More similar than different: Host cell protein production using three null CHO cell lines

Yuk, Inn H.; Nishihara, Julie C.; Walker, Donald E.; Huang, L. Eric; Gunawan, Feny; Subramanian, Jayashree; Pynn, Abigail F.J.; Yu, Xiaoyan; Zhu-Shimoni, Judith; Vanderlaan, Martin; Krawitz, Denise C.

doi:10.1002/bit.25615

Cited by 50 publications

(60 citation statements)

References 50 publications

(79 reference statements)

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“…These results suggest that, while final drug product HCP profiles are influenced by the innate identities and abundances of the host cell, many important differences exist. Given the findings herein plus recent results that showed high similarity between proteomic profiles of different null CHO cell lines and upstream processes, 44 variations in downstream processes are likely the primary cause of the significant differences we observed for final drug product HCP profiles as certain proteins will be more effectively purified than others (depending on the downstream process employed).…”

Section: Wwwtandfonlinecomsupporting

confidence: 50%

Toward the complete characterization of host cell proteins in biotherapeutics via affinity depletions, LC-MS/MS, and multivariate analysis

Farutin²,

Carbeau³

et al. 2015

mAbs

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Section: Wwwtandfonlinecomsupporting

confidence: 50%

Toward the complete characterization of host cell proteins in biotherapeutics via affinity depletions, LC-MS/MS, and multivariate analysis

Farutin²,

Carbeau³

et al. 2015

mAbs

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“…Hence, bacterial HCPs have the potential to influence the immunogenicity of the biotherapeutic by having adjuvant‐like activity. HCP contamination is also an issue for mammalian cell expression systems 6, 12, 13. However, non‐mammalian HCPs are more likely to pose a risk in patients, compared with their mammalian counterparts.…”

Section: Introductionmentioning

confidence: 99%

Influence of Escherichia coli chaperone DnaK on protein immunogenicity

et al. 2016

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SummaryThe production of anti‐drug antibodies can impact significantly upon the safety and efficacy of biotherapeutics. It is known that various factors, including aggregation and the presence of process‐related impurities, can modify and augment the immunogenic potential of proteins. The purpose of the investigations reported here was to characterize in mice the influence of aggregation and host cell protein impurities on the immunogenicity of a humanized single‐chain antibody variable fragment (scFv), and mouse albumin. Host cell protein impurities within an scFv preparation purified from Escherichia coli displayed adjuvant‐like activity for responses to the scFv in BALB/c strain mice. The 70 000 MW E. coli chaperone protein DnaK was identified as a key contaminant of scFv by mass spectrometric analysis. Preparations of scFv lacking detectable DnaK were spiked with recombinant E. coli DnaK to mimic the process‐related impurity. Mice were immunized with monomeric and aggregated preparations, with and without 0·1% DnaK by mass. Aggregation alone enhanced IgM and IgG2a antibody responses, but had no significant effect on total IgG or IgG1 responses. The addition of DnaK further enhanced IgG and IgG2a antibody responses, but only in the presence of aggregated protein. DnaK was shown to be associated with the aggregated scFv by Western blot analysis. Experiments with mouse albumin showed an overall increase in immunogenicity with protein aggregation alone, and the presence of DnaK increased the vigour of the IgG2a antibody response further. Collectively these data reveal that DnaK has the potential to modify and enhance immunogenicity when associated with aggregated protein.

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“…PLBL2 was identified and quantified in HCCF, with the Top 3 strategy 19 using a 4-point calibration curve of spiked internal standard protein (bovine carbonic anhydrase II). Table 1 shows the quantitation results obtained by DIA SWATH MS and by a PLBL2-specific ELISA 25 in five HCCF samples. Results showed that the measured PLBL2 levels by DIA SWATH MS quantification agreed well with those from an orthogonal analysis by PLBL2-specific ELISA ( Table 1).…”

Section: D Uhplc-ms/ms Strategies For Absolute Quantitation Of Hcps mentioning

confidence: 99%

“…This molar concentration was then normalized by the MW ratio of the HCP to the bovine carbonic anhydrase II to calculate the ppm level of these HCPs. Similarly, PLBL2 molar concentration was determined using the 4-point standard curve generated from the Top 3 peak area data of bovine carbonic anhydrase II, which was then converted to the mg/mL to compare with ELISA 25 results. Carbonic anhydrase II peptides used for quantification were unique to the bovine sequence of the protein.…”

Section: Quantitative Analysis Of Data Independent Swath Ms and Prm Datamentioning

confidence: 99%

A modular and adaptive mass spectrometry-based platform for support of bioprocess development toward optimal host cell protein clearance

Walker

Yang

Carver

et al. 2017

mAbs

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A modular and adaptive mass spectrometry (MS)-based platform was developed to provide fast, robust and sensitive host cell protein (HCP) analytics to support process development. This platform relies on one-dimensional ultra-high performance liquid chromatography (1D UHPLC) combined with several different MS data acquisition strategies to meet the needs of purification process development. The workflow was designed to allow HCP composition and quantitation for up to 20 samples per day, a throughput considered essential for real time bioprocess development support. With data-dependent acquisition (DDA), the 1D UHPLC-MS/MS method had excellent speed and demonstrated robustness in detecting unknown HCPs at 50 ng/mg (ppm) level. Combining 1D UHPLC with sequential window acquisition of all theoretical spectra (SWATH) MS enabled simultaneous detection and quantitation of all HCPs in single-digit ng/mg range within 1 hour, demonstrating for the first time the benefit of SWATH MS as a technique for HCP analysis. As another alternative, a targeted MS approach can be used to track the clearance of specific known HCP under various process conditions. This study highlights the importance of designing a robust LC-MS/MS workflow that not only allows HCP discovery, but also affords greatly improved process knowledge and capability in HCP removal. As an orthogonal and complementary detection approach to traditional HCP analysis by enzyme-linked immunosorbent assay, the reported LC-MS/MS workflow supports the development of bioprocesses with optimal HCP clearance and the production of safe and high quality therapeutic biopharmaceuticals.

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More similar than different: Host cell protein production using three null CHO cell lines

Cited by 50 publications

References 50 publications

Toward the complete characterization of host cell proteins in biotherapeutics via affinity depletions, LC-MS/MS, and multivariate analysis

Toward the complete characterization of host cell proteins in biotherapeutics via affinity depletions, LC-MS/MS, and multivariate analysis

Influence of Escherichia coli chaperone DnaK on protein immunogenicity

A modular and adaptive mass spectrometry-based platform for support of bioprocess development toward optimal host cell protein clearance

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