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Colocalization of multiple DNA double-strand breaks at a single Rad52 repair centre

机译:在一个Rad52维修中心将多个DNA双链断裂共定位

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摘要

DNA double-strand break repair (DSBR) is an essential process for preserving genomic integrity in all organisms. To investigate this process at the cellular level, we engineered a system of fluorescently marked DNA double-strand breaks (DSBs) in the yeast Saccharomyces cerevisiae to visualize in vivo DSBR in single cells. Using this system, we demonstrate for the first time that Rad52 DNA damage checkpoint-deficient cells provides direct evidence for coordination between DNA repair and subsequent release from checkpoint arrest. Finally, analyses of cells experiencing multiple DSBs demonstrate that Rad52 foci are centres of DNA repair capable of simultaneously recruiting more than one DSB.
机译:DNA双链断裂修复(DSBR)是维护所有生物体中基因组完整性的重要过程。为了在细胞水平上研究此过程,我们设计了酿酒酵母中荧光标记的DNA双链断裂(DSB)系统,以可视化单细胞的体内DSBR。使用该系统,我们首次证明Rad52 DNA损伤检查点缺陷细胞为DNA修复与随后从检查点逮捕释放之间的协调提供直接证据。最后,对经历多个DSB的细胞的分析表明,Rad52病灶是能够同时募集多个DSB的DNA修复中心。

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