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Construction of a recombinant plasmid expresses Mycobacterium tuberculosis A g85A fu sed to murine GM-CSF and it s expression in COS7 cells

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ã€Authorã€‘ XIE Yong en 1,BAO Lang 2,ZHANG Hui dong 2,CHEN Wei 2(1. Department of Pathophysiology,North Sichuan Medical College,Nanchong 63700 7,China;2. Research Unit of Infection and Immunity, School of Basical Medi cal Sciences, Sichuan University, Chengdu 610041, China) [

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ã€Abstractã€‘ Objective To find a new way of genetic modification for t uberculosis DNA vaccine.Methods The gene fragment encoding My cobacterium tuberculosis Ag85 A was obtained by using PCR and the cDNA encoding murine granulocyte macrophage clone stimulating factor(GM CSF)was obtained by using RT PCR , the two gene f rag ments were inserted into plasmid vector to construct recombinant plasmid , the r ecombinant plasmid was transferred into COS7 cells by using cationic liposomes. The fused expression product was determined by Western blotting analysis.Results A Recombinant plasmid which can express Mycobacterium tuber culosis Ag85A fuse d to murine Granulocyte Macrophage clone stimulating factor was successfully co n structed.Conclusion All these results provided the basis for fu rther study the immunogenicity and protective immunity of the recombinant plasmi d. [æ›´å¤š è¿˜åŽŸ