Bates H J, Farjah M, Osman T A, Buck K W
Department of Biology, Imperial College of Science, Technology and Medicine, London, UK.
J Gen Virol. 1995 Jun;76 ( Pt 6):1483-91. doi: 10.1099/0022-1317-76-6-1483.
A template-bound RNA polymerase was isolated from Nicotiana clevelandii plants infected with red clover necrotic mosaic dianthovirus (RCNMV) by differential centrifugation, solubilization with dodecyl beta-D-maltopyranoside, and chromatography on columns of Sephacryl S-400 and Q-Sepharose. Analysis of the purified polymerase by SDS-polyacrylamide gel electrophoresis, followed by silver staining or immunoblotting, showed that it contained virus-encoded proteins of molecular masses 27 kDa and 88 kDa together with several minor proteins possibly of host origin. After removal of endogenous RNA with micrococcal nuclease, the polymerase became template-dependent. It was also template-specific, being able to utilize as templates RNA of two strains of RCNMV, but not RNAs of three viruses in different taxonomic groups, namely cucumber mosaic cucumovirus, tomato bushy stunt tombusvirus and tomato mosaic tobamovirus. The products of RNA polymerase reactions were double-stranded RNAs corresponding to RCNMV RNAs 1 and 2. The ability of the template-dependent RNA polymerase to synthesize RNA was completely inhibited by antibodies to a peptide containing the GDD motif, whereas the activity of the template-bound enzyme was unaffected by these antibodies.
通过差速离心、用十二烷基-β-D-麦芽糖苷溶解以及在Sephacryl S-400和Q-Sepharose柱上进行层析,从感染了红三叶草坏死花叶病毒(RCNMV)的克利夫兰烟草植株中分离出一种模板结合型RNA聚合酶。通过SDS-聚丙烯酰胺凝胶电泳对纯化的聚合酶进行分析,随后进行银染或免疫印迹,结果表明它含有分子量为27 kDa和88 kDa的病毒编码蛋白以及几种可能源自宿主的次要蛋白。用微球菌核酸酶去除内源性RNA后,该聚合酶变得依赖模板。它也是模板特异性的,能够将两种RCNMV毒株的RNA用作模板,但不能将不同分类群中的三种病毒的RNA用作模板,即黄瓜花叶黄瓜病毒、番茄丛生矮缩番茄病毒和番茄花叶烟草花叶病毒。RNA聚合酶反应的产物是与RCNMV RNA 1和RNA 2相对应的双链RNA。含有GDD基序的肽的抗体完全抑制了模板依赖性RNA聚合酶合成RNA的能力,而模板结合型酶的活性不受这些抗体的影响。
