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人细胞提取物中一种对阿非迪霉素敏感的DNA聚合酶对腺嘌呤/8-氧代鸟嘌呤错配的碱基切除修复。

Base excision repair of adenine/8-oxoguanine mispairs by an aphidicolin-sensitive DNA polymerase in human cell extracts.

作者信息

Parlanti Eleonora, Fortini Paola, Macpherson Peter, Laval Jacques, Dogliotti Eugenia

机构信息

Laboratory of Comparative Toxicology and Ecotoxicology, Istituto Superiore di Sanita', Viale Regina Elena 299, 00161 Rome, Italy.

出版信息

Oncogene. 2002 Aug 8;21(34):5204-12. doi: 10.1038/sj.onc.1205561.

Abstract

Replication of DNA containing 8-oxo-7,8-dihydroguanine (8oxoG) can generate 8oxoG/A base pairs which, if uncorrected, lead to G-->T transversions. It is generally accepted that the repair of these promutagenic base pairs in human cells is initiated by the MutY DNA glycosylase homolog (hMYH). Here we provide biochemical evidence that human cell extracts perform base excision repair (BER) on both DNA strands of an 8oxoG/A mismatch. At early repair times the specificity of nucleotide incorporation indicates a preferential insertion of C opposite 8oxoG leading to the formation of 8oxoG/C pairs. This is followed by repair synthesis on the opposite DNA strand that is consistent with hOGG1-mediated correction of 8oxoG/C to G/C. Repair synthesis on either strand is completely inhibited by aphidicolin suggesting that a replicative DNA polymerase is involved in the gap filling. This is the first demonstration that repair of 8oxoG/A base pairs is by two BER events likely mediated by Poldelta/epsilon. We suggest that the Poldelta/epsilon-mediated BER is the general mode of repair when BER lesions are formed at replication forks.

摘要

含有8-氧代-7,8-二氢鸟嘌呤(8oxoG)的DNA复制可产生8oxoG/A碱基对,若不加以校正,会导致G→T颠换。人们普遍认为,人类细胞中这些前诱变碱基对的修复是由MutY DNA糖基化酶同源物(hMYH)启动的。在此,我们提供了生化证据,表明人类细胞提取物对8oxoG/A错配的两条DNA链都进行碱基切除修复(BER)。在修复早期,核苷酸掺入的特异性表明在8oxoG对面优先插入C,导致形成8oxoG/C对。随后在相反的DNA链上进行修复合成,这与hOGG1介导的将8oxoG/C校正为G/C一致。两条链上的修复合成均被阿非科林完全抑制,这表明复制性DNA聚合酶参与了缺口填补。这是首次证明8oxoG/A碱基对的修复是由可能由Poldelta/epsilon介导的两个BER事件完成的。我们认为,当在复制叉处形成BER损伤时,Poldelta/epsilon介导的BER是一般的修复模式。

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