4.7 Article

Host cell protein dynamics in recombinant CHO cells Impacts from harvest to purification and beyond

Journal

BIOENGINEERED
Volume 4, Issue 5, Pages 288-291

Publisher

LANDES BIOSCIENCE
DOI: 10.4161/bioe.23382

Keywords

host cell protein; Chinese hamster ovary (CHO); mammalian cell culture; downstream processing; protein A chromatography; monoclonal antibody; proteomics

Funding

  1. Biotechnology and Biological Sciences Research Council [BB/L002310/1, BB/G010307/1, BB/G010358/1] Funding Source: researchfish
  2. Biotechnology and Biological Sciences Research Council [BB/G010307/1, BB/G010358/1] Funding Source: Medline
  3. BBSRC [BB/G010358/1, BB/G010307/1, BB/L002310/1] Funding Source: UKRI

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During the production of recombinant protein products, such as monoclonal antibodies, manufacturers must demonstrate clearance of host cell impurities and contaminants to appropriate levels prior to use in the clinic. These include host cell DNA and RNA, product related contaminants such as aggregates, and importantly host cell proteins (HCPs). Despite the importance of HCP removal, the identity and dynamics of these proteins during cell culture and downstream processing (DSP) are largely unknown. Improvements in technologies such as SELDI-TOF mass spectrometry alongside the gold standard technique of ELISA has allowed semi-quantification of the total HCPs present. However, only recently have techniques been utilized in order to identify those HCPs present and align this with the development of approaches to monitor the dynamics of HCPs during both fermentation and downstream processing. In order to enable knowledge based decisions with regards to improving HCP clearance it is vital to identify potential problematic HCPs on a cell line and product specific basis. Understanding the HCP dynamics will in the future help provide a platform to rationally manipulate and engineer and/or select suitable recombinant CHO cell lines and downstream processing steps to limit problematic HCPs.

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