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小牛5'至3'外切/内切核酸酶必须从底物的5'末端滑动以进行结构特异性切割。

Calf 5' to 3' exo/endonuclease must slide from a 5' end of the substrate to perform structure-specific cleavage.

作者信息

Murante R S, Rust L, Bambara R A

机构信息

Department of Biochemistry, University of Rochester School of Medicine and Dentistry, New York 14642, USA.

出版信息

J Biol Chem. 1995 Dec 22;270(51):30377-83. doi: 10.1074/jbc.270.51.30377.

Abstract

Calf 5' to 3' exo/endonuclease, the counterpart of the human FEN-1 and yeast RTH-1 nucleases, performs structure-specific cleavage of both RNA and DNA and is implicated in Okazaki fragment processing and DNA repair. The substrate for endonuclease activity is a primer annealed to a template but with a 5' unannealed tail. The results presented here demonstrate that the nuclease must enter the 5' end of the unannealed tail and then slide to the region of hybridization where the cleavage occurs. The presence of bound protein or a primer at any point on the single-stranded tail prevents cleavage. However, biotinylation of a nucleotide at the 5' end or internal to the tail does not prevent cleavage. The sliding process is bidirectional. If the nuclease slides onto the tail, later binding of a primer to the tail traps the nuclease between the primer binding site and the cleavage site, preventing the nuclease from departing from the 5' end. A model for 5' entry, sliding, and cleavage is presented. The possible role of this unusual mechanism in Okazaki fragment processing, DNA repair, and protection of the replication fork from inappropriate endonucleolytic cleavage is presented.

摘要

小牛5'至3'外切/内切核酸酶,是人类FEN-1和酵母RTH-1核酸酶的对应物,可对RNA和DNA进行结构特异性切割,并参与冈崎片段加工和DNA修复。内切核酸酶活性的底物是与模板退火但带有5'未退火尾巴的引物。此处呈现的结果表明,核酸酶必须进入未退火尾巴的5'端,然后滑向发生切割的杂交区域。单链尾巴上任何位置存在结合蛋白或引物都会阻止切割。然而,在尾巴的5'端或内部对核苷酸进行生物素化不会阻止切割。滑动过程是双向的。如果核酸酶滑到尾巴上,随后引物与尾巴的结合会将核酸酶捕获在引物结合位点和切割位点之间,阻止核酸酶从5'端离开。本文提出了一个5'端进入、滑动和切割的模型。阐述了这种独特机制在冈崎片段加工、DNA修复以及保护复制叉免受不适当内切核酸酶切割方面可能发挥的作用。

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