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Novel nuclear and mitochondrial glycosylases revealed by disruption of the mouse Nth1 gene encoding an endonuclease III homolog for repair of thymine glycols

机译:通过破坏编码胸腺嘧啶二醇的内切核酸酶III同源物的小鼠Nth1基因而揭示的新型核和线粒体糖基化酶

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摘要

Endonuclease III, encoded by nth in Escherichia coli, removes thymine glycols (Tg), a toxic oxidative DNA lesion. To determine the biological significance of this repair in mammals, we established a mouse model with mutated mNth1, a homolog of nth, by gene targeting. The homozygous mNth1 mutant mice showed no detectable phenotypical abnormality. Embryonic cells with or without wild-type mNth1 showed no difference in sensitivity to menadione or hydrogen peroxide. Tg produced in the mutant mouse liver DNA by X-ray irradiation disappeared with time, though more slowly than in the wild-type mouse. In extracts from mutant mouse liver, we found, instead of mNTH1 activity, at least two novel DNA glycosylase activities against Tg. One activity is significantly higher in the mutant than in wild-type mouse in mitochondria, while the other is another nuclear glycosylase for Tg. These results underscore the importance of base excision repair of Tg both in the nuclei and mitochondria in mammals.
机译:在大肠杆菌中由nth编码的核酸内切酶III去除了胸腺嘧啶二醇(Tg),一种有毒的氧化性DNA损伤。为了确定这种修复在哺乳动物中的生物学意义,我们通过基因定位建立了具有突变的mNth1(第n个同源物)的小鼠模型。纯合mNth1突变小鼠显示未检测到表型异常。有或没有野生型mNth1的胚胎细胞对甲萘醌或过氧化氢的敏感性均无差异。 X射线辐射在突变小鼠肝DNA中产生的Tg随时间消失,尽管比野生型小鼠慢。在突变小鼠肝脏的提取物中,我们发现了至少两种针对Tg的新的DNA糖基化酶活性,而不是mNTH1活性。线粒体中突变体的一种活性明显高于野生型小鼠,而另一种是Tg的另一种核糖基化酶。这些结果强调了在哺乳动物的核和线粒体中Tg的碱基切除修复的重要性。

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