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与酵母DNA聚合酶α复合物相关的依赖DNA的ATP酶及DNA解旋活性的特性分析。

Characterization of the DNA-dependent ATPase and a DNA unwinding activity associated with the yeast DNA polymerase alpha complex.

作者信息

Biswas E E, Ewing C M, Biswas S B

机构信息

Department of Pediatrics, University of Maryland School of Medicine, Baltimore 21201.

出版信息

Biochemistry. 1993 Mar 30;32(12):3020-6. doi: 10.1021/bi00063a013.

DOI:10.1021/bi00063a013
PMID:8384485
Abstract

We have analyzed the ATPase and dATPase activities associated with the yeast DNA polymerase alpha complex. The ATPase/dATPase was primarily a single-stranded DNA-dependent ATPase. Analysis of the stimulatory effect of a large number of DNA substrates demonstrated that polynucleotides longer than 60 nucleotides (nts) had the maximal effect. The stimulation by oligonucleotides smaller than 60 nts, in general, decreased proportionally with decreased length of the oligomer. Poly- or oligopyrimidines were twice as stimulatory as the poly- or oligopurines of the same length. In addition to DNA, replication protein A (RP-A), a single-stranded DNA (ssDNA) binding protein, also stimulated the ATPase activity. Photo-cross-linking of the ATP binding component of the pol alpha complex to [alpha-32P]ATP at 0 degree C resulted in the exclusive labeling of a 90-kDa polypeptide. The labeling was inhibited by ATP and dATP but not by any other ribo- or deoxynucleotides, which suggest that the 90-kDa polypeptide is specific for ATP/dATP binding and possibly the active site for the ATPase/dATPase. We have also reported here a novel DNA unwinding activity associated with the multiprotein complex of DNA polymerase alpha. The complex was able to unwind M13mp19 ssDNA hybridized to an oligonucleotide (17-60 nucleotides long) with a protruding 3'-terminus. Regardless of the size of the duplex, the DNA unwinding was significantly stimulated by RP-A, while RP-A itself did not have any DNA unwinding activity. Consequently, it appeared that the DNA polymerase alpha complex possessed a putative RP-A-dependent helicase activity.(ABSTRACT TRUNCATED AT 250 WORDS)

摘要

我们分析了与酵母DNA聚合酶α复合物相关的ATP酶和dATP酶活性。该ATP酶/dATP酶主要是一种单链DNA依赖性ATP酶。对大量DNA底物的刺激作用分析表明,长度超过60个核苷酸(nts)的多核苷酸具有最大效应。一般来说,小于60 nts的寡核苷酸的刺激作用会随着寡聚物长度的减少而成比例降低。相同长度的聚嘧啶或寡嘧啶的刺激作用是聚嘌呤或寡嘌呤的两倍。除了DNA外,单链DNA(ssDNA)结合蛋白复制蛋白A(RP - A)也能刺激ATP酶活性。在0℃下,将pol α复合物的ATP结合成分与[α - 32P]ATP进行光交联,结果专一性地标记了一条90 kDa的多肽。该标记受到ATP和dATP的抑制,但不受任何其他核糖核苷酸或脱氧核苷酸的抑制,这表明90 kDa的多肽对ATP/dATP结合具有特异性,可能是ATP酶/dATP酶的活性位点。我们在此还报道了一种与DNA聚合酶α多蛋白复合物相关的新型DNA解旋活性。该复合物能够解开与一段寡核苷酸(17 - 60个核苷酸长)杂交且具有3'突出末端的M13mp19单链DNA。无论双链的大小如何,DNA解旋都受到RP - A的显著刺激,而RP - A本身没有任何DNA解旋活性。因此,似乎DNA聚合酶α复合物具有一种假定的依赖于RP - A的解旋酶活性。(摘要截短于250字)

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引用本文的文献

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Proc Natl Acad Sci U S A. 1993 Dec 15;90(24):11543-7. doi: 10.1073/pnas.90.24.11543.