Gdown1 与人类基因上 RNA 聚合酶 II 预定位点的功能关联。
Functional association of Gdown1 with RNA polymerase II poised on human genes.
机构信息
Molecular and Cellular Biology Program, University of Iowa, Iowa City, IA 52242, USA.
出版信息
Mol Cell. 2012 Jan 13;45(1):38-50. doi: 10.1016/j.molcel.2011.10.022.
Abstract
Most human genes are loaded with promoter-proximally paused RNA polymerase II (Pol II) molecules that are poised for release into productive elongation by P-TEFb. We present evidence that Gdown1, the product of the POLR2M gene that renders Pol II responsive to Mediator, is involved in Pol II elongation control. During in vitro transcription, Gdown1 specifically blocked elongation stimulation by TFIIF, inhibited the termination activity of TTF2, and influenced pausing factors NELF and DSIF, but did not affect the function of TFIIS or the mRNA capping enzyme. Without P-TEFb, Gdown1 led to the production of stably paused polymerases in the presence of nuclear extract. Supporting these mechanistic insights, ChIP-Seq demonstrated that Gdown1 mapped over essentially all poised polymerases across the human genome. Our results establish that Gdown1 stabilizes poised polymerases while maintaining their responsiveness to P-TEFb and suggest that Mediator overcomes a Gdown1-mediated block of initiation by allowing TFIIF function.
摘要
大多数人类基因都携带着靠近启动子的 RNA 聚合酶 II(Pol II)分子,这些分子准备被 P-TEFb 释放到有效的延伸中。我们提供的证据表明,POLR2M 基因的产物 Gdown1 参与了 Pol II 延伸控制,该基因使 Pol II 对中介体产生反应。在体外转录过程中,Gdown1 特异性地阻断了 TFIIF 对延伸的刺激,抑制了 TTF2 的终止活性,并影响了暂停因子 NELF 和 DSIF,但不影响 TFIIS 或 mRNA 加帽酶的功能。没有 P-TEFb 的情况下,Gdown1 在核提取物存在的情况下导致稳定暂停的聚合酶的产生。支持这些机制见解的是,ChIP-Seq 表明 Gdown1 映射到人类基因组中几乎所有的暂停聚合酶上。我们的结果表明,Gdown1 稳定了暂停的聚合酶,同时保持了它们对 P-TEFb 的反应性,并表明中介体通过允许 TFIIF 功能克服了 Gdown1 介导的起始阻断。
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