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在具有催化活性的芽孢杆菌DNA聚合酶晶体中观察DNA复制

Visualizing DNA replication in a catalytically active Bacillus DNA polymerase crystal.

作者信息

Kiefer J R, Mao C, Braman J C, Beese L S

机构信息

Department of Biochemistry, Duke University Medical Center, Durham, North Carolina 27710, USA.

出版信息

Nature. 1998 Jan 15;391(6664):304-7. doi: 10.1038/34693.

Abstract

DNA polymerases copy DNA templates with remarkably high fidelity, checking for correct base-pair formation both at nucleotide insertion and at subsequent DNA extension steps. Despite extensive biochemical, genetic and structural studies, the mechanism by which nucleotides are correctly incorporated is not known. Here we present high-resolution crystal structures of a thermostable bacterial (Bacillus stearothermophilus) DNA polymerase I large fragments with DNA primer templates bound productively at the polymerase active site. The active site retains catalytic activity, allowing direct observation of the products of several rounds of nucleotide incorporation. The polymerase also retains its ability to discriminate between correct and incorrectly paired nucleotides in the crystal. Comparison of the structures of successively translocated complexes allows the structural features for the sequence-independent molecular recognition of correctly formed base pairs to be deduced unambiguously. These include extensive interactions with the first four to five base pairs in the minor groove, location of the terminal base pair in a pocket of excellent steric complementarity favouring correct base-pair formation, and a conformational switch from B-form to underwound A-form DNA at the polymerase active site.

摘要

DNA聚合酶能以极高的保真度复制DNA模板,在核苷酸插入以及随后的DNA延伸步骤中检查碱基对的正确形成。尽管进行了广泛的生化、遗传和结构研究,但核苷酸正确掺入的机制仍不清楚。在此,我们展示了嗜热栖热放线菌DNA聚合酶I大片段的高分辨率晶体结构,其与DNA引物模板在聚合酶活性位点有效结合。活性位点保留了催化活性,从而能够直接观察几轮核苷酸掺入的产物。该聚合酶在晶体中也保留了区分正确和错误配对核苷酸的能力。对相继移位复合物结构的比较,使得能够明确推断出正确形成碱基对的序列无关分子识别的结构特征。这些特征包括与小沟中前四到五个碱基对的广泛相互作用、末端碱基对位于空间互补性极佳的口袋中以利于正确碱基对的形成,以及在聚合酶活性位点处从B型DNA到解旋的A型DNA的构象转换。

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