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脊髓灰质炎病毒蛋白酶2A诱导真核起始因子4F多肽p220的裂解。

Poliovirus proteinase 2A induces cleavage of eucaryotic initiation factor 4F polypeptide p220.

作者信息

Kräusslich H G, Nicklin M J, Toyoda H, Etchison D, Wimmer E

出版信息

J Virol. 1987 Sep;61(9):2711-8. doi: 10.1128/JVI.61.9.2711-2718.1987.

Abstract

Poliovirus infection of HeLa cells induces rapid shutoff of host protein synthesis, whereas translation of poliovirus RNA is not inhibited. It is presumed that shutoff is the result of proteolytic cleavage of component p220 of eucaryotic initiation factor 4F. To study whether poliovirus proteinase 2A is involved in this cleavage, we translated synthetic RNAs that contained the coding region for poliovirus-specific polypeptides P1 and 2A in vitro and assayed for cleavage of p220. We report here that cleavage of p220 occurred in all cases when active proteinase 2A was translated and that disruption of the coding sequence of 2A by linker insertion or deletion prevented processing of p220 in vitro. Activity of 2A was determined by its ability to cleave at the P1-P2 site of a segment of the poliovirus polyprotein. We also constructed a plasmid in which the 3'-most 500 nucleotides of the nontranslated region of encephalomyocarditis virus were linked to the coding sequence for poliovirus polypeptide 2A. Translation of the RNA transcript of this clone was very efficient and yielded a fusion protein that included 2A; this polypeptide also induced cleavage of p220. In vitro translation in the presence of antibodies against 2A specifically inhibited processing of p220, whereas incubation of in vitro translation products with antibodies against 2A after translation was completed did not prevent proteolysis of p220.

摘要

脊髓灰质炎病毒感染HeLa细胞会导致宿主蛋白质合成迅速关闭,而脊髓灰质炎病毒RNA的翻译不受抑制。据推测,这种关闭是真核起始因子4F的组分p220发生蛋白水解切割的结果。为了研究脊髓灰质炎病毒蛋白酶2A是否参与这种切割,我们在体外翻译了包含脊髓灰质炎病毒特异性多肽P1和2A编码区的合成RNA,并检测了p220的切割情况。我们在此报告,当翻译活性蛋白酶2A时,在所有情况下都会发生p220的切割,并且通过接头插入或缺失破坏2A的编码序列会阻止体外p220的加工。2A的活性通过其在脊髓灰质炎病毒多聚蛋白片段的P1-P2位点进行切割的能力来确定。我们还构建了一个质粒,其中脑心肌炎病毒非翻译区的最3'端500个核苷酸与脊髓灰质炎病毒多肽2A的编码序列相连。该克隆的RNA转录本的翻译非常有效,并产生了一种包含2A的融合蛋白;这种多肽也诱导了p220的切割。在存在抗2A抗体的情况下进行体外翻译会特异性抑制p220的加工,而在翻译完成后将体外翻译产物与抗2A抗体一起孵育并不会阻止p220 的蛋白水解。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/add5/255777/74a45f3328a4/jvirol00100-0067-a.jpg

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