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MRNIP是一种复制叉保护因子。

MRNIP is a replication fork protection factor.

作者信息

Bennett L G, Wilkie A M, Antonopoulou E, Ceppi I, Sanchez A, Vernon E G, Gamble A, Myers K N, Collis S J, Cejka P, Staples C J

机构信息

North West Cancer Research Institute, School of Medical Sciences, Bangor University, Bangor LL57 2UW, UK.

Institute for Research in Biomedicine, Faculty of Biomedical Sciences, Università della Svizzera italiana, 6500 Bellinzona, Switzerland.

出版信息

Sci Adv. 2020 Jul 10;6(28):eaba5974. doi: 10.1126/sciadv.aba5974. eCollection 2020 Jul.

Abstract

The remodeling of stalled replication forks to form four-way DNA junctions is an important component of the replication stress response. Nascent DNA at the regressed arms of these reversed forks is protected by RAD51 and the tumor suppressors BRCA1/2, and when this function is compromised, stalled forks undergo pathological MRE11-dependent degradation, leading to chromosomal instability. However, the mechanisms regulating MRE11 functions at reversed forks are currently unclear. Here, we identify the MRE11-binding protein MRNIP as a novel fork protection factor that directly binds to MRE11 and specifically represses its exonuclease activity. The loss of MRNIP results in impaired replication fork progression, MRE11 exonuclease-dependent degradation of reversed forks, persistence of underreplicated genomic regions, chemosensitivity, and chromosome instability. Our findings identify MRNIP as a novel regulator of MRE11 at reversed forks and provide evidence that regulation of specific MRE11 nuclease activities ensures protection of nascent DNA and thereby genome integrity.

摘要

停滞的复制叉重塑形成四向DNA连接是复制应激反应的重要组成部分。这些反向叉退化臂上的新生DNA由RAD51和肿瘤抑制因子BRCA1/2保护,当此功能受损时,停滞的叉会经历病理性MRE11依赖性降解,导致染色体不稳定。然而,目前尚不清楚调节MRE11在反向叉上功能的机制。在这里,我们鉴定出MRE11结合蛋白MRNIP是一种新型的叉保护因子,它直接与MRE11结合并特异性抑制其核酸外切酶活性。MRNIP的缺失导致复制叉进展受损、反向叉的MRE11核酸外切酶依赖性降解、未复制基因组区域的持续存在、化学敏感性和染色体不稳定。我们的研究结果确定MRNIP是反向叉上MRE11的新型调节因子,并提供证据表明特定MRE11核酸酶活性的调节可确保新生DNA的保护,从而保证基因组完整性。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/a68b/7439443/b01802d272ef/aba5974-F1.jpg

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