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从克隆DNA中拯救麻疹病毒。

Rescue of measles viruses from cloned DNA.

作者信息

Radecke F, Spielhofer P, Schneider H, Kaelin K, Huber M, Dötsch C, Christiansen G, Billeter M A

机构信息

Institut für Molekularbiologie, Abteilung I, Universität Zürich, Switzerland.

出版信息

EMBO J. 1995 Dec 1;14(23):5773-84. doi: 10.1002/j.1460-2075.1995.tb00266.x.

Abstract

A system has been established allowing the rescue of replicating measles viruses (MVs) from cloned DNA. On one hand, plasmids were constructed from which MV antigenomic RNAs with the correct termini are transcribed by phage T7 RNA polymerase. On the other hand, helper cells derived from the human embryonic kidney 293 cell line were generated constitutively expressing T7 RNA polymerase together with MV nucleocapsid protein and phosphoprotein. Simultaneous transfection of the helper cells with the MV antigenomic plasmid and with a plasmid encoding the MV polymerase under direction of a T7 promoter led to formation of syncytia from which MVs were easily recovered. A genetic tag comprising three nucleotide changes was present in the progeny virus. As a first application of reverse genetics, a segment of 504 nucleotides from the 5' non-coding region of the fusion gene was deleted, leading to an MV variant whose replication behaviour in Vero cells was indistinguishable from that of the laboratory Edmonston B strain. Since no helper virus is involved, this system, in principle, should be applicable to the rescue of any member of the large virus order Mononegavirales, i.e. viruses with a nonsegmented negative-strand RNA genome.

摘要

已建立了一个系统,可从克隆的DNA中拯救复制性麻疹病毒(MV)。一方面,构建了质粒,通过噬菌体T7 RNA聚合酶转录出具有正确末端的MV反基因组RNA。另一方面,构建了源自人胚肾293细胞系的辅助细胞,其可组成性表达T7 RNA聚合酶以及MV核衣壳蛋白和磷蛋白。用MV反基因组质粒和在T7启动子指导下编码MV聚合酶的质粒同时转染辅助细胞,导致形成多核巨细胞,从中可轻松回收MV。子代病毒中存在包含三个核苷酸变化的遗传标签。作为反向遗传学的首次应用,融合基因5'非编码区的504个核苷酸片段被删除,产生了一种MV变体,其在Vero细胞中的复制行为与实验室埃登斯顿B株无异。由于不涉及辅助病毒,该系统原则上应适用于拯救大型病毒目单股负链RNA病毒科的任何成员,即具有非节段性负链RNA基因组的病毒。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/1aa7/394696/7d27bfa30158/emboj00047-0030-a.jpg

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