On the function of the Dictyostelium Argonaute A protein (AgnA) in epigenetic gene regulation

Zhang, Xiaoxiao

Unknown Date

Univ., Diss., 2006--Kassel

Epigenetic repression of the NFATc1 transcription factor in human lymphomas

Akimzhanov, Askar M.

Unknown Date

University, Diss., 2005--Würzburg.

Epigenetic repression of the NFATc1 transcription factor in human lymphomas / Epigenetische Repression des NFATc1 Transkriptionsfakors in menschlichen Lymphomen

Akimzhanov, Askar M.

January 2005

We examined the regulation of NFATc1 in different lymphomas and observed an inversed correlation between the methylation status and expression of NFATc1. Our data demonstrate that aberrant DNA methylation associated with chromatin remodeling within nfatc1 locus is a major mechanism for the repression of NFATc1 expression, suggesting that the DNA methylation-mediated transcriptional silencing of NFATc1 may be a critical event in the tumorogenesis of ALCLs and cHLs. Furthermore, the DNA methylation of human nfatc1 promoter region could be used as a novel biomarker of tumor progression. Our results indicate a close link between the loss of immunoreceptor signaling and NFATc1 expression in human lymphomas. For both ALCLs and cHLs, defects in immunoreceptor signaling have been described which result in a loss of receptor-mediated gene expression programs (Schwering et al., 2003; Bonzheim et al., 2004; Marafioti et al., 2004). In T cells, one indicator gene of these programs appears to be the nfatc1 gene whose expression is controlled by TCR signals (Chuvpilo et al., 2002a). In contrast, in T cells NFATc1 expression is unaffected by TCR signals, and NFATc2 was found to be expressed at normal levels in ALCLs and cHLs (L.K., unpubl. data). Moreover, the activity of NF-kappaB factors which can bind to certain NFAT binding sites and share a distantly-related DNA binding domain with NFATs is strongly elevated in cHL cells (Bargou et al., 1997; Hinz et al., 2001; Hinz et al., 2002) suggesting that NFATs and NF-kappaBs exert very different effects on generation and maintenance of Hodgkin’s lymhomas. However, it should be mentioned that in Burkitt’s and further B cell lymphomas in which NFATc1 proteins are strongly expressed and controlled by receptor signals (Kondo et al., 2003), they could exert a promoting function in tumor development. The genes of p53 family members p63 and p73 are prominent examples for mammalian genes whose products can act both as oncoproteins and tumor suppressor genes (Hibi et al., 2000; Stiewe and Putzer, 2002), and it is likely that more genes exist which encode both tumor suppressors and oncoproteins. It remains to be shown whether the nfatc1 gene is one of them. / Wir haben die Regulation von NFATc1 in verschiedenen Lymphomen untersucht und beobachteten eine umgekehrte Korrelation zwischen dem Ausmaß an Methylierung und der Expression von NFATc1. Unsere Daten demonstrieren, dass eine aberrante DNA-Methylierung, die mit veränderter Chromatinstruktur innerhalb des nfatc1 Lokus assoziiert ist, der Hauptmechanismus für die Repression der NFATc1-Expression ist. Es wäre zu vermuten, dass die durch DNA-Methylierung verursachte transkriptionelle Abschaltung von NFATc1 der kritische Schritt bei der Tumorgenese von ALCLs und cHLs ist. Des weiteren könnte das Ausmaß der DNA-Methylierung in der humanen nfatc1-Promotorregion als neuer Biomarker für Tumorprogression genutzt werden. Unsere Daten indizieren eine enge Verbindung zwischen dem Verlust von Immunrezeptorsignalen und der NFATc1-Expression in humanen Lymphomen. Für sowohl ALCLs als auch cHLs wurden Defekte in der Immunrezeptorsignalgebung beschrieben, welche sich im Verlust des Rezeptor vermittelten Genexpressionsprogramms niederschlagen (Schwering et al., 2003; Bonzheim et al., 2004; Marafioti et al., 2004). In T-Zellen scheint das nfatc1-Gen eins der Indikatorgene dieses Programms zu sein, dessen Expression durch TCR-Signale kontrolliert wird (Chuvpilo et al., 2002a). Im Gegensatz dazu bleibt die NFATc2-Expression in T-Zellen unbeeinflusst von TCR-Signalen, weshalb NFATc2 in ALCLs und cHLs auch in normalem Ausmaß exprimiert wird (L.K., unpubl. data). Andererseits ist die Aktivität der NF-kappaB-Faktoren, die auch an bestimmte NFAT-Bindungsstellen binden können und deren DNA-Bindungsdomäne entfernt mit der der NFATs verwandt ist, in cHL-Zellen stark erhöht (Bargou et al., 1997; Hinz et al., 2001; Hinz et al., 2002). Das lässt vermuten, dass NFATc1 und die NF-kappa-Faktoren eine sehr unterschiedliche Rolle bei der Entstehung und dem Erhalt der Hodgkinlymphome spielen. Es sollte aber erwähnt werden, dass in Burkitts und anderen B-Zelllymphomen, in denen NFATc1-Proteine stark exprimiert und darüber hinaus durch Rezeptorsignale kontrolliert sind (Kondo et al., 2003), diese eine Tumor fördernde Funktion ausüben könnten. Die Gene der p53-Familienmitglieder p63 und p73 sind prominente Beispiele für Säugergene, deren Produkte sowohl als Onkoproteine als auch als Tumorsuppressoren fungieren können (Hibi et al., 2000; Stiewe and Putzer, 2002), und es ist wahrscheinlich, dass es noch weitere Gene gibt, die beide Funktionen ausüben. Es wird zu zeigen sein, ob das nfatc1-Gen eins von ihnen ist.

