Transcriptional repression by the methyl-CpG-binding protein MeCP2 involves a histone deacetylase complex

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作者
Xinsheng Nan
Huck-Hui Ng
Colin A. Johnson
Carol D. Laherty
Bryan M. Turner
Robert N. Eisenman
Adrian Bird
机构
[1] Institute of Cell and Molecular Biology,Department of Anatomy
[2] University of Edinburgh,Division of Basic Sciences
[3] The Medical School,undefined
[4] University of Birmingham,undefined
[5] Fred Hutchinson Cancer Research Center,undefined
来源
Nature | 1998年 / 393卷
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摘要
Cytosine residues in the sequence 5′CpG (cytosine–guanine) are often postsynthetically methylated in animal genomes. CpG methylation is involved in long-term silencing of certain genes during mammalian development1,2 and in repression of viral genomes3,4. The methyl-CpG-binding proteins MeCP1 (ref. 5) and MeCP2 (ref. 6) interact specifically with methylated DNA and mediate transcriptional repression7,8,9. Here we study the mechanism of repression by MeCP2, an abundant nuclear protein that is essential for mouse embryogenesis10. MeCP2 binds tightly to chromosomes in a methylation-dependent manner11,12. It contains a transcriptional-repression domain (TRD) that can function at a distance in vitro and in vivo9. We show that a region of MeCP2 that localizes with the TRD associates with a corepressor complex containing the transcriptional repressor mSin3A and histone deacetylases13,14,15,16,17,18,19. Transcriptional repression in vivo is relieved by the deacetylase inhibitor trichostatin A20, indicating that deacetylation of histones (and/or of other proteins) is an essential component of this repression mechanism. The data suggest that two global mechanisms of gene regulation, DNA methylation and histone deacetylation, can be linked by MeCP2.
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页码:386 / 389
页数:3
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