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作 者:马章亮[1] 杭长寿[1] 邱建明[1] 姚树元[1] 宋干[1]
机构地区:[1]中国预防医学科学院病毒学研究所
出 处:《病毒学报》1998年第3期221-228,共8页Chinese Journal of Virology
基 金:国家八五"863"生物计划资助
摘 要:为发展国产化肾综合征出血热(HFRS)病毒基因工程疫苗,选择了汉滩病毒A9株M基因片段为目的基因,构建转染质粒pJSBA9M。以携带Lac基因的重组病毒为亲本,使表达载体pJSB-A9M上的M片段与痘苗病毒内的Lac基因重组,将Lac置换成A9M片段。用蓝白斑法筛选重组痘苗病毒,经PCR扩增证实A9M片段重组入痘苗病毒基因组内。重组痘苗病毒感染的VeroE6细胞,用抗糖蛋白单克隆抗体(HCO2、11E10、3D5、16D2)间接免疫荧光法检测,呈阳性反应;放射免疫沉淀法(RIP)证实,表达产物可与抗G2的糖蛋白单克隆抗体出现特异性沉淀带;间接免疫荧光染色法检测表明,重组病毒免疫Balb/c小鼠的血清与A9株感染的VeroE6细胞有较好的特异性反应(1:320),说明A9M片段在痘苗中表达成功。In order to develope genetically engineered Chinese vaccine of HFRS,the hantaan virus A9 M genome segment of Chinese isolate was chosen as the target gene.The plasmid pJSBA9M,containing the M clone segment,was constructed and controlled by the promoter P11,and also was proved by restriction enzyme digestion.This expression plasmid pJSBA9M was transfected using lipofectin reagent into Vero cells,which were superinfected with the vaccinia virus containing the Lac Z gene in the TK region.The recombinant vaccinia viruses were isolated by plaque assay of transfected-cell lysate on Vero cells with 1% low-melting-point agarose overlay containing 300μg of X-gal per ml.White plaques were removed and subjected to six round plaque purification.From 16 white plaques,only one was identified as the recombinant vaccinia virus by PCR.In addition,immunofluorescent assay(IFA)and Radio-immunoprecipitation(RIP)were used to identify the products of the recombinant vaccinia virus.Furthermore,the neutralizing antibody against hantaan virus with the titer of 1:320 in sera of mice inoculated with the recombinant vaccinia virus was detected.All the above results proved the expression of A9M segment by the recombinant vaccinia virus, and it has great potential to be used as the vaccine against HFRS.
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