Viral clearance capacity by continuous Protein A chromatography step using Sequential MultiColumn Chromatography

单克隆抗体 色谱法 化学 亲和层析 抗体 生物 生物化学 免疫学
作者
Caroline Goussen,Laëtitia Goldstein,Corinne Brèque,Bruno You,Stéphane Boyer,Damien Bataille,Ludovic Burlot
出处
期刊:Journal of Chromatography B [Elsevier BV]
卷期号:1145: 122056-122056 被引量:9
标识
DOI:10.1016/j.jchromb.2020.122056
摘要

In response to the strong demand of biological protein therapeutics, such as monoclonal antibodies (MAbs), continuous downstream process was developed to deliver these molecules while maintaining desired product consistency and quality attributes, and providing manufacturing efficiency and flexibility. Viral safety is a critical quality attribute for biopharmaceuticals, such as MAbs. Evaluation of the viral clearance by the downstream process is a key component of risk mitigation. Protein A chromatography is typically used as an initial capture step for MAbs and efficient for the removal of process-related impurities like Host Cell Proteins (HCP). This step can also contribute to the clearance of potential viral contaminants. Murine Minute Virus (MMV)-spiking experiments were performed at small scale to investigate the impact on the viral clearance efficiency of the way the Protein A chromatography step is carried out, whether in batch or multicolumn mode. Protein A chromatography step using Novasep Sequential MultiColumn Chromatography (SMCC) technology demonstrated no statistical difference in the viral reduction with reduction factor (RF) of 3.7 log10 (vs. RF of 3.8 log10 for batch). The experiments showed also similar viral distribution over the purification cycles and columns. Data confirmed that the viral clearance capacity by the continuous Protein A chromatography step using SMCC technology is maintained and efficient.
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