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RecQ解旋酶的单分子可视化显示,进行性DNA解旋需要DNA解链、成核和组装。

Single-molecule visualization of RecQ helicase reveals DNA melting, nucleation, and assembly are required for processive DNA unwinding.

作者信息

Rad Behzad, Forget Anthony L, Baskin Ronald J, Kowalczykowski Stephen C

机构信息

Department of Microbiology and Molecular Genetics, University of California, Davis, CA 95616-8665; Department of Molecular and Cellular Biology, University of California, Davis, CA 95616-8665; Biophysics Graduate Group, University of California, Davis, CA 95616-8665.

Department of Microbiology and Molecular Genetics, University of California, Davis, CA 95616-8665; Department of Molecular and Cellular Biology, University of California, Davis, CA 95616-8665;

出版信息

Proc Natl Acad Sci U S A. 2015 Dec 15;112(50):E6852-61. doi: 10.1073/pnas.1518028112. Epub 2015 Nov 4.

Abstract

DNA helicases are motor proteins that unwind double-stranded DNA (dsDNA) to reveal single-stranded DNA (ssDNA) needed for many biological processes. The RecQ helicase is involved in repairing damage caused by DNA breaks and stalled replication forks via homologous recombination. Here, the helicase activity of RecQ was visualized on single molecules of DNA using a fluorescent sensor that directly detects ssDNA. By monitoring the formation and progression of individual unwinding forks, we observed that both the frequency of initiation and the rate of unwinding are highly dependent on RecQ concentration. We establish that unwinding forks can initiate internally by melting dsDNA and can proceed in both directions at up to 40-60 bp/s. The findings suggest that initiation requires a RecQ dimer, and that continued processive unwinding of several kilobases involves multiple monomers at the DNA unwinding fork. We propose a distinctive model wherein RecQ melts dsDNA internally to initiate unwinding and subsequently assembles at the fork into a distribution of multimeric species, each encompassing a broad distribution of rates, to unwind DNA. These studies define the species that promote resection of DNA, proofreading of homologous pairing, and migration of Holliday junctions, and they suggest that various functional forms of RecQ can be assembled that unwind at rates tailored to the diverse biological functions of RecQ helicase.

摘要

DNA解旋酶是一种驱动蛋白,可解开双链DNA(dsDNA)以暴露出许多生物过程所需的单链DNA(ssDNA)。RecQ解旋酶通过同源重组参与修复由DNA断裂和停滞的复制叉造成的损伤。在此,使用直接检测ssDNA的荧光传感器在单分子DNA上观察到了RecQ的解旋酶活性。通过监测单个解旋叉的形成和进展,我们观察到起始频率和解旋速率都高度依赖于RecQ浓度。我们确定解旋叉可以通过使dsDNA解链在内部起始,并且可以以高达40 - 60 bp/s的速度双向进行。这些发现表明起始需要RecQ二聚体,并且数千碱基的持续进行性解旋涉及DNA解旋叉处的多个单体。我们提出了一个独特的模型,其中RecQ在内部使dsDNA解链以起始解旋,随后在叉处组装成多种多聚体形式的分布,每种形式都包含广泛的速率分布,以解开DNA。这些研究确定了促进DNA切除、同源配对校对和霍利迪连接迁移的物质,并且表明可以组装各种功能形式的RecQ,它们以适合RecQ解旋酶不同生物学功能的速率解旋。

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本文引用的文献

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Structural mechanisms of DNA binding and unwinding in bacterial RecQ helicases.细菌RecQ解旋酶中DNA结合与解旋的结构机制。
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Translocation of E. coli RecQ helicase on single-stranded DNA.大肠杆菌 RecQ 解旋酶在单链 DNA 上的转位。
Biochemistry. 2012 Apr 3;51(13):2921-9. doi: 10.1021/bi3000676. Epub 2012 Mar 21.
9
Efficient coupling of ATP hydrolysis to translocation by RecQ helicase.RecQ 解旋酶将 ATP 水解与转运的有效偶联。
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