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脊髓灰质炎病毒2A(pro)对痘苗病毒基因表达的影响。

Effects of poliovirus 2A(pro) on vaccinia virus gene expression.

作者信息

Feduchi E, Aldabe R, Novoa I, Carrasco L

机构信息

Centro de Biología Molecular CSIC-UAM, Universidad Autónoma de Madrid, Spain.

出版信息

Eur J Biochem. 1995 Dec 15;234(3):849-54. doi: 10.1111/j.1432-1033.1995.849_a.x.

DOI:10.1111/j.1432-1033.1995.849_a.x
PMID:8575444
Abstract

The effects of transient expression of poliovirus 2A(pro) on p220 cleavage in COS cells have been analyzed. When 2A(pro) was cloned in plasmid pTM1 and transiently expressed in COS cells, efficient cleavage of p220 occurred after infection of these cells with a recombinant vaccinia virus bearing phage T7 RNA polymerase. High numbers of COS cells were transfected with pTM1-2A, as judged by p220 cleavage, thereby allowing an analysis of the effects of poliovirus 2A(pro) on vaccinia virus gene expression. A 40-50% cleavage of p220 by transfected poliovirus 2A(pro) was observed ten hours post infection and cleavage was almost complete (80-90%) 20-25 hours post infection with vaccinia virus. Profound inhibition of vaccinia virus protein synthesis was detectable ten hours post infection and was maximal 20-25 hours post infection. This inhibition resulted from neither a blockade of transcription of vaccinia virus nor a lack of translatability of the mRNAs present in cells that synthesize poliovirus 2A(pro). Addition of ara-C inhibited the replication of vaccinia virus and allowed the continued synthesis of cellular proteins. Under these conditions, 2A(pro) is expressed and blocks cellular translation. Finally, p220 cleavage by 2A(pro) did not inhibit the translation of a mRNA encoding poliovirus protein 2C, as directed by the 5' leader sequences of encephalomiocarditis virus. Therefore, these findings show a correlation between p220 cleavage and inhibition of translation from newly made mRNAs. Our results are discussed in the light of present knowledge of p220 function, and new approaches are considered that might provide further insights into the function(s) of initiation factor eIF-4F.

摘要

已分析脊髓灰质炎病毒2A(pro)瞬时表达对COS细胞中p220切割的影响。当将2A(pro)克隆到质粒pTM1中并在COS细胞中瞬时表达时,用携带噬菌体T7 RNA聚合酶的重组痘苗病毒感染这些细胞后,p220发生有效切割。根据p220切割情况判断,大量COS细胞用pTM1-2A转染,从而能够分析脊髓灰质炎病毒2A(pro)对痘苗病毒基因表达的影响。感染痘苗病毒后10小时观察到转染的脊髓灰质炎病毒2A(pro)对p220有40 - 50%的切割,感染后20 - 25小时切割几乎完全(80 - 90%)。感染后10小时可检测到痘苗病毒蛋白合成受到显著抑制,在感染后20 - 25小时达到最大抑制。这种抑制既不是由于痘苗病毒转录受阻,也不是由于合成脊髓灰质炎病毒2A(pro)的细胞中存在的mRNA缺乏可翻译性。添加阿糖胞苷抑制了痘苗病毒的复制并允许细胞蛋白的持续合成。在这些条件下,2A(pro)表达并阻断细胞翻译。最后,2A(pro)对p220的切割并不抑制由脑心肌炎病毒5'前导序列指导的编码脊髓灰质炎病毒蛋白2C的mRNA的翻译。因此,这些发现表明p220切割与对新合成mRNA翻译的抑制之间存在相关性。我们根据目前对p220功能的了解讨论了我们的结果,并考虑了可能为起始因子eIF - 4F的功能提供进一步见解的新方法。

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