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沃氏甲烷球菌的RadA的ATP酶活性需要第二个镁离子的结合。

Binding of a second magnesium is required for ATPase activity of RadA from Methanococcus voltae.

作者信息

Qian Xinguo, He Yujiong, Luo Yu

机构信息

Department of Biochemistry, University of Saskatchewan, A3 Health Sciences Building, 107 Wiggins Road, Saskatoon, Saskatchewan, Canada S7N 5E5.

出版信息

Biochemistry. 2007 May 22;46(20):5855-63. doi: 10.1021/bi6024098. Epub 2007 Apr 25.

DOI:10.1021/bi6024098
PMID:17455906
Abstract

RecA-like strand exchange proteins, which include closely related archaeal Rad51/RadA and eukaryal Rad51 and DMC1, play a key role in DNA repair by forming helical nucleoprotein filaments which promote a hallmark strand exchange reaction between homologous DNA substrates. Our recent crystallographic studies on a RadA recombinase from Methanococcus voltae (MvRadA) have unexpectedly revealed a secondary magnesium at the subunit interface approximately 11 A from the primary one coordinated by ATP and the canonical P-loop. The DNA-dependent ATPase activity of MvRadA appears to be dependent on the concentration of free Mg2+, while the strand exchange activity does not. We also made site-directed mutagenesis at the Mg2+-liganding residue Asp-246. The mutant proteins exhibited approximately 20-fold reduced ATPase activity but normal strand exchange activity. Structurally, the main chain carbonyl of the conserved catalytic residue Glu-151 is hydrogen bonded with one of the magnesium-liganding water molecules. Changes in the secondary magnesium site may therefore induce conformational changes around this catalytic glutamate and affect the ATPase activity without significantly altering the stability of the extended recombinase filament. Asp-246 is somewhat conserved among archaeal and eukaryal homologues, implying some homologues may share this allosteric site for ATPase function.

摘要

类RecA链交换蛋白,包括密切相关的古细菌Rad51/RadA以及真核生物Rad51和DMC1,通过形成螺旋核蛋白丝在DNA修复中发挥关键作用,该螺旋核蛋白丝促进同源DNA底物之间的标志性链交换反应。我们最近对来自沃氏甲烷球菌的RadA重组酶(MvRadA)的晶体学研究意外地揭示了在亚基界面处距离由ATP和典型P环配位的主要镁离子约11埃处存在一个二级镁离子。MvRadA的DNA依赖性ATP酶活性似乎取决于游离Mg2+的浓度,而链交换活性则不然。我们还对Mg2+配位残基Asp-246进行了定点诱变。突变蛋白的ATP酶活性降低了约20倍,但链交换活性正常。在结构上,保守催化残基Glu-151的主链羰基与其中一个与镁配位的水分子形成氢键。因此,二级镁离子位点的变化可能会在该催化谷氨酸周围诱导构象变化,并影响ATP酶活性,而不会显著改变延伸的重组酶丝的稳定性。Asp-246在古细菌和真核生物同源物中 somewhat conserved,这意味着一些同源物可能共享这个用于ATP酶功能的变构位点。 (注:“somewhat conserved”这里表述似乎不太准确,不太明确确切意思,按字面翻译为“有点保守” )

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