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微型抗体与多模式色谱方法:挑战与机遇的融合

Minibodies and Multimodal Chromatography Methods: A Convergence of Challenge and Opportunity.

作者信息

Gagnon Pete, Cheung Chia-Wei, Lepin Eric J, Wu Anna M, Sherman Mark A, Raubitschek Andrew A, Yazaki Paul J

机构信息

Pete Gagnon is principal consultant at Validated Biosystems Inc., 240 Avenida Vista Montana, Suite 7F, San Clemente, CA USA 92672; 1-949-276-7477, fax 1-949-606-1904; www.validated.com . Chia-Wei Cheung, Mark A. Sherman, Andrew A. Raubitschek, and Paul J. Yazaki are with the department of cancer immunotherapeutics and tumor immunology at the City of Hope Medical Center's Beckman Research Institute in Duarte, CA; www.cityofhope.org/research/beckman-research-institute . Eric J. Lepin and Anna M. Wu are with the Crump Institute for Molecular Imaging's department of molecular and medical pharmacology at UCLA's David Geffen School of Medicine in Los Angeles, CA; www.crump.ucla.edu.

出版信息

Bioprocess Int. 2010 Feb;8(2):26-35.

Abstract

This case study describes early phase purification process development for a recombinant anticancer minibody produced in mammalian cell culture. The minibody did not bind to protein A. Cation-exchange, anion-exchange, hydrophobic-interaction, and hydroxyapatite (eluted by phosphate gradient) chromatographic methods were scouted, but the minibody coeluted with BSA to a substantial degree on each. Hydroxyapatite eluted with a sodium chloride gradient separated BSA and also removed a dimeric contaminant, but BSA consumed so much binding capacity that this proved impractical as a capture tool. Capto MMC media proved capable of supporting adequate capture and significant dimer removal, although both loading and elution selectivity varied dramatically with the amount of supernatant applied to the column. An anion-exchange step was included to fortify overall virus and DNA removal. These results illustrate the value of multimodal chromatography methods when affinity chromatography methods are lacking and conventional alternatives prove inadequate.

摘要

本案例研究描述了在哺乳动物细胞培养中生产的重组抗癌微型抗体的早期纯化工艺开发。该微型抗体不与蛋白A结合。研究了阳离子交换、阴离子交换、疏水相互作用和羟基磷灰石(用磷酸盐梯度洗脱)色谱方法,但该微型抗体在每种方法中都与牛血清白蛋白(BSA)大量共洗脱。用氯化钠梯度洗脱的羟基磷灰石分离了BSA,还去除了一种二聚体污染物,但BSA消耗了太多的结合容量,以至于作为捕获工具被证明不切实际。Capto MMC介质被证明能够支持充分的捕获并显著去除二聚体,尽管上样量和洗脱选择性都随上样到柱上的上清液量而显著变化。加入了一个阴离子交换步骤以加强整体病毒和DNA的去除。这些结果说明了在缺乏亲和色谱方法且传统替代方法证明不足时,多模式色谱方法的价值。

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