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作 者:仝莉莉[1] 秦鄂德[1] 李同据[1] 杨佩英[1] 于曼[1]
机构地区:[1]军事医学科学院微生物学流行病学研究所,北京100850
出 处:《军事医学科学院院刊》1999年第4期276-279,317,共5页Bulletin of the Academy of Military Medical Sciences
基 金:国家自然科学基金!资助课题(39770036)
摘 要:目的:构建我国登革2 型病毒43 株(D2-43)的PrM-E基因片段,观察其在哺乳动物细胞中的表达。方法:采用RT-PCR和分子克隆技术构建PrM-E基因片段,包括编码PrM 的信号肽序列、完整的PrM 蛋白和去除羧基端跨膜疏水区部分氨基酸的97.8% E蛋白的基因片段。用电穿孔法将构建的含有PrM-E基因的pCMV-ME真核重组质粒导入哺乳动物细胞中进行表达。采用蛋白印迹和间接免疫荧光法对表达产物进行特异性鉴定。结果与结论:构建的PrM-E基因全长2 019个核苷酸,序列分析证明其核苷酸序列是正确的。PrM-E基因在BHK-21 细胞中获得高效表达,表达蛋白可与D2-43 多克隆抗体起特异反应,且表达蛋白主要位于细胞浆中。Objective: To construct the PrM E gene fragment of dengue 2 virus strain 43(D 2 43)isolated in China and to observe its expression in mammalian cells. Methods: The PrM E gene, containing the PrM signal sequence, whole PrM and 97.8% E, was constructed by RT PCR and molecular cloning technologies. The recombinant eukaryotic expression plasmid pCMV ME, containing the PrM E gene fragment, was transfected into BHK 21 cell by electroporation to express the PrM E gene. The specificity of the expressed products was identified by Western blotting and the location of the expressed products in the cell was confirmed by indirect immunofluorescence analysis. Results and Conclusion: The constructed PrM E gene was 2 019 nts in length and consistent with the reported sequence,which was proved by DNA sequencing analysis. The SDS PAGE and indirect immunofluorescence analyses showed that the gene was expressed highly in BHK 21 cell and the expressed products mostly located at the cytoplasm. Western blot analysis further confirmed that the expressed protein was capable of reacting with the polyclonal antibody against the D 2 43 virus.
关 键 词:登革病毒 PrM-E基因 基因表达 哺乳动物细胞
分 类 号:R373.33[医药卫生—病原生物学]
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