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Membrane Adsorber for the Fast Purification of a Monoclonal Antibody Using Protein A Chromatography

机译:膜吸附剂用于使用蛋白A色谱法快速纯化单克隆抗体

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摘要

Monoclonal antibodies are conquering the biopharmaceutical market because they can be used to treat a variety of diseases. Therefore, it is very important to establish robust and optimized processes for their production. In this article, the first step of chromatography (Protein A chromatography) in monoclonal antibody purification was optimized with a focus on the critical elution step. Therefore, different buffers (citrate, glycine, acetate) were tested for chromatographic performance and product quality. Membrane chromatography was evaluated because it promises high throughputs and short cycle times. The membrane adsorber Sartobind Protein A 2 mL was used to accelerate the purification procedure and was further used to perform a continuous chromatographic run with a four-membrane adsorber-periodic counter-current chromatography (4MA-PCCC) system. It was found that citrate buffer at pH 3.5 and 0.15 M NaCl enabled the highest recovery of >95% and lowest total aggregate content of 0.26%. In the continuous process, the capacity utilization of the membrane adsorber was increased by 20%.
机译:单克隆抗体正在征服生物制药市场,因为它们可用于治疗多种疾病。因此,建立强大而优化的生产过程非常重要。在本文中,对单克隆抗体纯化中的层析(蛋白质A层析)的第一步进行了优化,重点是关键洗脱步骤。因此,测试了不同的缓冲液(柠檬酸盐,甘氨酸,乙酸盐)的色谱性能和产品质量。对膜色谱法进行了评估,因为它保证了高通量和较短的循环时间。膜吸附器Sartobind Protein A 2 mL用于加速纯化过程,并进一步用于通过四膜吸附器-周期性逆流色谱(4MA-PCCC)系统进行连续色谱分析。发现在pH 3.5和0.15 M NaCl的柠檬酸盐缓冲液中,回收率最高> 95%,总聚集体最低含量为0.26%。在连续过程中,膜吸附器的容量利用率提高了20%。

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