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作 者:王宏卫[1] 夏辉明[1] 张东升[1] 高晓东[1] 李红乐[1] 鲁桂琛 孙颖
机构地区:[1]河南医科大学病理生理学教研室,郑州4500522 [2]中国医学科学院药物研究所合成室,北京100050
出 处:《河南医科大学学报》1999年第4期8-10,共3页Journal of Henan Medical University
基 金:卫生部科学研究基金;河南省自然科学基金 资助项目
摘 要:目的:人抑制素βB亚基单克隆抗体(单抗)的制备和鉴定。方法:以化学合成人抑制素βB(1- 28) 和(85-115)多肽片段和粗提猪卵泡抑制素免疫BALB/c 小鼠,经细胞融合与筛选,得到分泌单抗的细胞株,诱生腹水后采用特定的免疫学方法进行鉴定。结果:获得4 株能分泌单抗的细胞株,ELISA 检测腹水效价为1 ×10-4 ~1 ×10- 6,与α、βA亚基片段及其他多肽激素无交叉反应,3 株McAb( 抗INHβB(85- 115)) 识别同一抗原位点。相对亲和力3E8>5E11>7B9。腹水中的抗体能明显地被人卵泡液,猪卵泡液和βB(85 -115)BSA 中和而呈抑制曲线。Aims: To prepare the McAb againsting the INH βB subunits and to identify them. Methods:BALB/c mice were immunized with crude preparation of porcine inhibin by intra peritoneal injection,and followed by injection with chemically synthetic peptide INHβB (1-28) and βB(85-115) directly into the spleen of the immunized BALB/c mice 3 days before fusion. After fusion,selection and cloning producers,we got the cell lines which can secret McAbs,and used them to induce the ascites, then identified the McAb using specific immunological methods. Results:4 hybridoma cell lines which can secret McAbs were successfully obstained. The titer of ascites were 1×10\+\{-4\}~1×10\+\{-6\}, and the McAbs had no cross reaction with the α and βA subunits and other polypeptide hormones. Epitope specificity analysis proved that three cell lines (against INHβΒ(85-114)) recognized the same epitope. Relative affinity of them were 3E8>5E11>7B9. Antigen competitive inhibition test showed that the antibodies could be blocked by preincubating with human follicle fluid, porcine follicule fluid and INHβB(85-115) BSA. Conclusion: We first estabolished the cell lines which can secret the INH βB subunit's antibodies having high specificity and high affinity in China.
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