Production of lentivirus of LMP1 and GFP recombinant gene

    LI Xianª²Mao, ZHAO Tong£¬ ZHU Meiª²Gang£¬ ZHANG Sanª²Quan£¬ZHANG Jinª²Hua

    Department of Pathology, School of Basic Medicine, Southern Medical University, Guangzhou 510515, China

    ¡¾Abstract¡¿ AIM: To produce lentivirus of latentmembrane protein 1 (LMP1) and green fluorescent protein (GFP) recombinant gene. METHODS: The fragment including all the exons of LMP1 was amplified by RTª²PCR and was recombined to the downstream of CMV promoter in the lentivirus vector FUGW. The three plasmids expressing lentivirus [packaging plasmid pCMV.¡÷8.9, envelope plasmid VSVG and target plasmid FUGWª²LMP1] were packaged into virus packaging cell line 293FT using lipofectamine method. The virusª²producing cell supernatant was harvested and concentrated. RESULTS: It was proved that the sequence of the RTª²PCR product was totally consistent with the data of GenBank by DNA sequencing analysis. The LMP1 cDNA fragment was cloned in the vector FUGW in the right direction and the open reading fragment of LMP1 was maintained. The three plasmids were effectively transferred into 293FT. Much green fluorescence was observed by fluorescence microscopy. CONCLUSION: The lentivirus of LMP1 and GFP recombinant gene are successfully produced. ......