Playing TET

Methylation of the fifth carbon of cytosine was the first epigenetic modification to be discovered in DNA. Recently, three new DNA modifications have come to light: hydroxymethylcytosine, formylcytosine, and carboxylcytosine, all generated by oxidation of methylcytosine by Ten Eleven Translocation (TET) enzymes. These modifications can initiate full DNA demethylation, but they are also likely to participate, like methylcytosine, in epigenetic signalling per se. A scenario is emerging in which coordinated regulation at multiple levels governs the participation of TETs in a wide range of physiological functions, sometimes via a mechanism unrelated to their enzymatic activity. Although still under construction, a sophisticated picture is rapidly forming where, according to the function to be performed, TETs ensure epigenetic marking to create specific landscapes, and whose improper build-up can lead to diseases such as cancer and neurodegenerative disorders. © 2014 The Authors.SCOPUS: re.jFLWINinfo:eu-repo/semantics/publishe

DNA methylation profiling identifies epigenetic dysregulation in pancreatic islets from type 2 diabetic patients

The first genome-scale DNA methylation study on pancreatic islets from type 2 diabetic patients identifies disease-associated DNA methylation pattern that translate into aberrant gene expression in novel factors relevant for β-cell function and survival

Methylglyoxal: a novel upstream regulator of DNA methylation.

peer reviewed[en] BACKGROUND: Aerobic glycolysis, also known as the Warburg effect, is predominantly upregulated in a variety of solid tumors, including breast cancer. We have previously reported that methylglyoxal (MG), a very reactive by-product of glycolysis, unexpectedly enhanced the metastatic potential in triple negative breast cancer (TNBC) cells. MG and MG-derived glycation products have been associated with various diseases, such as diabetes, neurodegenerative disorders, and cancer. Glyoxalase 1 (GLO1) exerts an anti-glycation defense by detoxifying MG to D-lactate. METHODS: Here, we used our validated model consisting of stable GLO1 depletion to induce MG stress in TNBC cells. Using genome-scale DNA methylation analysis, we report that this condition resulted in DNA hypermethylation in TNBC cells and xenografts. RESULTS: GLO1-depleted breast cancer cells showed elevated expression of DNMT3B methyltransferase and significant loss of metastasis-related tumor suppressor genes, as assessed using integrated analysis of methylome and transcriptome data. Interestingly, MG scavengers revealed to be as potent as typical DNA demethylating agents at triggering the re-expression of representative silenced genes. Importantly, we delineated an epigenomic MG signature that effectively stratified TNBC patients based on survival. CONCLUSION: This study emphasizes the importance of MG oncometabolite, occurring downstream of the Warburg effect, as a novel epigenetic regulator and proposes MG scavengers to reverse altered patterns of gene expression in TNBC

Regulation of DNA Methylation Patterns by CK2-Mediated Phosphorylation of Dnmt3a

DNA methylation is a central epigenetic modification that is established by de novo DNA methyltransferases. The mechanisms underlying the generation of genomic methylation patterns are still poorly understood. Using mass spectrometry and a phosphospecific Dnmt3a antibody, we demonstrate that CK2 phosphorylates endogenous Dnmt3a at two key residues located near its PWWP domain, thereby downregulating the ability of Dnmt3a to methylate DNA. Genome-wide DNA methylation analysis shows that CK2 primarily modulates CpG methylation of several repeats, most notably of Alu SINEs. This modulation can be directly attributed to CK2-mediated phosphorylation of Dnmt3a. We also find that CK2-mediated phosphorylation is required for localization of Dnmt3a to heterochromatin. By revealing phosphorylation as a mode of regulation of de novo DNA methyltransferase function and by uncovering a mechanism for the regulation of methylation at repetitive elements, our results shed light on the origin of DNA methylation patterns

Etude des mécanismes moléculaires par lesquels les méthyltransférases de l'ADN établissent les profils de méthylation

