Home > Archive>Volume , Issue 2, 2000 >79-81. DOI:10.7671/j.issn.1001-411X.2000.02.023
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Rapid Construction of the Gene Transfer Vector of Pseudorabies Virus and Its Transient Expression in vitro
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S858.285.3 S858.282.5

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    Abstract:

    A gene expression cassette with molecular size of the insert, a recombinant plasmid containing the PK gene of PRV,equal to vector was cloned through partial repair of the terminal ends of insert and vector, thus transforming them from nonadherent to adherent ones. The constructed gene expression vector of PRV with the report gene was further identified by endonuclear enzyme analysis and the biological activity of expression vector was recognized directly through transfecting cells to detect its transient expression in vitro.

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LUO Man-lin, DING Jian-hua, LIU Zhen-ming, YUAN Shao-hua, ZHANG Chu-yu, WANG Jia-fu. Rapid Construction of the Gene Transfer Vector of Pseudorabies Virus and Its Transient Expression in vitro[J]. Journal of South China Agricultural University,2000,(2):79-81

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  • Revised:September 29,1999
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