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端粒酶修复端粒处崩溃的复制叉。

Telomerase Repairs Collapsed Replication Forks at Telomeres.

机构信息

Marseille Cancer Research Centre (CRCM), U1068 INSERM, UMR7258 CNRS, UM105 Aix-Marseille University, Institut Paoli-Calmettes, Ligue Nationale Contre le Cancer (équipe labellisée) Marseille, F-13009, France.

Institut Curie, PSL Research University, CNRS, UMR3348, F-91405 Orsay, France; University Paris Sud, Paris-Saclay University, CNRS, UMR3348, F-91405 Orsay, France.

出版信息

Cell Rep. 2020 Mar 10;30(10):3312-3322.e3. doi: 10.1016/j.celrep.2020.02.065.

Abstract

Telomeres are difficult-to-replicate sites whereby replication itself may threaten telomere integrity. We investigate, in fission yeast, telomere replication dynamics in telomerase-negative cells to unmask problems associated with telomere replication. Two-dimensional gel analysis reveals that replication of telomeres is severely impaired and correlates with an accumulation of replication intermediates that arises from stalled and collapsed forks. In the absence of telomerase, Rad51, Mre11-Rad50-Nbs1 (MRN) complex, and its co-factor CtIP become critical to maintain telomeres, indicating that homologous recombination processes these intermediates to facilitate fork restart. We further show that a catalytically dead mutant of telomerase prevents Ku recruitment to telomeres, suggesting that telomerase and Ku both compete for the binding of telomeric-free DNA ends that are likely to originate from a reversed fork. We infer that Ku removal at collapsed telomeric forks allows telomerase to repair broken telomeres, thereby shielding telomeres from homologous recombination.

摘要

端粒是难以复制的位点,复制本身可能会威胁端粒的完整性。我们在裂殖酵母中研究了端粒酶缺失细胞中端粒的复制动态,以揭示与端粒复制相关的问题。二维凝胶分析显示,端粒的复制受到严重损害,并与复制中间体的积累相关,这些中间体是由停滞和崩溃的叉头引起的。在没有端粒酶的情况下,Rad51、Mre11-Rad50-Nbs1(MRN)复合物及其共因子 CtIP 对维持端粒至关重要,表明同源重组过程将这些中间体转化为促进叉头重新启动。我们进一步表明,端粒酶的催化失活突变体阻止 Ku 向端粒募集,这表明端粒酶和 Ku 都竞争结合可能来自反转叉头的游离端粒 DNA。我们推断,在崩溃的端粒叉头处去除 Ku 允许端粒酶修复断裂的端粒,从而使端粒免受同源重组的影响。

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