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水泡性口炎病毒体相关转录酶活性在体外被一种合成的21个氨基酸的寡肽所抑制,该寡肽是为模拟NS蛋白的羧基末端而制备的。

Vesicular stomatitis virion-associated transcriptase activity was suppressed in vitro by a synthetic 21 amino acid oligopeptide prepared to mimic the carboxy-terminus of NS protein.

作者信息

Yamashita T, Kawai A

机构信息

Department of Molecular Microbiology, Faculty of Pharmaceutical Sciences, Kyoto University, Japan.

出版信息

Virology. 1990 Sep;178(1):166-73. doi: 10.1016/0042-6822(90)90390-d.

Abstract

To study the biological function of the NS protein of vesicular stomatitis virus (VSV), we prepared 21 species of synthetic oligopeptides with 11-21 amino acid residues, corresponding to every portion of the amino acid sequence of NS protein (Indiana serotype), and tested their effects on the VS virion (VSV) transcriptase activity in vitro. Only one peptide affected the virion-associated transcriptase activity of VSV Indiana, by reducing the incorporation of [3H]GMP into acid-insoluble fraction (IC50 = 26 microM). This peptide, the amino acid sequence of which corresponded to the carboxy (C)-terminal region of NS protein, also inhibited the New Jersey serotype virus transcriptase activity, as expected from a high degree of homology found between the amino acid sequences of the C-terminal regions of NS protein of both serotype viruses. Electrophoretic analysis on acrylamide gels of RNA transcripts revealed that the inhibitory synthetic peptide decreased the frequency of the initiation of transcription with no apparent effect on the chain-elongation process of viral transcription. As expected from its highly conserved amino acid sequence, these results suggest that the C-terminal domain of VSV NS protein is involved in initiating viral RNA synthesis.

摘要

为研究水疱性口炎病毒(VSV)NS蛋白的生物学功能,我们制备了21种含11 - 21个氨基酸残基的合成寡肽,它们对应于NS蛋白(印第安纳血清型)氨基酸序列的各个部分,并在体外测试了它们对VS病毒粒子(VSV)转录酶活性的影响。只有一种肽影响了VSV印第安纳株病毒粒子相关的转录酶活性,它通过减少[3H]GMP掺入酸不溶性部分来实现(IC50 = 26 microM)。该肽的氨基酸序列对应于NS蛋白的羧基(C)末端区域,正如预期的那样,由于两种血清型病毒NS蛋白C末端区域的氨基酸序列具有高度同源性,它也抑制了新泽西血清型病毒的转录酶活性。对RNA转录本进行的丙烯酰胺凝胶电泳分析表明,具有抑制作用的合成肽降低了转录起始频率,而对病毒转录的链延伸过程没有明显影响。从其高度保守的氨基酸序列来看,这些结果表明VSV NS蛋白的C末端结构域参与启动病毒RNA合成。

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