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B型组蛋白乙酰转移酶Hat1p募集至染色质与DNA双链断裂有关。

Recruitment of the type B histone acetyltransferase Hat1p to chromatin is linked to DNA double-strand breaks.

作者信息

Qin Song, Parthun Mark R

机构信息

Department of Molecular and Cellular Biochemistry, The Ohio State University, Columbus, Ohio 43210, USA.

出版信息

Mol Cell Biol. 2006 May;26(9):3649-58. doi: 10.1128/MCB.26.9.3649-3658.2006.

DOI:10.1128/MCB.26.9.3649-3658.2006
PMID:16612003
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC1447429/
Abstract

Type B histone acetyltransferases are thought to catalyze the acetylation of the NH(2)-terminal tails of newly synthesized histones. Although Hat1p has been implicated in cellular processes, such as telomeric silencing and DNA damage repair, the underlying molecular mechanisms by which it functions remain elusive. In an effort to understand how Hat1p is involved in the process of DNA double-strand break (DSB) repair, we examined whether Hat1p is directly recruited to sites of DNA damage. Following induction of the endonuclease HO, which generates a single DNA DSB at the MAT locus, we found that Hat1p becomes associated with chromatin near the site of DNA damage. The nuclear Hat1p-associated histone chaperone Hif1p is also recruited to an HO-induced DSB with a similar distribution. In addition, while the acetylation of all four histone H4 NH(2)-terminal tail domain lysine residues is increased following DSB formation, only the acetylation of H4 lysine 12, the primary target of Hat1p activity, is dependent on the presence of Hat1p. Kinetic analysis of Hat1p localization indicates that it is recruited after the phosphorylation of histone H2A S129 and concomitant with the recombinational-repair factor Rad52p. Surprisingly, Hat1p is still recruited to chromatin in strains that cannot repair an HO-induced double-strand break. These results indicate that Hat1p plays a direct role in DNA damage repair and is responsible for specific changes in histone modification that occur during the course of recombinational DNA repair.

摘要

B型组蛋白乙酰转移酶被认为可催化新合成组蛋白氨基末端尾巴的乙酰化反应。尽管Hat1p与细胞过程有关,如端粒沉默和DNA损伤修复,但其发挥作用的潜在分子机制仍不清楚。为了了解Hat1p如何参与DNA双链断裂(DSB)修复过程,我们研究了Hat1p是否直接被招募到DNA损伤位点。在内切核酸酶HO诱导后,其在MAT基因座产生单个DNA DSB,我们发现Hat1p与DNA损伤位点附近的染色质相关联。核内与Hat1p相关的组蛋白伴侣Hif1p也以类似的分布被招募到HO诱导的DSB处。此外,虽然在DSB形成后所有四个组蛋白H4氨基末端尾巴结构域赖氨酸残基的乙酰化都增加了,但只有H4赖氨酸12(Hat1p活性的主要靶点)的乙酰化依赖于Hat1p的存在。Hat1p定位的动力学分析表明,它在组蛋白H2A S129磷酸化后被招募,并与重组修复因子Rad52p同时出现。令人惊讶的是,Hat1p在无法修复HO诱导的双链断裂的菌株中仍被招募到染色质上。这些结果表明,Hat1p在DNA损伤修复中起直接作用,并负责重组DNA修复过程中发生的组蛋白修饰的特定变化。

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Distinct roles for the RSC and Swi/Snf ATP-dependent chromatin remodelers in DNA double-strand break repair.RSC和Swi/Snf ATP依赖的染色质重塑因子在DNA双链断裂修复中的不同作用。
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