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Repair of a minimal DNA double-strand break by NHEJ requires DNA-PKcs and is controlled by the ATM/ATR checkpoint

机译:NHEJ修复最小的DNA双链断裂需要DNA-PKcs,并由ATM / ATR检查点控制

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摘要

Mammalian cells primarily rejoin DNA double-strand breaks (DSBs) by the non-homologous end-joining (NHEJ) pathway. The joining of the broken DNA ends appears directly without template and accuracy is ensured by the NHEJ factors that are under ATM/ATR regulated checkpoint control. In the current study we report the engineering of a mono-specific DNA damaging agent. This was used to study the molecular requirements for the repair of the least complex DSB in vivo. Single-chain PvuII restriction enzymes fused to protein delivery sequences transduce cells efficiently and induce blunt end DSBs in vivo. We demonstrate that beside XRCC4/LigaseIV and KU, the DNA-PK catalytic subunit (DNA-PKcs) is also essential for the joining of this low complex DSB in vivo. The appearance of blunt end 3'-hydroxyl and 5'-phosphate DNA DSBs induces a significantly higher frequency of anaphase bridges in cells that do not contain functional DNA-PKcs, suggesting an absolute requirement for DNA-PKcs in the control of chromosomal stability during end joining. Moreover, these minimal blunt end DSBs are sufficient to induce a p53 and ATM/ATR checkpoint function.
机译:哺乳动物细胞主要通过非同源末端连接(NHEJ)途径重新结合DNA双链断裂(DSB)。断裂的DNA末端的连接直接出现而没有模板,并且由ATM / ATR调节的检查点控制下的NHEJ因子确保了准确性。在当前的研究中,我们报告了单特异性DNA损伤剂的工程设计。这用于研究修复体内最不复杂的DSB的分子要求。与蛋白质递送序列融合的单链PvuII限制酶可有效地转导细胞并在体内诱导平末端DSB。我们证明,除了XRCC4 / LigaseIV和KU外,DNA-PK催化亚基(DNA-PKcs)对于体内这种低复杂度DSB的连接也是必不可少的。 3'-末端羟基和5'-磷酸末端DNA DSB钝化的出现在不包含功能性DNA-PKcs的细胞中诱导后期桥的频率明显升高,这提示在控制染色体稳定性时绝对需要DNA-PKcs结束加入。而且,这些最小的钝端DSB足以诱导p53和ATM / ATR检查点功能。

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