deletion of Hdac3 in second heart field progenitors bypasses these defects, instead causing malformations in the outflow tract and semilunar valves, with lethality prior to birth. Affected semilunar valves and outflow tract vessels exhibit extracellular matrix and EndMT defects and activation of the Tgfβ1 signaling pathway. In normal second heart field development, Hdac3 represses Tgfβ1 transcription, independent of its deacetylase activity, by recruiting the PRC2 methyltransferase complex to methylate the Tgfβ1 promoter. Importantly, knockouts of Hdac3 in differentiated cardiac cells do not fully recapitulate the progenitor-specific knockout phenotypes. These results illustrate spatiotemporal roles of Hdac3, both deacetylase-dependent and deacetylase-independent, in cardiac development, suggesting that dysregulation of Hdac3 in cardiac progenitor cells could be a contributing factor in congenital heart disease pathogenesis.

Hdac3

histone deacetylase

cardiac development

heart

congenital heart disease

primary heart field

second heart field

progenitor cells

development

chromatin

epigenetics

gene regulation

Tbx5

Tgf-beta

Cell and Developmental Biology

Cell Biology

Developmental Biology

Molecular Genetics

The role of DNA methylation in regulating LHX3 gene expression

Malik, Raleigh Elizabeth

25 February 2014

Indiana University-Purdue University Indianapolis (IUPUI) / LIM homeodomain 3 (LHX3) is an important regulator of pituitary and nervous system development. To date, twelve LHX3 gene mutations have been identified in patients with combined pituitary hormone deficiency disease (CPHD). Understanding the molecular mechanisms governing LHX3/Lhx3 gene regulation will provide critical insights into organ development pathways and associated diseases. DNA methylation has been implicated in gene regulation in multiple physiological systems. This dissertation examines the role of DNA methylation in regulating the murine Lhx3 gene. To determine if demethylation of the Lhx3 gene promoter would induce its expression, murine pre-somatotrope pituitary cells that do not normally express Lhx3 (Pit-1/0 cells) were treated with the demethylating reagent, 5-Aza-2’-deoxycytidine. This treatment lead to activation of the Lhx3 gene and thus suggested that methylation contributes to Lhx3 gene regulation. Proteins that modify chromatin, such as histone deacetylases (HDACs) have also been shown to affect DNA methylation patterns and subsequent gene activation. Pit-1/0 pituitary cells treated with a combination of the demethylating reagent and the HDAC inhibitor, Trichostatin A led to activation of the Lhx3 gene, suggesting crosstalk between DNA methylation and histone modification processes. To assess DNA methylation levels, treated and untreated Pit-1/0 genomic DNA were subjected to bisulfite conversion and sequencing. Treated Pit-1/0 cells had decreased methylation compared to untreated cells. Chromatin immunoprecipitation assays demonstrated interactions between the methyl-binding protein, MeCP2 and the Lhx3 promoter regions in the Pit-1/0 cell line. Overall, the study demonstrates that DNA methylation patterns of the Lhx3 gene are associated with its expression status.

LHX3

DNA Methylation

Developmental neurophysiology

Histone deacetylase

Chromatin -- Research

Nucleotide sequence

Genetic regulation -- Research

Adenohypophysis

Acetylation

Design, Synthesis and Biological Evaluation of Histone Deacetylase Inhibitors and SARS-CoV-2 Main Protease Inhibitors

Banerjee, Riddhidev

11 July 2022

No description available.

Chemistry

Biochemistry

Medicine

Pharmacy Sciences

Optimisation d'antiœstrogènes dans le traitement du cancer du sein positif pour le récepteur des œstrogènes