Lymphom

T-Lymphozyt

Transkriptionsfaktor

Methylierung

Epigenese

ddc:570

Epigenetic switch induced by MYC in Non-Small-Cell Lung Cancer / Durch MYC induzierte epigenetische Veränderung im Nichtkleinzelligen Bronchialkarzinom

Cardoso e Castro, Inês Sofia

January 2012

Non–Small-Cell Lung Cancer (NSCLC) is the most frequent human lung cancer and a major cause of death due to its high rate of metastasis1. These facts emphasize the urgent need for the investigation of new targets for anti-metastatic therapy. Up to now a number of genes and gene products have been identified that positively or negatively affect the probability of established human tumor cell lines to metastasize2. Previously, together with the group of Professor Ulf Rapp, we have described the first conditional mouse model for metastasis of NSCLC and identified a gene, c-MYC, that is able to orchestrate all steps of this process. We could identify potential markers for detection of metastasis and highlighted GATA4, which is exclusively expressed during lung development, as a target for future therapeutic intervention2. However, the mechanism underlying this metastatic conversion remained to be identified, and was therefore the focus of the present work. Here, GATA4 is identified as a MYC target in the development of metastasis and epigenetic alterations at the GATA4 promoter level are shown after MYC expression in NSCLC in vivo and in vitro. Such alterations include site-specific demethylation that accompanies the displacement of the MYC-associated zinc finger protein (MAZ) from the GATA4 promoter, which leads to GATA4 expression. Histone modification analysis of the GATA4 promoter revealed a switch from repressive histone marks to active histone marks after MYC binding, which corresponds to active GATA4 expression. This work identifies a novel epigenetic mechanism by which MYC activates GATA4 leading to metastasis in NSCLC, suggesting novel potential targets for the development of anti-metastatic therapy. / Das nichtkleinzellige Bronchialkarzinom (Non-Small-Cell Lung Cancer/NSCLC) ist die häufigste Form des Lungenkrebs und ist aufgrund seiner hohen Metastasierungsrate für die meisten krebsbedingten Todesfälle verantwortlich1. Bisher konnte eine Vielzahl von Genen und Genprodukten identifiziert werden, die einen Einfluss auf das Metastasierungspotenzial von humanen Tumorzelllinien in vitro haben2. Vor kurzem gelang es uns unter der Leitung von Prof. Ulf R. Rapp das erste konditionelle Modell der Metastasierung von NSCLC zu beschreiben. Wir identifizierten u.a. das Gen c-MYC, welches in der Lage ist, in alle Schritte des Prozesses manipulierend einzugreifen. Im Rahmen dieser Arbeit konnten wir potentielle Marker zur Detektion der Metastasierung identifizieren. Unser Hauptaugenmerk lag dabei auf GATA4, ein Gen, das nur während der Lungenentwicklung exprimiert wird. Als potentielles Ziel für spätere therapeutische Eingriffe erscheint es daher besonders geeignet2. Die der Metastasierung zugrunde liegenden Mechanismen sind bisher weitestgehend ungeklärt und stellen daher einen Fokus dieser Arbeit dar. Im Rahmen der vorliegenden Arbeit wurde GATA4 als ein von MYC regulierter Faktor identifiziert, der an der Entwicklung von Metastasen beteiligt ist. Epigenetische Veränderungen am GATA4-Promotor nach der Expression von MYC konnten sowohl in vitro als auch in vivo nachgewiesen werden. Die Veränderungen beinhalten ortsspezifische Methylierungen, die einhergehen mit der Dislokation des MYC-assoziierten zinc finger protein (MAZ), die zur Expression von GATA4 führt. Die Analyse der Histon-Modifikationen am GATA4-Promotor ergab, dass nach der Bindung von MYC ein Wechsel von reprimierenden Histon-Markierungen zu aktiven stattfindet, der mit der GATA4-Expression korreliert. Im Rahmen dieser Arbeit konnte also ein neuartiger epigenetischer Mechanismus identifiziert werden, mit dem MYC GATA4 aktiviert und auf diese Weise zur Metastasenbildung bei NSCLC führt. Gleichzeitig wurden dadurch neue potentielle Zielstrukturen für die Entwicklung von anti-metastasierenden Therapeutika gefunden.

