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Replication fork integrity and intra-S phase checkpoint suppress gene amplification

机译:复制叉完整性和S内阶段检查点抑制基因扩增

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摘要

Gene amplification is a phenotype-causing form of chromosome instability and is initiated by DNA double-strand breaks (DSBs). Cells with mutant p53 lose G1/S checkpoint and are permissive to gene amplification. In this study we show that mammalian cells become proficient for spontaneous gene amplification when the function of the DSB repair protein complex MRN (Mre11/Rad50/Nbs1) is impaired. Cells with impaired MRN complex experienced severe replication stress and gained substrates for gene amplification during replication, as evidenced by the increase of replication-associated single-stranded breaks that were converted to DSBs most likely through replication fork reversal. Impaired MRN complex directly compromised ATM/ATR-mediated checkpoints and allowed cells to progress through cell cycle in the presence of DSBs. Such compromised intra-S phase checkpoints promoted gene amplification independently from mutant p53. Finally, cells adapted to endogenous replication stress by globally suppressing genes for DNA replication and cell cycle progression. Our results indicate that the MRN complex suppresses gene amplification by stabilizing replication forks and by securing DNA damage response to replication-associated DSBs.
机译:基因扩增是导致染色体不稳定的表型形式,并由DNA双链断裂(DSB)启动。带有突变体p53的细胞会丢失G1 / S检查点,并且允许基因扩增。在这项研究中,我们表明当DSB修复蛋白复合物MRN(Mre11 / Rad50 / Nbs1)的功能受损时,哺乳动物细胞会熟练地进行自发基因扩增。 MRN复合物受损的细胞在复制过程中会遭受严重的复制压力,并获得了用于基因扩增的底物,这与复制相关的单链断裂的增加所证明,这种断裂最有可能通过复制叉逆转转化为DSB。受损的MRN复合物直接损害了ATM / ATR介导的检查点,并允许细胞在存在DSB的情况下经历细胞周期。这种受损的S内相检查点独立于突变体p53促进了基因扩增。最后,细胞通过全局抑制DNA复制和细胞周期进程的基因来适应内源性复制压力。我们的结果表明,MRN复合物通过稳定复制叉和通过确保DNA损伤对复制相关DSB的应答来抑制基因扩增。

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