Diennet, Marine

10 1900

Deux tiers des cancers du sein expriment le récepteur des œstrogènes alpha (ERα), un facteur de transcription ligand dépendant responsable de la prolifération oncogénique de ces cellules. Ces tumeurs, dites ER positives (ER+), bénéficient de thérapies endocrines comme les antiœstrogènes (AE). Les AE sont des ligands compétitifs de ERα qui inhibent son activité transcriptionnelle. Le tamoxifène est l’antiœstrogène le plus utilisé en première ligne de traitement chez les patientes ayant un cancer du sein ER+. Malgré un bon pronostique initial, plus du tiers d’entre elles finiront par développer une résistance, parfois après de nombreuses années. L’absence de résistance croisée avec le tamoxifène place le fulvestrant comme seul dé-régulateur sélectif de ER (SERD) autorisé en clinique contre les tumeurs mammaires avancées résistantes. Malgré son profil antagoniste pur, le fulvestrant ne s’est pas révélé supérieur au tamoxifène en première ligne de traitement, cela étant attribué à sa faible biodisponibilité. D’autres SERD oralement disponibles sont en cours d’évaluation clinique. Des mutations du gène ESR1 (ERα) sont retrouvées dans environ 20% des tumeurs avancées résistantes à l’hormonothérapie et contribuent à la résistance au fulvestrant. Les mutations sont toutes retrouvées dans le domaine de liaison au ligand. La maladie progressera éventuellement avec le développement de métastases qui sont incurables. Il est donc crucial de (1) comprendre les mécanismes moléculaires médiant l’antiestrogénicité pure et l’impact des altérations génétiques impliquées dans la résistance aux AE pour (2) développer des thérapies ciblées plus efficaces qui pourraient lutter contre les tumeurs avancées résistantes. Les résultats prometteurs de plusieurs études in vitro et en clinique combinant un AE avec un inhibiteur d’histones désacétylases (HDACi) ont mené à la création de molécules hybrides combinant les deux fonctionnalités en une seule molécule. Nos travaux montrent que ces molécules hybrides dérivées du tamoxifène démontrent des propriétés inhibitrices améliorées par l’ajout d’un groupe fonctionnel inhibiteur des HDAC sur le squelette du tamoxifène. Ces composés sont antagonistes contre ERα et plusieurs HDAC et l’un d’eux possède une activité antiproliférative accrue par rapport aux composés parentaux dans les cellules de cancer du sein ER+ MCF-7. Notre étude fournit une preuve de concept que la combinaison d’une fonction pharmacologique HDACi sur le noyau d’un AE est prometteuse. Afin de mieux comprendre les déterminants moléculaires liés à l’induction de la SUMOylation de ERα et l’inhibition de son activité transcriptionnelle par le fulvestrant, nous avons testé l’impact de différentes mutations sur l’activité de plusieurs SERD, comprenant le fulvestrant. Nos résultats valident l’importance du résidu L536 dans la SUMOylation et la répression transcriptionnelle de ERα en réponse aux SERD. Les mutations ponctuelles L536P, Q et R, trouvées en clinique, compromettent la réponse au fulvestrant et à une sélection de SERD oraux in vitro. En résumé, nos résultats participent à une meilleure compréhension des caractéristiques moléculaires liées au mécanisme d’action du fulvestrant et de plusieurs SERD oraux de nouvelle génération. L’ensemble de nos résultats devraient aider au développement de nouvelles molécules plus efficaces contre les tumeurs résistantes, y compris des composés avec une double fonction inhibitrice AE-HDACi. / Two thirds of breast tumors are classified as positive for estrogen receptor alpha (ERα), a ligand-dependent transcription factor driving breast cancer cell proliferation. ER-positive (ER+) tumors benefit from endocrine therapies such as antiestrogens (AE). AE compete with ERα natural ligands and inhibit its transcriptional activity. Tamoxifen is the gold-standard for antiestrogenic therapy in patients with primary ER+ breast cancer. Despite a good initial prognosis, more than one-third will eventually develop resistance, sometimes after long periods of latency. Fulvestrant, known as a “pure” AE, is the only selective ER deregulator (SERD) approved in advanced breast cancer even after development of resistance to tamoxifen. Despite its pure antagonistic profile, fulvestrant has not proven superior to tamoxifen in first-line treatment, which is attributed to poor pharmacological properties. New generation SERDs with orally bioavailable properties are currently tested in the clinic. Mutations of ERα are found in about 20% of hormone-resistant advanced tumors and contribute to resistance to fulvestrant. The mutations are all located in the ligand binding domain. Resistant tumors will eventually progress and develop metastases which are deadly. It is therefore crucial to (1) understand the molecular determinants of pure antiestrogenicity and the impact of genetic alterations involved in AE resistance to (2) develop treatments with improved cytotoxic activities to achieve a more efficient suppression of advanced tumors. Promising results from several in vitro and clinical studies combining an AE with a histone deacetylase inhibitor (HDACi) have led to the design of hybrid molecules combining both functionalities into a single molecule. Our work shows that tamoxifen-derived hybrids display properties by the addition of an HDAC inhibitory functional group (HDACi) on the tamoxifen backbone. These compounds have inhibitory activities against ERα and several HDACs. One hybrid exhibits an improved cytotoxic activity against ER+ MCF-7 breast cancer cells compared to parental molecules. Our study provides proof of concept that combining HDACi function to the core of an AE is promising. To better understand the molecular determinants related to the induction of ERα SUMOylation and transcriptional repression by fulvestrant, we evaluated the impact of different mutations on the activity of several SERDs, including fulvestrant. Our results validate the importance of residue L536 in SUMOylation and transcriptional repression of ERα in response to SERDs. L536P, Q, and R point mutations are found in the clinic compromise the response to fulvestrant and to several oral SERDs in vitro. In summary, our results give better insights into the mechanism of action of fulvestrant and new generation oral SERDs and on the impact of naturally occurring mutations on transcriptional responses to these AE. Taken together, our results should help in the design of more efficient molecules, including compounds with dual AE-HDACi inhibitory function.

Cancer du sein

Récepteur des œstrogènes alpha

Antiœstrogènes

Inhibiteur d’histone désacétylase

Molécules hybrides

Mutations

SUMOylation

Répression transcriptionnelle

Breast cancer

Estrogen receptor alpha

Antiestrogens

Histone deacetylase inhibitor

Hybrid molecules

Transcriptional repression