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采用四级错流中空纤维膜洗涤步骤的连续沉淀-过滤工艺,初始捕获单克隆抗体产品。

Continuous precipitation-filtration process for initial capture of a monoclonal antibody product using a four-stage countercurrent hollow fiber membrane washing step.

机构信息

Department of Chemical Engineering, The Pennsylvania State University, State College, Pennsylvania, USA.

Department of Chemical and Biological Engineering, Rensselaer Polytechnic Institute, Troy, New York, USA.

出版信息

Biotechnol Bioeng. 2024 Aug;121(8):2258-2268. doi: 10.1002/bit.28525. Epub 2023 Aug 10.

DOI:10.1002/bit.28525
PMID:37565527
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC10858288/
Abstract

The significant increase in product titers, coupled with the growing focus on continuous bioprocessing, has renewed interest in using precipitation as a low-cost alternative to Protein A chromatography for the primary capture of monoclonal antibody (mAb) products. In this work, a commercially relevant mAb was purified from clarified cell culture fluid using a tubular flow precipitation reactor with dewatering and washing provided by tangential flow microfiltration. The particle morphology was evaluated using an inline high-resolution optical probe, providing quantitative data on the particle size distribution throughout the precipitation process. Data were obtained in both a lab-built 2-stage countercurrent washing system and a commercial countercurrent contacting skid that provided 4 stages of continuous washing. The processes were operated continuously for 2 h with overall mAb yield of 92 ± 3% and DNA removal of nearly 3 logs in the 4-stage system. The high DNA clearance was achieved by selective redissolution of the mAb using a low pH acetate buffer. Host cell protein clearance was 0.59 ± 0.08 logs, comparable to that based on model predictions. The process mass intensity was slightly better than typical Protein A processes and could be significantly improved by preconcentration of the antibody feed material.

摘要

产物滴度的显著提高,加上对连续生物加工的日益关注,使得沉淀作为单克隆抗体 (mAb) 产品初始捕获的低成本替代方案(优于 Protein A 层析)重新受到关注。在这项工作中,使用带有切向流微滤脱水和洗涤功能的管状流沉淀反应器,从澄清的细胞培养液中纯化出一种具有商业相关性的 mAb。使用在线高分辨率光学探头评估颗粒形态,提供沉淀过程中整个粒径分布的定量数据。在实验室构建的 2 级逆流洗涤系统和商业逆流接触撬装设备中均获得了数据,后者提供了 4 级连续洗涤。该过程连续运行 2 小时,总 mAb 收率为 92±3%,在 4 级系统中 DNA 去除率接近 3 个对数。通过使用低 pH 醋酸盐缓冲液选择性重新溶解 mAb,实现了高 DNA 清除率。宿主细胞蛋白清除率为 0.59±0.08 个对数,与基于模型预测的结果相当。该工艺的质量强度略优于典型的 Protein A 工艺,通过预浓缩抗体进料材料,可显著提高该工艺的质量强度。

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