Global ETD Search

41	GENETIC AND BIOCHEMICAL ANALYSIS OF THE ROLE OF EXTRA SEX COMBS-LIKE IN POLYCOMB SILENCING IN DROSOPHILA MELANOGASTER Kurzhals, Rebeccah Lynn 28 March 2006 (has links) No description available. Biology, Genetics Polycomb Drosophila chromatin histone methylation ESC ESCL E(Z)
42	Etude de la protéine de liaison à l’ARN LIF2, partenaire de la protéine chromatinienne LHP1, chez Arabidopsis thaliana / Study oh the RNA-binding protein LIF2, partner of the chromatin component LHP1, in Arabidopsis t haliana Leroux, Clémentine 08 February 2013 (has links) La dynamique chromatinienne joue un rôle central dans les contrôles développementaux, la différenciation cellulaire ou les réponses des organismes à l’environnement. Chez les animaux, les protéines du groupe Polycomb sont impliquées dans l’établissement d’états chromatiniens silencieux. Chez les plantes, des données récentes suggèrent que la protéine LIKE HETEROCHROMATIN PROTEIN 1 (LHP1) participerait à un complexe de type Polycomb. Nous nous sommes intéressés aux complexes LHP1 en étudiant un de ses partenaires, LHP1 INTERACTING FACTOR 2 (LIF2). L’objectif de ce travail de thèse a été de poursuivre la caractérisation de LIF2. LIF2 se caractérise par la présence de domaines de liaison à l’ARN, suggérant la participation d’une composante ARN dans les complexes LHP1. Nous avons recherché des ARN ligands de LIF2 et étudié les interactions LIF2/ARN par différentes approches dont la technologie Biacore. En analysant le transcriptome du mutant lif2, nous avons remarqué un enrichissement pour des gènes impliqués dans la réponse aux stress biotiques et abiotiques. Nous avons étudié la fonction de LIF2 dans la réponse aux pathogènes et avons pu mettre en évidence que LIF2 joue un rôle dans l’immunité innée des plantes et est essentiel pour réguler négativement les réactions de défenses en l’absence de pathogènes. / Chromatin dynamics play a central role in developmental control, cell differentiation or responses of the organisms to environment. In animals, Polycomb group proteins are involved in the establishment of silent chromatin states. In plants, recent data suggest that LIKE HETEROCHROMATIN PROTEIN 1 (LHP1) participates to a Polycomb-like complex. We focused on LHP1 complexes by studying one of its partners, LHP1 INTERACTING FACTOR 2 (LIF2). The aim of this thesis was to pursue the characterization of LIF2. LIF2 is composed of RNA-binding domains, suggesting the participation of an RNA component in LHP1 complexes. We have searched for LIF2 RNA-ligands and studied LIF2/RNA interactions with different approaches including Biacore technology. By analyzing the transcriptome profile of lif2, we have noticed an enrichment for genes involved in responses to abiotic and biotic stresses stimuli. We investigated the LIF2 functions in response to pathogens infection and we have been able to highlight that LIF2 plays a role in plant innate immunity and is essential to negatively regulate defense responses in the absence of pathogens. Chromatine Polycomb LHP1 Protéine de liaison à l’ARN LIF2 Immunité innée Chromatin Polycomb LHP1 RNA-binding protein LIF2 Innate immunity
43	Computational Biology: Insights into Hemagglutinin and Polycomb Repressive Complex 2 Function January 2012 (has links) Influenza B virus hemagglutinin (HA) is a major surface glycoprotein with frequent amino-acid substitutions. However, the roles of antibody selection in the amino-acid substitutions of HA were still poorly understood. An analysis was conducted on a total of 271 HA 1 sequences of influenza B virus strains isolated during 1940âˆ¼2007 finding positively selected sites all located in the four major epitopes (120-loop, 150-loop, 160-loop and 190-helix) supporting a predominant role of antibody selection in HA evolution. Of particular significance is the involvement of the 120-loop in positive selection. Influenza B virus HA continues to evolve into new sublineages, within which the four major epitopes were targeted selectively in positive selection. Thus, any newly emerging strains need to be placed in the context of their evolutionary history in order to understand and predict their epidemic potential. As key epigenetic regulators, polycomb group (PcG) proteins are responsible