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肌细胞生成素位点特异性去甲基化的动态变化与其表达以及肌肉分化密切相关。

The dynamics of myogenin site-specific demethylation is strongly correlated with its expression and with muscle differentiation.

作者信息

Lucarelli M, Fuso A, Strom R, Scarpa S

机构信息

Department of Cellular Biotechnologies and Hematology and I Department of Surgery, University of Rome "La Sapienza," Rome, Italy.

出版信息

J Biol Chem. 2001 Mar 9;276(10):7500-6. doi: 10.1074/jbc.M008234200. Epub 2000 Nov 28.

DOI:10.1074/jbc.M008234200
PMID:11096088
Abstract

The molecular mechanisms underlying the activation of tissue-specific genes have not yet been fully clarified. We analyzed the methylation status of specific CCGG sites in the 5'-flanking region and exon 1 of myogenin gene, a very important myogenic differentiation factor. We demonstrated a loss of methylation, at the onset of C2C12 muscle cell line differentiation, limited to the CCGG site of myogenin 5'-flanking region, which was strongly correlated with the transcriptional activation of this gene and with myogenic differentiation. The same CCGG site was also found to be hypomethylated, in vivo, in embryonic mouse muscle (a myogenin-expressing tissue), as opposed to nonmuscle (nonexpressing) tissues that had a fully methylated site. In a C2C12-derived clone with enhanced myogenic ability, demethylation occurred within 2 h of induction of differentiation, suggesting the involvement of some active demethylation mechanism(s) that occur in the absence of DNA replication. Exposure to drugs that inhibit DNA methylation by acting on the S-adenosylmethionine metabolism produced a further reduction, to a few minutes, in the duration of the demethylation dynamics. These effects suggest that the final site-specific DNA methylation pattern of tissue-specific genes is defined through a continuous, relatively fast interplay between active DNA demethylation and re-methylation mechanisms.

摘要

组织特异性基因激活背后的分子机制尚未完全阐明。我们分析了肌细胞生成素基因(一种非常重要的肌源性分化因子)5'-侧翼区域和外显子1中特定CCGG位点的甲基化状态。我们证明,在C2C12肌肉细胞系分化开始时,甲基化缺失仅限于肌细胞生成素5'-侧翼区域的CCGG位点,这与该基因的转录激活和肌源性分化密切相关。在体内,相同的CCGG位点在胚胎小鼠肌肉(一个表达肌细胞生成素的组织)中也被发现是低甲基化的,与之形成对比的是,非肌肉(不表达)组织中的该位点是完全甲基化的。在一个具有增强肌源性能力的C2C12衍生克隆中,去甲基化在诱导分化后2小时内发生,这表明在没有DNA复制的情况下,存在一些活跃的去甲基化机制。暴露于通过作用于S-腺苷甲硫氨酸代谢来抑制DNA甲基化的药物,使去甲基化动力学的持续时间进一步缩短至几分钟。这些效应表明,组织特异性基因最终的位点特异性DNA甲基化模式是通过活跃的DNA去甲基化和重新甲基化机制之间持续、相对快速的相互作用来定义的。

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