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RA 诱导分化的 NT2 细胞在贴壁和非贴壁培养条件下 Oct4 调控区的比较表观遗传学分析。

Comparative epigenetic analysis of Oct4 regulatory region in RA-induced differentiated NT2 cells under adherent and non-adherent culture conditions.

机构信息

Department of Genetics, Reproductive Biomedicine Center, Royan Institute for Reproductive Biomedicine, ACECR, P.O. Box 19395-4644, Tehran, Iran.

出版信息

Mol Cell Biochem. 2012 Apr;363(1-2):129-34. doi: 10.1007/s11010-011-1165-y. Epub 2011 Dec 9.

DOI:10.1007/s11010-011-1165-y
PMID:22160855
Abstract

Oct4 is a POU domain homeobox gene, expressed in undifferentiated embryonal carcinoma and embryonic stem cells and is quickly down-regulated upon induction of differentiation. Transcriptional repression of Oct4 is followed by pronounced epigenetic changes on the regulatory region of the gene. Oct4 has a long upstream regulatory region of about 2,600 bp, consisting of proximal enhancer (PE), distal enhancer (DE), and proximal promoter (PP). In this study, we induced differentiation of a human embryonic carcinoma cell line, NT2, under two different adherent and non-adherent culture conditions, and compared histone modifications as the epigenetic marks on the regulatory region of Oct4 gene after 3 days of differentiation. Using chromatin immunoprecipitation coupled with real-time PCR technique, it was shown that the after induction of differentiation the repressive epigenetic marks of hypoacetylation and methylation on lysine-9 of histone H3 occurred very effectively on the upstream of Oct4, especially in PP region. Also, comparing the two culturing systems it was shown that methylation of lysine-9 of H3 histone was more drastic in PE region of adherent cells rather than suspension cells. This epigenetic profile was in agreement with the difference observed in the expression level of Oct4 in these two culturing systems. The current study clearly shows the effective role of cell culture condition on the epigenetic regulation of gene expression.

摘要

Oct4 是一个 POU 结构域同源盒基因,在未分化的胚胎癌细胞和胚胎干细胞中表达,并在诱导分化时迅速下调。Oct4 的转录抑制伴随着基因调控区明显的表观遗传变化。Oct4 具有约 2600bp 的长上游调控区,包括近端增强子(PE)、远端增强子(DE)和近端启动子(PP)。在这项研究中,我们在两种不同的贴壁和非贴壁培养条件下诱导人类胚胎癌细胞系 NT2 的分化,并在分化 3 天后比较了 Oct4 基因调控区的组蛋白修饰作为表观遗传标记。使用染色质免疫沉淀结合实时 PCR 技术,结果表明,分化诱导后,Oct4 上游的组蛋白 H3 赖氨酸 9 的去乙酰化和甲基化等抑制性表观遗传标记非常有效,尤其是在 PP 区域。此外,比较两种培养系统表明,在贴壁细胞而非悬浮细胞的 PE 区域,H3 组蛋白赖氨酸 9 的甲基化更为剧烈。这种表观遗传特征与这两种培养系统中观察到的 Oct4 表达水平的差异一致。本研究清楚地表明细胞培养条件对基因表达的表观遗传调控有明显的作用。

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