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Purification of a human immunoglobulin G1 monoclonal antibody from transgenic tobacco using membrane chromatographic processes

机译:使用膜色谱法从转基因烟草中纯化人免疫球蛋白G1单克隆抗体

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摘要

Efficient purification of protein biopharmaceuticals from transgenic plants is a major challenge, primarily due to low target protein expression levels, and high impurity content in the feed streams. These challenges may be addressed by using membrane chromatography. This paper discusses the use of cation-exchange and Protein A affinity-based membrane chromatographic techniques, singly and in combination for the purification of an anti-Pseudomonas aerugenosa O6ad human IgG1 monoclonal antibody from transgenic tobacco. Protein A membrane chromatography on its own was unable to provide a pure product, mainly due to extensive non-specific binding of impurities. Moreover, the Protein A membrane showed severe fouling tendency and generated high back-pressure. With cation-exchange membrane chromatography, minimal membrane fouling and high permeability were observed but high purity could not be achieved using one-step. Therefore, by using a combination of the cation-exchange and Protein A membrane chromatography, in that order, both high purity and recovery were achieved with high permeability. The antibody purification method was first systematically optimized using a simulated feed solution. Anti-P. aeruginosa human IgG1 type monoclonal antibody was then purified from transgenic tobacco juice using this optimized method. (c) 2008 Elsevier B.V. All rights reserved.
机译:从转基因植物中高效纯化蛋白质生物制药是一项重大挑战,这主要是由于目标蛋白质表达水平低和进料流中杂质含量高。这些挑战可以通过使用膜色谱法来解决。本文分别讨论了阳​​离子交换和基于蛋白质A亲和力的膜色谱技术的用途,以及结合使用这些技术从转基因烟草中纯化抗铜绿假单胞菌O6ad人IgG1单克隆抗体的方法。蛋白质A膜层析本身无法提供纯净的产品,这主要是由于杂质的广泛非特异性结合所致。此外,蛋白A膜显示出严重的结垢趋势并产生高背压。使用阳离子交换膜色谱法,可以观察到最小的膜污染和高渗透性,但是使用一步法无法获得高纯度。因此,通过组合使用阳离子交换膜和蛋白A膜色谱法,可以同时获得高纯度和高渗透率的回收率。首先使用模拟进料溶液系统地优化抗体纯化方法。反P。然后使用这种优化方法从转基因烟草汁中纯化铜绿人IgG1型单克隆抗体。 (c)2008 Elsevier B.V.保留所有权利。

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