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在无辅助病毒的情况下产生鼠冠状病毒的重组感染性缺陷颗粒。

The production of recombinant infectious DI-particles of a murine coronavirus in the absence of helper virus.

作者信息

Bos E C, Luytjes W, van der Meulen H V, Koerten H K, Spaan W J

机构信息

Department of Virology, Leiden University, Leiden, 2300 AH, The Netherlands.

出版信息

Virology. 1996 Apr 1;218(1):52-60. doi: 10.1006/viro.1996.0165.

Abstract

We have studied the production and release of infectious DI-particles in vaccinia-T7-polymerase recombinant virus-infected L cells that were transfected with five different plasmids expressing the synthetic DI RNA MIDI-HD and the four structural proteins (M, N, S, and E) of the murine coronavirus MHV-A59. The DI cDNA contains the hepatitis delta ribozyme sequences to generate in the transfected cells a defined 3' end. In EM studies of transfected cells virus-like particles (VLP) were observed in vesicles. Release of the particles into the medium was studied by immunoprecipitations of proteins released into the culture supernatant. Particle release was independent of S or N, but required M and E. Coexpression of E and M was sufficient for particle release. Coexpression of the structural proteins and the MIDI-HD RNA resulted in the production and release of infectious DI-particles. Infectivity of the DI-particles was determined by adding helper virus MHV-A59 to the medium containing the VLPs and using this mixture to infect new L cells. Intracellular RNA of several subsequent undiluted passages was isolated to detect the MIDI-HD RNA. Passage of the MIDI-HD RNA was dependent on the expression of the structural proteins of MHV-A59 in the transfected cells. In the absence of either E or M, MIDI-HD RNA could not be passaged to fresh L cells. We have thus developed a system in which we can produce coronavirus-like particles and an assay to test their infectivity.

摘要

我们研究了痘苗-T7-聚合酶重组病毒感染的L细胞中感染性DI颗粒的产生和释放情况,这些L细胞被转染了五种不同的质粒,分别表达合成的DI RNA MIDI-HD以及鼠冠状病毒MHV-A59的四种结构蛋白(M、N、S和E)。DI cDNA包含丁型肝炎核酶序列,以便在转染细胞中产生确定的3'末端。在对转染细胞的电子显微镜研究中,在囊泡中观察到了病毒样颗粒(VLP)。通过对释放到培养上清液中的蛋白质进行免疫沉淀来研究颗粒释放到培养基中的情况。颗粒释放不依赖于S或N,但需要M和E。E和M的共表达足以实现颗粒释放。结构蛋白与MIDI-HD RNA的共表达导致了感染性DI颗粒的产生和释放。通过向含有VLP的培养基中添加辅助病毒MHV-A59,并使用该混合物感染新的L细胞来测定DI颗粒的感染性。分离了几个后续未稀释传代的细胞内RNA以检测MIDI-HD RNA。MIDI-HD RNA的传代依赖于转染细胞中MHV-A59结构蛋白的表达。在没有E或M的情况下,MIDI-HD RNA无法传递到新鲜的L细胞中。我们因此开发了一个系统,在该系统中我们可以产生冠状病毒样颗粒,并建立了一种检测其感染性的方法。

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