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recA protein-catalyzed strand assimilation: stimulation by Escherichia coli single-stranded DNA-binding protein.

机译:recA蛋白催化的链同化:大肠杆菌单链DNA结合蛋白的刺激。

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摘要

The single-stranded DNA-binding protein of Escherichia coli significantly alters the strand assimilation reaction catalyzed by recA protein [McEntee, K., Weinstock, G. M. & Lehman, I. R. (1979) Proc. Natl. Acad. Sci. USA 76, 2615--2619]. The binding protein (i) increases the rate and extent of strand assimilation into homologous duplex DNA, (ii) enhances the formation of a complex between recA protein and duplex DNA in the presence of homologous or heterologous single-stranded DNA, (iii) reduces the rate and extent of ATP hydrolysis catalyzed by recA protein in the presence of single-stranded DNA, (iv) reduces the high concentration of recA protein required for strand assimilation, and (v) permits detection of strand assimilation in the presence of the ATP analog, adenosine 5'-O-(O-thiotriphosphate). Single-stranded DNA-binding protein purified from a binding protein mutant (lexC) is considerably less effective than wild-type binding protein in stimulating strand assimilation, a result which suggests that single-stranded DNA-binding protein participates in general recombination in vivo.
机译:大肠杆菌的单链DNA结合蛋白显着改变了recA蛋白催化的链同化反应[McEntee,K.,Weinstock,G.M。和Lehman,I.R。(1979)Proc.Natl.Acad.Sci.USA 90:5873-5877。 Natl。学院科学USA 76,2615--2619]。结合蛋白(i)增加了链同化成同源双链DNA的速率和程度,(ii)在存在同源或异源单链DNA的情况下增强了recA蛋白与双链DNA之间复合物的形成,(iii)降低了单链DNA存在下recA蛋白催化ATP水解的速率和程度,(iv)降低了链同化所需的recA蛋白的高浓度,并且(v)允许在ATP存在下检测链同化类似物,腺苷5'-O-(O-硫代三磷酸)。从结合蛋白突变体(lexC)纯化的单链DNA结合蛋白在刺激链同化方面远不如野生型结合蛋白有效,结果表明,单链DNA结合蛋白参与体内的一般重组。

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