首页> 外文OA文献 >Kinetic measurement of 2-aminopurine X cytosine and 2-aminopurine X thymine base pairs as a test of DNA polymerase fidelity mechanisms.
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Kinetic measurement of 2-aminopurine X cytosine and 2-aminopurine X thymine base pairs as a test of DNA polymerase fidelity mechanisms.

机译:动力学测量2-氨基嘌呤X胞嘧啶和2-氨基嘌呤X胸腺嘧啶碱基对,作为DNA聚合酶保真度机制的测试。

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摘要

Enzyme kinetic measurements are presented showing that Km rather than maximum velocity (Vmax) discrimination governs the frequency of forming 2-aminopurine X cytosine base mispairs by DNA polymerase alpha. An in vitro system is used in which incorporation of dTMP or dCMP occurs opposite a template 2-aminopurine, and values for Km and Vmax are obtained. Results from a previous study in which dTTP and dCTP were competing simultaneously for insertion opposite 2-aminopurine indicated that dTMP is inserted 22 times more frequently than dCMP. We now report that the ratio of Km values KCm/KTm = 25 +/- 6, which agrees quantitatively with the dTMP/dCMP incorporation ratio obtained previously. We also report that VCmax is indistinguishable from VTmax. These Km and Vmax data are consistent with predictions from a model, the Km discrimination model, in which replication fidelity is determined by free energy differences between matched and mismatched base pairs. Central to this model is the prediction that the ratio of Km values for insertion of correct and incorrect nucleotides specifies the insertion fidelity, and the maximum velocities of insertion are the same for both nucleotides.
机译:提出的酶动力学测量结果表明,Km而不是最大速度(Vmax)区分控制着DNA聚合酶α形成2-氨基嘌呤X胞嘧啶碱基错对的频率。使用体外系统,其中在模板2-氨基嘌呤对面发生dTMP或dCMP的掺入,并且获得Km和Vmax的值。先前研究中dTTP和dCTP同时竞争与2-氨基嘌呤相反的插入的结果表明,dTMP的插入频率是dCMP的22倍。我们现在报告,Km值的比值KCm / KTm = 25 +/- 6,这在数量上与先前获得的dTMP / dCMP掺入比吻合。我们还报告说VCmax与VTmax是无法区分的。这些Km和Vmax数据与模型(Km判别模型)的预测一致,其中复制保真度由匹配和不匹配碱基对之间的自由能差异决定。该模型的核心是预测,正确和错误核苷酸插入的Km值之比指定了插入保真度,并且两个核苷酸的最大插入速度相同。

著录项

  • 作者

    Watanabe, S M; Goodman, M F;

  • 作者单位
  • 年度 1982
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  • 原文格式 PDF
  • 正文语种 en
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