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影响酿酒酵母中CHA1启动子转录抑制和染色质结构的组蛋白H3中的分散突变。

Dispersed mutations in histone H3 that affect transcriptional repression and chromatin structure of the CHA1 promoter in Saccharomyces cerevisiae.

作者信息

He Qiye, Yu Cailin, Morse Randall H

机构信息

Department of Biomedical Sciences, State University of New York at Albany School of Public Health, Wadsworth Center, Albany, NY 12201-2002, USA.

出版信息

Eukaryot Cell. 2008 Oct;7(10):1649-60. doi: 10.1128/EC.00233-08. Epub 2008 Jul 25.

Abstract

The histone H3 amino terminus, but not that of H4, is required to prevent the constitutively bound activator Cha4 from remodeling chromatin and activating transcription at the CHA1 gene in Saccharomyces cerevisiae. Here we show that neither the modifiable lysine residues nor any specific region of the H3 tail is required for repression of CHA1. We then screened for histone H3 mutations that cause derepression of the uninduced CHA1 promoter and identified six mutants, three of which are also temperature-sensitive mutants and four of which exhibit a sin(-) phenotype. Histone mutant levels were similar to that of wild-type H3, and the mutations did not cause gross alterations in nucleosome structure. One specific and strongly derepressing mutation, H3 A111G, was examined in depth and found to cause a constitutively active chromatin configuration at the uninduced CHA1 promoter as well as at the ADH2 promoter. Transcriptional derepression and altered chromatin structure of the CHA1 promoter depend on the activator Cha4. These results indicate that modest perturbations in distinct regions of the nucleosome can substantially affect the repressive function of chromatin, allowing activation in the absence of a normal inducing signal (at CHA1) or of Swi/Snf (resulting in a sin(-) phenotype).

摘要

在酿酒酵母中,为了防止组成型结合的激活因子Cha4重塑染色质并激活CHA1基因的转录,需要组蛋白H3的氨基末端,但不需要H4的氨基末端。我们在此表明,抑制CHA1既不需要可修饰的赖氨酸残基,也不需要H3尾巴的任何特定区域。然后,我们筛选了导致未诱导的CHA1启动子去抑制的组蛋白H3突变体,并鉴定出六个突变体,其中三个也是温度敏感突变体,四个表现出sin(-)表型。组蛋白突变体水平与野生型H3相似,并且这些突变不会导致核小体结构的明显改变。我们深入研究了一个特定且强烈去抑制的突变体H3 A111G,发现它在未诱导的CHA1启动子以及ADH2启动子处导致组成型活性染色质构型。CHA1启动子的转录去抑制和染色质结构改变依赖于激活因子Cha4。这些结果表明,核小体不同区域的适度扰动可显著影响染色质的抑制功能,从而在没有正常诱导信号(在CHA1处)或没有Swi/Snf的情况下允许激活(导致sin(-)表型)。

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