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关于大肠杆菌DNA聚合酶I的持续合成机制

On the processive mechanism of Escherichia coli DNA polymerase I.

作者信息

Uyemura D, Bambara R, Lehman I R

出版信息

J Biol Chem. 1975 Nov 25;250(22):8577-84.

PMID:1102539
Abstract

A procedure has been developed to assess whether polymerization of nucleotides by DNA polymerases is processive, that is, whether a succession of polymerization steps occurs without release of the enzyme from the template. The method involves measurement of the ratio of deoxyguanylate to deocycytidylate incorporated in the course of replicating a segment of the right hand cohesive end of phage lambaDNA with the sequence 5'-G-G-G-C-G-G-C-G-3'. In the case of the Escherichia coli DNA polymerase I, each enzyme molecule completes synthesis of the sequence before dissociation occurs. Furthermore, at both 6 and 22 degrees, the polymerase remains bound to the lambdaDNA template after synthesis has completed. Template challenge experiments, in which the polymerase is allowed to begin synthesis in the presence of a molar excess of lambdaDNA before addition of a very large excess of calf thymus DNA, show that under the conditions used, productive binding of polymerase to lambdaDNA is a slow process requiring 1 to 2 hours. After synthesis has been completed, polymerase remains bound to the lambdaDNA in spite of the availability of new primer termini. The association, polymerization, and dissociation rates measured in these experiments suggest that the polymerization reaction catalyzed by DNA polymerase I is processive, and that hundreds of nucleotides may be polymerized between each association and dissociation.

摘要

已开发出一种程序来评估DNA聚合酶使核苷酸聚合的过程是否具有持续性,也就是说,一连串的聚合步骤是否在酶不脱离模板的情况下发生。该方法涉及测量在复制噬菌体λDNA右手粘性末端的一段序列(5'-G-G-G-C-G-G-C-G-3')过程中掺入的脱氧鸟苷酸与脱氧胞苷酸的比率。就大肠杆菌DNA聚合酶I而言,每个酶分子在解离发生之前完成该序列的合成。此外,在6℃和22℃时,合成完成后聚合酶仍与λDNA模板结合。模板挑战实验中,在加入非常大量的小牛胸腺DNA之前,先让聚合酶在存在摩尔过量的λDNA的情况下开始合成,结果表明在所使用的条件下,聚合酶与λDNA的有效结合是一个缓慢的过程,需要1至2小时。合成完成后,尽管有新的引物末端可用,聚合酶仍与λDNA结合。在这些实验中测得的结合、聚合和解离速率表明,DNA聚合酶I催化的聚合反应是持续的,并且在每次结合和解离之间可能有数百个核苷酸聚合。

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