for the control of cell proliferation and differentiation as well as stem cell pluripotency and self-renewal. To facilitate experimental identification of PcG target genes, which are poorly understood, we propose a novel computational method, EpiPredictor , which models transcription factor interaction using a non-linear kernel. The resulting targets suggests that multiple transcription factor networking at the cis -regulatory elements is critical for PcG recruitment, while high GC content and high conservation level are also important features of PcG target genes. To try to translate the EpiPredictor into human data, we performed a computational study utilizing 22 human genome-wide CHIP data to identify DNA motifs and genome features that would potentially specify PRC2 using five motif discovery algorithms, Jaspar known transcription binding motifs, and other whole genome data. We have found multiple motifs within the various subgroups of experimental categories that have much higher enrichment against CHIP identified gene promoter than among random gene promoters. Specifically, we have identified Low CpG content CpG Islands (LeG's) as being critical in the separation of Cancer cell line identified targets from Embryonic Stem cell line identified targets. Additionally, there are differences between human and mouse ES cell predictions using the same motifs and features suggesting relevant evolutionary divergence. Applied sciences Biological sciences Polycomb Polycomb response element Hemagglutinin Motif discovery Positive selective pressure Viral evolution Biomedical engineering Bioinformatics
44	Reprogrammation cellulaire et morphogenèse épithéliale pendant le développement embryonnaire chez la drosophile / Reprogramming and epithelial morphogenesis during drosophila embryo development Roumengous, Solange 11 December 2015 (has links) Les changements de forme et les mouvements des cellules constituant les tissus relèvent de la morphogenèse épithéliale. Dans les tissus segmentés les compartiments antérieurs et postérieurs représentent des domaines morphogénétiques indépendants constitués de lignées cellulaires distinctes et séparées par des barrières biophysiques. Le laboratoire a montré que lors de la fermeture dorsale de l’embryon de drosophile, certaines cellules des segments centraux de l’ectoderme, appelées « Cellules Mixer » (CMs), sont reprogrammées pour traverser la frontière segmentale dans un phénomène qui prend le nom de « mixing ». La reprogrammation des CMs est JNK dépendante induisant l’expression de novo du gène engrailed (en). La mise au point de nouveaux outils génétiques a permis de révéler le rôle de deux familles de gènes impliqués dans les mécanismes de reprogrammation et de mixing : le gène Polycomb (Pc) et les gènes Hox. La technique de DNA-FISH, qui analyse l’interaction entre Pc et le PRE d’en, a ainsi montré que la voie JNK induit l’expression de novo d’en par dé-répression de l’activité Pc dans les CMs. De manière intéressante l’analyse approfondie des mutants Pc a dévoilé que les gènes Hox abdominal-A (abdA) et Abdominal-B (AbdB) contrôlent le domaine du mixing. Des expériences de gain et perte de fonction ont par la suite confirmé le rôle positif d’abdA et le rôle négatif d’AbdB dans le mixing. En conclusion, l’ensemble des résultats obtenus ont permis de dévoiler la présence d’un réseau génétique composé de par JNK, en, Pc et les gènes Hox contrôlant les mécanismes de reprogrammation cellulaire et de remodelage des frontières segmentales au cours du développement normal. / Tissue morphogenesis relies on patterned cell shape changes and movements taking place in specific morphogenetic domains. In segmented tissues, anterior and posterior compartments represent independent morphogenetic domains which are made of distinct lineages separated by boundaries. We previously reported on a rare event leading to the exchange of specific ‘Mixer Cells’ (MCs) between compartments of the ectoderm. During dorsal closure, MCs, which are of anterior origin, cross the boundary to integrate the adjacent posterior compartment through de novo expression of the posterior determinant Engrailed (En). This reprograming process is dependent on JNK signalling and is restricted to the central abdominal