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甲型肝炎病毒(HAV)的减毒及细胞培养适应性:一项利用HAV cDNA的基因分析

Attenuation and cell culture adaptation of hepatitis A virus (HAV): a genetic analysis with HAV cDNA.

作者信息

Cohen J I, Rosenblum B, Feinstone S M, Ticehurst J, Purcell R H

机构信息

Laboratory of Infectious Diseases, National Institute of Allergy and Infectious Diseases, Bethesda, Maryland 20892.

出版信息

J Virol. 1989 Dec;63(12):5364-70. doi: 10.1128/JVI.63.12.5364-5370.1989.

Abstract

RNA transcripts of hepatitis A virus (HAV) HM-175 cDNA from attenuated, cell culture-adapted HAV were infectious in cell culture. A full-length HAV cDNA from wild-type HAV (propagated in marmosets in vivo) was constructed. Chimeric cDNAs that contained portions of both wild-type and attenuated genomes were produced. Oligonucleotide-directed mutagenesis was used to engineer a point mutation into the VP1 gene of attenuated HAV cDNA, so that the sequence of this capsid protein would be identical to that of the wild-type virus. Transfection of monkey kidney cells with RNA transcripts from several of the chimeric cDNAs and from the mutagenized cDNA induced production of HAV. Comparison of the growth of attenuated, wild-type, chimeric, and mutant viruses in vitro indicated that the P2-P3 (nonstructural protein) region is important for cell culture adaptation of the virus; the 5' noncoding region may also contribute to adaptation, but to a lesser extent. Inoculation of marmosets with transfection-derived virus also suggested that the P2-P3 region plays an important role in attenuation of HAV HM-175.

摘要

来自减毒的、细胞培养适应型甲型肝炎病毒(HAV)HM - 175 cDNA的RNA转录本在细胞培养中具有感染性。构建了来自野生型HAV(在狨猴体内传代)的全长HAV cDNA。制备了包含野生型和减毒基因组部分的嵌合cDNA。使用寡核苷酸定向诱变技术在减毒HAV cDNA的VP1基因中引入一个点突变,使得这种衣壳蛋白的序列与野生型病毒相同。用几种嵌合cDNA和诱变cDNA的RNA转录本转染猴肾细胞可诱导产生HAV。减毒病毒、野生型病毒、嵌合病毒和突变病毒在体外生长情况的比较表明,P2 - P3(非结构蛋白)区域对病毒的细胞培养适应性很重要;5'非编码区域也可能有助于适应性,但作用较小。用转染衍生病毒接种狨猴也表明,P2 - P3区域在HAV HM - 175的减毒过程中起重要作用。

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Molecular cloning and characterization of hepatitis A virus cDNA.甲型肝炎病毒cDNA的分子克隆与特性分析
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