首页> 外文期刊>Journal of Virology >Characterization and translation of methylated and unmethylated vesicular stomatitis virus mRNA synthesized in vitro by ribonucleoprotein particles from vesicular stomatitis virus-infected L cells.
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Characterization and translation of methylated and unmethylated vesicular stomatitis virus mRNA synthesized in vitro by ribonucleoprotein particles from vesicular stomatitis virus-infected L cells.

机译:核糖蛋白颗粒来自脉络膜炎病毒感染L细胞的体外甲基化和未甲基化囊泡膜病毒mRNA的表征及翻译。

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Ribonucleoprotein particles isolated from extracts of vesicular stomatitis virus (VSV) -infected L cells synthesized in vitro four classes of polyadenylated RNA sedimenting at 29S, 19S, 17S, and 13S. When synthesized in vitro in the presence of the methyl donor S-adenosyl methionine, these RNA species contained the following 5'-terminal structures: (i) m7G5ppp5'AmpAp(70%) ; (ii) m7G5'ppp5'AmpAmpNp (20%) and (iii) pppAp (10%). In the presence of the methylation inhibitor S-adenosylhomocysteine, however, the mRNA contained the 5'-terminal structures G5'ppp5'Ap (80%) and pppAp (20%). The mRNA's synthesized in vitro were translated in the homologous ascites and the heterologous wheat embryo cell-free systems. In both, the products were shown by sodium dodecyl sulfate gel electrophoresis and by immunoprecipitation to contain all five viral proteins, L, G, N, NS, and M. The presumed precursor to the G protein (G*) was also identified by fingerprint analysis. Methylated VSV mRNA was more active in protein synthesis than unmethylated mRNA in both the ascites system and the wheat embryo systems. Addition of S-adenosylmethionine stimulated translation of unmethylated mRNA in the wheat embryo but not in the ascites extract. S-adenosylhomocysteine, however, by preventing mRNA methylation inhibited the translation of unmethylated VSV mRNA in both systems. The mRNA methylating activity present in wheat embryo S-30 extracts was recovered in the ribosome-free supernatant fraction (S-150) and was insensitive to the protein synthesis inhibitor pactamycin.
机译:从囊泡口炎病毒(VSV)的提取物中分离的核糖核糖蛋白颗粒 - 在体外四种多腺苷酸化RNA沉淀在29s,19s,17s和13s中合成。当在甲基供体S-腺苷蛋白存在下在体外合成时,这些RNA物种含有以下5'-末端结构:(I)M7G5PPP5'AMPAP(70%); (ii)M7G5'PPP5'ampampnPNP(20%)和(III)PPPAP(10%)。然而,在甲基化抑制剂S-腺苷基肌细胞内的存在下,MRNA含有5'-末端结构G5'PPP5'AP(80%)和PPPAP(20%)。体外合成的mRNA在同源腹水和异源小麦胚胎细胞系统中翻译。在两者中,产十二烷基硫酸钠凝胶电泳显示并通过免疫沉淀,含有所有五种病毒蛋白,L,G,N,NS和M.对于G蛋白(G *)的假定前体也被指纹鉴定分析。在腹水系统和小麦胚胎系统中,甲基化的VSV mRNA在蛋白质合成中更活跃。在小麦胚胎中加入S-腺苷甲基硫醚刺激翻译未甲基化mRNA但不在腹水提取物中。然而,通过防止mRNA甲基化抑制在两个系统中未甲基化的VSV mRNA的翻译。在无核糖体上清液级分(S-150)中回收小麦胚胎S-30提取物中的mRNA甲基化活性,并对蛋白质合成抑制剂螯嘧啶不敏感。

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