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hGM-CSF基因在哺乳动物细胞中稳定转染表达质粒的构建和鉴定

Construction and Identification of hGM CSF Expressing Plasmid Which can be Stably Expressed in Mammalian Cells
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摘要 目的:获得具有天然糖基化结构的重组人粒细胞巨噬细胞集落刺激因子(rhGM-CSF)。方法:采用含sRα启动子和新霉素抗性基因的真核细胞表达载体pMEneo,接上XhoI接头,与XhoI酶切hGM-CSFcDNA片段连接,构建了可在哺乳动物细胞中稳定表达的pMEneo-hGM-CSF质粒。结果:22个pMEneo重构载体克隆中,8个含有hGM-CSFcDNA片段,酶切鉴定插入方向为5个顺式,1个顺式串珠,2个反式。结论:将上述各式以DEAE法转染COS细胞,瞬时表达鉴定,用TF1细胞MTT法测定培养液上清的hGM-CSF活性,顺式和顺式串珠培养上清活性为1×(103~104)U/ml。 Obiective:The recombinant human glanulocyte macrophage colony stimulating factor (rhGM CSF) with natural glycosylation structure was to be obtained.Method:The eukaryocyte expressing vetor containing sRa promotor and neomycin resistance gene was used,and then it was connected to Xhol enzyme digested hGM CSF cDNA fragment,thereby pMEneo hGM CSF plasmid which could stably experss recombinant hGM CSF in mammalian cells was constructed.Results:8 of 22 pMEneo reconstructed clones contained hGM CSF cDNA fragment.Determined by enzyme digestion,the plasmids had five cis forms,one cisroasary and two trans insertions.Conclusion:The cos cells transfected by DEAE method in the mentioned above forms could traniently express the identification.The activity of hGM CSF in culture supernatant in cis form and cis rosary form was (1×10 3~1×10 4)U/ml,and there was no activity of the culture supernatant in trans insertion.
出处 《中国输血杂志》 CAS CSCD 北大核心 1998年第3期119-121,共3页 Chinese Journal of Blood Transfusion
关键词 HGM-CSF 基因表达 哺乳动物细胞 hGM CSF Gene expression Mammalian cells
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