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RecD2 解旋酶在乏养古生球菌中解旋 DNA 的动力学研究。

Kinetics of DNA unwinding by the RecD2 helicase from Deinococcus radiodurans.

机构信息

Department of Chemistry and Biochemistry, University of Maryland, College Park, Maryland 20742, USA.

出版信息

J Biol Chem. 2010 Jun 4;285(23):17292-300. doi: 10.1074/jbc.M110.111427. Epub 2010 Mar 31.

Abstract

RecD2 from Deinococcus radiodurans is a superfamily 1 DNA helicase that is homologous to the Escherichia coli RecD protein but functions outside the context of RecBCD enzyme. We report here on the kinetics of DNA unwinding by RecD2 under single and multiple turnover conditions. There is little unwinding of 20-bp substrates by preformed RecD2-dsDNA complexes when excess ssDNA is present to trap enzyme molecules not bound to the substrate. A shorter 12-bp substrate is unwound rapidly under single turnover conditions. The 12-bp unwinding reaction could be simulated with a mechanism in which the DNA is unwound in two kinetic steps with rate constant of k(unw) = 5.5 s(-1) and a dissociation step from partially unwound DNA of k(off) = 1.9 s(-1). These results indicate a kinetic step size of about 3-4 bp, unwinding rate of about 15-20 bp/s, and low processivity (p = 0.74). The reaction time courses with 20-bp substrates, determined under multiple turnover conditions, could be simulated with a four-step mechanism and rate constant values very similar to those for the 12-bp substrate. The results indicate that the faster unwinding of a DNA substrate with a forked end versus only a 5'-terminal single-stranded extension can be accounted for by a difference in the rate of enzyme binding to the DNA substrates. Analysis of reactions done with different RecD2 concentrations indicates that the enzyme forms an inactive dimer or other oligomer at high enzyme concentrations. RecD2 oligomers can be detected by glutaraldehyde cross-linking but not by size exclusion chromatography.

摘要

耐辐射球菌 RecD2 是一个超家族 1 的 DNA 解旋酶,与大肠杆菌 RecD 蛋白同源,但在 RecBCD 酶的背景之外发挥作用。我们在此报告 RecD2 在单轮和多轮条件下的 DNA 解旋动力学。当存在过量的 ssDNA 以捕获未结合到底物上的酶分子时,预先形成的 RecD2-dsDNA 复合物对 20bp 底物的解旋作用很小。在单轮条件下,较短的 12bp 底物迅速解旋。12bp 解旋反应可以用一个机制来模拟,其中 DNA 在两个动力学步骤中解旋,速率常数 k(unw) = 5.5 s(-1),从部分解旋的 DNA 中解离的速率常数 k(off) = 1.9 s(-1)。这些结果表明,动力学步长约为 3-4bp,解旋速率约为 15-20bp/s,且低的延伸性(p = 0.74)。在多轮条件下测定的 20bp 底物的反应时间过程可以用一个四步机制来模拟,并且速率常数值与 12bp 底物非常相似。结果表明,分叉末端的 DNA 底物比只有 5'端单链延伸的底物更快地解旋,可以用酶与 DNA 底物结合的速率差异来解释。用不同浓度的 RecD2 进行的反应分析表明,酶在高酶浓度下形成无活性的二聚体或其他寡聚体。RecD2 寡聚体可以通过戊二醛交联检测到,但不能通过分子筛层析检测到。

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