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Quantitative analysis of DNA methylation at all human imprinted regions reveals preservation of epigenetic stability in adult somatic tissue

机译:对所有人类印迹区域的DNA甲基化的定量分析表明在成年体细胞组织中表观遗传稳定性得以保留

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摘要

BackgroundGenes subject to genomic imprinting are mono-allelically expressed in a parent-of-origin dependent manner. Each imprinted locus has at least one differentially methylated region (DMR) which has allele specific DNA methylation and contributes to imprinted gene expression. Once DMRs are established, they are potentially able to withstand normal genome reprogramming events that occur during cell differentiation and germ-line DMRs are stably maintained throughout development. These DMRs, in addition to being either maternally or paternally methylated, have differences in whether methylation was acquired in the germ-line or post fertilization and are present in a variety of genomic locations with different Cytosine-phosphate guanine (CpG) densities and CTCF binding capacities. We therefore examined the stability of maintenance of DNA methylation imprints and determined the normal baseline DNA methylation levels in several adult tissues for all imprinted genes. In order to do this, we first developed and validated 50 highly specific, quantitative DNA methylation pyrosequencing assays for the known DMRs associated with human imprinted genes.
机译:以基因组印记的背景基因以原代依赖的方式单等位表达。每个印迹的基因座具有至少一个差异甲基化区域(DMR),该区域具有等位基因特异性DNA甲基化并有助于印迹的基因表达。一旦建立了DMR,它们就有可能承受细胞分化过程中发生的正常基因组重编程事件,并且在整个发育过程中稳定地维持种系DMR。这些DMR除在母体或父体中被甲基化外,在种系中还是在受精后都获得甲基化方面也存在差异,并且存在于具有不同胞嘧啶-磷酸鸟嘌呤(CpG)密度和CTCF结合的各种基因组位置能力。因此,我们检查了DNA甲基化印记维持的稳定性,并确定了所有印记基因在几个成年组织中的正常基线DNA甲基化水平。为此,我们首先开发和验证了50种高度特异性的,定量的DNA甲基化焦磷酸测序分析方法,用于与人类印迹基因相关的已知DMR。

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