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小鼠细胞DNA中对无嘌呤/无嘧啶位点具有特异性的线粒体核酸内切酶活性。

Mitochondrial endonuclease activities specific for apurinic/apyrimidinic sites in DNA from mouse cells.

作者信息

Tomkinson A E, Bonk R T, Linn S

机构信息

Department of Biochemistry, University of California, Berkeley 94720.

出版信息

J Biol Chem. 1988 Sep 5;263(25):12532-7.

PMID:2457585
Abstract

Endonuclease activity which specifically cleaves baseless (apurinic/apyrimidinic (AP] sites in supercoiled DNA has been purified from mitochondria of the mouse plasmacytoma cell line, MPC-11. Two variant forms separate upon purification; these have small but reproducible differences in catalytic and chromatographic properties, but similar physical properties. Both have a sedimentation coefficient of 4.0, corresponding to a molecular weight of 61,000 (assuming a globular configuration) and a peptide molecular weight of about 65,000 as determined by immunoblot analysis with antiserum raised against the major AP endonuclease from HeLa cells. Thus mitochondrial AP endonuclease appears to be a monomer of about 65 kDa, making it distinguishable from the major AP endonuclease of MPC-11 cells which, like those of other mammalian cells, appears to be a monomer of about 41 kDa. A possible 82-kDa precursor form was also detected by immunoblot analysis of a crude mitochondrial fraction. Mitochondrial AP endonuclease activity is greatly stimulated by divalent cations, has a pH optimum between 6.5 and 8.5, and cleaves the AP site by a class II mechanism to generate a 3'-OH nucleotide residue. These properties resemble those of the major mammalian AP endonucleases but, unlike those enzymes, mitochondrial AP endonuclease activity is neither inhibited by adenine or NAD+ nor stimulated by Triton X-100. Since the mitochondrial activity generates active primer termini for DNA synthesis, it could function in base excision DNA repair; alternatively, it might have a role in eliminating damaged mitochondrial genomes from the gene pool.

摘要

已从小鼠浆细胞瘤细胞系MPC - 11的线粒体中纯化出一种内切核酸酶活性,该活性可特异性切割超螺旋DNA中的无碱基(脱嘌呤/脱嘧啶(AP))位点。纯化后分离出两种变体形式;它们在催化和色谱性质上有微小但可重复的差异,但物理性质相似。两者的沉降系数均为4.0,对应分子量为61,000(假设为球状结构),通过用针对来自HeLa细胞的主要AP内切核酸酶产生的抗血清进行免疫印迹分析确定,其肽分子量约为65,000。因此,线粒体AP内切核酸酶似乎是一种约65 kDa的单体,这使其与MPC - 11细胞的主要AP内切核酸酶不同,后者与其他哺乳动物细胞的类似,似乎是一种约41 kDa的单体。通过对粗线粒体部分的免疫印迹分析还检测到一种可能的82 kDa前体形式。线粒体AP内切核酸酶活性受到二价阳离子的极大刺激,最适pH在6.5至8.

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