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痘苗病毒颗粒蛋白I8R具有DNA和RNA解旋酶活性:对痘苗病毒转录的影响

Vaccinia virion protein I8R has both DNA and RNA helicase activities: implications for vaccinia virus transcription.

作者信息

Bayliss C D, Smith G L

机构信息

Sir William Dunn School of Pathology, University of Oxford, United Kingdom.

出版信息

J Virol. 1996 Feb;70(2):794-800. doi: 10.1128/JVI.70.2.794-800.1996.

Abstract

A nucleic acid-dependent ATPase was purified from vaccinia virions and shown to have both DNA:DNA and RNA:RNA helicase activities. This is only the third helicase to be identified that can unwind both DNA and RNA duplexes. The DNA helicase activity copurified with nucleoside triphosphate phosphohydrolase II (NPHII), an RNA helicase encoded by gene I8R (S. Shuman, Proc. Natl. Acad. Sci. USA 89:10935-10939, 1992). Immunodepletion with two antisera to NPHII and analysis of recombinant NPHII protein (C. H. Gross and S. Shuman, J. Virol. 69:4727-4736, 1995) confirmed that the DNA helicase activity was encoded by the I8R gene. The I8R DNA helicase unwound DNA in a 3'-to-5' direction only, unwound duplexes of 35 bp but not 45 bp, and could be stimulated to unwind longer duplexes by the Escherichia coli single-stranded DNA-binding protein. DNA helicase activity was not stimulated by salt and was sensitive to 100 mM NaCl or KCl. The I8R protein has amino acid similarity to human RNA helicase A and to nuclear DNA helicase II, a bovine DNA and RNA helicase. On the basis of the phenotype of I8R temperature-sensitive mutants, it was suggested that the I8R protein is not required for DNA replication but might aid in the extrusion of early mRNA from the virus core. The DNA helicase activity of the I8R protein allows another interpretation of the mutant phenotype, namely, that the I8R DNA helicase activity is required for initiation of early transcription from within vaccinia virions.

摘要

从痘苗病毒颗粒中纯化出一种依赖核酸的ATP酶,它具有DNA:DNA和RNA:RNA解旋酶活性。这是已鉴定出的第三种既能解开DNA双链又能解开RNA双链的解旋酶。DNA解旋酶活性与核苷三磷酸磷酸水解酶II(NPHII)共纯化,NPHII是由I8R基因编码的一种RNA解旋酶(S. 舒曼,《美国国家科学院院刊》89:10935 - 10939,1992)。用两种针对NPHII的抗血清进行免疫去除以及对重组NPHII蛋白的分析(C. H. 格罗斯和S. 舒曼,《病毒学杂志》69:4727 - 4736,1995)证实,DNA解旋酶活性由I8R基因编码。I8R DNA解旋酶仅沿3'至5'方向解开DNA,能解开35 bp的双链但不能解开45 bp的双链,并且可被大肠杆菌单链DNA结合蛋白刺激以解开更长的双链。DNA解旋酶活性不受盐的刺激,对100 mM NaCl或KCl敏感。I8R蛋白与人类RNA解旋酶A以及核DNA解旋酶II(一种牛的DNA和RNA解旋酶)具有氨基酸相似性。基于I8R温度敏感突变体的表型,有人提出I8R蛋白对于DNA复制不是必需的,但可能有助于早期mRNA从病毒核心中挤出。I8R蛋白的DNA解旋酶活性对突变体表型有另一种解释,即I8R DNA解旋酶活性是痘苗病毒颗粒内早期转录起始所必需的。

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