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INO80复合物与组蛋白伴侣之间的合作决定了酿酒酵母中应激基因转录的适应性。

Cooperation between the INO80 complex and histone chaperones determines adaptation of stress gene transcription in the yeast Saccharomyces cerevisiae.

作者信息

Klopf Eva, Paskova Ludmila, Solé Carme, Mas Gloria, Petryshyn Andriy, Posas Francesc, Wintersberger Ulrike, Ammerer Gustav, Schüller Christoph

机构信息

Department of Biochemistry and Cell Biology, Max F Perutz Laboratories, University of Vienna, Vienna, Austria.

出版信息

Mol Cell Biol. 2009 Sep;29(18):4994-5007. doi: 10.1128/MCB.01858-08. Epub 2009 Jul 20.

DOI:10.1128/MCB.01858-08
PMID:19620280
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC2738301/
Abstract

In yeast, environmental stresses provoke sudden and dramatic increases in gene expression at stress-inducible loci. Stress gene transcription is accompanied by the transient eviction of histones from the promoter and the transcribed regions of these genes. We found that mutants defective in subunits of the INO80 complex, as well as in several histone chaperone systems, exhibit extended expression windows that can be correlated with a distinct delay in histone redeposition during adaptation. Surprisingly, Ino80 became associated with the ORFs of stress genes in a stress-specific way, suggesting a direct function in the repression during adaptation. This recruitment required elongation by RNA polymerase (Pol) II but none of the histone modifications that are usually associated with active transcription, such as H3 K4/K36 methylation. A mutant lacking the Asf1-associated H3K56 acetyltransferase Rtt109 or Asf1 itself also showed enhanced stress-induced transcript levels. Genetic data, however, suggest that Asf1 and Rtt109 function in parallel with INO80 to restore histone homeostasis, whereas Spt6 seems to have a function that overlaps that of the chromatin remodeler. Thus, chromatin remodeling by INO80 in cooperation with Spt6 determines the shape of the expression profile under acute stress conditions, possibly by an elongation-dependent mechanism.

摘要

在酵母中,环境胁迫会引发应激诱导基因座处基因表达的突然显著增加。应激基因转录伴随着组蛋白从这些基因的启动子和转录区域的短暂移除。我们发现,INO80复合物亚基以及几个组蛋白伴侣系统存在缺陷的突变体表现出延长的表达窗口,这与适应过程中组蛋白重新沉积的明显延迟相关。令人惊讶的是,Ino80以应激特异性方式与应激基因的开放阅读框(ORF)相关联,这表明其在适应过程中的抑制作用具有直接功能。这种招募需要RNA聚合酶(Pol)II进行延伸,但不需要通常与活跃转录相关的任何组蛋白修饰,如H3 K4/K36甲基化。缺乏与Asf1相关的H3K56乙酰转移酶Rtt109或Asf1本身的突变体也表现出应激诱导转录水平增强。然而,遗传数据表明,Asf1和Rtt109与INO80并行发挥作用以恢复组蛋白稳态,而Spt6似乎具有与染色质重塑因子重叠的功能。因此,INO80与Spt6协同进行的染色质重塑可能通过一种依赖延伸的机制决定急性应激条件下表达谱的形状。

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本文引用的文献

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FACT and Asf1 regulate nucleosome dynamics and coactivator binding at the HO promoter.FACT和Asf1调节HO启动子处的核小体动力学及共激活因子结合。
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Chromatin- and transcription-related factors repress transcription from within coding regions throughout the Saccharomyces cerevisiae genome.染色质和转录相关因子在整个酿酒酵母基因组的编码区域内抑制转录。
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