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Identification and characterization of mitochondrial abasic (AP)-endonuclease in mammalian cells

机译:哺乳动物细胞中线粒体无碱基(AP)-核酸内切酶的鉴定和表征

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摘要

Abasic (AP)-endonuclease (APE) is responsible for repair of AP sites, and single-strand DNA breaks with 3' blocking groups that are generated either spontaneously or during repair of damaged or abnormal bases via the DNA base excision repair (BER) pathway in both nucleus and mitochondria. Mammalian cells express only one nuclear APE, 36 kDa APE1, which is essential for survival. Mammalian mitochondrial (mt) BER enzymes other than mtAPE have been characterized. In order to identify and characterize mtAPE, we purified the APE activity from beef liver mitochondria to near homogeneity, and showed that the mtAPE which has 3-fold higher specific activity relative to APE1 is derived from the latter with deletion of 33 N-terminal residues which contain thenuclear localization signal. The mtAPE-sized product could be generated by incubating 35S-labeled APE1 with crude mitochondrial extract, but not with cytosolic or nuclear extract, suggesting that cleavage of APE1 by a specific mitochondria-associated N-terminal peptidase is a prerequisite for mitochondrial import. The low abundance of mtAPE, particularly in cultured cells might be the reason for its earlier lack of detection by western analysis.
机译:Abasic(AP)核酸内切酶(APE)负责AP位点的修复,单链DNA断裂带有3'封闭基团,这些断裂是在DNA碱基切除修复(BER)的过程中自发或在修复受损或异常碱基时产生的核和线粒体中的通路。哺乳动物细胞仅表达一种核APE,36 kDa APE1,这对于存活至关重要。除mtAPE以外,哺乳动物的线粒体(mt)BER酶已被鉴定。为了鉴定和表征mtAPE,我们从牛肉肝线粒体中纯化了APE活性至接近均一,并显示比活性比APE1高3倍的mtAPE来源于后者,并缺失了33个N端残基其中包含核定位信号。 mtAPE大小的产物可以通过将35S标记的APE1与粗线粒体提取物一起温育,而不是与胞质或核提取物一起温育来生产,这表明线粒体相关N末端肽酶对A​​PE1的切割是线粒体导入的前提条件。 mtAPE的丰度低,尤其是在培养的细胞中,可能是其早期无法通过Western分析检测到的原因。

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