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Flap核酸内切酶-1对含错配核苷酸底物的切割。对哺乳动物冈崎片段加工的影响。

Cleavage of substrates with mismatched nucleotides by Flap endonuclease-1. Implications for mammalian Okazaki fragment processing.

作者信息

Rumbaugh J A, Henricksen L A, DeMott M S, Bambara R A

机构信息

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

出版信息

J Biol Chem. 1999 May 21;274(21):14602-8. doi: 10.1074/jbc.274.21.14602.

DOI:10.1074/jbc.274.21.14602
PMID:10329652
Abstract

Flap endonuclease-1 (FEN1) is proposed to participate in removal of the initiator RNA of mammalian Okazaki fragments by two pathways. In one pathway, RNase HI removes most of the RNA, leaving a single ribonucleotide adjacent to the DNA. FEN1 removes this ribonucleotide exonucleolytically. In the other pathway, FEN1 removes the entire primer endonucleolytically after displacement of the 5'-end region of the Okazaki fragment. Cleavage would occur beyond the RNA, a short distance into the DNA. The initiator RNA and an adjacent short region of DNA are synthesized by DNA polymerase alpha/primase. Because the fidelity of DNA polymerase alpha is lower than that of the DNA polymerases that complete DNA extension, mismatches occur relatively frequently near the 5'-ends of Okazaki fragments. We have examined the ability of FEN1 to repair such errors. Results show that mismatched bases up to 15 nucleotides from the 5'-end of an annealed DNA strand change the pattern of FEN1 cleavage. Instead of removing terminal nucleotides sequentially, FEN1 appears to cleave a portion of the mismatched strand endonucleolytically. We propose that a mismatch destabilizes the helical structure over a nearby area. This allows FEN1 to cleave more efficiently, facilitating removal of the mismatch. If mismatches were not introduced during synthesis of the Okazaki fragment, helical disruption would not occur, nor would unnecessary degradation of the 5'-end of the fragment.

摘要

瓣内切核酸酶-1(FEN1)被认为通过两条途径参与去除哺乳动物冈崎片段的起始RNA。在一条途径中,核糖核酸酶H I去除大部分RNA,在DNA相邻处留下单个核糖核苷酸。FEN1通过核酸外切作用去除该核糖核苷酸。在另一条途径中,FEN1在冈崎片段5'端区域被置换后,通过核酸内切作用去除整个引物。切割将发生在RNA之外,进入DNA的短距离处。起始RNA和相邻的短DNA区域由DNA聚合酶α/引发酶合成。由于DNA聚合酶α的保真度低于完成DNA延伸的DNA聚合酶,错配在冈崎片段5'端附近相对频繁地发生。我们已经研究了FEN1修复此类错误的能力。结果表明,与退火DNA链5'端距离达15个核苷酸的错配碱基会改变FEN1的切割模式。FEN1似乎不是依次去除末端核苷酸,而是通过核酸内切作用切割错配链的一部分。我们提出,错配会使附近区域的螺旋结构不稳定。这使得FEN1能够更有效地切割,促进错配的去除。如果在冈崎片段合成过程中不引入错配,就不会发生螺旋破坏,片段5'端也不会发生不必要的降解。

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