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激活处于暂停状态的依赖 RNA 聚合酶 II 的启动子需要 SAGA 和中介体。

Activation of a poised RNAPII-dependent promoter requires both SAGA and mediator.

机构信息

Department of Biochemistry and Molecular Biology, Colorado State University, Fort Collins, Colorado 80523, USA.

出版信息

Genetics. 2010 Mar;184(3):659-72. doi: 10.1534/genetics.109.113464. Epub 2010 Jan 4.

Abstract

A growing number of promoters have key components of the transcription machinery, such as TATA-binding protein (TBP) and RNA polymerase II (RNAPII), present at the promoter prior to activation of transcription. Thus, while transcriptional output undergoes a dramatic increase between uninduced and induced conditions, occupancy of a large portion of the transcription machinery does not. As such, activation of these poised promoters depends on rate-limiting steps after recruitment of TBP and RNAPII for regulated expression. Little is known about the transcription components required in these latter steps of transcription in vivo. To identify components with critical roles in transcription after recruitment of TBP in Saccharomyces cerevisiae, we screened for loss of gene expression activity from promoter-tethered TBP in >100 mutant strains deleted for a transcription-related gene. The assay revealed a dramatic enrichment for strains containing deletions in genes encoding subunits of the Spt-Ada-Gcn5-acetyltransferase (SAGA) complex and Mediator. Analysis of an authentic postrecruitment-regulated gene (CYC1) reveals that SAGA occupies the promoter under both uninduced and induced conditions. In contrast, Mediator is recruited only after transfer to inducing conditions and correlates with activation of the preloaded polymerase at CYC1. These studies indicate the critical functions of SAGA and Mediator in the mechanism of activation of genes with rate-limiting steps after recruitment of TBP.

摘要

越来越多的启动子在转录激活之前就有转录机器的关键成分,如 TATA 结合蛋白 (TBP) 和 RNA 聚合酶 II (RNAPII),存在于启动子上。因此,虽然转录产物在未诱导和诱导条件下会发生显著增加,但大部分转录机器的占据并不增加。因此,这些处于静止状态的启动子的激活取决于 TBP 和 RNAPII 募集后的限速步骤,以进行调节表达。对于体内这些转录后步骤所需的转录成分知之甚少。为了在酿酒酵母中鉴定 TBP 募集后转录中具有关键作用的成分,我们筛选了 >100 种转录相关基因缺失的突变株中,从启动子连接的 TBP 上失去基因表达活性的情况。该测定方法对编码 Spt-Ada-Gcn5-乙酰转移酶 (SAGA) 复合物和 Mediator 亚基的基因缺失的菌株进行了显著富集。对一个真实的募集后调节基因 (CYC1) 的分析表明,SAGA 在未诱导和诱导条件下都占据启动子。相比之下,Mediator 仅在转移到诱导条件后才被募集,并且与预加载聚合酶在 CYC1 上的激活相关。这些研究表明,SAGA 和 Mediator 在 TBP 募集后的限速步骤基因激活机制中具有关键功能。

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