首页> 美国卫生研究院文献>Nucleic Acids Research >Expression of largest RNA segment and synthesis of VP1 protein of bluetongue virus in insect cells by recombinant baculovirus: association of VP1 protein with RNA polymerase activity.
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Expression of largest RNA segment and synthesis of VP1 protein of bluetongue virus in insect cells by recombinant baculovirus: association of VP1 protein with RNA polymerase activity.

机译:重组杆状病毒在昆虫细胞中表达蓝舌病毒最大RNA片段并合成蓝舌病毒VP1蛋白:VP1蛋白与RNA聚合酶活性的关联。

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摘要

The bluetongue virus core particles have been shown to contain an RNA-directed RNA polymerase (1). To identify the protein responsible for the virion RNA polymerase activity, the complete 3.9 Kb DNA clone representing the largest RNA segment 1 (L1) of bluetongue virus (BTV-10) was placed under control of the polyhedrin promoter of Autographa californica nuclear polyhedrosis virus (AcNPV). The derived recombinant virus was used to infect Spodoptera frugiperda cells. As demonstrated by stained polyacrylamide gel electrophoresis and by the use of bluetongue virus antibody, infected insect cells synthesized the largest protein of BTV-10 (VP1, 150 k Da). Antibody raised in rabbit to recombinant VP1 protein recognized bluetongue virus VP1 protein. The recombinant virus infected cell lysate had significantly inducible levels of RNA polymerase enzymatic activity as determined by a poly (U)-oligo (A) polymerase assay. The availability of enzymatically active bluetongue virus RNA polymerase provides a system in which we can precisely delineate the role this protein plays in the regulation of bluetongue replication.
机译:蓝舌病毒核心颗粒已显示含有RNA定向的RNA聚合酶(1)。为了鉴定负责病毒体RNA聚合酶活性的蛋白质,将代表蓝舌病病毒(BTV-10)的最大RNA片段1(L1)的完整3.9 Kb DNA克隆置于加利福尼亚州卷柏核多角体病毒多面体启动子的控制下( AcNPV)。衍生的重组病毒用于感染草地贪夜蛾细胞。如通过染色的聚丙烯酰胺凝胶电泳和使用蓝舌病毒抗体所证明,被感染的昆虫细胞合成了最大的BTV-10蛋白(VP1,150 k Da)。在兔中产生的针对重组VP1蛋白的抗体识别了蓝舌病毒VP1蛋白。重组病毒感染的细胞裂解液具有可诱导水平的RNA聚合酶酶活性,如通过聚(U)-寡(A)聚合酶测定法所确定的。具有酶活性的蓝舌病病毒RNA聚合酶的可用性提供了一个系统,在该系统中,我们可以精确地描述该蛋白在调节蓝舌病复制中的作用。

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