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在由高度纯化的蛋白质重构的复制系统中对大肠杆菌DnaAcos蛋白的特性分析。

Characterization of Escherichia coli DnaAcos protein in replication systems reconstituted with highly purified proteins.

作者信息

Katayama T, Crooke E, Sekimizu K

机构信息

Department of Biochemistry, Stanford University School of Medicine, California 94305, USA.

出版信息

Mol Microbiol. 1995 Dec;18(5):813-20. doi: 10.1111/j.1365-2958.1995.18050813.x.

Abstract

Excessive initiation of chromosomal replication occurs in the dnaAcos mutant at 30 degrees C. Whereas purified wild-type DnA protein binds ATP and ADP tightly, DnaAcos protein is defective for such nucleotide binding. As initiation is a multistep reaction and DnaA protein functions at each step, activities of DnaAcos protein need to be examined precisely. DnaAcos protein specifically bound a DNA fragment containing the chromosomal replication origin with an affinity similar to that seen with the wild-type protein. In a system reconstituted with purified proteins at 30 degrees C, the mutant protein initiated replication of single-stranded DNA that contains a DnA-binding hairpin structure. Thus, DnaAcos protein basically sustains affinity to a DnaA-binding sequence and functions in the loading of DnaB helicase onto single-stranded DNA. Thermal stabilities of wild-type DnA and DnaAcos activities were comparable. Unlike wild-type DnaA protein, DnaAcos protein was inactive for minichromosomal replication in systems reconstituted with purified proteins in which the ATP-bound form of DnaA protein is required for initiation. Taken together, the data indicate that the prominent defect in DnaAcos protein appears to be the inability to bind nucleotide.

摘要

在30℃时,dnaAcos突变体中发生了染色体复制的过度起始。纯化的野生型Dna蛋白能紧密结合ATP和ADP,而DnaAcos蛋白在这种核苷酸结合方面存在缺陷。由于起始是一个多步骤反应,且DnaA蛋白在每个步骤中都发挥作用,因此需要精确检测DnaAcos蛋白的活性。DnaAcos蛋白特异性结合了一个包含染色体复制起点的DNA片段,其亲和力与野生型蛋白相似。在30℃用纯化蛋白重建的系统中,突变蛋白起始了含有Dna结合发夹结构的单链DNA的复制。因此,DnaAcos蛋白基本上维持了对DnaA结合序列的亲和力,并在将DnaB解旋酶加载到单链DNA上发挥作用。野生型Dna和DnaAcos活性的热稳定性相当。与野生型DnaA蛋白不同,在需要DnaA蛋白的ATP结合形式进行起始的用纯化蛋白重建的系统中,DnaAcos蛋白对微型染色体复制无活性。综上所述,数据表明DnaAcos蛋白的主要缺陷似乎是无法结合核苷酸。

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