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三种方法纯化生物工程抗体片段的比较
引用本文:韩焕兴,陆慧琦,姜波,安峰,叶伟民,曾万杰,罗荣城. 三种方法纯化生物工程抗体片段的比较[J]. 解放军医学杂志, 2003, 28(3): 266-267
作者姓名:韩焕兴  陆慧琦  姜波  安峰  叶伟民  曾万杰  罗荣城
作者单位:200003,上海,第二军医大学长征医院;第二军医大学长海医院;第一军医大学南方医院
基金项目:上海科委资助课题 (编号 0 0 4 31 92 0 8)
摘    要:比较3种不同纯化体系纯化生物工程抗-HBsFab的效率和效果,寻求高效,经济的生物工程产品批量纯化方法,采用增菌发酵抗-HBsFab阳性克隆,超声破菌法制备Fab上清,分别缓冲平衡抗Fab -Sepharose亲合胶,链球菌蛋白G(prot.G)-Sepharose胶和Ni-NTA离子螯合胶,对Fab上清进行过柱纯化,紫外光检测目的蛋白得率,SDS-PAGE鉴定产物的纯度并用HBsAg包被ELISA检测其生物活性,结果显示,等容积不同类别的胶体对目的蛋白的纯化效率依次为:Ni-NTA离子螯合胶>prot.G-Sepharose胶>抗-FabSepharose亲合胶;在各胶体饱和结合能力之内,3种方法中获高纯度产品,在SDS-PAGE中呈现单一区带:HBsAg包被ELISA检测结果为3种方法纯化制备的Fab在抗原结合能力上未显示明显差别,提示,3种纯化方法各有优势和应用限制,Ni-NTA法在经济性,实用性和纯化效率上明显优于其他两种方法。

关 键 词:生物工程抗HBsFab  亲合纯化  Ni-NTA离子螯合纯化  SDS-PAGE
修稿时间:2002-08-20

COMPARATIVE STUDIES ON PURIFICATION OF ENGINEERED ANTI-HBSFAB WITH 3 DIFFERENT METHODS
Han Huanxing,Lu Huiqi,Jiang Bo et al. COMPARATIVE STUDIES ON PURIFICATION OF ENGINEERED ANTI-HBSFAB WITH 3 DIFFERENT METHODS[J]. Medical Journal of Chinese People's Liberation Army, 2003, 28(3): 266-267
Authors:Han Huanxing  Lu Huiqi  Jiang Bo et al
Affiliation:Han Huanxing,Lu Huiqi,Jiang Bo et al. Changzheng Hospital,Second Military Medical University,Shanghai 200433,China
Abstract:The purpose of this study was to compare the efficiency of 3 different methods in purifying engineered anti-HBsFab. Anti-HBsFab Supernatants containing anti-HBsFab were prepared by ultrasound lysis of host cells of anti-HBsFab positive clone. Anti-Fab-sepharose gel, streptococcal protein G-sepharose gel (Prot G gel) and Ni-NTA-agarose gel were used to purify Fabs according to the reagents protocols. Then the concentrations of purified proteins were determined. SDS-PAGE was used for the measurement of purified Fabs'purity. HBsAg based ELISA was chosen to determine the Fabs' bio-activity. The results indicated that Fab recovery of different gels in equal volume were different. The recovery of Ni-NTA GEL was greater than that of Prot G gel, and the recovery of Prot G gel was greater than that of anti-Fab gel. Purity of the Fab isolated by 3 different gels was confirmed by SDS-PAGE. The binding capacity of anti-HBs Fab to HBsAg of these three gels had no signifticant difference. Our data suggested that each method had its advantage and usage limitation, Ni-NTA method demonstrated much better performance in economy, management, and efficiency over the other two methods.
Keywords:engineered anti-HbsFab  protein affinity purification  Ni-NTA gel purification  SDS-PAGE
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