La méthylation des cytosines de l’ADN est un niveau de contrôle essentiel de la transcription génique. Elle joue un rôle primordial dans plusieurs étapes du développement comme l’inactivation du chromosome X et l’empreinte génomique. De plus, il est de plus en plus évident que la méthylation de l’ADN participe à la cancérogenèse.Actuellement, le monde de la méthylation de l’ADN n’en est encore qu’à l'aube de son histoire. En effet, les mécanismes moléculaires la gouvernant sont encore peu connus. La méthylation de l’ADN est caractérisée par deux concept clés :le verrouillage de la transcription des gènes et le ciblage en des régions spécifiques du génome. Au cours de notre travail de thèse de doctorat, nous avons poursuivi les avancées réalisées dans ces deux domaines.Dans un premier temps, nous nous sommes attachés à l’étude de la répression transcriptionnelle entraînée par la méthylation de l’ADN. Grâce à plusieurs études récentes, il paraît de plus en plus clair que la méthylation agit de paire avec la structure de la chromatine. Nous avons donc concentré nos recherches sur l’interconnexion de celle-ci avec deux machineries impliquées dans la régulation de son degré de compaction :la désacétylation et la méthylation des histones. Par diverses expérimentations, nous avons démontré un lien étroit entre ces machineries répressives pour l’imposition d’un état silencieux de la transcription.Dans la deuxième partie de ce travail, nous avons dirigé notre attention sur le ciblage des Dnmt. Pour cela, nous avons mené deux stratégies de front. La première est une approche ciblée et consiste en l’étude de l’association des Dnmt avec l’oncoprotéine bien connue, Myc. La seconde approche est plus large. Grâce à l’utilisation de la technique du double hybride en levure, nous avons identifié de nouveaux partenaires des Dnmt, dont un qui pourrait s’avéré particulièrement intéressant :le protéine Cart1 (cartilage homeoproteine 1) impliquée dans le développement du système nerveux central.En conclusion, notre travail de doctorat devrait permettre une meilleure compréhension des mécanismes moléculaires de la méthylation de l’ADN ainsi que son implication dans les divers processus physiologiques mais aussi pathologiques auxquels elle participe.Doctorat en sciences biomédicalesinfo:eu-repo/semantics/nonPublishe

Etude des mécanismes moléculaires par lesquels les méthyltransférases de l'ADN établissent les profils de méthylation

La méthylation des cytosines de l’ADN est un niveau de contrôle essentiel de la transcription génique. Elle joue un rôle primordial dans plusieurs étapes du développement comme l’inactivation du chromosome X et l’empreinte génomique. De plus, il est de plus en plus évident que la méthylation de l’ADN participe à la cancérogenèse.Actuellement, le monde de la méthylation de l’ADN n’en est encore qu’à l'aube de son histoire. En effet, les mécanismes moléculaires la gouvernant sont encore peu connus. La méthylation de l’ADN est caractérisée par deux concept clés :le verrouillage de la transcription des gènes et le ciblage en des régions spécifiques du génome. Au cours de notre travail de thèse de doctorat, nous avons poursuivi les avancées réalisées dans ces deux domaines.Dans un premier temps, nous nous sommes attachés à l’étude de la répression transcriptionnelle entraînée par la méthylation de l’ADN. Grâce à plusieurs études récentes, il paraît de plus en plus clair que la méthylation agit de paire avec la structure de la chromatine. Nous avons donc concentré nos recherches sur l’interconnexion de celle-ci avec deux machineries impliquées dans la régulation de son degré de compaction :la désacétylation et la méthylation des histones. Par diverses expérimentations, nous avons démontré un lien étroit entre ces machineries répressives pour l’imposition d’un état silencieux de la transcription.Dans la deuxième partie de ce travail, nous avons dirigé notre attention sur le ciblage des Dnmt. Pour cela, nous avons mené deux stratégies de front. La première est une approche ciblée et consiste en l’étude de l’association des Dnmt avec l’oncoprotéine bien connue, Myc. La seconde approche est plus large. Grâce à l’utilisation de la technique du double hybride en levure, nous avons identifié de nouveaux partenaires des Dnmt, dont un qui pourrait s’avéré particulièrement intéressant :le protéine Cart1 (cartilage homeoproteine 1) impliquée dans le développement du système nerveux central.En conclusion, notre travail de doctorat devrait permettre une meilleure compréhension des mécanismes moléculaires de la méthylation de l’ADN ainsi que son implication dans les divers processus physiologiques mais aussi pathologiques auxquels elle participe.Doctorat en sciences biomédicalesinfo:eu-repo/semantics/nonPublishe

Playing TETris with DNA modifications

Methylation of the fifth carbon of cytosine was the first epigenetic modification to be discovered in DNA. Recently, three new DNA modifications have come to light: hydroxymethylcytosine, formylcytosine, and carboxylcytosine, all generated by oxidation of methylcytosine by Ten Eleven Translocation (TET) enzymes. These modifications can initiate full DNA demethylation, but they are also likely to participate, like methylcytosine, in epigenetic signalling per se. A scenario is emerging in which coordinated regulation at multiple levels governs the participation of TETs in a wide range of physiological functions, sometimes via a mechanism unrelated to their enzymatic activity. Although still under construction, a sophisticated picture is rapidly forming where, according to the function to be performed, TETs ensure epigenetic marking to create specific landscapes, and whose improper build-up can lead to diseases such as cancer and neurodegenerative disorders. © 2014 The Authors.SCOPUS: re.jFLWINinfo:eu-repo/semantics/publishe

