Illuminating a biologics development challenge: systematic characterization of CHO cell-derived hydrolases identified in monoclonal antibody formulations

中国仓鼠卵巢细胞 化学 单克隆抗体 生物过程 生物化学 丝氨酸水解酶 亲和层析 重组DNA 丝氨酸 抗体 生物 免疫学 古生物学 受体 基因
作者
Michael K. Maier,Linus Weiß,Nikolas Zeh,Valerie Schmieder‐Todtenhaupt,Alireza Dehghani,Marius Nicolaus Felix,Daniel Heinzelmann,Benjamin Lindner,Moritz J. Schmidt,Joey Studts,Patrick Schulz,Bernd Reisinger,Kerstin Otte,Matthias Franzreb,Daniel Lakatos,Simon Fischer
出处
期刊:mAbs [Informa]
卷期号:16 (1) 被引量:1
标识
DOI:10.1080/19420862.2024.2375798
摘要

Monoclonal antibodies (mAb) and other biological drugs are affected by enzymatic polysorbate (PS) degradation that reduces product stability and jeopardizes the supply of innovative medicines. PS represents a critical surfactant stabilizing the active pharmaceutical ingredients, which are produced by recombinant Chinese hamster ovary (CHO) cell lines. While the list of potential PS-degrading CHO host cell proteins (HCPs) has grown over the years, tangible data on industrially relevant HCPs are still scarce. By means of a highly sensitive liquid chromatography-tandem mass spectrometry method, we investigated seven different mAb products, resulting in the identification of 12 potentially PS-degrading hydrolases, including the strongly PS-degrading lipoprotein lipase (LPL). Using an LPL knockout CHO host cell line, we were able to stably overexpress and purify the remaining candidate hydrolases through orthogonal affinity chromatography methods, enabling their detailed functional characterization. Applying a PS degradation assay, we found nine mostly secreted, PS-active hydrolases with varying hydrolytic activity. All active hydrolases showed a serine-histidine-aspartate/glutamate catalytical triad. Further, we subjected the active hydrolases to pH-screenings and revealed a diverse range of activity optima, which can facilitate the identification of residual hydrolases during bioprocess development. Ultimately, we compiled our dataset in a risk matrix identifying PAF-AH, LIPA, PPT1, and LPLA2 as highly critical hydrolases based on their cellular expression, detection in purified antibodies, active secretion, and PS degradation activity. With this work, we pave the way toward a comprehensive functional characterization of PS-degrading hydrolases and provide a basis for a future reduction of PS degradation in biopharmaceutical drug products.
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