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Hpy188I-DNA pre- and post-cleavage complexes-snapshots of the GIY-YIG nuclease mediated catalysis

机译:Hpy188I-DNA裂解前后复合物-GIY-YIG核酸酶介导的催化快照

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摘要

The GIY-YIG nuclease domain is present in all kingdoms of life and has diverse functions. It is found in the eukaryotic flap endonuclease and Holliday junction resolvase Slx1-Slx4, the prokaryotic nucleotide excision repair proteins UvrC and Cho, and in proteins of 'selfish' genetic elements. Here we present the structures of the ternary pre- and post-cleavage complexes of the type II GIY-YIG restriction endonuclease Hpy188I with DNA and a surrogate or catalytic metal ion, respectively. Our structures suggest that GIY-YIG nucleases catalyze DNA hydrolysis by a single substitution reaction. They are consistent with a previous proposal that a tyrosine residue (which we expect to occur in its phenolate form) acts as a general base for the attacking water molecule. In contrast to the earlier proposal, our data identify the general base with the GIY and not the YIG tyrosine. A conserved glutamate residue (Glu149 provided in trans in Hpy188I) anchors a single metal cation in the active site. This metal ion contacts the phosphate proS oxygen atom and the leaving group 3'-oxygen atom, presumably to facilitate its departure. Taken together, our data reveal striking analogy in the absence of homology between GIY-YIG and beta beta alpha-Me nucleases.
机译:GIY-YIG核酸酶结构域存在于所有生命王国中,并具有多种功能。在真核皮瓣内切核酸酶和霍利迪连接分辨酶Slx1-Slx4,原核核苷酸切除修复蛋白UvrC和Cho以及“自私”遗传元件蛋白中发现了它。在这里,我们介绍了II型GIY-YIG限制性核酸内切酶Hpy188I与DNA和替代或催化金属离子的三元裂解前后的复合物的结构。我们的结构表明,GIY-YIG核酸酶通过单个取代反应催化DNA水解。它们与以前的建议一致,即酪氨酸残基(我们期望以酚盐的形式出现)充当攻击性水分子的一般碱。与早先的提议相反,我们的数据确定了GIY而不是YIG酪氨酸的一般基础。保守的谷氨酸残基(Hpy188I中反式提供的Glu149)将单个金属阳离子锚定在活性位点。该金属离子与磷酸proS氧原子和离去基团3'-氧原子接触,以促进其离开。综上所述,我们的数据揭示了在GIY-YIG与beta beta alpha-Me核酸酶之间没有同源性的惊人相似之处。

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