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人副流感病毒3型基因组RNA合成类似物的拯救

Rescue of synthetic analogs of genome RNA of human parainfluenza virus type 3.

作者信息

De B P, Banerjee A K

机构信息

Department of Molecular Biology, Research Institute, Cleveland Clinic Foundation, Ohio 44195.

出版信息

Virology. 1993 Sep;196(1):344-8. doi: 10.1006/viro.1993.1486.

Abstract

A simple system that allows expression and packaging of a foreign gene by human parainfluenza virus type 3 (HPIV-3) has been described. First, a cDNA was constructed to encode an internally deleted version of HPIV-3 genome RNA. The viral genes were replaced with a negative sense copy of the bacterial chloramphenicol acetyl transferase (CAT) reporter gene. In vitro run-off transcription with T7 RNA polymerase synthesized an 870 nucleotide RNA that contained the antisense coding region of the CAT gene flanked by the transcription regulatory sequences and the 3' and 5' end extracistronic sequences of the HPIV-3 genome. When introduced into cells that are infected with HPIV-3, this RNA was amplified and the reporter gene was expressed, as measured by the CAT activity in the cell extract. Furthermore, the synthetic RNA was packaged into infectious virions. The addition of two extra nucleotides at the 5' end of the parental trailer region decreased the CAT activity by more than 90%, suggesting a requirement for the intact 5'-regulatory domain in the viral replicative cycle. Interestingly, the addition of one extra nucleotide to the 3' end totally abolished the CAT activity indicating that an exact 3' terminus is critical in this process.

摘要

一种可通过3型人副流感病毒(HPIV-3)实现外源基因表达和包装的简单系统已被描述。首先,构建了一个cDNA来编码HPIV-3基因组RNA的内部缺失版本。病毒基因被细菌氯霉素乙酰转移酶(CAT)报告基因的反义拷贝所取代。用T7 RNA聚合酶进行体外 runoff转录合成了一个870个核苷酸的RNA,其包含CAT基因的反义编码区,两侧是转录调控序列以及HPIV-3基因组的3'和5'端顺反子外序列。当将该RNA引入感染了HPIV-3的细胞中时,如通过细胞提取物中的CAT活性所测定的,该RNA被扩增且报告基因得以表达。此外,合成RNA被包装进感染性病毒粒子中。在亲本拖尾区域的5'端添加两个额外核苷酸使CAT活性降低了90%以上,这表明在病毒复制周期中需要完整的5'调控域。有趣的是,在3'端添加一个额外核苷酸完全消除了CAT活性,这表明精确的3'末端在此过程中至关重要。

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