采用绿色荧光蛋白腺病毒载体表达HBsAgCTL优势表位肽MHC单链三聚体 Expression of a single-chain trimer of MHC restricted HBsAg CTL epitope using adenovirus vector containing GFP-report gene期刊界 All Journals 搜尽天下杂志传播学术成果专业期刊搜索期刊信息化学术搜索

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采用绿色荧光蛋白腺病毒载体表达HBsAgCTL优势表位肽MHC单链三聚体

引用本文：	陈心春,刘威龙,杨桂林,刘勇军,朱秀云,张红梅,周伯平.采用绿色荧光蛋白腺病毒载体表达HBsAgCTL优势表位肽MHC单链三聚体[J].中华实验和临床病毒学杂志,2002,23(1):161-164.

作者姓名：	陈心春刘威龙杨桂林刘勇军朱秀云张红梅周伯平

作者单位：	深圳市第三人民医院,518020;Depamnem af Immunology,University of Arimna,USA;

摘要：	目的采用携带GFP报告基因腺病毒载体表达HBsAg细胞毒性T细胞(CIL)表位MHC单链三聚体,为增强HBV特异性免疫提供新方法.方法构建小鼠MHC Ⅰ类分子(H-2Ld)限制的HBsAg优势CTL表位肽与MHCⅠ类分子重链(Ld)和β2M链(β2-microglobulin,β2微球蛋白)的单链三聚体(HBsAg-SCT).并将HBsAg-SCT亚克隆到GFP标记腺病毒载体,以HBsAg和OVA-SCT作为对照,转染293A细胞,包装产生携带HBsAs-SCT,HBsAg和OVA-SCT的重组腺病毒.结果经双酶切和克隆测序鉴定,HBsAg-SCT能成功克隆到编码GFP标记的腺病毒载体,通过荧光显微镜观察到转染的293A细胞含有绿色荧光素蛋白.通过Western Blot进一步证实表达的重组蛋白HBsAg-SCT能与抗-腿抗体发生反应.结论编码HBsAg-SCT的荧光蛋白腺病毒载体成功构建,并能在293A细胞中完整包装成重组腺病毒颗粒.
关键词：	肝炎表面抗原乙型重组遗传腺病毒人免疫显性表位基因 MHCⅠ类 T淋巴细胞细胞毒性荧光抗体技术 Genes MHC class Ⅰ
Expression of a single-chain trimer of MHC restricted HBsAg CTL epitope using adenovirus vector containing GFP-report gene

Lybarger Lonnie,CHEN Xin-chun,LIU Wei-long,YANG Gui-lin,LIU Yong-jun,ZHU Xiu-yun,ZHANG Hong-mei,ZHOU Bo-ping,Lybarger Lonnie.Expression of a single-chain trimer of MHC restricted HBsAg CTL epitope using adenovirus vector containing GFP-report gene[J].Chinese Journal of Experimental and Clinical Virology,2002,23(1):161-164.

Authors:	Lybarger Lonnie CHEN Xin-chun LIU Wei-long YANG Gui-lin LIU Yong-jun ZHU Xiu-yun ZHANG Hong-mei ZHOU Bo-ping Lybarger Lonnie

Abstract:	Objective To generate a recombinant Adenovh'us encoding a GFP (green fluorescent protein)-report gene and a single-chain trimer of MHC restricted HBsAg CTL epitope. Methods An oligonucleotide encoding H-2Ld restricted HBsAg CTL epitopo was synthesized and fused with H-2Ld DNA molecule to construct the eukaryotic expression vector carrying the HBsAg-SCT gene. The HBsAg-SCT gene was subcloned into a GFP adenovirus expression vector,which was transfeeted into Ad293 cells for packaging and amplification of recombinant adenovirus encoding HBsAg-SCT. Results HBsAg-SCT has been cloned into an adenovirus vector encoding GFP report gene successfully as confirmed by double enzyme digestion and direct sequencing. HBsAg-SCT was expressed by infected Ad293 ceils demonstrated by western blot assay. Conclusion A recombinant adenovirus expressing HBsAg-SCT and green fluorescent protein report gene has been generated.

Keywords:	Hepatitis B surface antigensRecombinant geneticAdenoviruses humanImmunodominant epitopesT-Lymphocytes cytotoxicFluorescent antibody technique

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