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痘苗病毒DNA引发酶的产物及底物/模板使用情况

Products and substrate/template usage of vaccinia virus DNA primase.

作者信息

De Silva Frank S, Paran Nir, Moss Bernard

机构信息

Laboratory of Viral Diseases, National Institute of Allergy and Infectious Diseases, National Institutes of Health, Bethesda, MD 20892-0445, USA.

出版信息

Virology. 2009 Jan 5;383(1):136-41. doi: 10.1016/j.virol.2008.10.008. Epub 2008 Nov 12.

DOI:10.1016/j.virol.2008.10.008
PMID:19007959
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC2630392/
Abstract

Vaccinia virus encodes a 90-kDa protein conserved in all poxviruses, with DNA primase and nucleoside triphosphatase activities. DNA primase products, synthesized with a single stranded varphiX174 DNA template, were resolved as dinucleotides and long RNAs on denaturing polyacrylamide and agarose gels. Following phosphatase treatment, the dinucleotides GpC and ApC in a 4:1 ratio were identified by nearest neighbor analysis in which (32)P was transferred from [alpha-(32)P]CTP to initiating purine nucleotides. Differences in the nucleotide binding sites for initiation and elongation were suggested by the absence of CpC and UpC dinucleotides as well as the inability of deoxynucleotides to mediate primer synthesis despite their incorporation into mixed RNA/DNA primers. Strong primase activity was detected with an oligo(dC) template. However, there was only weak activity with an oligo(dT) template and none with oligo(dA) or oligo(dG). The absence of stringent template specificity is consistent with a role for the enzyme in priming DNA synthesis at the replication fork.

摘要

痘苗病毒编码一种在所有痘病毒中都保守的90 kDa蛋白,具有DNA引发酶和核苷三磷酸酶活性。用单链φX174 DNA模板合成的DNA引发酶产物,在变性聚丙烯酰胺和琼脂糖凝胶上被解析为二核苷酸和长RNA。磷酸酶处理后,通过邻位分析鉴定出比例为4:1的二核苷酸GpC和ApC,其中(32)P从[α-(32)P]CTP转移到起始嘌呤核苷酸上。起始和延伸的核苷酸结合位点的差异表现为不存在CpC和UpC二核苷酸,以及脱氧核苷酸尽管能掺入混合RNA/DNA引物中但无法介导引物合成。用寡聚(dC)模板检测到强引发酶活性。然而,用寡聚(dT)模板时活性较弱,用寡聚(dA)或寡聚(dG)时则无活性。缺乏严格的模板特异性与该酶在复制叉处引发DNA合成的作用一致。

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