Concentrating all helper protein functions on a single entity allows rescue of recombinant measles virus by transfection of just two plasmids

生物 麻疹病毒 病毒学 质粒 重组DNA 单反病毒 辅助病毒 溶瘤病毒 病毒 麻疹病毒 基因组 内部核糖体进入位点 转染 基因 分子生物学 副粘病毒科 遗传学 病毒复制 信使核糖核酸 麻疹 翻译(生物学) 病毒性疾病 接种疫苗
作者
Arne Auste,Michael D. Mühlebach
出处
期刊:Journal of General Virology [Microbiology Society]
卷期号:103 (11)
标识
DOI:10.1099/jgv.0.001815
摘要

The generation of recombinant measles virus (MeV) from manipulated genomes on plasmid DNA is quite a complex and inefficient process. As a member of the order Mononegavirales its single-stranded ssRNA genome in negative sense orientation is not infectious, but requires co-availability of the viral RNA-dependent RNA polymerase L, the polymerase co-factor phosphoprotein P, and the nucleocapsid protein N in defined relative amounts to establish infectious centres in transfected cell cultures that release replication-competent recombinant MeV particles. For this so-called rescue, different rescue systems were developed that rely on at least four different components. In this work, we establish a functional MeV rescue system just being composed of two components: the plasmid encoding the (modified) viral genome, and a one-helper-plasmid bundling all helper functions. In contrast to a rescue-system for Newcastle Disease Virus, another paramyxovirus, co-expression of all helper proteins by the same promoter failed. Instead, adaptation of the strength of the respective promoters to drive each helper gene´s expression to the relative expression found in MeV-infected cells or other rescue systems, which indeed adjusted respective mRNA and protein expression, yielded success, albeit not yet to the same efficacy as the four-component system. Thereby, our study paves the way for the development of easier and, after further optimization, more efficient rescue systems to generate recombinant MeV for e.g. the application as a vaccine platform or oncolytic virus, for example.

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