首页 | 本学科首页   官方微博 | 高级检索  
     

GST与FGF23C末端71个氨基酸融合蛋白的表达、纯化及其免疫原性
引用本文:陈玉斌,刘孝菊,姚娜,孙常文,田海山,张键,刘敏,李校堃. GST与FGF23C末端71个氨基酸融合蛋白的表达、纯化及其免疫原性[J]. 吉林大学学报(医学版), 2012, 38(2): 225-229
作者姓名:陈玉斌  刘孝菊  姚娜  孙常文  田海山  张键  刘敏  李校堃
作者单位:吉林农业大学生物反应器与药物开发教育部工程研究中心,吉林长春130118;吉林农业大学生命科学学院,吉林长春130118;吉林农业大学生物反应器与药物开发教育部工程研究中心,吉林长春130118;吉林大学公共卫生学院卫生部放射生物学重点实验室,吉林长春130021;温州医学院药学院生物技术制药工程重点实验室,浙江温州325035;吉林农业大学生物反应器与药物开发教育部工程研究中心,吉林长春,130118;吉林农业大学生物反应器与药物开发教育部工程研究中心,吉林长春130118;温州医学院药学院生物技术制药工程重点实验室,浙江温州325035;吉林农业大学生物反应器与药物开发教育部工程研究中心,吉林长春130118;吉林农业大学生命科学学院,吉林长春130118;吉林大学公共卫生学院卫生部放射生物学重点实验室,吉林长春130021;温州医学院药学院生物技术制药工程重点实验室,浙江温州325035
基金项目:国家863计划资助课题,浙江省温州市第4期科技项目资助课题,浙江省温州市科技局项目资助课题
摘    要:目的:构建和表达谷胱甘肽-S-转移酶(GST)与成纤维细胞生长因子23(FGF-23)的活性片段-C末端71个氨基酸(FGF23CTR)融合蛋白的基因工程菌,并检测融合蛋白的免疫原性,为制备FGF23特异性单克隆抗体以及研发慢性肾病诊断试剂提供实验数据。方法:以质粒pET22b-fgf23为模板利用PCR方法扩增FGF23CTR的基因片段,将该基因与表达载体pGEX-4T-1连接后转化至BL21宿主细胞中,通过IPTG诱导获得可溶性表达,将GST-FGF23CTR融合蛋白用Glutathione Sepharose4B亲和层析法纯化,Western blotting法鉴定蛋白。该融合蛋白免疫Balb/C小鼠制备抗血清,采用ELISA法检测抗血清的效价。结果:构建GST-FGF23CTR融合蛋白的表达载体,纯化后得到纯度90%以上的融合蛋白,并与商品化的FGF23多克隆抗体呈阳性反应,ELISA法证实融合蛋白具有良好的免疫原性。结论:成功构建GST-FGF23CTR融合蛋白基因工程菌,并纯化得到具有良好免疫原性的融合蛋白,以此方法制备的抗原可用于FGF23特异性单克隆抗体的制备和FGF23生物学功能研究。

关 键 词:成纤维细胞生长因子23  免疫原性  基因工程菌
收稿时间:2011-10-25

Expression and purification of GST and FGF23 C termination fusion protein and its immunogenicity
CHEN Yu-bin , LIU Xiao-ju , YAO Na , SHUN Chang-wen , TIAN Hai-shan , ZHANG Jian , LIU Min , LI Xiao-kun. Expression and purification of GST and FGF23 C termination fusion protein and its immunogenicity[J]. Journal of Jilin University: Med Ed, 2012, 38(2): 225-229
Authors:CHEN Yu-bin    LIU Xiao-ju    YAO Na    SHUN Chang-wen    TIAN Hai-shan    ZHANG Jian    LIU Min    LI Xiao-kun
Affiliation:1,2,3,4(1.Engineering Research Center of Bioreactor and Pharmaceutical Development,Ministry of Education,Jilin Agricultural University,Changchun 130118,China;2.School of Life Science,Jilin Agricultural University,Changchun 130118,China;3.Key Laboratory of Radiobiology,Ministry of Health,School of Public Health,Jilin University,Changchun 130021,China;4.Key Laboratory of Biotechnology Pharmaceutical Engineering,School of Pharmacy,Wenzhou Medical College,Wenzhou 325035,China)
Abstract:Objective To construct the genetic engineering bacteria highly expressing fusion protein of glutathione-S-transferase(GST) and C-terminal 71 amino acids of fibroblast growth factor 23(FGF23CTR),and to test the immunogenicity of the fusion protein and to provide experimental data for FGF23 specific monoclonal antibodies and the development of diagnosis reagent for chronic kidney disease.Methods After FGF23CTR gene fragment was obtained by PCR,it was fused with GST by expression vector pGEX-4T-1,then was transformed in E.coli BL21(DE3).By inducing with 1IPTG,the fusion proteins were expressed solubly.The fused protein was purified by Glutathione Sepharose4B.The purity of GST-FGF23CTR by SDS-PAGE was shown to be higher than 90%.The Balb/C mice were immuned with fusion protein to pepare antiserum,then ELISA was used to assay antiserum titer.Results The GSTFGF23CTR expression vector was constructed successfully.The purity of fusion protein was more than 90% after purification,and it positively reacted to the commercialization of FGF23 polyclonal antibody.The ELISA result showed that the confirmed fusion protein had good immunogenicity.Conclusion The genetic engineering bacteria of GSTFGF23CTR is successfully constructed and the purified protein has good immunogenicity.The fused protein can be used for the FGF23 monoclonal antibody preparation and research on the biological function of FGF23.
Keywords:fibroblast growth factor 23  immunogenicity  genetic engineering bacteria
本文献已被 CNKI 万方数据 等数据库收录!
点击此处可从《吉林大学学报(医学版)》浏览原始摘要信息
点击此处可从《吉林大学学报(医学版)》下载全文
设为首页 | 免责声明 | 关于勤云 | 加入收藏

Copyright©北京勤云科技发展有限公司  京ICP备09084417号