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Flp重组过程中活性位点酪氨酸介导的反式DNA切割:在交换链之前切换蛋白质伴侣。

DNA cleavage in trans by the active site tyrosine during Flp recombination: switching protein partners before exchanging strands.

作者信息

Chen J W, Lee J, Jayaram M

机构信息

Department of Microbiology, University of Texas, Austin 78712.

出版信息

Cell. 1992 May 15;69(4):647-58. doi: 10.1016/0092-8674(92)90228-5.

Abstract

Each recombination event mediated by the Flp recombinase is the sum of four strand breakage and reunion reactions executed in two steps of two-strand exchanges. The reaction requires four Flp monomers. The key catalytic residue in Flp is Tyr-343. Arg-191, His-305, and Arg-308 appear to facilitate the cleavage and exchange steps of recombination. These four residues constitute the invariant tetrad of the Int family site-specific recombinases. Complementation tests between "step-arrest" mutants of Flp suggest that each Flp protomer harbors a "fractional active site." Hybrid "half site-recombinase" complexes reveal that efficient catalysis occurs when the Arg-His-Arg triad is present on one Flp monomer and the active site Tyr on a second monomer. Strand cleavage by an Flp monomer occurs virtually exclusively on the half site to which its partner protein is bound (cleavage in trans), and almost never on the half site to which it is bound (cleavage in cis). Trans-cleavage by Flp can provide a means for functionally exchanging Flp monomers between two DNA partners. Such a mechanism would be germane to recombination, since cleavage and rejoining in cis can only restore the parental substrate configuration and cannot yield recombinants.

摘要

由Flp重组酶介导的每个重组事件都是在两步双链交换中执行的四个链断裂和重新连接反应的总和。该反应需要四个Flp单体。Flp中的关键催化残基是Tyr-343。Arg-191、His-305和Arg-308似乎促进了重组的切割和交换步骤。这四个残基构成了Int家族位点特异性重组酶的不变四联体。Flp的“步骤阻断”突变体之间的互补测试表明,每个Flp原体都含有一个“部分活性位点”。杂交“半位点重组酶”复合物表明,当Arg-His-Arg三联体存在于一个Flp单体上而活性位点酪氨酸存在于第二个单体上时,会发生高效催化。Flp单体的链切割几乎只发生在与其伴侣蛋白结合的半位点上(反式切割),而几乎从不发生在其自身结合的半位点上(顺式切割)。Flp的反式切割可以提供一种在两个DNA伴侣之间功能性交换Flp单体的方法。这样的机制与重组密切相关,因为顺式切割和重新连接只能恢复亲本底物构型,而不能产生重组体。

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