region. Here, we show that JNK signalling represses Polycomb (Pc) expression and that loss of Pc leads to an absence of MCs reprogramming. FISH-DNA coupled to immunostaining further shows that MCs fate transition is accompanied by a release of the en promoter from the repressing Pc bodies. Interestingly, our genetic data reveal that spatial control of MCs reprograming depends on the activity of the Hox genes abdominal-A (abdA) and Abdominal-B (AbdB). In their respective domains, abd-A promotes mixing while abd-B behaves as a strong repressor, thus restricting cell mixing to the central abdominal region. Together, these results provide new insights into the mechanisms of developmental reprogramming, showing that segment boundary plasticity relies on regional control of cell remodelling involving a gene regulatory network composed of JNK, en, Pc, and Hox activities. Reprogrammation Fermeture dorsale Morphogenèse JNK Polycomb Abdominal-A Abdominal-B Hox Reprogramming Dorsal closure Morphogenesis JNK Polycomb Abdominal-A Abdominal-B Hox
45	Investigação molecular e funcional de proteínas do Grupo Polycomb e seu envolvimento com a neurogênese olfatória / Molecular and functional investigation of Polycomb Group proteins and their involvement in olfactory neurogenesis Souza, Mateus Augusto de Andrade, 1989- 03 December 2015 (has links) Orientador: Fabio Papes / Dissertação (mestrado) - Universidade Estadual de Campinas, Instituto de Biologia / Made available in DSpace on 2018-08-27T05:41:39Z (GMT). No. of bitstreams: 1 Souza_MateusAugustodeAndrade_M.pdf: 6121419 bytes, checksum: a603ea19d560e8cfebddccca9b7d824a (MD5) Previous issue date: 2015 / Resumo: Em mamíferos, os neurônios sensoriais do Sistema Olfatório (OSNs) se encontram no interior da cavidade nasal, mas estão diretamente expostos ao ambiente externo. Por um lado, tal localização permite a esses neurônios o acesso imediato aos estímulos químicos ambientais, tomando vantagem do fluxo respiratório. Por outro lado, esses neurônios estão constantemente sujeitos a injúrias por agentes nocivos, como toxinas e patógenos, capazes de destruir essas células sensoriais. Sua perda constante, contudo, é contrabalanceada pela geração de novos OSNs durante toda a vida do indivíduo, fato que torna o Sistema Olfatório um dos poucos locais do organismo com neurogênese contínua na idade adulta. A regeneração dos OSNs tem atraído a atenção da comunidade científica tanto pelo seu potencial uso como modelo de estudo do Sistema Nervoso quanto pela sua potencial aplicação para o tratamento de doenças neurodegenerativas. Nesse sentido, muito conhecimento já foi produzido sobre a dinâmica de fatores de transcrição que acompanha a diferenciação dos progenitores neuronais olfatórios em OSNs. Porém, uma grande lacuna no conhecimento diz respeito a outros elementos capazes de coordenar esse processo, como os fatores moduladores da cromatina. Diante desse cenário, escolhemos como objeto de estudo as proteínas do Grupo Polycomb (PcG), que constituem uma maquinaria de controle transcricional relacionada a modificações na organização da cromatina. Neste trabalho, genes PcG selecionados foram caracterizados molecular e funcionalmente no epitélio olfatório principal de camundongos (MOE). Através de ensaios de hibridação in situ, cinco dos seis genes avaliados apresentaram expressão ubíqua por todo o epitélio (Cbx2, Cbx4, Phc2, Ezh1, Bcl6), enquanto um (Ezh2) mostrou-se expresso somente nos estratos basais do MOE. Em ensaios de colocalização, provamos que Ezh2 é expresso exclusivamente nos progenitores olfatórios, onde o processo de diferenciação se inicia, e em parte dos OSNs recém-diferenciados, ainda não funcionais. Esta foi a primeira vez que a expressão de um gene PcG foi analisada detalhadamente no Sistema Olfatório. O interessante perfil de expressão de Ezh2 foi sugestivo de um possível papel funcional relacionado à diferenciação dos progenitores olfatórios. Para investigar essa hipótese, utilizamos como ferramenta experimental a habilidade do MOE em se regenerar após a indução de injúrias específicas. Para isso, o MOE de camundongos foi lesionado quimicamente com o composto diclobenil, que leva à perda abrupta de OSNs, estimulando a proliferação e a diferenciação dos progenitores