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在大肠杆菌中没有 Holliday junction resolvases 的情况下进行重组修复。

Recombinational repair in the absence of holliday junction resolvases in E. coli.

机构信息

CNRS, UMR7242 Biotechnologie et Signalisation Cellulaire, 300 Bld Sébastien Brant, CS10413 F - 67412 ILLKIRCH Cedex, France.

Department of Biology, Carleton University, 1125 Colonel By Drive, Ottawa, ON K1S 5B6, Canada.

出版信息

Mutat Res. 2021 Jan-Jun;822:111740. doi: 10.1016/j.mrfmmm.2021.111740. Epub 2021 Feb 13.

DOI:10.1016/j.mrfmmm.2021.111740
PMID:33740684
Abstract

Cells possess two major DNA damage tolerance pathways that allow them to duplicate their genomes despite the presence of replication blocking lesions: translesion synthesis (TLS) and daughter strand gap repair (DSGR). The TLS pathway involves specialized DNA polymerases that are able to synthesize past DNA lesions while DSGR relies on Recombinational Repair (RR). At least two mechanisms are associated with RR: Homologous Recombination (HR) and RecA Mediated Excision Repair (RAMER). While HR and RAMER both depend on RecFOR and RecA, only the HR mechanism should involve Holliday Junctions (HJs) resolvase reactions. In this study we investigated the role of HJ resolvases, RuvC, TopIII and RusA on the balance between RAMER and HR in E. coli MG1655 derivatives. Using UV survival measurements, we first clearly establish that, in this genetic background, topB and ruvC define two distinct pathways of HJ resolution. We observed that a recA mutant is much more sensitive to UV than the ruvC topB double mutant which is deficient in HR because of its failure to resolve HJs. This difference is independent of RAMER, the SOS system, RusA, and the three TLS DNA polymerases, and may be accounted for by Double Strand Break repair mechanisms such as Synthesis Dependent Strand Annealing, Single Strand Annealing, or Break Induced Replication, which are independent of HJ resolvases. We then used a plasmid-based assay, in which RR is triggered by a single blocking lesion present on a plasmid molecule, to establish that while HR requires topB, ruvC or rusA, RAMER is independent of these genes and, as expected, requires a functional UvrABC excinuclease. Surprisingly, analysis of the RR events in a strain devoid of HJ resolvases reveals that the UvrABC dependent repair of the single lesion present on the plasmid molecule can generate an excision track potentially extending to dozens of nucleotides.

摘要

细胞拥有两种主要的 DNA 损伤容忍途径,使它们能够在复制受阻的情况下复制基因组:跨损伤合成(TLS)和子链间隙修复(DSGR)。TLS 途径涉及能够合成过去 DNA 损伤的专门 DNA 聚合酶,而 DSGR 依赖于重组修复(RR)。RR 至少有两种机制与之相关:同源重组(HR)和 RecA 介导的切除修复(RAMER)。虽然 HR 和 RAMER 都依赖于 RecFOR 和 RecA,但只有 HR 机制应涉及 Holliday 结(HJ)解旋酶反应。在这项研究中,我们研究了 HJ 解旋酶、RuvC、TopIII 和 RusA 在大肠杆菌 MG1655 衍生物中 RAMER 和 HR 之间平衡中的作用。使用 UV 生存测量,我们首先明确确立了,在这种遗传背景下,topB 和 ruvC 定义了两种不同的 HJ 分辨率途径。我们观察到,recA 突变体对 UV 比 ruvC topB 双突变体敏感得多,因为它不能解决 HJ,所以 HR 缺陷。这种差异与 RAMER、SOS 系统、RusA 和三种 TLS DNA 聚合酶无关,可能是由双链断裂修复机制(如合成依赖性链退火、单链退火或断裂诱导复制)引起的,这些机制与 HJ 解旋酶无关。然后,我们使用基于质粒的测定法,其中 RR 由质粒分子上存在的单个阻断损伤引发,以确定虽然 HR 需要 topB、ruvC 或 rusA,但 RAMER 独立于这些基因,并且如预期的那样,需要功能性 UvrABC 外切核酸酶。令人惊讶的是,在缺乏 HJ 解旋酶的菌株中分析 RR 事件表明,UvrABC 对质粒分子上存在的单个损伤的依赖性修复可以产生一个切除轨迹,该轨迹可能延伸至数十个核苷酸。

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