Nicht-kleinzelliges Bronchialkarzinom

Metastase

Gen

Myc

Epigenese

ddc:570

Die epigenetische Regulation des C4-Syndroms belichtungsabhängige Chromatinveränderungen am Promotor der Phosphoenolpyruvat Carboxylase aus Mais (Zea mays L.) /

Kalamajka, Rainer.

Unknown Date

Techn. Hochsch., Diss., 2005--Aachen.

Analysis of an epigenetic regulator in mouse embryonic stem cell self-renewal and differentiation / Analyse eines epigenetischen Regulators bei der Selbsterneuerung und Differenzierung muriner embryonaler Stammzellen

Lubitz, Sandra

10 January 2006

Mammals have two orthologs, Mll and Trx2, for the Drososphila protein Trithorax (TRX), which is the founding member of the trithorax group (TrxG) of epigenetic regulators. TrxG proteins are characterized by an evolutionary conserved SET domain. A major function of all SET domain- containing proteins is to modulate gene activity, but the underlying mechanisms are poorly understood. Apparently TRX, Mll and Trx2 are histone H3 lysine 4 specific methyltransferases. So far all evidence points to roles in expression of specific target genes. However, target genes and function of the epigenetic regulator Trx2 were still unknown. Homozygous trx2 mutant embryos arrest in development because of severe and widespread defects {Glaser, 2005 #296}. Thus mouse embryonic stem (ES) cells carrying a null mutation of trx2 were used as an alternative model system to address the implication of Trx2 in differentiation. This study showed that Trx2 is redundant for ES cell self-renewal. Homozygous trx2 knockout ES cells did not exhibit cell cycle defects. However, loss of Trx2 resulted in reduced proliferation and increased apoptosis rates in trx2-/- ES cells. Due to the fact that differentiation requires an appropriate rate of population growth, trx2-/- cells were affected adversely upon in vitro differentiation. Neurogeneic differentiation of trx2 mutant cells generated fewer mature neurons than wild type cells. Moreover a temporal delay in the developmental progression to differentiation became apparent. Cardiac differentiation of trx2-/- cells confirmed the developmental defect and temporal delay. Notably differentiation of trx2-/- cells was merely delayed or impaired but it was not absent, implying that Trx2 is not required for gene expression programs specific for neurons or cardiac myocytes. We propose that differentiation of trx2-/- ES cells is impaired because apoptosis is disturbing differentiation. Apart from analyzing the phenotype of trx2 mutant cells, this work was focused on the identification of Trx2 target genes. Oligonucleotide expression arrays were used to identify genes whose expression levels were affected by the absence of Trx2. In general, loss of Trx2 function resulted in more genes with decreased than increased expression levels. This is consistent with the hypothesis that Trx2 functions as a transcriptional activator. Comparison of gene expression profiles for constitutive and conditional trx2 mutant cells enabled a distinction between direct and indirect target genes for Trx2. As a result Magoh2 was identified as the key candidate target gene for Trx2. Interaction between Trx2 and Magoh2 suggested a potential regulatory role for Trx2 in alternative splicing. Furthermore this work provided evidence that Trx2 could be involved in the maintenance of CpG island promoter gene expression, thus providing a potent regulatory mechanism for ubiquitously expressed genes.