olfatórios para repovoar as regiões lesionadas. Os animais assim tratados receberam, por via intranasal, o fármaco GSK126, uma molécula inibidora específica da atividade da proteína EZH2. Acompanhando a regeneração subsequente do MOE, observamos que a inibição da atividade de EZH2 levou ao incremento de OSNs no epitélio, favorecendo a sua regeneração. Interessantemente, esse incremento também foi observado em MOEs não lesionados, mostrando que o efeito de GSK126 não é dependente da indução de injúrias prévias. Através dessa investigação molecular e funcional, buscamos contribuir para o melhor entendimento da diferenciação neuronal do MOE, e apontamos as proteína PcG como elementos importantes para esse processo / Abstract: In mammals, the olfactory sensory neurons (OSNs) are located inside the nasal cavity, but they are directly exposed to the external environment. Taking advantage of the respiratory flux, this location favors the access to the chemical stimuli presented by the environment. On the other hand, it leads OSNs to be continually damaged by pathogens and toxic substances carried by the inhaled air. However, the persistence of neuronal progenitors in the olfactory epithelium makes the constant reposition of the OSNs possible. This unique ability of regeneration makes the Olfactory System one of the few sites of neurogenesis throughout the adult life. Olfactory regeneration has attracted the attention scientific community because of its potential as a model of study of the Nervous System and application in the treatment of neurodegenerative diseases. A great amount of knowledge has been accumulated about the transcription factor dynamics that follows the differentiation of neuronal progenitors into OSNs. However, there is a great gap about other elements that could coordinate this process, such as chromatin modulator factors. In this scenario, we decided to study the Polycomb Group (PcG) proteins, a transcription control machinery involved in chromatin structure organization. In the present study, selected PcG genes were molecular and functionally analyzed in the mouse main olfactory epithelium (MOE). Using in situ hybridization assays, we characterized the expression of six PcG genes. Five of them were shown to be expressed throughout the MOE (Cbx2, Cbx4, Phc2, Ezh1, Bcl6), while one (Ezh2) was found only in the basal layers of this epithelium. Using colocalization strategies, we proved that Ezh2 gene is expressed exclusively in the olfactory progenitor cells, where the differentiation process begins, and in part of the newly differentiated OSNs that are still not functional. It was the first time that a PcG gene expression profile was finely analyzed in the Olfactory System. This interesting expression profile presented by Ezh2 suggested a possible involvement with the MOE neuronal progenitor differentiation. For this functional investigation, we used MOE¿s neuronal regeneration after specific injuries as an experimental tool. For this purpose, the MOE was chemically damaged by the compound dichlobenil, which causes a great loss of OSNs, stimulating proliferation and differentiation of neuronal progenitor cells, leading to the repopulation of the damaged tissue. Next, mice received by intranasal route the pharmacological inhibitor GSK126, which blocks EZH2 protein activity. The observation of the MOE regeneration that followed showed us that GSK126 application resulted in an increased number of OSNs, improving MOE regeneration. Interestingly, this increase was also found in intact MOEs, pointing that GSK126¿s effects do not depend on previous olfactory injuries. By this molecular and functional investigation, we aimed at a better understanding of olfactory neuronal differentiation, and we targeted the PcG proteins as relevant elements to this process / Mestrado / Genetica Animal e Evolução / Mestre em Genética e Biologia Molecular Neurogênese Neurônios receptores olfatórios Proteínas do Grupo Polycomb Sistema nervoso - Regeneração Neurogenesis Olfactory receptor neurons Polycomb-Group proteins Nervous system - Regeneration
