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The Construction of Schistosoma Japonicum Vaccine BCG Sj26GST and Its Identification
Authors:HUANGFU Yongmu  ZHENG Bo  CHENG Jizhong  LIANG Juqing  FENG Zuohua
Institution:HUANGFU Yongmu,ZHENG Bo,CHENG Jizhong,LIANG Juqing,FENG Zuohua Department of Medical Molecular Biology,Research Center of Experimental Medicine,Tongji Medical University,Wuhan 430030
Abstract:Summary: The expression of foreign gene, Schistosoma Japonicum 26 ku antigen (Sj26GST), in Bacillus Calmette Guerin (BCG), Mycobacterium ( M. smegmatis ) and Escherichia coli ( E. coli ) were studied. The cDNA fragment encoding Sj26GST was amplified by PCR using plasmid pGEX, which could express Sj26GST in E. coli as template. The Sj26GST cDNA was cloned into the downstream of human M. tuberculosis heat shock protein (hsp) 70 promoter with correct reading frame, and then the DNA fragment containing hsp70 promoter and Sj26GST gene were subcloned together into E. coli Mycobacteria shuttle plasmid pBCG 2000 to construct the expression shuttle plasmid pBCG Sj26. The recombinant BCG and M. smegmatis mc 2 155, which were electroplated with pBCG Sj26, could express Sj26GST and the recombinant Schistosoma Japonicum vaccine BCG Sj26GST was made. The recombinant Sj26GST (rSj26GST) were soluble and could be observed on SDS PAGE at molecular weight of 26 ku. The content of rSj26GST accounted for 15 % and 10 % of total bacterial protein in BCG and M. smegmatis respectively. The results of Western blot showed the combination of rSj26GST with antibody of GST.
Keywords:BCG    M  smegmatis  shuttle plasmid  Schistosoma Japonicum  26ku antigen gene  vaccine  gene expression
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