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Cloning and expression of foreign genes in vaccinia virus using a host range selection system.

机译:使用宿主范围选择系统在牛痘病毒中克隆和表达外源基因。

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摘要

A simple selection system has been developed for the cloning and expression of open reading frames in vaccinia virus. The selection system is based on a conditional lethal (host range) mutant of vaccinia virus. A deletion mutant of the vaccinia virus WR strain was generated by insertion of the neomycin resistance gene from transposon Tn5 and selection with the antibiotic G418. This deletion recombinant, vP293, lacked approximately 21.7 kilobases of DNA beginning 3.8 kilobases from the left end of the genome, vP293, was capable of plaquing on primary chicken embryo fibroblasts and two monkey cell lines (BSC-40 and Vero) but was defective in replication in the human cell line MRC-5. Insertion of the host range gene K1L into vP293 restored the ability to grow on MRC-5 cells. A series of plasmids were constructed which in addition to the K1L gene contained a vaccinia virus early-late promoter, H6, followed by a unique polylinker sequence, translational initiation and termination signals, and an early transcription termination signal. These plasmids, pHES1 through 4, allowed for rapid single-step cloning and expression of any open reading frame when recombined in vivo with vP293 and scored for growth on MRC-5 cells.
机译:已经开发了一种简单的选择系统,用于在牛痘病毒中克隆和表达开放阅读框。选择系统基于痘苗病毒的条件致死(宿主范围)突变体。通过插入来自转座子Tn5的新霉素抗性基因并用抗生素G418选择来产生牛痘病毒WR株的缺失突变体。这种缺失的重组体vP293从基因组左端3.8 kb开始缺少大约21.7 kb的DNA,能够在初级鸡胚成纤维细胞和两个猴细胞系(BSC-40和Vero)上噬菌斑,但在在人细胞系MRC-5中复制。将宿主范围基因K1L插入vP293恢复了在MRC-5细胞上生长的能力。构建了一系列质粒,除了K1L基因外,还包含痘苗病毒早期启动子H6,其后是独特的多接头序列,翻译起始和终止信号以及早期转录终止信号。这些质粒pHES1至4可在体内与vP293重组并在MRC-5细胞上生长时对其进行快速单步克隆并表达任何开放阅读框。

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