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人DNA聚合酶β在体外对O6-甲基鸟嘌呤的复制。对O6-甲基鸟嘌呤无效的细胞毒性修复和诱变的见解。

Replication across O6-methylguanine by human DNA polymerase beta in vitro. Insights into the futile cytotoxic repair and mutagenesis of O6-methylguanine.

作者信息

Singh J, Su L, Snow E T

机构信息

Nelson Institute of Environmental Medicine, New York University Medical Center, Tuxedo, New York 10987, USA.

出版信息

J Biol Chem. 1996 Nov 8;271(45):28391-8. doi: 10.1074/jbc.271.45.28391.

DOI:10.1074/jbc.271.45.28391
PMID:8910463
Abstract

Replication in vivo across unrepaired O6-methylguanine (m6dG) lesions by mammalian DNA polymerase beta (pol beta) during short patch repair may contribute to the cytotoxicity and mutagenesis of m6dG. We have employed in vitro steady state kinetic analysis to investigate the replication of oligonucleotide templates containing site-specific m6dG by human pol beta. Our results show that m6dG is a strong but not absolute block to replication by pol beta. pol beta exhibits mixed kinetic discrimination during overall replication across dG and m6dG. pol beta preferentially inserts dTMP rather than dCMP opposite m6dG. However, pol beta extends from the dC-m6dG base pair more efficiently than from the dT-m6dG base pair. This is in strong contrast to other polymerases such as the exonuclease-deficient Klenow fragment of Escherichia coli DNA polymerase I (exo-KF) that preferentially extends dT-m6dG by a factor of 10 over dC-m6dG. When both insertion and extension are considered, pol beta has a 15-fold overall preference for incorporation of the mutagenic substrate dTTP rather than the nonmutagenic substrate dCTP during replication across m6dG. This suggests that pol beta, in concert with the T:G-specific thymine DNA glycosylase, may be intricately involved in the futile cytotoxic repair induced by m6dG. Our results also suggest that replication across m6dG by pol beta may contribute to m6dG-induced G --> A transition mutations.

摘要

在短片段修复过程中,哺乳动物DNA聚合酶β(pol β)在体内跨越未修复的O6-甲基鸟嘌呤(m6dG)损伤进行复制,可能会导致m6dG的细胞毒性和诱变作用。我们采用体外稳态动力学分析方法,研究人pol β对含位点特异性m6dG的寡核苷酸模板的复制情况。我们的结果表明,m6dG是pol β复制的一个强大但非绝对的障碍。pol β在跨越dG和m6dG的整体复制过程中表现出混合动力学歧视。pol β在m6dG对面优先插入dTMP而非dCMP。然而,pol β从dC-m6dG碱基对延伸的效率高于从dT-m6dG碱基对延伸的效率。这与其他聚合酶形成强烈对比,例如大肠杆菌DNA聚合酶I的核酸外切酶缺陷型Klenow片段(exo-KF),它优先延伸dT-m6dG的效率比dC-m6dG高10倍。当同时考虑插入和延伸时,在跨越m6dG复制过程中,pol β总体上对诱变底物dTTP而非非诱变底物dCTP的掺入偏好为15倍。这表明pol β与T:G特异性胸腺嘧啶DNA糖基化酶协同作用,可能复杂地参与了由m6dG诱导的无效细胞毒性修复。我们的结果还表明,pol β跨越m6dG的复制可能导致m6dG诱导的G→A转换突变。

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