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DNA Methylation Density Influences the Stability of an Epigenetic Imprint and Dnmt3a/b-Independent De Novo Methylation

机译:DNA甲基化密度影响表观遗传印记和Dnmt3a / b独立的De Novo甲基化的稳定性

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DNA methylation plays an important role in transcriptional repression. To gain insight into the dynamics of demethylation and de novo methylation, we introduced a proviral reporter, premethylated at different densities, into a defined chromosomal site in murine erythroleukemia cells and monitored the stability of the introduced methylation and reporter gene expression. A high density of methylation was faithfully propagated in vivo. In contrast, a low level of methylation was not stable, with complete demethylation and associated transcriptional activation or maintenance-coupled de novo methylation and associated silencing occurring with equal probability. Deletion of the proviral enhancer increased the probability of maintenance-coupled de novo methylation, suggesting that this enhancer functions in part to antagonize such methylation. The DNA methyltransferases (MTases) Dnmt3a and Dnmt3b are thought to be the sole de novo MTases in the mammalian genome. To determine whether these enzymes are responsible for maintenance-coupled de novo methylation, the unmethylated or premethylated proviral reporter was introduced into DNA MTase-deficient embryonic stem cells. These studies revealed the presence of a Dnmt3a/Dnmt3b-independent de novo methyltransferase activity that is stimulated by the presence of preexisting methylation.
机译:DNA甲基化在转录抑制中起重要作用。为了深入了解去甲基化和从头甲基化的动力学,我们将在不同密度下预甲基化的原病毒报告基因引入鼠类红细胞白血病细胞中定义的染色体位点,并监测所引入甲基化和报告基因表达的稳定性。高密度的甲基化被忠实地在体内传播。相反,低水平的甲基化是不稳定的,完全脱甲基和相关的转录激活或维持偶联的从头甲基化和相关的沉默发生的可能性均等。删除前病毒增强剂增加了维持偶联的从头甲基化的可能性,表明该增强剂部分地拮抗了这种甲基化。 DNA甲基转移酶(MTase)Dnmt3a和Dnmt3b被认为是哺乳动物基因组中唯一的从头MTase。为了确定这些酶是否负责维持偶联的从头甲基化,将未甲基化或预甲基化的原病毒报道分子引入DNA MTase缺陷型胚胎干细胞中。这些研究表明存在Dnmt3a / Dnmt3b的从头甲基转移酶活性被存在的甲基化刺激了。

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