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用于产生经典猪瘟病毒的新型单步反向遗传学系统的开发。

Development of a novel single-step reverse genetics system for the generation of classical swine fever virus.

作者信息

Li Ling, Pang Huining, Wu Rui, Zhang Yanwen, Tan Yiluo, Pan Zishu

机构信息

State Key Laboratory of Virology, College of Life Sciences, Wuhan University, Wuhan, 430072, China.

出版信息

Arch Virol. 2016 Jul;161(7):1831-8. doi: 10.1007/s00705-016-2851-6. Epub 2016 Apr 11.

Abstract

We describe an alternative reverse genetics system for generating classical swine fever virus (CSFV) based on swine RNA polymerase I promoter (pSPI)-mediated vRNA transcription. The recombinant plasmid pSPTI/SM harboring a full-length CSFV Shimen strain cDNA, flanked by a swine RNA polymerase I (pol I) promoter sequence at the 5' end and a murine pol I terminator sequence at the 3' end, was constructed. When the plasmid pSPTI/SM was introduced into PK-15 cells by transfection, an infectious CSFV with termini identical to those of the parental virus was generated directly. CSFV rescued from this reverse genetics system exhibited similar growth kinetics and plaque formation compared with the parental CSFV. When the novel reverse genetics system was used to generate the CSFV vaccine C-strain, infectious virus was detected in the supernatant of PK-15 cells transfected with the recombinant plasmid pSPTI/C. This novel reverse genetics system is a simple and efficient tool for the investigation of the structure and function of the viral genome, for molecular pathogenicity studies, and for the development of genetically engineered vaccines for CSFV.

摘要

我们描述了一种基于猪RNA聚合酶I启动子(pSPI)介导的vRNA转录来产生经典猪瘟病毒(CSFV)的替代反向遗传学系统。构建了重组质粒pSPTI/SM,其携带全长CSFV石门株cDNA,在5'端侧翼为猪RNA聚合酶I(pol I)启动子序列,在3'端侧翼为鼠pol I终止子序列。当通过转染将质粒pSPTI/SM导入PK-15细胞时,直接产生了一种末端与亲本病毒相同的感染性CSFV。从该反向遗传学系统拯救的CSFV与亲本CSFV相比,表现出相似的生长动力学和蚀斑形成。当使用这种新型反向遗传学系统来产生CSFV疫苗C株时,在用重组质粒pSPTI/C转染的PK-15细胞的上清液中检测到了感染性病毒。这种新型反向遗传学系统是用于研究病毒基因组的结构和功能、进行分子致病性研究以及开发CSFV基因工程疫苗的一种简单而有效的工具。

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