The DNA methyltransferases associate with HP1 and the SUV39H1 histone methyltransferase

The DNA methyltransferases, Dnmts, are the enzymes responsible for methylating DNA in mammals, which leads to gene silencing. Repression by DNA methylation is mediated partly by recruitment of the methyl-CpG-binding protein MeCP2. Recently, MeCP2 was shown to associate and facilitate histone methylation at Lys9 of H3, which is a key epigenetic modification involved in gene silencing. Here, we show that endogenous Dnmt3a associates primarily with histone H3-K9 methyltransferase activity as well as, to a lesser extent, with H3-K4 enzymatic activity. The association with enzymatic activity is mediated by the conserved PHD-like motif of Dnmt3a. The H3-K9 histone methyltransferase that binds Dnmt3a is likely the H3-K9 specific SUV39H1 enzyme since we find that it interacts both in vitro and in vivo with Dnmt3a, using its PHD-like motif. We find that SUV39H1 also binds to Dnmt1 and, consistent with these interactions, SUV39H1 can purify DNA methyltransferase activity from nuclear extracts. In addition, we show that HP1β, a SUV39H1-interacting partner, binds directly to Dnmt1 and Dnmt3a and that native HP1β associates with DNA methyltransferase activity. Our data show a direct connection between the enzymes responsible for DNA methylation and histone methylation. These results further substantiate the notion of a self-reinforcing repressive chromatin state through the interplay between these two global epigenetic modifications

Functional and Direct Connection between Deimination and Deacetylation of Histone

Histone methylation plays key roles in the regulation of chromatin structure and function. The recent identification of enzymes that antagonize or remove histone methylation offers new opportunities to appreciate histone methylation plasticity in the regulation of epigenetic pathways. Peptidylarginine deiminase 4 (PADI4) was the first enzyme shown to antagonize histone methylation. PADI4 functions as a histone deiminase converting a methylarginine residue to citrulline at specific sites on the tail of histones H3 and H4. This activity is linked to repression of the estrogen-regulated pS2 promoter. Very little is known as to how PADI4 silences gene expression. To investigate the mechanisms by which histone demethylation and in particular PADI4 functions, and as no PADI4 interactors have been described so far, in vitro interaction assays and coimmunoprecipitations were performed. We found that the histone deacetylase HDAC1 interacts with PADI4, both in vitro and in vivo, and associates with PADI4-mediated histone deiminase activity. Chromatin immunoprecipitations in MDA-ER66 cells using antibodies against PADI4, HDAC1, citrulline H3 and acetylated histones show that PADI4 and HDAC1 appear transiently and in a cyclic manner on the estrogen-responsive promoter pS2, in the presence of estradiol. Their presence correlates with the loss of arginine methylation, acquisition of citrulline, histone deacetylation, and disengagement of RNA polymerase II from the pS2 promoter. Furthermore, sequential ChIP further indicated that PADI4 and HDAC1 bind together to the pS2 promoter in the presence of estrogen. These results further substantiate the “transcriptional clock” concept, highlighting the dynamic interplay between deimination and deacetylation of histones.info:eu-repo/semantics/nonPublishe

Functional Connection between Deimination and Deacetylation of Histones▿

Histone methylation plays key roles in regulating chromatin structure and function. The recent identification of enzymes that antagonize or remove histone methylation offers new opportunities to appreciate histone methylation plasticity in the regulation of epigenetic pathways. Peptidylarginine deiminase 4 (PADI4; also known as PAD4) was the first enzyme shown to antagonize histone methylation. PADI4 functions as a histone deiminase converting a methylarginine residue to citrulline at specific sites on the tails of histones H3 and H4. This activity is linked to repression of the estrogen-regulated pS2 promoter. Very little is known as to how PADI4 silences gene expression. We show here that PADI4 associates with the histone deacetylase 1 (HDAC1). Kinetic chromatin immunoprecipitation assays revealed that PADI4 and HDAC1, and the corresponding activities, associate cyclically and coordinately with the pS2 promoter during repression phases. Knockdown of HDAC1 led to decreased H3 citrullination, concomitantly with increased histone arginine methylation. In cells with a reduced HDAC1 and a slightly decreased PADI4 level, these effects were more pronounced. Our data thus suggest that PADI4 and HDAC1 collaborate to generate a repressive chromatin environment on the pS2 promoter. These findings further substantiate the “transcriptional clock” concept, highlighting the dynamic connection between deimination and deacetylation of histones