中华实验和临床病毒学杂志
中華實驗和臨床病毒學雜誌
중화실험화림상병독학잡지
CHINESE JOURNAL OF EXPERIMENTAL AND CLINICAL VIROLOGY
2008年
3期
228-230
,共3页
牟劲松%王慧芬%王江华%潘孝本%张璐%魏来
牟勁鬆%王慧芬%王江華%潘孝本%張璐%魏來
모경송%왕혜분%왕강화%반효본%장로%위래
肝炎病毒,乙型%肝炎表面抗原,乙型%转染%细胞系
肝炎病毒,乙型%肝炎錶麵抗原,乙型%轉染%細胞繫
간염병독,을형%간염표면항원,을형%전염%세포계
Hepatitis B virus%Hepatitis B surface antigesn%Transfection%Cell line
目的 构建可表达乙型肝炎病毒(HBV)HBsAg-EGFP融合蛋白的真核表达载体;获得重组质粒稳定转染的Chang Liver细胞系.方法 利用PCR技术从HBV基因组中扩增出HBsAg基因片段,BamH I/EcoR l双酶切后连接到经同样酶切的pEGFP-N1真核表达载体,转化TG1菌株感受态细胞,获得阳性重组质粒pEGFPNl.HBsAg.将阳性克隆用脂质体法转染Chang Liver细胞,经持续G418压力选择和有限稀释法克隆化获得稳定转染的细胞系.结果 成功构建了真核表达载体pEGFPN1-HBsAg;建立了其重组质粒稳定转染的Chang Liver细胞系.结论 重组质粒稳定转染的Chang Liver细胞系可表达HBsAg-EGFP融合蛋白;该细胞系可以用于筛选HBsAg转染细胞后,差异表达的蛋白质研究,为深入研究HBsAg可能的致病机制提供依据.
目的 構建可錶達乙型肝炎病毒(HBV)HBsAg-EGFP融閤蛋白的真覈錶達載體;穫得重組質粒穩定轉染的Chang Liver細胞繫.方法 利用PCR技術從HBV基因組中擴增齣HBsAg基因片段,BamH I/EcoR l雙酶切後連接到經同樣酶切的pEGFP-N1真覈錶達載體,轉化TG1菌株感受態細胞,穫得暘性重組質粒pEGFPNl.HBsAg.將暘性剋隆用脂質體法轉染Chang Liver細胞,經持續G418壓力選擇和有限稀釋法剋隆化穫得穩定轉染的細胞繫.結果 成功構建瞭真覈錶達載體pEGFPN1-HBsAg;建立瞭其重組質粒穩定轉染的Chang Liver細胞繫.結論 重組質粒穩定轉染的Chang Liver細胞繫可錶達HBsAg-EGFP融閤蛋白;該細胞繫可以用于篩選HBsAg轉染細胞後,差異錶達的蛋白質研究,為深入研究HBsAg可能的緻病機製提供依據.
목적 구건가표체을형간염병독(HBV)HBsAg-EGFP융합단백적진핵표체재체;획득중조질립은정전염적Chang Liver세포계.방법 이용PCR기술종HBV기인조중확증출HBsAg기인편단,BamH I/EcoR l쌍매절후련접도경동양매절적pEGFP-N1진핵표체재체,전화TG1균주감수태세포,획득양성중조질립pEGFPNl.HBsAg.장양성극륭용지질체법전염Chang Liver세포,경지속G418압력선택화유한희석법극륭화획득은정전염적세포계.결과 성공구건료진핵표체재체pEGFPN1-HBsAg;건립료기중조질립은정전염적Chang Liver세포계.결론 중조질립은정전염적Chang Liver세포계가표체HBsAg-EGFP융합단백;해세포계가이용우사선HBsAg전염세포후,차이표체적단백질연구,위심입연구HBsAg가능적치병궤제제공의거.
Objective To construct a eukaryotic expression vector for expressing hepatitis B virus (HBV) recombinant HBsAg-EGFP fusion protein and obtain a stable transfocted Chang Liver cell line. Methods The coding region of HBsAg gene of HBV was amplified by PCR and was digested by BamH I/EcoR I. This fragment was inserted into pEGFPN1 with T4 ligase and transformed E-coli TG1. The positive recombinant plasmid was selected, then the recombinant plasmid was transfocted into Chang Liver cell by Lipofectamine 2000 cells containing stable transformants were selected by the ability of resistance to G418 and isolated with a limited dilution. The stable transfected cell line expressing high level HBsAg-EGFP fusion protein was obtained. Results The eukaryotic expression vector named pEGFPN1-HBsAg was successfully constructed and the stable transfected Chang Liver celI line could express pEGFPN1-HBsAg fusion protein was obtained. Conclusion The stable transfected Chang Liver cell line could express pEGFPN1-HBsAg fusion protein, could be used to screen the proteins differentially expressed in HBsAg expression Chang Liver cells, which brought some new clues for studying the potential molecular mechanism of HBsAg protein.
