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如何开启马达:单分子水平下的RNA聚合酶起始步骤。

How to switch the motor on: RNA polymerase initiation steps at the single-molecule level.

作者信息

Marchetti M, Malinowska A, Heller I, Wuite G J L

机构信息

Department of Physics and Astronomy and LaserLaB Amsterdam, Vrije Universiteit Amsterdam, Amsterdam, The Netherlands.

出版信息

Protein Sci. 2017 Jul;26(7):1303-1313. doi: 10.1002/pro.3183. Epub 2017 May 12.

DOI:10.1002/pro.3183
PMID:28470684
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC5477531/
Abstract

RNA polymerase (RNAP) is the central motor of gene expression since it governs the process of transcription. In prokaryotes, this holoenzyme is formed by the RNAP core and a sigma factor. After approaching and binding the specific promoter site on the DNA, the holoenzyme-promoter complex undergoes several conformational transitions that allow unwinding and opening of the DNA duplex. Once the first DNA basepairs (∼10 bp) are transcribed in an initial transcription process, the enzyme unbinds from the promoter and proceeds downstream along the DNA while continuously opening the helix and polymerizing the ribonucleotides in correspondence with the template DNA sequence. When the gene is transcribed into RNA, the process generally is terminated and RNAP unbinds from the DNA. The first step of transcription-initiation, is considered the rate-limiting step of the entire process. This review focuses on the single-molecule studies that try to reveal the key steps in the initiation phase of bacterial transcription. Such single-molecule studies have, for example, allowed real-time observations of the RNAP target search mechanism, a mechanism still under debate. Moreover, single-molecule studies using Förster Resonance Energy Transfer (FRET) revealed the conformational changes that the enzyme undergoes during initiation. Force-based techniques such as scanning force microscopy and magnetic tweezers allowed quantification of the energy that drives the RNAP translocation along DNA and its dynamics. In addition to these in vitro experiments, single particle tracking in vivo has provided a direct quantification of the relative populations in each phase of transcription and their locations within the cell.

摘要

RNA聚合酶(RNAP)是基因表达的核心动力,因为它掌控着转录过程。在原核生物中,这种全酶由RNAP核心和一个σ因子组成。在接近并结合DNA上的特定启动子位点后,全酶-启动子复合物会经历几次构象转变,从而使DNA双链解旋并打开。一旦在初始转录过程中转录出前10个左右的DNA碱基对,酶就会从启动子上解离,并沿着DNA向下游移动,同时持续打开螺旋并根据模板DNA序列聚合核糖核苷酸。当基因转录为RNA时,该过程通常会终止,RNAP也会从DNA上解离。转录起始的第一步被认为是整个过程的限速步骤。本综述聚焦于试图揭示细菌转录起始阶段关键步骤的单分子研究。例如,此类单分子研究使得实时观察RNAP的靶标搜索机制成为可能,而该机制仍存在争议。此外,利用荧光共振能量转移(FRET)的单分子研究揭示了酶在起始过程中所经历的构象变化。诸如扫描力显微镜和磁镊等基于力的技术能够对驱动RNAP沿DNA转位的能量及其动力学进行量化。除了这些体外实验,体内单粒子追踪还能直接量化转录各阶段的相对群体数量及其在细胞内的位置。

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本文引用的文献

1
Backtracked and paused transcription initiation intermediate of Escherichia coli RNA polymerase.大肠杆菌RNA聚合酶的回溯与暂停转录起始中间体
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RNA Polymerase Pausing during Initial Transcription.初始转录过程中的RNA聚合酶暂停
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Local and global regulation of transcription initiation in bacteria.细菌中转录起始的局部和全局调控。
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Single molecule microscopy reveals mechanistic insight into RNA polymerase II preinitiation complex assembly and transcriptional activity.单分子显微镜揭示了对RNA聚合酶II预起始复合物组装和转录活性的机制性见解。
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Live-cell superresolution microscopy reveals the organization of RNA polymerase in the bacterial nucleoid.活细胞超分辨率显微镜揭示了细菌类核中RNA聚合酶的组织方式。
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Structural basis of transcription initiation by bacterial RNA polymerase holoenzyme.细菌RNA聚合酶全酶转录起始的结构基础
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