Identification and classification of host cell proteins during biopharmaceutical process development.

Biotechnol Prog

The Advanced Centre for Biochemical Engineering, Department of Biochemical Engineering, University College London, London, UK.

Published: January 2022

AI Article Synopsis

  • Significant advancements in volumetric antibody productivity have led to challenges in recovering harvest materials, prompting a need for integration of upstream and downstream processing to address purification issues early on.
  • Research on CHO-expressed IgG1 showed that as cell culture duration increased, product quality declined with higher levels of host cell proteins (HCPs) detected during purification, indicating problematic trends related to longer cultivation times.
  • Mass spectrometry analysis identified specific types of HCPs that increase with culture duration, offering valuable insights for improving mAb purification processes and overall product quality.

Article Abstract

As significant improvements in volumetric antibody productivity have been achieved by advances in upstream processing over the last decade, and harvest material has become progressively more difficult to recover with these intensified upstream operations, the segregation of upstream and downstream processing has remained largely unchanged. By integrating upstream and downstream process development, product purification issues are given consideration during the optimization of upstream operating conditions, which mitigates the need for extensive and expensive clearance strategies downstream. To investigate the impact of cell culture duration on critical quality attributes, CHO-expressed IgG1 was cultivated in two 2 L bioreactors with samples taken on days 8, 10, 13, 15, and 17. The material was centrifuged, filtered and protein A purified on a 1 ml HiTrap column. Host cell protein (HCP) identification by mass spectrometry (MS) was applied to this system to provide insights into cellular behavior and HCP carryover during protein A purification. It was shown that as cultivation progressed from day 8 to 17 and antibody titer increased, product quality declined due to an increase in post-protein A HCPs (from 72 to 475 peptides detected by MS) and a decrease in product monomer percentage (from 98% to 95.5%). Additionally, the MS data revealed an increase in the abundance of several classes of post-protein A HCPs (e.g., stress response proteins and indicators of cell age), particularly on days 15 and 17 of culture, which were associated with significant increases in total overall HCP levels. This provides new insight into the specific types of HCPs that are retained during mAb purification and may be used to aid process development strategies.

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Source
http://www.ncbi.nlm.nih.gov/pmc/articles/PMC11475378PMC
http://dx.doi.org/10.1002/btpr.3224DOI Listing

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