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大肠杆菌核酸外切酶VII的亚基结构。

Subunit structure of Escherichia coli exonuclease VII.

作者信息

Vales L D, Rabin B A, Chase J W

出版信息

J Biol Chem. 1982 Aug 10;257(15):8799-805.

PMID:6284744
Abstract

Exonuclease VII has been purified 7,500-fold to 87% homogeneity from Escherichia coli K12 using a new purification procedure. The enzyme has been shown to be composed of two nonidentical subunits of 10,500 and 54,000 daltons. This has been confirmed by restoration of exonuclease VII activity after renaturation of denatured and purified subunits. The structure of the native enzyme consists of one large subunit and four small subunits. We have previously isolated exonuclease VII mutant strains containing defects which map at two distinct loci. Subunit-mixing experiments utilizing wild type enzyme and temperature-sensitive enzyme produced by an xseB mutant strain have shown that the xseB gene codes for the small subunit of the enzymes.

摘要

利用一种新的纯化方法,已从大肠杆菌K12中纯化出核酸外切酶VII,纯化倍数达7500倍,纯度为87%。该酶已被证明由两个不同的亚基组成,分子量分别为10500和54000道尔顿。变性和纯化后的亚基复性后核酸外切酶VII活性的恢复证实了这一点。天然酶的结构由一个大亚基和四个小亚基组成。我们之前分离出了核酸外切酶VII突变菌株,这些菌株含有位于两个不同位点的缺陷。利用野生型酶和xseB突变菌株产生的温度敏感型酶进行的亚基混合实验表明,xseB基因编码该酶的小亚基。

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