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连接酶 Ku 因子在双链断裂游离的复制叉末端切除中起作用。

The end-joining factor Ku acts in the end-resection of double strand break-free arrested replication forks.

机构信息

Institut Curie, PSL Research University, CNRS, UMR3348, Orsay, F-91405, France.

University Paris Sud, Paris-Saclay University, CNRS, UMR3348, Orsay, F-91405, France.

出版信息

Nat Commun. 2017 Dec 7;8(1):1982. doi: 10.1038/s41467-017-02144-5.

Abstract

Replication requires homologous recombination (HR) to stabilize and restart terminally arrested forks. HR-mediated fork processing requires single stranded DNA (ssDNA) gaps and not necessarily double strand breaks. We used genetic and molecular assays to investigate fork-resection and restart at dysfunctional, unbroken forks in Schizosaccharomyces pombe. Here, we report that fork-resection is a two-step process regulated by the non-homologous end joining factor Ku. An initial resection mediated by MRN-Ctp1 removes Ku from terminally arrested forks, generating ~110 bp sized gaps obligatory for subsequent Exo1-mediated long-range resection and replication restart. The mere lack of Ku impacts the processing of arrested forks, leading to an extensive resection, a reduced recruitment of RPA and Rad51 and a slower fork-restart process. We propose that terminally arrested forks undergo fork reversal, providing a single DNA end for Ku binding. We uncover a role for Ku in regulating end-resection of unbroken forks and in fine-tuning HR-mediated replication restart.

摘要

复制需要同源重组 (HR) 来稳定和重新启动末端停滞的叉。HR 介导的叉处理需要单链 DNA (ssDNA) 缺口,而不一定需要双链断裂。我们使用遗传和分子测定法来研究在裂殖酵母中功能失调、未断裂的叉处的叉切除和重新启动。在这里,我们报告叉切除是由非同源末端连接因子 Ku 调控的两步过程。MRN-Ctp1 介导的初始切除将 Ku 从末端停滞的叉上移除,产生大约 110 bp 大小的缺口,这是随后 Exo1 介导的长距离切除和复制重新启动所必需的。仅仅缺乏 Ku 就会影响被阻断的叉的处理,导致广泛的切除、RPA 和 Rad51 的募集减少以及叉重新启动过程的减慢。我们提出,末端停滞的叉会发生叉反转,为 Ku 结合提供一个单链 DNA 末端。我们揭示了 Ku 在调节未断裂的叉的末端切除以及精细调控 HR 介导的复制重新启动中的作用。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/2cc9/5719404/4f46ac18168e/41467_2017_2144_Fig1_HTML.jpg

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