从克隆的互补DNA中完全拯救出一种分节段的负链RNA病毒。
Rescue of a segmented negative-strand RNA virus entirely from cloned complementary DNAs.
作者信息
Bridgen A, Elliott R M
机构信息
Institute of Virology, University of Glasgow, Scotland.
出版信息
Proc Natl Acad Sci U S A. 1996 Dec 24;93(26):15400-4. doi: 10.1073/pnas.93.26.15400.
Abstract
We provide the first report, to our knowledge, of a helper-independent system for rescuing a segmented, negative-strand RNA genome virus entirely from cloned cDNAs. Plasmids were constructed containing full-length cDNA copies of the three Bunyamwera bunyavirus RNA genome segments flanked by bacteriophage T7 promoter and hepatitis delta virus ribozyme sequences. When cells expressing both bacteriophage T7 RNA polymerase and recombinant Bunyamwera bunyavirus proteins were transfected with these plasmids, full-length antigenome RNAs were transcribed intracellularly, and these in turn were replicated and packaged into infectious bunyavirus particles. The resulting progeny virus contained specific genetic tags characteristic of the parental cDNA clones. Reassortant viruses containing two genome segments of Bunyamwera bunyavirus and one segment of Maguari bunyavirus were also produced following transfection of appropriate plasmids. This accomplishment will allow the full application of recombinant DNA technology to manipulate the bunyavirus genome.
摘要
据我们所知,我们首次报道了一种无需辅助病毒的系统,该系统能够完全从克隆的cDNA中拯救出分节段的负链RNA基因组病毒。构建了质粒,其包含三个布尼亚姆韦拉布尼亚病毒RNA基因组片段的全长cDNA拷贝,两侧分别为噬菌体T7启动子和丁型肝炎病毒核酶序列。当用这些质粒转染同时表达噬菌体T7 RNA聚合酶和重组布尼亚姆韦拉布尼亚病毒蛋白的细胞时,全长反基因组RNA在细胞内被转录,这些反基因组RNA进而被复制并包装成有感染性的布尼亚病毒颗粒。产生的子代病毒含有亲代cDNA克隆特有的特定遗传标签。转染适当的质粒后,还产生了含有两个布尼亚姆韦拉布尼亚病毒基因组片段和一个马瓜里布尼亚病毒片段的重配病毒。这一成果将使重组DNA技术得以全面应用于操纵布尼亚病毒基因组。
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