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Distinct DNA methylation patterns characterize differentiated human embryonic stem cells and developing human fetal liver.

机译:不同的 DNA 甲基化模式表征了分化的人类胚胎干细胞和发育中的人类胎儿肝脏。

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摘要

To investigate the role of DNA methylation during human development, we developed Methyl-seq, a method that assays DNA methylation at more than 90,000 regions throughout the genome. Performing Methyl-seq on human embryonic stem cells (hESCs), their derivatives, and human tissues allowed us to identify several trends during hESC and in vivo liver differentiation. First, differentiation results in DNA methylation changes at a minimal number of assayed regions, both in vitro and in vivo (2-11). Second, in vitro hESC differentiation is characterized by both de novo methylation and demethylation, whereas in vivo fetal liver development is characterized predominantly by demethylation. Third, hESC differentiation is uniquely characterized by methylation changes specifically at H3K27me3-occupied regions, bivalent domains, and low density CpG promoters (LCPs), suggesting that these regions are more likely to be involved in transcriptional regulation during hESC differentiation. Although both H3K27me3-occupied domains and LCPs are also regions of high variability in DNA methylation state during human liver development, these regions become highly unmethylated, which is a distinct trend from that observed in hESCs. Taken together, our results indicate that hESC differentiation has a unique DNA methylation signature that may not be indicative of in vivo differentiation.
机译:为了研究DNA甲基化在人类发育过程中的作用,我们开发了Methyl-seq,这是一种在整个基因组中超过90,000个区域检测DNA甲基化的方法。对人类胚胎干细胞(hESCs)、其衍生物和人体组织进行甲基测序使我们能够确定hESC和体内肝脏分化过程中的几个趋势。首先,分化导致体外和体内(2%-11%)最小数量的测定区域的DNA甲基化变化。其次,体外hESC分化的特征是新甲基化和去甲基化,而体内胎儿肝脏发育的主要特征是去甲基化。第三,hESC 分化的独特特征是 H3K27me3 占据区域、二价结构域和低密度 CpG 启动子 (LCP) 的甲基化变化,表明这些区域更有可能参与 hESC 分化过程中的转录调控。尽管 H3K27me3 占据的结构域和 LCP 也是人类肝脏发育过程中 DNA 甲基化状态高度变异的区域,但这些区域变得高度非甲基化,这与在 hESC 中观察到的趋势截然不同。综上所述,我们的结果表明,hESC分化具有独特的DNA甲基化特征,这可能并不表示体内分化。

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