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一种刺激大肠杆菌Rep蛋白解旋酶活性的蛋白质的鉴定与纯化。

Identification and purification of a protein that stimulates the helicase activity of the Escherichia coli Rep protein.

作者信息

Smith K R, Yancey J E, Matson S W

机构信息

Department of Biology, University of North Carolina, Chapel Hill 27599.

出版信息

J Biol Chem. 1989 Apr 15;264(11):6119-26.

PMID:2522929
Abstract

A polypeptide (Mr = 15,000) has been purified from Escherichia coli cell extracts that significantly stimulates the duplex DNA unwinding reaction catalyzed by E. coli Rep protein. The Rep helicase unwinding reaction was stimulated by as much as 20-fold, upon addition of the stimulatory protein, using either a 71-base pair or a 343-base pair partial duplex DNA molecule as a substrate. The purified Rep helicase stimulatory protein (RHSP) had no intrinsic helicase activity or ATP hydrolysis activity and did not stimulate the single-stranded DNA-dependent ATP hydrolysis reaction catalyzed by Rep protein. It is likely that RHSP stimulates the Rep helicase unwinding reaction by stoichiometric binding to single-stranded DNA. However, a specific interaction between Rep protein and RHSP cannot be ruled out, since RHSP did not stimulate the duplex DNA unwinding reactions catalyzed by E. coli helicase I or the recently discovered 75-kDa helicase. RHSP did stimulate the duplex DNA unwinding reaction catalyzed by E. coli helicase II. The identification and subsequent purification of RHSP from cell extracts demonstrates the feasibility of using direct helicase assays to purify stimulatory proteins.

摘要

已从大肠杆菌细胞提取物中纯化出一种多肽(分子量 = 15,000),它能显著刺激大肠杆菌Rep蛋白催化的双链DNA解旋反应。使用71碱基对或343碱基对的部分双链DNA分子作为底物,加入刺激蛋白后,Rep解旋酶的解旋反应被刺激了多达20倍。纯化的Rep解旋酶刺激蛋白(RHSP)没有内在的解旋酶活性或ATP水解活性,也不刺激Rep蛋白催化的单链DNA依赖性ATP水解反应。RHSP可能通过与单链DNA化学计量结合来刺激Rep解旋酶的解旋反应。然而,不能排除Rep蛋白与RHSP之间存在特异性相互作用,因为RHSP不刺激大肠杆菌解旋酶I或最近发现的75 kDa解旋酶催化的双链DNA解旋反应。RHSP确实刺激了大肠杆菌解旋酶II催化的双链DNA解旋反应。从细胞提取物中鉴定并随后纯化RHSP证明了使用直接解旋酶测定法纯化刺激蛋白的可行性。

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