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An infectious clone of human parainfluenza virus type 3.

机译:3型人副流感病毒的感染性克隆。

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摘要

A full-length clone of the human parainfluenza virus type 3 (HPIV-3) genome (called pHPIV-3) was constructed, and recombinant, infectious HPIV-3 was generated by transfecting pHPIV-3 and support plasmids encoding the HPIV-3 NP, P, and L proteins into HeLa cells infected with a vaccinia virus recombinant which expresses T7 RNA polymerase. T7 RNA polymerase promoters on the transfected plasmids direct the synthesis of transcripts encoding the NP, P, and L proteins and a full-length, positive-sense copy of the HPIV-3 genome. Generation of virus was dependent on transfection of pHPIV-3 and the HPIV-3 P- and L-encoding plasmids. However, a plasmid encoding the NP protein was not required since NP was expressed from pHPIV-3. Recovered virus was neutralized by anti-HPIV-3 antisera and shown to contain specific base substitutions characteristic of pHPIV-3. Recombination was shown to occur during recovery, as viruses with two distinct genotypes and phenotypes were isolated. The ability to produce infectious HPIV-3 engineered to contain specific alterations within the HPIV-3 genes and cis-acting elements expedites the study of all aspects of the virus replication cycle. Additionally, analysis of mutations may lead to the identification of attenuating genotypes, a key step in the development of a live virus vaccine.
机译:构建了人类副流感病毒3型(HPIV-3)基因组的全长克隆(称为pHPIV-3),并通过转染pHPIV-3和编码HPIV-3 NP的支持质粒产生了具有感染力的重组HPIV-3 ,P和L蛋白进入感染了表达T7 RNA聚合酶的牛痘病毒重组体的HeLa细胞。转染质粒上的T7 RNA聚合酶启动子指导编码NP,P和L蛋白的转录本以及HPIV-3基因组的全长正义拷贝的合成。病毒的产生取决于pHPIV-3和HPIV-3 P和L编码质粒的转染。但是,由于NP是从pHPIV-3表达的,因此不需要编码NP蛋白的质粒。回收的病毒被抗HPIV-3抗血清中和,并显示含有pHPIV-3特有的特异性碱基取代。由于分离出具有两种不同基因型和表型的病毒,重组在重组过程中发生。产生感染性HPIV-3的能力被改造成包含HPIV-3基因和顺式作用元件内的特定变化,从而加快了病毒复制周期各个方面的研究。另外,突变分析可能导致鉴定减毒基因型,这是开发活病毒疫苗的关键步骤。

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