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IPTG-dependent vaccinia virus: identification of a virus protein enabling virion envelopment by Golgi membrane and egress.

机译:IPTG依赖的痘苗病毒:鉴定一种病毒蛋白可通过高尔基体膜和出口包裹病毒体。

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摘要

A novel method has been developed to study the functional roles of individual vaccinia virus gene products that is neither limited by the possible essentiality of the target gene nor by the availability of conditional lethal mutants. The system utilises the E. coli lac repressor protein, the operator sequence to which it binds and the specific inducer IPTG. It allows the generation of recombinant viruses in which the expression of any chosen gene, and hence virus replication, can be externally controlled. In principle, this system is broadly applicable to the functional analysis of genes in any large DNA virus. This approach has demonstrated that the gene encoding the 14 kDa membrane protein of vaccinia virus is non-essential for the production of infectious intracellular virus particles, but essential for the envelopment of intracellular virions by Golgi membrane and for egress of mature extracellular viral particles. This is the first vaccinia virus protein shown to be specifically required for these processes. In vivo this system may prove useful as a means of attenuating recombinant vaccinia virus vaccines by preventing virus spread without reducing the amount of the foreign antigen expressed in each infected cell. Attenuation of other live virus vaccines may be developed in a similar way.
机译:已经开发出一种新的方法来研究单个痘苗病毒基因产物的功能作用,该作用既不受靶基因可能的必要性的限制,也不受条件致死突变体的可用性的限制。该系统利用了大肠杆菌的lac阻遏蛋白,与其结合的操纵基因序列和特异性诱导物IPTG。它允许产生重组病毒,其中可以从外部控制任何选定基因的表达以及因此病毒的复制。原则上,该系统可广泛应用于任何大型DNA病毒中基因的功能分析。这种方法已证明,编码痘苗病毒14 kDa膜蛋白的基因对于生产感染性细胞内病毒颗粒不是必需的,但对于高尔基膜包裹细胞内病毒体以及成熟的细胞外病毒颗粒的散发是必不可少的。这是这些过程特别需要的第一个牛痘病毒蛋白。在体内,通过防止病毒传播而不减少每个感染细胞中表达的外源抗原的量,该系统可被证明是减毒重组牛痘病毒疫苗的一种手段。可以以类似方式开发其他活病毒疫苗的衰减。

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