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作 者:李强[1] 葛永红[2] 孟尧[1] 姚明明[1] 刘兰军[2] 沈富兵[2] 王黔川[2] 孟延发[1]
机构地区:[1]四川大学生命科学院,成都610064 [2]卫生部成都生物制品研究所,成都610040
出 处:《四川大学学报(自然科学版)》2004年第5期1046-1049,共4页Journal of Sichuan University(Natural Science Edition)
摘 要:重组EPO细胞灌注法培养的收获液,用Q SepharoseXL,C4反相疏水和Superdex75层析柱纯化表达的EPO.经SDS PAGE、PAGE和HPLC分析纯度达98%以上,总回收率为17%.经SDS PAGE分析其表观分子量为32~40kD.用IEF方法测得pI为3.75~4.15.网织红细胞计数法测得体内比活大于1.5×105IU,用ELISA测得体外活性为1.5×106~1.6×106IU.纯化的EPO的氨基酸组成和其它一些性质也进行了研究.Gene-engineering CHO-cells with the capacity to express recombinant human erythropoietin (rhEPO) were cultured in a perfusion mode. The rhEPO from culture supernatent was isolated and purified by a three-step purification process:Q Sephorose XL anion exchange chromatography-C4 reverse-phase chromatography and Superdex 75 molecular sieve chromatography. The purified rhEPO was showed to be homogeneous with a single protein band or a single peak by SDS-PAGE under reducing or non-reducing conditions, PAGE and HPLC. pI 3.75~4.15 of rhEPO was tested by polyacrylamide gel isoelectric focusing. The apparent molecular weight of rhEPO was identified to be 32~40kD by SDS-PAGE under reducing or non-reducing conditions. The western blot result revealed that rhEPO possessed the antigen of native erythropoietin. The specific activity of rhEPO in vitro was estimated 1.5×10~6~1.6×10~6IU by ELISA and more than 1.5×10~5 IU in vivo by Reticulocyte count method.
关 键 词:EPO 重组人促红细胞生成素 网织红细胞计数 体内 体外活性 ELISA 纯化 IEF SDS-PAGE分析
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