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Real-time observation of the transition from transcription initiation to elongation of the RNA polymerase

机译:实时观察从转录起始到RNA聚合酶延伸的过渡

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摘要

The transition from initiation to elongation of the RNA polymerase (RNAP) is an important stage of transcription that often limits the production of the full-length RNA. Little is known about the RNAP transition kinetics and the steps that dictate the transition rate, because of the challenge in monitoring subpopulations of the transient and heterogeneous transcribing complexes in rapid and real time. Here, we have dissected the complete transcription initiation pathway of T7 RNAP by using kinetic modeling of RNA synthesis and by determining the initiation (IC) to elongation (EC) transition kinetics at each RNA polymerization step using single-molecule and stopped-flow FRET methods. We show that the conversion of IC to EC in T7 RNAP consensus promoter occurs only after 8- to 12-nt synthesis, and the 12-nt synthesis represents a critical juncture in the transcriptional initiation pathway when EC formation is most efficient. We show that the slow steps of transcription initiation, including DNA scrunching/RNAP–promoter rotational changes during 5- to 8-nt synthesis, not the major conformational changes, dictate the overall rate of EC formation in T7 RNAP and represent key steps that regulate the synthesis of full-length RNA.
机译:RNA聚合酶(RNAP)从起始到伸长的过渡是重要的转录阶段,通常会限制全长RNA的产生。对于RNAP过渡动力学和决定过渡速率的步骤知之甚少,因为在快速,实时地监测瞬时和异源转录复合物的亚群方面存在挑战。在这里,我们通过使用RNA合成的动力学模型并通过使用单分子和停流FRET方法确定每个RNA聚合步骤中起始(IC)到伸长(EC)转变动力学的方式,来剖析T7 RNAP的完整转录起始途径。 。我们表明,IC到T7 RNAP共有启动子中的EC的转换仅在8至12-nt合成后发生,而12-nt合成代表了EC形成最有效时转录起始途径中的关键时刻。我们显示,转录起始的缓慢步骤(包括5至8 nt合成过程中的DNA收缩/ RNAP-启动子旋转变化,而不是主要构象变化)决定了T7 RNAP中EC形成的总体速率,并代表了调节全长RNA的合成。

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