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在明确的蛋白质体系和 E. coli topA 突变株中,转录偶联的 DNA 超螺旋。

Transcription-coupled DNA supercoiling in defined protein systems and in E. coli topA mutant strains.

机构信息

Department of Chemistry and Biochemistry, Florida International University, FL 33199, USA.

出版信息

IUBMB Life. 2013 Jul;65(7):615-22. doi: 10.1002/iub.1179. Epub 2013 Jun 12.

DOI:10.1002/iub.1179
PMID:23757201
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC5992920/
Abstract

Transcription by RNA polymerases can stimulate (-) DNA supercoiling both in vitro and in Escherichia coli topA strains. This phenomenon has been successfully explained by a "twin-supercoiled-domain" model of transcription in which (+) supercoils are produced in front of the transcribing RNA polymerase and (-) supercoils behind it. Previously, it has been shown that certain sequence-specific DNA-binding proteins potently stimulate transcription-coupled DNA supercoiling (TCDS) in an in vitro protein system. These results are consistent with a topological barrier model where certain nucleoprotein complexes can form topological barriers that impede the diffusion and merger of independent chromosomal supercoil domains. Indeed, recent biochemical and single-molecule results demonstrated the existence of nucleoprotein-based DNA topological barriers, which are capable of dividing a DNA molecule into different topological domains. Additionally, recent in vivo studies showed that a transcriptional ensemble (including the transcribing RNA polymerase and the RNA transcript) alone is sufficient to cause a change in local DNA superhelicity. This topological change in local chromosome structure should have a great impact on the conformation and function of critical DNA sequence elements, such as promoters and DNA replication origins. In this article, we will also review recent progress by which TCDS is a critical stimulating force to activate transcription initiation from weak promoters, such as the Salmonella typhimurium leu-500 promoter.

摘要

RNA 聚合酶转录可以在体外和大肠杆菌 topA 菌株中刺激 (-) DNA 超螺旋。这一现象已经通过“双超螺旋域”转录模型得到了成功解释,该模型认为 (+) 超螺旋在前转录 RNA 聚合酶处产生,(-) 超螺旋在其后产生。先前的研究表明,某些序列特异性 DNA 结合蛋白在体外蛋白系统中能够强烈刺激转录偶联的 DNA 超螺旋化 (TCDS)。这些结果与拓扑障碍模型一致,即某些核蛋白复合物可以形成拓扑障碍,阻碍独立染色质超螺旋域的扩散和合并。事实上,最近的生化和单分子研究结果证明了基于核蛋白的 DNA 拓扑障碍的存在,这些障碍能够将 DNA 分子划分为不同的拓扑域。此外,最近的体内研究表明,转录复合物(包括正在转录的 RNA 聚合酶和 RNA 转录本)本身足以引起局部 DNA 超螺旋性的变化。局部染色体结构的这种拓扑变化应该对关键 DNA 序列元件(如启动子和 DNA 复制起始点)的构象和功能产生重大影响。在本文中,我们还将回顾 TCDS 作为一种关键的刺激力量,如何激活弱启动子(如鼠伤寒沙门氏菌 leu-500 启动子)转录起始的最新进展。

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Dependence of transcription-coupled DNA supercoiling on promoter strength in Escherichia coli topoisomerase I deficient strains.转录偶联的 DNA 超螺旋对大肠杆菌拓扑异构酶 I 缺陷菌株中启动子强度的依赖性。
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