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The mammary gland of mice serves as a model system for studying differentiation in an adult animal. With the beginning of pregnancy the mammary epithelial cells undergo functional differentiation to produce milk for nourishment of the young. The transcription factor STAT5 mediates the cytokine-induced induction of the milk proteins during pregnancy and lactation in response to the lactogenic hormone prolactin. In addition to transcription factors that mediate transcription of their target genes by recruitment of the general transcription machinery to the DNA-regulator regions, specific post-translational modifications on the N-terminal tails of histones also influence expression. These histone modifications can affect chromatin structure, which is a main control barrier to transcription, by directly altering accessibility of the chromatin and by providing binding surfaces for protein complexes that can further modulate chromatin structure and regulate transcription. In this work N-terminal histone modification marks that associate with open, permissive and repressed chromatin where investigated in different regions of two milk protein genes during mammary gland development. Using the chromatin-immunoprecipitation (ChIP) assays increased acetylation of histone H3 and H4 at the 5’ region, promoter and transcribed regions of β-casein and whey acidic protein (WAP) gene were observed during pregnancy and lactation when these genes are expressed. The presence of these histone marks, which are associated with a relaxed chromatin structure, correlates with the recruitment of STAT5A and STAT5B to the promoter containing regulatory regions as well as the detection of the phosphorylated RNA polymerase II in the transcribed gene region. Both di- and tri-methylation of histone H3 lysine 4, that mark permissive and active chromatin respectively, were enriched in tissue from pregnant and lactating mice. In comparison tri-methylation of histone H3 lysine 27, a mark associated with repressed chromatin, could be observed during all stages of mammary gland tissue investigated, but appears slightly elevated in the tissue from virgin mice when β-casein and WAP are not expressed. Together these results illustrate that the expression of the two milk proteins genes at distinct stages of mammary gland differentiation correlate with specific changes in histone modifications. In mammary gland tissue STAT5A is important for the mammary gland epithelial cell differentiation and survival during lactation. Yet many genomic target regions that STAT5A actually bind and which are involved in regulation of gene expression during lactation still remain unknown. Therefore, the second part of this thesis was focused on the identification of novel STAT5-binding sites that are differentiation specifically bound by STAT5A in mammary gland tissue during lactation. In summary, the results demonstrate that the ChIP cloning method was employed successfully for the cloning of a STAT5A library and the identification of new STAT5 targets in mammary gland tissue from lactating mice. Nine of the newly identified STAT5-binding targets were verified to differentiation specifically bind STAT5A and STAT5B in vivo during pregnancy and lactation. Even though the selection of the tested clones was biased towards STAT5-binding sites near or at known genes and for multiple STAT5 binding sites, only one out of the nine validated STAT5-binding regions is located in a traditional defined proximal promoter. Except for two STAT5-binding regions, which are located at least 10 kb from the next annotated known gene, six are located in the intronic regions of annotated mRNA or EST transcripts. Three, out of four verified STAT5-binding regions tested in reporter gene assays for functionality, display the ability to drive reporter gene activity in a STAT5 dependent manner. This transcriptional activity is due to the STAT5-binding sites within the cloned regions as determined by mutational analysis. Of special interest is a STAT5-binding region that contains one STAT5 and three STAT-like sites within a 339 bp region that is evolutionary conserved by approximately 80% between the mouse and human genome. This STAT5-binding region lies about 62 kb 5 prime of the nuclear factor I/B gene. The expression of the NFI/B mRNA transcript correlates with the in vivo association of STAT5A to the conserved region during the mammary gland differentiation. Together, these results suggest that this STAT5-binding might be a cis-regulatory region that potentially mediates STAT5 induced NFI/B gene expression in mice during lactation.
A plethora of data has highlighted the role of epigenetics in the development of cancer. Initiation and progression of different cancer types are associated with a variety of changes of epigenetic mechanisms, including aberrant DNA methylation, histone modifications, and miRNA expression. At the same time, advances in the available epigenetic tools allow to investigate and reverse these epigenetic changes and form the basis for the development of anticancer drugs in human oncology. Although human and canine cancer shares several common features, only recently that studies emerged investigating the epigenetic landscape in canine cancer and applying epigenetic modulators to canine cancer. This review focuses on the existing studies involving epigenetic changes in different types of canine cancer and the use of small-molecule inhibitors in canine cancer cells.
DNA methylation reader MECP2 : cell type- and differentiation stage-specific protein distribution
(2014)
Background: Methyl-CpG binding protein 2 (MECP2) is a protein that specifically binds methylated DNA, thus regulating transcription and chromatin organization. Mutations in the gene have been identified as the principal cause of Rett syndrome, a severe neurological disorder. Although the role of MECP2 has been extensively studied in nervous tissues, still very little is known about its function and cell type specific distribution in other tissues.
Results: Using immunostaining on tissue cryosections, we characterized the distribution of MECP2 in 60 cell types of 16 mouse neuronal and non-neuronal tissues. We show that MECP2 is expressed at a very high level in all retinal neurons except rod photoreceptors. The onset of its expression during retina development coincides with massive synapse formation. In contrast to astroglia, retinal microglial cells lack MECP2, similar to microglia in the brain, cerebellum, and spinal cord. MECP2 is also present in almost all non-neural cell types, with the exception of intestinal epithelial cells, erythropoietic cells, and hair matrix keratinocytes. Our study demonstrates the role of MECP2 as a marker of the differentiated state in all studied cells other than oocytes and spermatogenic cells. MECP2-deficient male (Mecp2−/y) mice show no apparent defects in the morphology and development of the retina. The nuclear architecture of retinal neurons is also unaffected as the degree of chromocenter fusion and the distribution of major histone modifications do not differ between Mecp2−/y and Mecp2wt mice. Surprisingly, the absence of MECP2 is not compensated by other methyl-CpG binding proteins. On the contrary, their mRNA levels were downregulated in Mecp2−/y mice.
Conclusions: MECP2 is almost universally expressed in all studied cell types with few exceptions, including microglia. MECP2 deficiency does not change the nuclear architecture and epigenetic landscape of retinal cells despite the missing compensatory expression of other methyl-CpG binding proteins. Furthermore, retinal development and morphology are also preserved in Mecp2-null mice. Our study reveals the significance of MECP2 function in cell differentiation and sets the basis for future investigations in this direction.