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Comparison of Turnip Crinkle Virus RNA-Dependent RNA Polymerase Preparations Expressed in Escherichia coli or Derived from Infected Plants

机译:在大肠杆菌中表达或衍生自被感染植物的芜菁皱纹病毒RNA依赖性RNA聚合酶制剂的比较

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摘要

Turnip crinkle virus (TCV) is a small, plus-sense, single-stranded RNA virus of plants. A virus-coded protein, p88, which is required for replication has been expressed and purified from Escherichia coli. In vitro assays revealed that the recombinant p88 has an RNA-dependent RNA polymerase (RdRp) activity and can also bind to RNA. Deletion of the N-terminal region in p88 resulted in a more active RdRp, while further deletions abolished RdRp activity. Comparison of the E. coli-expressed p88, the N-terminal deletion mutant of p88, and a TCV RdRp preparation obtained from infected plants revealed that these preparations show remarkable similarities in RNA template recognition and usage. Both the recombinant and the plant TCV RdRp preparations are capable of de novo initiation on both plus- and minus-strand satC and satD templates, which are small parasitic RNAs associated with TCV infections. In addition, these RdRp preparations can efficiently recognize the related Tomato bushy stunt virus promoter sequences, including the minus- and plus-strand initiation promoters. Heterologous viral and artificial promoters are recognized poorly by the recombinant and the plant TCV RdRps. Further comparison of the single-component recombinant TCV RdRp and the multicomponent plant TCV RdRp will help dissect the functions of various components of the TCV replicase.
机译:芜菁皱纹病毒(TCV)是植物的一种小巧的单链RNA病毒。从大肠杆菌表达并纯化了复制所需的病毒编码蛋白p88。体外测定显示重组p88具有RNA依赖性RNA聚合酶(RdRp)活性,并且还可以与RNA结合。 p88中N末端区域的删除导致更活跃的RdRp,而进一步的删除则取消了RdRp的活性。比较大肠杆菌表达的p88,p88的N末端缺失突变体和从受感染植物中获得的TCV RdRp制剂,发现这些制剂在RNA模板识别和使用方面显示出显着的相似性。重组和植物TCV RdRp制剂均能够在正链和负链satC和satD模板上从头启动,这些模板是与TCV感染相关的小型寄生RNA。此外,这些RdRp制剂可以有效识别相关的番茄浓密特技病毒启动子序列,包括负链和正链启动子。重组和植物TCV RdRps对异源病毒和人工启动子的识别较差。单组分重组TCV RdRp和多组分植物TCV RdRp的进一步比较将有助于剖析TCV复制酶各种组分的功能。

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