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金属诱导的 DNA 易位导致 DNA 聚合酶构象激活。

Metal-induced DNA translocation leads to DNA polymerase conformational activation.

机构信息

Laboratory of Structural Biology, NIEHS, Research Triangle Park, NC 27709, USA.

出版信息

Nucleic Acids Res. 2012 Apr;40(7):2974-83. doi: 10.1093/nar/gkr1218. Epub 2011 Dec 14.

Abstract

Binding of the catalytic divalent ion to the ternary DNA polymerase β/gapped DNA/dNTP complex is thought to represent the final step in the assembly of the catalytic complex and is consequently a critical determinant of replicative fidelity. We have analyzed the effects of Mg(2+) and Zn(2+) on the conformational activation process based on NMR measurements of [methyl-(13)C]methionine DNA polymerase β. Unexpectedly, both divalent metals were able to produce a template base-dependent conformational activation of the polymerase/1-nt gapped DNA complex in the absence of a complementary incoming nucleotide, albeit with different temperature thresholds. This conformational activation is abolished by substituting Glu295 with lysine, thereby interrupting key hydrogen bonds necessary to stabilize the closed conformation. These and other results indicate that metal-binding can promote: translocation of the primer terminus base pair into the active site; expulsion of an unpaired pyrimidine, but not purine, base from the template-binding pocket; and motions of polymerase subdomains that close the active site. We also have performed pyrophosphorolysis studies that are consistent with predictions based on these results. These findings provide new insight into the relationships between conformational activation, enzyme activity and polymerase fidelity.

摘要

结合催化二价离子到三元 DNA 聚合酶 β/缺口 DNA/dNTP 复合物被认为代表了催化复合物组装的最后一步,因此是复制保真度的关键决定因素。我们已经基于 [methyl-(13)C]methionine DNA 聚合酶 β 的 NMR 测量分析了 Mg(2+) 和 Zn(2+) 对构象激活过程的影响。出乎意料的是,尽管温度阈值不同,但两种二价金属都能够在没有互补进入核苷酸的情况下产生模板碱基依赖性的聚合酶/1-nt 缺口 DNA 复合物的构象激活。这种构象激活被用赖氨酸取代 Glu295 所破坏,从而中断了稳定封闭构象所必需的关键氢键。这些和其他结果表明,金属结合可以促进:引物末端碱基对进入活性位点的易位;从模板结合口袋中逐出未配对的嘧啶而不是嘌呤碱基;以及关闭活性位点的聚合酶亚结构域的运动。我们还进行了焦磷酸解研究,这些研究与基于这些结果的预测一致。这些发现为构象激活、酶活性和聚合酶保真度之间的关系提供了新的见解。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/88d9/3326329/37b0cc991683/gkr1218f1.jpg

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