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首页> 外文期刊>Journal of Huazhong University of Science and Technology >E Sequence Analysis of Persistently Infected Mutant Japanese Encephalitis Virus Strains
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E Sequence Analysis of Persistently Infected Mutant Japanese Encephalitis Virus Strains

机译:持续感染的突变型日本脑炎病毒株的E序列分析

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摘要

A persistent infection model was established after human hepatoma cells infected by Japanese encephalitis viruses were subcultured for several times. Viral liters of mutant viruses in persistently infected cells were examined by plaque methods using BHK cells. Nucleotides of the E coding region of two wild and two mutant viruses were amplified by RT-PCR. PCR products were sequenced by ABI-PRSM™310 sequencing system. Compared to JaGAr-01 wild strains, four amino acids were replaced (E61Tyr鶤sp, E219His→Tyr, E384Val→Glu, E418Pro→Ala) in the E sequence of JaGAr-01 persistently-infected mutant strains. Eleven amino acid replacement (E51Arg →Ser, E61Tyr→Asp, E83Lys→Glu, E123Ser→Arg, E209Arg→Lys, E227Pro→Ser, E276Asp→Ser, E290Arg→Lys, E387Lys→Arg, E418Leu→Pro, E454Arg→Gly) was also noted when we compared the E sequence between persistently infected Nakayama and its wild strains. A lot of similarities of amino acid sequence between mutant strains JaGAr-01 and Nakayama were also noted. It was concluded that geno-variation existed in E region of mutant viruses and the mutant protein encoded by E region, especially the mutation of E61 (Tyr→Asp) may contribute to the maintenance of the persistent infection of Japanese encephalitis virus.
机译:将受日本脑炎病毒感染的人肝癌细胞传代培养数次后,建立了持久性感染模型。使用BHK细胞通过噬菌斑方法检查了持续感染细胞中的病毒升突变病毒。通过RT-PCR扩增了两种野生和两种突变病毒的E编码区的核苷酸。 PCR产物通过ABI-PRSM TM 310测序系统测序。与JaGAr-01野生株相比,在JaGAr-01持续感染突变株的E序列中置换了四个氨基酸(E61Tyr鹍sp,E219His→Tyr,E384Val→Glu,E418Pro→Ala)。十一个氨基酸替换(E51Arg→Ser,E61Tyr→Asp,E83Lys→Glu,E123Ser→Arg,E209Arg→Lys,E227Pro→Ser,E276Asp→Ser,E290Arg→Lys,E387Lys→Arg,E418Leu→Pro,E454Arg→Gly)还指出,当我们比较持续感染的中山及其野生株之间的E序列时。还注意到突变菌株JaGAr-01和Nakayama之间的氨基酸序列有很多相似性。结论:突变病毒E区存在基因变异,E区编码的突变蛋白,特别是E61的突变(Tyr→Asp)可能有助于维持日本脑炎病毒的持续感染。

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