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A three-step pathway of transcription initiation leading to promoter clearance at an activation RNA polymerase II promoter.

机译:转录起始的三步途径导致激活RNA聚合酶II启动子清除启动子。

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摘要

The progress of transcription bubbles during inhibition in vitro was followed in order to learn how RNA polymerase II begins transcription at the activated adenovirus E4 promoter. The issues addressed include the multiple roles of ATP, the potential effect of polymerase C-terminal domain phosphorylation, and the ability of polymerase to clear the promoter for reinitiation. The results lead to a three-step model for the transition from closed complex to elongation complex, two steps of which use ATP independently. In the first step, studied previously, ATP is hydrolyzed to open the DNA strands over the start site. In a second step, apparently independent of ATP, transcription bubbles move into the initial transcribed region where RNA synthesis can stall. In the third step, transcripts can be made as polymerase is released from these stalled positions with the assistance of an ATP-dependent process, likely phosphorylation of the polymerase C-terminal domain. After this third step, the promoter becomes cleared, allowing for the reinitiation of transcription.
机译:为了了解RNA聚合酶II如何在活化的腺病毒E4启动子处开始转录,追踪了体外抑制过程中转录气泡的进展。解决的问题包括ATP的多种作用,聚合酶C末端结构域磷酸化的潜在作用以及聚合酶清除启动子以重新启动的能力。结果导致从封闭复合物到伸长复合物的转变的三步模型,其中两步独立地使用ATP。在先前研究的第一步中,将ATP水解以在起始位点上打开DNA链。在第二个步骤中,转录气泡显然独立于ATP,移动到最初转录的区域,RNA合成可能在那里停滞。在第三步中,可以在依赖于ATP的过程(可能是聚合酶C末端结构域的磷酸化)的帮助下,从这些停滞的位置释放聚合酶,从而生成转录本。第三步之后,启动子被清除,从而允许转录的重新初始化。

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