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rhIL-6大肠杆菌高效表达的影响因素及其产品中试的研究 被引量:4

Study on the Influential Factors of High Expression of rhIL-6 E. coli and Its Middle Scale of Products
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摘要 研究自构建的重组人白细胞介素- 6(rhIL-6)基因工程菌株高效表达的影响因素及其rhIL-6产品中试工艺。方法:①将rhL-6-PBV重组质粒转化至RRI、JM103和 DH5 a不同宿主菌中,在M9CA和 LB培养基中,42℃诱导培养不同时间(3~6 h),观测 rhIL-6不同表达效率。②采用 10 L发酵罐诱导培养,经破菌-洗包-溶包初步纯化后,再经三步柱层析纯化,提取rhIL-6。结果:①rhIL-6在DH5 a大肠杆菌中(SDH-945株)表达效率高;可达 39%,用 M9CA培基,42℃诱导培养 5h可使表达效率提高到41%,②SDH-945菌株在5批 10L M9CA发酵诱导培养 5 h,rhIL-6表达效率可达 35. 87±2. 65%。经初步纯化后,rhIL-6的纯度达 74. 87±3. 68%,再经三步柱层析后,纯度可达 95%以上,比活性达 4 × 108 U/mg,总得率稍低可达 23.1%.结论:①SDH-945工程菌株在 M9CA培养基巾,42℃诱导培养 5 h,rhIL-6表达效率最佳。②10 L发酵和纯化工艺可获高效价、高比活性、高纯度的rhIL-6合格生物制品。 Purpose: To study influential factors of the high expression of rhlL-6 E. coli constructed by our department and its middle scale of product. Methods: ① We transformate rhIL-pBV plasmid into different hosts of RRI, JM103 and DH5 a. and observe their different expression rate under the conditions of different media (M9 CA or LB) and different time of inducing cultivation (three-six hours) at 42℃ ②After inducing cultivation in 10L fermentation tank, carry on primary purification through breaking E. coli-Washing inclusion bodies-soluting inclusion bodies, and further purification by sephadex G50 - DEAE-Fibre column-sephacry S 200 to get rhIL-6. Results: ①The expression rate of rhIL-6 is higher in DH5 a E. coli (SDH-945), and reach 39%, while using M9 CA media for five hours at 42℃, it can improve to 41 %. ②SDH-945 carry 5 lots of inducing cultivation for five hours in the 10L fermentation tank, its expression rate can reach 35. 87±2. 65 %. After primary purification, the purity of rhIL-6 reach 74. 87 ± 3. 68%, and after further three steps purifying, the purity reach 95%, the contrast activity reaches 4 × 108 U/mg, the total output is lower and reach 23. 1 %. Conclusion: ①The expression rate of rhlL-6 is best by cultivating SDH-945 under the conditions that at 42 ℃ in the media of M9CA for 5 hours. ②This technic of 10L fermentation tank and purity can get qualified product of rhIL-6 of high efficiency. high contrast activity and high purity.
作者 杨吉成 盛伟华 张云
机构地区 苏州医学院基因工程研究室
出处 《中国生化药物杂志》 CAS CSCD 1999年第1期23-27,共5页 Chinese Journal of Biochemical Pharmaceutics
关键词 hIL-6 大肠杆菌 高效表达 发酵 纯化 rhIL-6, E. coli, High expression, Fermentation, Purification
分类号 R392-33 [医药卫生—免疫学]
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中国生化药物杂志
1999年 第1期

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