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源自克隆互补DNA的传染性麻疹病毒。

Infectious measles virus from cloned cDNA.

作者信息

Ballart I, Eschle D, Cattaneo R, Schmid A, Metzler M, Chan J, Pifko-Hirst S, Udem S A, Billeter M A

机构信息

Institut für Molekularbiologie I, Universität Zürich, Switzerland.

出版信息

EMBO J. 1990 Feb;9(2):379-84. doi: 10.1002/j.1460-2075.1990.tb08121.x.

Abstract

The study of measles virus (MV) and of negative strand RNA viruses in general has been hampered by the lack of an experimental system for genetic manipulation. Here we describe a procedure for generating infectious MV from cloned MV cDNA. First we assembled a genetically marked DNA copy of the MV genome in plasmids, under the control of phage T3 or T7 promoters, allowing production of transcripts almost identical to the MV genome or antigenome. Incubation of these linearized plasmid DNAs with the appropriate phage polymerase and only two ribonucleoside triphosphates yielded committed transcription complexes. Microinjection of these complexes into the cytoplasm of helper cells which provide the proteins necessary for MV genome encapsidation and transcription/replication, reproducibly give rise to lytic MVs. The transcripts of one of these viruses were analysed by sequencing after reverse transcription followed by DNA amplification, and found to contain the genetic tags. The described procedure permits the analysis of a negative strand RNA virus with the same genetic tools previously applicable only to positive strand RNA viruses and retroviruses.

摘要

麻疹病毒(MV)以及一般的负链RNA病毒的研究,一直因缺乏用于基因操作的实验系统而受到阻碍。在此,我们描述了一种从克隆的MV cDNA产生感染性MV的方法。首先,我们在噬菌体T3或T7启动子的控制下,在质粒中组装了一个带有遗传标记的MV基因组DNA拷贝,从而能够产生几乎与MV基因组或反基因组相同的转录本。将这些线性化的质粒DNA与合适的噬菌体聚合酶以及仅两种核糖核苷三磷酸一起温育,产生了稳定的转录复合物。将这些复合物显微注射到辅助细胞的细胞质中,这些辅助细胞提供MV基因组包装以及转录/复制所需的蛋白质,可重复性地产生裂解性MV。其中一种病毒的转录本在逆转录后通过测序分析,然后进行DNA扩增,发现含有遗传标签。所描述的方法允许使用以前仅适用于正链RNA病毒和逆转录病毒的相同遗传工具来分析负链RNA病毒。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/6a85/551677/9a69197a592c/emboj00229-0076-a.jpg

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