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克隆猪中,甲基化的H3赖氨酸4或乙酰化的H3与乙酰化的H4的比例变化以及DNA甲基化与组织特异性基因表达相关。

Coordinated change of a ratio of methylated H3-lysine 4 or acetylated H3 to acetylated H4 and DNA methylation is associated with tissue-specific gene expression in cloned pig.

作者信息

Kang Jae-Ku, Park Kwang-Wook, Chung Yeon-Gu, You Jueng-Soo, Kim Yong-Kee, Lee Seung-Hyeon, Hong Seung-Pyo, Choi Ki-Myung, Heo Ki-Nam, Seol Jae-Goo, Lee Jong-Ho, Jin Dong-Il, Park Chang-Sik, Seo Jeong-Sun, Lee Hyang-Woo, Han Jeung-Whan

机构信息

Department of Biochemistry and Molecular Biology, College of Pharmacy, Sungkyunkwan University, Suwon 440-746, Korea.

出版信息

Exp Mol Med. 2007 Feb 28;39(1):84-96. doi: 10.1038/emm.2007.10.

DOI:10.1038/emm.2007.10
PMID:17334232
Abstract

Various cell types in higher multicellular organisms are genetically homogenous, but are functionally and morphologically heterogeneous due to the differential expression of genes during development, which appears to be controlled by epigenetic mechanisms. However, the exact molecular mechanisms that govern the tissue-specific gene expression are poorly understood. Here, we show that dynamic changes in histone modifications and DNA methylation in the upstream coding region of a gene containing the transcription initiation site determine the tissue-specific gene expression pattern. The tissue-specific expression of the transgene correlated with DNA demethylation at specific CpG sites as well as significant changes in histone modifications from a low ratio of methylated H3- lysine 4 or acetylated H3-lysine 9, 14 to acetylated H4 to higher ratios. Based on the programmed status of transgene silenced in cloned mammalian ear-derived fibroblasts, the transgene could be reprogrammed by change of histone modification and DNA methylation by inhibiting both histone deacetylase and DNA methylation, resulting in high expression of the transgene. These findings indicate that dynamic change of histone modification and DNA methylation is potentially important in the establishment and maintenance of tissue-specific gene expression.

摘要

高等多细胞生物中的各种细胞类型在基因上是同质的,但由于发育过程中基因的差异表达,它们在功能和形态上是异质的,而这种差异表达似乎受表观遗传机制控制。然而,调控组织特异性基因表达的确切分子机制仍知之甚少。在此,我们表明,在含有转录起始位点的基因的上游编码区,组蛋白修饰和DNA甲基化的动态变化决定了组织特异性基因表达模式。转基因的组织特异性表达与特定CpG位点的DNA去甲基化以及组蛋白修饰的显著变化相关,即从低比例的甲基化H3-赖氨酸4或乙酰化H3-赖氨酸9、14到乙酰化H4转变为更高比例。基于克隆的哺乳动物耳源成纤维细胞中转基因沉默的编程状态,通过抑制组蛋白脱乙酰酶和DNA甲基化,改变组蛋白修饰和DNA甲基化,转基因可以被重新编程,从而导致转基因的高表达。这些发现表明,组蛋白修饰和DNA甲基化的动态变化在组织特异性基因表达的建立和维持中可能具有重要意义。

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