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首页> 外文期刊>Journal of Virology >Isolation and Characterization of an RNA-Dependent RNA Polymerase from Black Beetle Virus-Infected Drosophila melanogaster Cells
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Isolation and Characterization of an RNA-Dependent RNA Polymerase from Black Beetle Virus-Infected Drosophila melanogaster Cells

机译:来自黑甲虫病毒感染的RNA依赖性RNA聚合酶的分离和表征来自黑甲虫病毒感染的果蝇细胞

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摘要

Crude lysates of black beetle virus (BBV)-infected cells of Drosophila melanogaster contain an RNA-dependent RNA polymerase activity not detectable in uninfected cells. The activity (designated BBV polymerase) sedimented at 20,000 × g, indicating an association with particulate material. It was solubilized from the pellet by sonication in a magnesium-deficient buffer. Differential centrifugation resulted in a 43-fold purification with 84% recovery of polymerase activity. The effects of divalent and monovalent cations, time, temperature, and pH on the activity of the partially purified polymerase were examined. RNA synthesis was not stimulated by the addition of exogenous BBV RNA, suggesting that an enzyme-template complex existed. Analysis of the RNA products of the RNA polymerase reaction indicated that full-length “negative” strand BBV RNAs were synthesized.
机译:黑甲虫病毒(BBV)的粗裂解物 - 果蝇黑素转渣的感染细胞含有在未感染的细胞中未检测到的RNA依赖性RNA聚合酶活性。将活性(指定的BBV聚合酶)沉淀在20,000× G ,表明与颗粒材料相关联。它通过在缺镁缓冲液中通过超声处理从颗粒中溶解。差动离心导致43倍纯化,聚合酶活性84%回收率。研究了二价和单价阳离子,时间,温度和pH对部分纯化聚合酶活性的影响。通过添加外源BBV RNA没有刺激RNA合成,表明存在酶模板复合物。 RNA聚合酶反应的RNA产物分析表明,合成了全长的“阴性”链BBV RNA。

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