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首页> 外文期刊>Virus Research: An International Journal of Molecular and Cellular Virology >RECOMBINANT-BACULOVIRUS-EXPRESSED PB2 SUBUNIT OF THE INFLUENZA A VIRUS RNA POLYMERASE BINDS CAP GROUPS AS AN ISOLATED SUBUNIT
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RECOMBINANT-BACULOVIRUS-EXPRESSED PB2 SUBUNIT OF THE INFLUENZA A VIRUS RNA POLYMERASE BINDS CAP GROUPS AS AN ISOLATED SUBUNIT

机译:重组杆状病毒表达的PB2亚型流感病毒RNA聚合酶将帽基团作为一个分离的亚基

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摘要

The influenza A virus RNA-dependent RNA polymerase catalyzes several reactions in transcription and replication of the genome RNA. The first step in viral mRNA synthesis is the recognition of the 5' end cap structure of host cell hnRNA and the cleavage of the RNA substrate between 10 and 14 nucleotides from the 5' end to generate capped primers for initiation of transcription of virus-specific mRNAs. This report describes the use of an in vitro UV crosslinking and protein renaturation assay to identify the polymerase subunits which interact with the 5' end cap structure of an artificial RNA substrate. Our results showed, for the first time; that purified polymerase subunit PB2 expressed by recombinant baculovirus in insect cells possessed cap-binding activity by itself after renaturation by Escherichia coli thioredoxin, whereas cleavage of the artificial capped substrate required the holoenzyme expressed in insect cells triply-infected with baculovirus containing all three polypeptide components, PB1, PB2, and PA. Purified polyclonal anti-PB2 IgG inhibited the binding activity; anti-PB1 and anti-PA IgGs did not.
机译:甲型流感病毒RNA依赖性RNA聚合酶催化基因组RNA的转录和复制中的若干反应。病毒mRNA合成的第一步是识别宿主细胞hnRNA的5'末端帽结构,并从5'末端切割10到14个核苷酸之间的RNA底物,以产生用于引发病毒特异性转录的带帽引物mRNA。该报告描述了使用体外紫外线交联和蛋白质复性测定法来鉴定与人工RNA底物的5'端帽结构相互作用的聚合酶亚基。我们的结果首次显示;重组杆状病毒在昆虫细胞中表达的纯化的聚合酶亚基PB2在被大肠杆菌硫氧还蛋白复性后具有自身的帽结合活性,而人工带帽底物的裂解则需要在含有所有三种多肽成分的杆状病毒三次感染的昆虫细胞中表达的全酶,PB1,PB2和PA。纯化的多克隆抗PB2 IgG抑制了结合活性。抗PB1和抗PA IgG则没有。

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