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机构地区:[1]贵阳医学院免疫学教研室,贵州贵阳550004 [2]贵州省疾病预防控制中心 [3]河南省商丘医学高等专科学校
出 处:《贵阳医学院学报》2009年第4期357-359,365,共4页Journal of Guiyang Medical College
基 金:国家973计划前期研究专项项目(2008CB517408);国家自然科学基金资助项目(30560148)
摘 要:目的:克隆登革2型病毒NGC株NS1基因部分序列,构建NS1基因部分序列的真核表达载体。方法:用PCR技术扩增登革2型病毒NGC株NS1基因部分序列,并定向克隆入pcDNA3.1(+)的kpnⅠ、xhoⅠ位点,构建真核重组载体pcDNA3.1(+)-NS1,转化EcoliDH5a。阳性重组质粒用PCR、酶切及序列测定等方法鉴定。电穿孔法将真核重组载体转染COS-7细胞,RT-PCR鉴定其表达情况。结果:阳性质粒经kpnⅠ及xhoⅠ双酶切及PCR获得了1个核苷酸长度为413 bp的基因,序列测定证实与NGC株NS1基因部分基因序列有99%同源,重组真核质粒转染COS-7细胞经RT-PCR鉴定证实有表达。结论:成功构建了含有登革2型病毒NGC株NS1基因部分序列基因的真核重组载体pcDNA3.1(+)-NS1。Objective: To clone partial sequence of NS1 gene of DEN-2 virus, strain NGC (NDN) and to construct its eukaryotic expression vector. Methods: NDN sequence was amplified with PCR, and the products were cloned into eukaryotic expression vector pcDNA3.1 ( + ), then transferred into E. coli DH5a. The positive recombinant plasmids were identified by PCR, restriction enzyme digesting and sequence analysis. The recombinant plasmid was transferred into mammalian COS-7 ceils by electroporation and its mRNA was identified by RT-PCR. Results: Digesting results with restriction enzymes kpn I and xho I , and sequence analysis, showed a fragment of 413 bp was obtained of which the sequence was 99% homology with partial sequence of NDN and pcDNA3.1 ( + )-NS1 mRNA expressed in COS-7 cells. Conclusion : The constretion of pcDNA3.1 ( + ) -NS1 is successful, which may facilitate further functional study of NS1 partial gene sequence.
分 类 号:R373.33[医药卫生—病原生物学]
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