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Targeted detection of in vivo endogenous DNA base damage reveals preferential base excision repair in the transcribed strand

机译:体内内源性DNA碱基损伤的靶向检测揭示了转录链中优先的碱基切除修复

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Endogenous DNA damage is removed mainly via base excision repair (BER), however, whether there is preferential strand repair of endogenous DNA damage is still under intense debate. We developed a highly sensitive primer-anchored DNA damage detection assay (PADDA) to map and quantify in vivo endogenous DNA damage. Using PADDA, we documented significantly higher levels of endogenous damage in Saccharomyces cerevisiae cells in stationary phase than in exponential phase. We also documented that yeast BER-defective cells have significantly higher levels of endogenous DNA damage than isogenic wild-type cells at any phase of growth. PADDA provided detailed fingerprint analysis at the single-nucleotide level, documenting for the first time that persistent endogenous nucleotide damage in CAN1 co-localizes with previously reported spontaneous CAN1 mutations. To quickly and reliably quantify endogenous strand-specific DNA damage in the constitutively expressed CAN1 gene, we used PADDA on a real-time PCR setting. We demonstrate that wild-type cells repair endogenous damage preferentially on the CAN1 transcribed strand. In contrast, yeast BER-defective cells accumulate endogenous damage preferentially on the CAN1 transcribed strand. These data provide the first direct evidence for preferential strand repair of endogenous DNA damage and documents the major role of BER in this process.
机译:内源性DNA损伤主要通过碱基切除修复(BER)去除,但是,是否存在内源性DNA损伤的优先链修复仍在激烈的争论中。我们开发了一种高度敏感的引物锚定DNA损伤检测测定(PADDA),以绘制和量化体内内源性DNA损伤。使用PADDA,我们记录了酿酒酵母细胞在稳定期的内源性损伤水平明显高于指数期。我们还证明,在任何生长阶段,酵母BER缺陷细胞均比同基因野生型细胞具有更高水平的内源性DNA损伤。 PADDA在单核苷酸水平上提供了详细的指纹分析,首次记录了CAN1中持续的内源性核苷酸损伤与先前报道的自发CAN1突变共定位。为了快速可靠地定量组成性表达的CAN1基因中的内源链特异性DNA损伤,我们在实时PCR设置中使用了PADDA。我们证明,野生型细胞优先在CAN1转录链上修复内源性损伤。相反,酵母BER缺陷细胞优先在CAN1转录的链上积累内源性损伤。这些数据为内源性DNA损伤的优先链修复提供了首个直接证据,并证明了BER在此过程中的主要作用。

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