Stammzellen

Epigenetik

Histone

Histonmethyltransferase

Trx2

Trithorax

in vitro Differenzierung

stem cells

epigenetic

histones

histonemethyltransferase

Trx2

trithorax

in vitro differentiation

ddc:570

rvk:WX 6500

rvk:WG 3700

Embryonale Stammzelle

Epigenese

Genregulation

Histon-Methyltransferase

Histone

In vitro

TRX2

Trithorax

Analysis of an epigenetic regulator in mouse embryonic stem cell self-renewal and differentiation

Lubitz, Sandra

06 December 2005

Mammals have two orthologs, Mll and Trx2, for the Drososphila protein Trithorax (TRX), which is the founding member of the trithorax group (TrxG) of epigenetic regulators. TrxG proteins are characterized by an evolutionary conserved SET domain. A major function of all SET domain- containing proteins is to modulate gene activity, but the underlying mechanisms are poorly understood. Apparently TRX, Mll and Trx2 are histone H3 lysine 4 specific methyltransferases. So far all evidence points to roles in expression of specific target genes. However, target genes and function of the epigenetic regulator Trx2 were still unknown. Homozygous trx2 mutant embryos arrest in development because of severe and widespread defects {Glaser, 2005 #296}. Thus mouse embryonic stem (ES) cells carrying a null mutation of trx2 were used as an alternative model system to address the implication of Trx2 in differentiation. This study showed that Trx2 is redundant for ES cell self-renewal. Homozygous trx2 knockout ES cells did not exhibit cell cycle defects. However, loss of Trx2 resulted in reduced proliferation and increased apoptosis rates in trx2-/- ES cells. Due to the fact that differentiation requires an appropriate rate of population growth, trx2-/- cells were affected adversely upon in vitro differentiation. Neurogeneic differentiation of trx2 mutant cells generated fewer mature neurons than wild type cells. Moreover a temporal delay in the developmental progression to differentiation became apparent. Cardiac differentiation of trx2-/- cells confirmed the developmental defect and temporal delay. Notably differentiation of trx2-/- cells was merely delayed or impaired but it was not absent, implying that Trx2 is not required for gene expression programs specific for neurons or cardiac myocytes. We propose that differentiation of trx2-/- ES cells is impaired because apoptosis is disturbing differentiation. Apart from analyzing the phenotype of trx2 mutant cells, this work was focused on the identification of Trx2 target genes. Oligonucleotide expression arrays were used to identify genes whose expression levels were affected by the absence of Trx2. In general, loss of Trx2 function resulted in more genes with decreased than increased expression levels. This is consistent with the hypothesis that Trx2 functions as a transcriptional activator. Comparison of gene expression profiles for constitutive and conditional trx2 mutant cells enabled a distinction between direct and indirect target genes for Trx2. As a result Magoh2 was identified as the key candidate target gene for Trx2. Interaction between Trx2 and Magoh2 suggested a potential regulatory role for Trx2 in alternative splicing. Furthermore this work provided evidence that Trx2 could be involved in the maintenance of CpG island promoter gene expression, thus providing a potent regulatory mechanism for ubiquitously expressed genes.

info:eu-repo/classification/ddc/570

ddc:570