Tsuchihashi Z, Kornberg A
Department of Biochemistry, Stanford University School of Medicine, California 94305.
J Biol Chem. 1989 Oct 25;264(30):17790-5.
The tau and gamma subunits of the DNA polymerase III holoenzyme of Escherichia coli were each isolated in large quantities as oligomers from overproducing cells in which their genes (dnaZ and X) were under the control of a T7 phage promoter. The 52-kDa gamma subunit (encoded by the dnaZ sequence) contains three-forths of the N-terminal residues of the 71-kDa tau subunit (encoded by the dnaX sequence). Both gamma and tau share a binding site for ATP (or dATP). A DNA-dependent ATPase activity (Lee, S.H., and Walker, J.R. (1987) Proc. Natl. Acad. Sci. U. S. A. 84, 2713-2717) exhibited only by the tau subunit, presumably requires a DNA-binding site in the C-terminal domain lacking in the gamma subunit. Among ATPases dependent on single-stranded DNA, the tau activity is remarkable in the failure of homopolymers (e.g. poly(dA) or poly(dT)) to replace natural DNAs. The presumed need for certain secondary structures may reflect a feature of template binding in the crucial contribution that tau makes to the high processivity of polymerase III holoenzyme. Limited tryptic digestion of tau generates a fragment that resembles gamma in: (i) size, (ii) binding of ATP without ATPase activity, and (iii) a level of complementing holoenzyme activity in extracts of dnaZ-mutant cells that is higher than that of tau.
大肠杆菌DNA聚合酶III全酶的τ和γ亚基均从过量表达细胞中大量分离得到,呈寡聚体形式,在这些细胞中,它们的基因(dnaZ和X)受T7噬菌体启动子控制。52 kDa的γ亚基(由dnaZ序列编码)包含71 kDa的τ亚基(由dnaX序列编码)四分之三的N端残基。γ和τ都有一个ATP(或dATP)结合位点。一种仅由τ亚基表现出的依赖DNA的ATP酶活性(Lee, S.H., and Walker, J.R. (1987) Proc. Natl. Acad. Sci. U. S. A. 84, 2713 - 2717),推测需要γ亚基所缺乏的C端结构域中的一个DNA结合位点。在依赖单链DNA的ATP酶中,τ的活性在同聚物(如聚(dA)或聚(dT))不能替代天然DNA方面表现突出。对某些二级结构的推测需求可能反映了模板结合的一个特征,这是τ对聚合酶III全酶的高持续性起关键作用的体现。用胰蛋白酶对τ进行有限消化会产生一个片段,该片段在以下方面与γ相似:(i)大小,(ii)结合ATP但无ATP酶活性,以及(iii)在dnaZ突变体细胞提取物中补充全酶活性的水平高于τ。
