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对酿酒酵母中聚合酶II的一个亚基Rpb4进行全基因组募集分析,揭示了其在转录延伸中的作用。

Genomewide recruitment analysis of Rpb4, a subunit of polymerase II in Saccharomyces cerevisiae, reveals its involvement in transcription elongation.

作者信息

Verma-Gaur Jiyoti, Rao Sudha Narayana, Taya Toshiki, Sadhale Parag

机构信息

Department of Microbiology and Cell biology, Indian Institute of Science, Bangalore 560 012, India.

出版信息

Eukaryot Cell. 2008 Jun;7(6):1009-18. doi: 10.1128/EC.00057-08. Epub 2008 Apr 25.

Abstract

The Rpb4/Rpb7 subcomplex of yeast RNA polymerase II (Pol II) has counterparts in all multisubunit RNA polymerases from archaebacteria to higher eukaryotes. The Rpb4/7 subcomplex in Saccharomyces cerevisiae is unique in that it easily dissociates from the core, unlike the case in other organisms. The relative levels of Rpb4 and Rpb7 in yeasts affect the differential gene expression and stress response. Rpb4 is nonessential in S. cerevisiae and affects expression of a small number of genes under normal growth conditions. Here, using a chromatin immunoprecipitation ("ChIP on-chip") technique, we compared genomewide binding of Rpb4 to that of a core Pol II subunit, Rpb3. Our results showed that in spite of being nonessential for survival, Rpb4 was recruited on coding regions of most transcriptionally active genes, similar to the case with the core Pol II subunit, Rpb3, albeit to a lesser extent. The extent of Rpb4 recruitment increased with increasing gene length. We also observed Pol II lacking Rpb4 to be defective in transcribing long, GC-rich transcription units, suggesting a role for Rpb4 in transcription elongation. This role in transcription elongation was supported by the observed 6-azauracil (6AU) sensitivity of the rpb4Delta mutant. Unlike most phenotypes of rpb4Delta, the 6AU sensitivity of the rpb4Delta strain was not rescued by overexpression of RPB7. This report provides the first instance of a distinct role for Rpb4 in transcription, which is independent of its interacting partner, Rpb7.

摘要

酵母RNA聚合酶II(Pol II)的Rpb4/Rpb7亚复合物在从古细菌到高等真核生物的所有多亚基RNA聚合酶中都有对应物。酿酒酵母中的Rpb4/7亚复合物很独特,因为它很容易从核心解离,这与其他生物体的情况不同。酵母中Rpb4和Rpb7的相对水平影响基因的差异表达和应激反应。Rpb4在酿酒酵母中不是必需的,并且在正常生长条件下影响少数基因的表达。在这里,我们使用染色质免疫沉淀(“芯片上的ChIP”)技术,比较了Rpb4与核心Pol II亚基Rpb3在全基因组范围内的结合情况。我们的结果表明,尽管Rpb4对生存不是必需的,但它与核心Pol II亚基Rpb3一样,被募集到大多数转录活跃基因的编码区域,尽管程度较小。Rpb4的募集程度随着基因长度的增加而增加。我们还观察到缺乏Rpb4的Pol II在转录长的、富含GC的转录单元时存在缺陷,这表明Rpb4在转录延伸中发挥作用。rpb4Delta突变体对6-氮杂尿嘧啶(6AU)的敏感性支持了其在转录延伸中的作用。与rpb4Delta的大多数表型不同,rpb4Delta菌株对6AU的敏感性不能通过过表达RPB7来挽救。本报告首次揭示了Rpb4在转录中具有独立于其相互作用伙伴Rpb7的独特作用。

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