DNA聚合酶III与大肠杆菌诱变基因mutD产物的相互作用。
The interaction of DNA polymerase III and the product of the Escherichia coli mutator gene, mutD.
作者信息
DiFrancesco R, Bhatnagar S K, Brown A, Bessman M J
出版信息
J Biol Chem. 1984 May 10;259(9):5567-73.
A comparison of DNA polymerase III core enzyme (McHenry, C. S., and Crow, W. (1979) J. Biol. Chem. 254, 1748-1753) prepared from wild type Escherichia coli and a strain harboring the mutator gene, mutD5 (Degnen, G. E., and Cox, E. C. (1974) J. Bacteriol. 17, 477-487) has revealed several differences in their properties. Among these are alterations in the heat stability, divalent cation requirement, pH optimum, 3'----5'-single strand exonuclease activity, and DNA-dependent conversion of a deoxynucleoside triphosphate to its corresponding monophosphate ("turnover"). The decrease in the 3'-single strand exonuclease and turnover indicate a defect in the editing function of the mutD strain, which is at least in part responsible for the high spontaneous mutation rate in mutD. Transformation of mutD by a hybrid plasmid, pRD3, constructed from an EcoRI restriction fragment of E. coli and pBR322, cures mutD of its abnormally high mutation rate, and simultaneously restores its 3'-exonuclease activity. These observations are consistent with the notion that the mutD gene product is a subunit of DNA polymerase III, and it either contains the catalytic site for the 3'-exonuclease or modulates its activity. From a consideration of the known molecular weights of the subunits in DNA polymerase III core (McHenry C. S., and Crow, W. (1979) J. Biol. Chem. 254, 1748-1753) the molecular weights of the two proteins translated in maxicells transformed with pRD3, and from a comparison of our results with those obtained with the mutator dnaQ (Horiuchi, T., Maki, H., Maruyama, M., and Sekiguchi, M. (1981) Proc. Natl. Acad. Sci. U. S. A. 78, 3770-3774) and the work of Cox and Horner (Cox, E. C., and Horner, D. L. (1983) Proc. Natl. Acad. Sci. U. S. A. 80, 2295-2299) as well as Echols et al. (Echols, H., Lu, C., and Burgers, P. M. J. (1983) Proc. Natl. Acad. Sci. U. S. A. 80, 2189-2192) we tentatively assign the mutD gene product to the epsilon subunit of DNA polymerase III.
对从野生型大肠杆菌以及携带突变基因mutD5的菌株中制备的DNA聚合酶III核心酶(麦克亨利,C.S.,和克劳,W.(1979年)《生物化学杂志》254卷,1748 - 1753页)进行比较,发现它们在性质上存在若干差异。其中包括热稳定性、二价阳离子需求、最适pH值、3'→5'单链外切核酸酶活性以及脱氧核苷三磷酸向其相应单磷酸的DNA依赖性转化(“周转”)的改变。3'单链外切核酸酶和周转的降低表明mutD菌株的编辑功能存在缺陷,这至少部分导致了mutD中高自发突变率。用由大肠杆菌的EcoRI限制片段和pBR322构建的杂交质粒pRD3转化mutD,可消除其异常高的突变率,并同时恢复其3'外切核酸酶活性。这些观察结果与以下观点一致,即mutD基因产物是DNA聚合酶III的一个亚基,它要么包含3'外切核酸酶的催化位点,要么调节其活性。通过考虑DNA聚合酶III核心中亚基的已知分子量(麦克亨利,C.S.,和克劳,W.(1979年)《生物化学杂志》254卷,1748 - 1753页)、用pRD3转化的最大细胞中翻译的两种蛋白质的分子量,以及将我们的结果与用突变体dnaQ(堀内,T.,牧木,H.,丸山,M.,和关口,M.(1981年)《美国国家科学院院刊》78卷,3770 - 3774页)以及考克斯和霍纳(考克斯,E.C.,和霍纳,D.L.(1983年)《美国国家科学院院刊》80卷,2295 - 2299页)以及埃科尔斯等人(埃科尔斯,H.,卢,C.,和伯格斯,P.M.J.(1983年)《美国国家科学院院刊》80卷,2189 - 2192页)的研究结果进行比较,我们初步将mutD基因产物归为DNA聚合酶III的ε亚基。
Zotero 插件