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源自大肠杆菌的人白细胞介素-1受体拮抗剂:大规模微生物培养与蛋白质纯化

Human IL-1 receptor antagonist from Escherichia coli: large-scale microbial growth and protein purification.

作者信息

Zanette D, Dundon W, Soffientini A, Sottani C, Marinelli F, Akeson A, Sarubbi E

机构信息

Lepetit Research Center, Gerenzano, VA, Italy.

出版信息

J Biotechnol. 1998 Oct 8;64(2-3):187-96. doi: 10.1016/s0168-1656(98)00111-4.

DOI:10.1016/s0168-1656(98)00111-4
PMID:9821675
Abstract

Interleukin-1 receptor antagonist (IL-1ra) is a recently discovered cytokine which specifically inhibits IL-1 pro-inflammatory activities in various experimental conditions. In this work, the growth conditions of a recombinant E. coli strain which in laboratory studies expressed human IL-1ra mostly in insoluble form, have been optimized at the level of 6-1 bioreactors and then scaled up to a 50-1 process. As a result, a high amount (0.43 g l-1 of microbial culture) of soluble, active IL-1ra has been directly obtained in the large-scale cell lysate with no need for protein solubilization. Also, an efficient purification procedure has been developed for the soluble protein, based on cation exchange expanded bed adsorption directly followed by anion exchange chromatography. This process, which does not include any intermediate dialysis step or gradient elutions, can be easily scaled up to larger production volumes and is therefore well-suited for manufacturing. As a result of the overall optimization study, more than 12 g of pure IL-1ra have been obtained from a single 50-1 fermentation run, without any denaturation/renaturation process. The final product, whose identity and purity have been checked also by MALDI-TOF and ESI-MS, shows full biological activity both in cellular assays and in in vivo experiments with Cynomolgus monkeys.

摘要

白细胞介素-1受体拮抗剂(IL-1ra)是一种最近发现的细胞因子,在各种实验条件下能特异性抑制IL-1的促炎活性。在本研究中,对一株重组大肠杆菌菌株的生长条件进行了优化,该菌株在实验室研究中表达的人IL-1ra大多为不溶性形式,首先在6-1生物反应器水平进行优化,然后扩大到50-1规模的工艺。结果,在大规模细胞裂解物中直接获得了大量(0.43 g l-1微生物培养物)可溶性、有活性的IL-1ra,无需蛋白质溶解。此外,基于阳离子交换扩张床吸附直接继以阴离子交换色谱,开发了一种针对可溶性蛋白的高效纯化程序。该工艺不包括任何中间透析步骤或梯度洗脱,可轻松扩大到更大的生产规模,因此非常适合大规模生产。通过整体优化研究,单次50-1发酵运行可获得超过12 g的纯IL-1ra,无需任何变性/复性过程。最终产品的身份和纯度也通过基质辅助激光解吸电离飞行时间质谱(MALDI-TOF)和电喷雾电离质谱(ESI-MS)进行了检测,在细胞试验和食蟹猴体内实验中均显示出完全的生物活性。

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