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中国汉坦病毒H8205株G2糖蛋白基因的克隆及在真核细胞中的瞬时表达 被引量:3

Cloning and Transient Expression of the Gene Encoding Human Hantavirus H8205 Strain G2 Glycoprotein in Mammalian Cells
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摘要 从感染病毒乳鼠脑组织提取总 RNA,采用 RT- PCR和分子克隆技术将扩增到的 G2糖蛋白基因插入含 CMV启动子的 pc DNA3.1/ His质粒载体中 ,通过脂质体介导转染 COS- 7细胞 ,用 SDS- PAGE、 Western- blot及 IFIA方法分别测定表达产物的相对分子量及特异性。结果证明获得正向插入的 G2 - pc DNA3.1/ His重组表达质粒 ,表达产物的相对分子量为 5 6 ku,与理论预期大小一致 ,并且可与汉坦病毒 H82 0 5株的腹水抗体起特异反应。表明构建的 G2 - pc DNA3.1/His重组质粒所表达的蛋白为中国汉坦病毒株特有 ,能在哺乳动物细胞中表达并具有抗原性 ,重组质粒可应用于汉坦病毒的 Total RNA from the brain tissue of the young mice infected with virus was extracted. The G2 glycoprotein gene was amplified and cloned into the plasmid vector pCDNA3 1/His containing CMV promoter by using RT PCR and molecular cloning technique,the recombinant plasmid G2 pCDNA3.1/His was transfected into eukaryotic COS 7 cells by lipofectine mediated transfection. SDS PAGE, Western blot and indirective FIA analysis were used to analyze the molecular weight and specificity of the expressed protein respectively. The results showed that the positive recombinant plasmid harbouring the right inserted G2 glycoprotein gene fragment was abtained. The protein expressed in mammalian cells COS 7 was about 56 ku, corresponding to the estimated molecular size of the G2 glycoprotein, and could react with the Hantavirus H8205 strain hyoerimmune mouse ascites. It was suggested that the G2 glycoprotein gene could be expressed in mammalian cells transiently and reserved Chinese specific antigenicity, indicating that the recombinant plasmid G2 pCDNA3 1/His could be used to develope DNA vaccine against Hantavirus.
出处 《华中科技大学学报(医学版)》 CAS CSCD 北大核心 2002年第3期230-233,共4页 Acta Medicinae Universitatis Scientiae et Technologiae Huazhong
基金 国家自然科学基金资助项目 (No. 30 170 819)
关键词 中国 汉坦病毒 H8205株 G2糖蛋白 DNA疫苗 基因表达 基因克隆 真核细胞 Hantavirus G2 glycoprotein DNA based vaccine gene expression
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  • 1姜泊 张亚历.分子生物学常用实验方法[M].北京:人民军医出版社,1997.50.

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