46	Dynamic Polycomb Chromatin Suppresses Aberrant Transcription in Drosophila Immunity Streeck, Robert 10 August 2020 (has links) Die Modifikation von Chromatin und Histonen sind vielmehr zentrale Ereignisse in der Regulation der Geneexpression. Es ist gut etabliert, dass die Trimethylierung von Histon H3 Lysin 27 (H3K27me3) durch ‚Polycomb group’ (PcG) Proteine epigenetisches Gedächtnis aufrechterhält. Genomweite Analysen haben jedoch gezeigt, dass ein großer Teil des nicht-exprimierten Genoms die H3K27me3 Modifikation trägt. In dieser Arbeit habe ich RNA-seq und ChIP-seq auf Drosophila Plasmatozyten angewendet und ein hochauflösendes Chromatinprofil generiert. Ich konnte zeigen, dass eine Gruppe von Immungenen, die durch H3K27me3 markiert sind, nach einer Immunstimulierung rasch hochreguliert wird. Weiterhin konnte ich durch die Anwendung eines neu entwickelten Genomanalyse-Algorithmus zeigen, dass diese H3K27me3 positiven Gene in einem Chromatinzustand sind, der sich von kanonischem Polycomb Chromatin unterscheidet. Dieser Chromatinzustand hat zwei wichtige Eigenschaften: Erstens beweise ich, dass H3K27me3 als Antwort auf physiologische Stimuli dynamisch reguliert wird. Zweitens weise ich nach, dass es für den Erhalt eines reprimierten Genezustands instruktiv ist. Daher bezeichne ich diesen Chromatinzustand als dynamisches Polycomb Chromatin. Meine weiteren Analysen haben gezeigt, dass dieses dynamisches Polycomb Chromatin in Drosophila Plasmatozyten mit einer großen Zahl anderer dynamisch regulierter Gene assoziieret ist. Einige dieser Gene wurden ebenfalls nach der Depletion von H3K27me3 hochreguliert. Deshalb schlage ich vor, dass dynamisches Polycomb Chromatin einen neuartigen Chromatinzustand darstellt, der an Genen zu finden ist, deren Transkription durch unvorhersehbare Ereignisse ausgelöst wird. Die Reprimierung durch dynamisches Polycomb Chromatin bildet demnach eine Aktivierungschwelle gegen aberrante Transkription, die aber trotzdem eine rasche Geninduktion in physiologisch relevanten Situationen erlaubt. / Modification of chromatin and histones are central events in regulating gene expression. It is clearly established that histone H3 lysine 27 trimethylation (H3K27me3) by Polycomb group (PcG) proteins maintains the repressed state in epigenetic memory. Genome wide analysis revealed that much of the non-transcribed genome carries the H3K27me3 modification. This raises the question, whether this modification is functionally relevant outside of development to preclude activation of genes through physiological signaling. Here, I applied RNA-seq and ChIP-seq to Drosophila plasmatocytes generating a high resolution epigenetic landscape. Thereby, I demonstrated that a set of H3K27me3 marked immune genes was rapidly transcriptionally induced upon challenge. By applying a newly developed genome clustering algorithm, I demonstrated that these H3K27me3 positive genes are in a chromatin state that is distinct from the canonical Polycomb chromatin. This state has two important properties: First, by demonstrating that in plasmatocytes H3K27me3 is depleted specifically at immune genes after activation, I showed that it is dynamically regulated in response to physiological stimulation. Second, by establishing that immune genes were up-regulated when H3K27me3 was depleted, I confirmed that it is instructive in maintaining a silenced gene state. Therefore, I termed this novel chromatin state dynamic Polycomb chromatin. Further analysis revealed that this dynamic Polycomb chromatin state is also associated with a large number of other dynamically regulated genes. Some of these genes were also up-regulated when H3K27me3 is depleted by genetic manipulation. Hence, I propose that dynamic Polycomb chromatin is a novel chromatin state that targets genes which are triggered by non-predetermined signaling events. Silencing by dynamic Polycomb chromatin thresholds such genes against aberrant gene activation, but permits rapid induction in physiologically relevant situations. Genregulation Polycomb H3K27me3 Drosophila gene regulation polycomb H3K27me3 drosophila 570 Biologie WE 4500 WG 1950 ddc:570
