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植物中表达的疏水蛋白-蛋白 A 融合蛋白通过双水相萃取高效地从植物提取物中纯化抗西尼罗河病毒单克隆抗体。

Hydrophobin-Protein A Fusion Protein Produced in Plants Efficiently Purified an Anti-West Nile Virus Monoclonal Antibody from Plant Extracts via Aqueous Two-Phase Separation.

机构信息

The Biodesign Institute and School of Life Sciences, Arizona State University, Mail Zone 5401, 1001 S. McAllister Avenue, Tempe, AZ 85287, USA.

VTT Technical Research Centre of Finland Ltd, Espoo, Finland.

出版信息

Int J Mol Sci. 2020 Mar 20;21(6):2140. doi: 10.3390/ijms21062140.

DOI:10.3390/ijms21062140
PMID:32244994
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC7139538/
Abstract

The development of monoclonal antibodies (mAbs) has provided vast opportunities to treat a wide range of diseases from cancer to viral infections. While plant-based production of mAbs has effectively lowered the upstream cost of mAb production compared to mammalian cell cultures, further optimization of downstream processing, especially in extending the longevity of Protein A resin by an effective bulk separation step, will further reduce the overall prohibitive cost of mAb production. In this study, we explored the feasibility of using aqueous two-phase separation (ATPS) in capturing and separating plant-made mAbs from host proteins. Our results demonstrated that an anti-West Nile virus mAb (E16) was efficiently separated from most plant host proteins by a single ATPS step, comprising the mixing of plant extracts containing Hydrophobin-Protein A fusion protein (HPA) and E16 and the subsequent incubation with an inexpensive detergent. This simple ATPS step yielded a highly enriched E16 mAb preparation with a recovery rate comparable to that of Protein A chromatography. The ATPS-enriched E16 retained its structural integrity and was fully functional in binding its target antigen. Notably, HPA-based ATPS was also effective in enriching E16 from plant host proteins when both HPA and E16 were produced in the same leaves, supporting the potential of further streamlining the downstream purification process. Thus, ATPS based on plant-produced HPA in unpurified extract is a cost-effective yet efficient initial capture step for purifying plant-made mAbs, which may significantly impact the approach of mAb purification.

摘要

单克隆抗体(mAbs)的发展为治疗从癌症到病毒感染等各种疾病提供了广阔的机会。虽然与哺乳动物细胞培养相比,植物生产 mAbs 有效地降低了 mAb 生产的上游成本,但进一步优化下游加工过程,特别是通过有效的批量分离步骤延长 Protein A 树脂的寿命,将进一步降低 mAb 生产的整体高成本。在这项研究中,我们探索了利用双水相分离(ATPS)从宿主蛋白中捕获和分离植物制造的 mAbs 的可行性。我们的结果表明,通过单次 ATPS 步骤可以有效地将抗西尼罗河病毒 mAb(E16)从大多数植物宿主蛋白中分离出来,该步骤包括含有 Hydrophobin-Protein A 融合蛋白(HPA)和 E16 的植物提取物的混合,以及随后与廉价洗涤剂孵育。这种简单的 ATPS 步骤可获得高度富集的 E16 mAb 制剂,回收率可与 Protein A 层析相媲美。ATPS 富集的 E16 保留了其结构完整性,并能完全结合其靶抗原。值得注意的是,当 HPA 和 E16 都在同一叶片中生产时,基于 HPA 的 ATPS 也能有效地从植物宿主蛋白中富集 E16,这支持了进一步简化下游纯化过程的潜力。因此,基于未经纯化的植物生产的 HPA 的 ATPS 是一种经济有效的初始捕获步骤,用于纯化植物制造的 mAbs,这可能会显著影响 mAb 纯化的方法。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/0b62/7139538/d6fefbc8381a/ijms-21-02140-g005.jpg
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