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解析小角 X 射线散射(SAXS)研究来自耐辐射球菌的 RecQ 及其与连接 DNA 底物的复合物。

Solution small angle X-ray scattering (SAXS) studies of RecQ from Deinococcus radiodurans and its complexes with junction DNA substrates.

机构信息

From the Beijing Synchrotron Radiation Facility, Institute of High Energy Physics, Chinese Academy of Sciences, Beijing 100049, China.

the Department of Plant Sciences, College of Agriculture and Nature Resources, University of Connecticut, Storrs, Connecticut 06269.

出版信息

J Biol Chem. 2013 Nov 8;288(45):32414-32423. doi: 10.1074/jbc.M113.502112. Epub 2013 Sep 25.

Abstract

RecQ helicases, essential enzymes for maintaining genome integrity, possess the capability to participate in a wide variety of DNA metabolisms. They can initiate the homologous recombination repair pathway by unwinding damaged dsDNA and suppress hyper-recombination by promoting Holliday junction (HJ) migration. To learn how DrRecQ participates in the homologous recombination repair pathway, solution structures of Deinococcus radiodurans RecQ (DrRecQ) and its complexes with DNA substrates were investigated by small angle x-ray scattering. We found that the catalytic core and the most N-terminal HRDC (helicase and RNase D C-terminal) domain (HRDC1) undergo a conformational change to a compact state upon binding to a junction DNA. Furthermore, models of DrRecQ in complexes with two kinds of junction DNA (fork junction and HJ) were built based on the small angle x-ray scattering data, and together with the EMSA results, possible binding sites were proposed. It is demonstrated that two DrRecQ molecules bind to the opposite arms of HJ. This architecture is similar to the RuvAB complex and is hypothesized to be highly conserved in the other HJ migration proteins. This work provides us new clues to understand the roles DrRecQ plays in the RecFOR pathway.

摘要

RecQ 解旋酶是维持基因组完整性的必需酶,具有参与多种 DNA 代谢的能力。它们可以通过解开受损的双链 DNA 来启动同源重组修复途径,并通过促进 Holliday junction (HJ) 迁移来抑制超重组。为了了解 DrRecQ 如何参与同源重组修复途径,通过小角度 X 射线散射研究了 Deinococcus radiodurans RecQ(DrRecQ)及其与 DNA 底物复合物的溶液结构。我们发现,当与连接 DNA 结合时,催化核心和最 N 端 HRDC(解旋酶和 RNase D C 端)结构域(HRDC1)发生构象变化,形成紧凑状态。此外,根据小角度 X 射线散射数据构建了 DrRecQ 与两种连接 DNA(叉连接和 HJ)复合物的模型,并结合 EMSA 结果,提出了可能的结合位点。结果表明,两个 DrRecQ 分子结合到 HJ 的相反臂上。这种结构类似于 RuvAB 复合物,并且假设在其他 HJ 迁移蛋白中高度保守。这项工作为我们理解 DrRecQ 在 RecFOR 途径中所起的作用提供了新的线索。

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