47	Identification and characterization of Polycomb repressed gene-enhancer loops / Identification et caractérisation des boucles entre les promoteurs des gènes réprimés par Polycomb et les enhancers dans les cellules souches embryonnaires des souris Souaid, Charbel 25 January 2019 (has links) Dans les cellules souches embryonnaires de souris (mESCs), le groupe de protéines Polycomb (PcG) répriment les gènes de développement en participant ainsi à la maintenance de l’état de pluripotence. Ce complexe dépose la H3K27me3au niveau des éléments régulateurs induisant une compaction de la chromatine. Cette marque forme en plus des marquesactives H3K4me3 présentes des domaines bivalents. Etrangement, des boucles d’ADN dites entre le promoteur et enhancer, généralement associé à l’activation du gènes, sont observées au niveau des gènes bivalents avant leur activation.On suppose que la fonction du PcG pourrait être de neutraliser l'enhancer conférant une future activation rapide des gènes.Au cours de ma thèse, j’ai identifié les boucles d’ADN formé par les réprimés par PcG dans les mESCs. Pour cela,j’ai effectué un profilage épigénomique de 4 marques d'histones et identifié près de 2500 promoteurs bivalents et 13000enhancers. En utilisant des données publiées de Hi-C à haute résolution, j’ai identifié toutes les boucles formées par les domaines bivalents. Etonnement, j’ai pu identifier que de nombreux gènes réprimés par PcG interagissent avec des enhancers actifs. Cette observation a été suivie d'une validation par le 4C-seq. De plus, j’ai effectué une caractérisation fonctionnelle des boucles en utilisant deux approches. Tout d'abord, j'ai mis en place, en collaboration avec D. Bourc'his(Institut Curie), un système de culture de mESCs (2i + VitC) où le taux de H3K27me3 est réduit. J'ai effectué un profilage épigénomique similaire révélant que les promoteurs réprimés par PcG ont perdu la marque H3K27me3. En RNA-seq, j’ai démontré que l’expression des gènes ne change pas après le PcG soit détacher des promoteurs.. Ensuite, par la réalisation de plusieurs validations en 4C-seq j’ai démontré que les interactions avec les enhancers ne sont pas affecté alors que la moitié des enhancers interagissant perdent leurs marques activatrices. Dans le système 2i+VitC, ces gènes semblent être réprimés par un autre mécanisme suite à la perte du PcG. De plus, j’utilise une approche ciblée pour enlever localement laH3K27me3 de deux gènes bivalents en utilisant le système Cette technique est en cours d’optimisation.Notre étude est la plus systématique au niveau génomique des boucles d'ADN dans le cadre de la régulation des gènes PcG. Notre étude révèle une nouvelle fonction du PcG qui est la répression de boucle d’ADN déjà établies entre promoteurs et enhancers. / In the mouse embryonic stem cells (mESCs), Polycomb Group Proteins (PcG) repress developmental genes and thereby participating in the maintenance of the pluripotency. PcG repress genes by depositing the H3K27me3 histone marks on their regulatory elements, followed by chromatin compaction. In addition to the H3K27me3 marks, those genes carry H3K4me3 active marks and were characterized as bivalent. Intriguingly, at many PcG repressed genes, DNA loops can be observed with enhancer elements, which are normally thought to have an activating function. The aim of my project is to both describe and mechanistically dissect the function of Polycomb repressed promoter – enhancer loops.During my PhD, I aimed firstly to identify all promoter–enhancer loops involved by PcG repressed genes in mESCs. I have performed ChIP-seq profiling of 4 histone marks and identified around 2500 PcG repressed promoters and 13000 enhancers. Using a recently published high-resolution Hi-C data in mESCs, I have identified all DNA loops that are formed by PcG repressed promoters. Surprisingly, a high percentage of bivalent promoters were found to contact active enhancers. The presence of those loops were validated by ultra-high 4C-seq on selected genes and imply a small significant increase of the gene expression without leading to a complete activation of the gene. I have established a more physiological ESC model (2i+VitC) where H3K27me3 is reduced at all promoters. I have performed ChIP-seq, where bivalent promoters were all classified as H3K27me3 negative. RNA-seq experiments have showed that those genes do not become activated. 