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Pif1 和复制依赖性链位移产生的分叉长 ssDNA 瓣背后的 DNA2 加工。

Dna2 processes behind the fork long ssDNA flaps generated by Pif1 and replication-dependent strand displacement.

机构信息

IFOM (Fondazione Istituto FIRC di Oncologia Molecolare), Via Adamello 16, Milan, 20139, Italy.

Dipartimento di Oncologia ed Emato-Oncologia, Universita' degli Studi di Milano, Via Festa del Perdono 7, Milan, 20122, Italy.

出版信息

Nat Commun. 2018 Nov 16;9(1):4830. doi: 10.1038/s41467-018-07378-5.

Abstract

Dna2 is a DNA helicase-endonuclease mediating DSB resection and Okazaki fragment processing. Dna2 ablation is lethal and rescued by inactivation of Pif1, a helicase assisting Okazaki fragment maturation, Pol32, a DNA polymerase δ subunit, and Rad9, a DNA damage response (DDR) factor. Dna2 counteracts fork reversal and promotes fork restart. Here we show that Dna2 depletion generates lethal DNA structures activating the DDR. While PIF1 deletion rescues the lethality of Dna2 depletion, RAD9 ablation relieves the first cell cycle arrest causing genotoxicity after few cell divisions. Slow fork speed attenuates DDR in Dna2 deprived cells. Electron microscopy shows that Dna2-ablated cells accumulate long ssDNA flaps behind the forks through Pif1 and fork speed. We suggest that Dna2 offsets the strand displacement activity mediated by the lagging strand polymerase and Pif1, processing long ssDNA flaps to prevent DDR activation. We propose that this Dna2 function has been hijacked by Break Induced Replication in DSB processing.

摘要

Dna2 是一种 DNA 解旋酶内切酶,可介导 DSB 切除和 Okazaki 片段加工。Dna2 缺失是致命的,可通过失活 Pif1、一种有助于 Okazaki 片段成熟的解旋酶、DNA 聚合酶 δ 亚基 Pol32 和 DNA 损伤反应 (DDR) 因子 Rad9 来挽救。Dna2 可拮抗叉反转并促进叉重新启动。本文研究表明,Dna2 耗竭会产生激活 DDR 的致死性 DNA 结构。虽然 PIF1 缺失挽救了 Dna2 缺失的致死性,但 RAD9 缺失可缓解第一个细胞周期停滞,从而在经过几次细胞分裂后导致遗传毒性。缓慢的叉速度会减轻 Dna2 缺乏细胞中的 DDR。电子显微镜显示,Dna2 缺失的细胞通过 Pif1 和叉速度在叉后积累长的单链 DNA 瓣。本文提出,Dna2 抵消了由滞后链聚合酶和 Pif1 介导的链位移活性,加工长的单链 DNA 瓣以防止 DDR 激活。本文还提出,这种 Dna2 功能已在 DSB 加工的断裂诱导复制中被劫持。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/37f9/6240037/7d099986ef74/41467_2018_7378_Fig1_HTML.jpg

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