4C-seq experiments have revealed that those loops do not disappear after PcG removal, whereas the half of interacted enhancer loose their H3K27ac active marks. Those genes seem to remain repressed by an unknown mechanism. These results argue for a possible role of PcG in preparing the gene for their activation by blocking the productivity of such DNA loops. Secondly, I aimed to functionally characterize those DNA loops by using a CRISPR/dCas9 approach to completely remove H3K27me3 from two PcG repressed genes that contact active enhancers Pax6 and Nkx1-1 genes. This system is still under optimization steps.My project revealed the most systematic characterization of DNA loops under the regulation of PcG, providing important insight how PcG function to inactivate such loops. I have highlighted an additional function of PcG which the involvement in the repression of already establish loops between active enhancers and promoters and thereby blocking the productivity of such activating loops. This function is an addition to the already described repressive function of PcG on both promoters and poised enhancers. Cellules souches Régulation des gènes Épigénétique Génomique Enhancers Protéines du groupe Polycomb Stem cells Gene regulation Epigenetics Genomics Enhancers Polycomb group proteins
48	The Role of Polycomb Repressive Complex 2 in Epidermal Homeostasis and Hair Growth Asamaowei, Inemo E. January 2017 (has links) Polycomb repressive complex 2 (PRC2) catalyses the methylation of ‘Lys-27’ of histone H3, leading to transcriptional repression of target genes through its catalytic subunit Enhancer of zeste homolog 1/2 (EZH1/2). PRC2 functions as a critical regulator of stem cells in mouse embryonic and adult tissues. However, the role of PRC2 in human skin remains largely unknown. This study investigated the role of PRC2 in human epidermal homeostasis and hair growth. The expression of EZH2 was elevated in differentiating suprabasal layers of the human epidermis. Consistently, EZH1/2 expression and enzymatic activity was upregulated in differentiating primary human keratinocytes (NHEKs) in vitro. Inhibition of EZH2 and Embryonic ectoderm development (EED) in NHEKs stimulated the expression of differentiation-associated genes, therefore leading to their premature differentiation; while inhibition of EZH1/2 reduced cell proliferation and promoted apoptosis. Silencing of EZH2 in NHEKs induced complex changes in gene expression programmes, including the upregulation of terminal differentiation genes, such as Filaggrin. EZH2 expression was downregulated in aged keratinocytes accompanied with upregulation of senescence-associated genes, p16INK4A and p19INK4D, suggesting EZH2 involvement in epidermal aging. In human anagen hair follicle (HF), EZH2 was detected in stem and progenitor cells; and hair matrix keratinocytes. Silencing EZH2 in HFs accelerated anagen-catagen transition and retarded hair growth accompanied by decreased proliferation and increased apoptosis. Silencing EZH2 in outer root sheath keratinocytes resulted in upregulation of p14ARF and K15, suggesting EZH2 involvement in regulating proliferation and stem cell activity. Thus, this study demonstrates that PRC2-mediated repression is crucial for epidermal homeostasis and hair growth. Modulating the activities of PRC2 in skin might offer a new therapeutic approach for disorders of epidermal differentiation and hair growth. Skin Epidermis Hair folicle Polycomb group proteins EZH2 Differentiation Epidermal homeostasis Hair growth Polycomb repressive complex 2 (PRC2)
49	Inhibition of Hox function by the cell cycle regulator geminin / Inhibition der Hox-Funktion durch den Zellzyklus-Regulator Geminin Luo, Lingfei 25 October 2004 (has links) No description available. 570 Biowissenschaften, Biologie Mathematics and Computer Science Inhibition Geminin Polycomb Hox Zellzyklus Embryogenese Inhibition Geminin Polycomb Hox Cell Cycle Embryogenesis 42.13 Molekularbiologie WK 000: Entwicklungsbiologie
50	Protein dynamics in the nucleus: Implications for gene expression / Proteindynamik im Zellkern: Auswirkungen auf die Genexpression Ficz, Gabriella 16 July 2005 (has links) No description available. Polycomb Gruppen Proteine FRAP Inverse FRAP iFRAP Transkription Repression homeotische Gene Polycomb group proteins FRAP Inverse FRAP iFRAP Transcription Repression Homeotic genes

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