Literature DB >> 26280711

Quantitative host cell protein analysis using two dimensional data independent LC-MS(E).

Amy Farrell1,2, Stefan Mittermayr1, Brian Morrissey1, Niaobh Mc Loughlin1, Natalia Navas Iglesias3, Ian W Marison2, Jonathan Bones1.   

Abstract

Host cell proteins (HCPs) are bioprocess-related impurities arising from cell-death or secretion from nonhuman cells used for recombinant protein production. Clearance of HCPs through downstream purification (DSP) is required to produce safe and efficacious therapeutic proteins. While traditionally measured using anti-HCP ELISA, more in-depth approaches for HCP characterization may ensure that risks to patients from HCPs are adequately assessed. Mass spectrometry methods provide rationale for targeted removal strategies through the provision of both qualitative and quantitative HCP information. A high pH, low pH, reversed-phase data independent 2D-LC-MS(E) proteomic platform was applied to determine HCP repertoires in the Protein A purified monoclonal antibody (mAb) samples as a function of culture harvest time, elution buffer used for DSP and also following inclusion of additional DSP steps. Critical quality attributes (CQAs) were examined for mAbs purified with different Protein A elution buffers to ensure that the selected buffers not only minimized the HCP profile but also exhibited no adverse effect on product quality. Results indicated that an arginine based Protein A elution buffer minimized the levels of HCPs identified and quantified in a purified mAb sample and also demonstrated no impact on product CQAs. It was also observed that mAbs harvested at later stages of cell culture contained higher concentrations of HCPs but that these were successfully removed by the addition of DSP steps complementary to Protein A purification. Taken together, our results showed how mass spectrometry based methods for HCP determination in conjunction with careful consideration of processing parameters such as harvest time, Protein A elution buffers, and subsequent DSP steps can reduce the HCP repertoire of therapeutic mAbs.

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Year:  2015        PMID: 26280711     DOI: 10.1021/acs.analchem.5b01377

Source DB:  PubMed          Journal:  Anal Chem        ISSN: 0003-2700            Impact factor:   6.986


  8 in total

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2.  A Retrospective Evaluation of the Use of Mass Spectrometry in FDA Biologics License Applications.

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4.  ELISA reagent coverage evaluation by affinity purification tandem mass spectrometry.

Authors:  Scott M Henry; Elissa Sutlief; Oscar Salas-Solano; John Valliere-Douglass
Journal:  MAbs       Date:  2017-07-14       Impact factor: 5.857

5.  An HS-MRM Assay for the Quantification of Host-cell Proteins in Protein Biopharmaceuticals by Liquid Chromatography Ion Mobility QTOF Mass Spectrometry.

Authors:  Catalin Doneanu; Jing Fang; Yun Alelyunas; Ying Qing Yu; Mark Wrona; Weibin Chen
Journal:  J Vis Exp       Date:  2018-04-17       Impact factor: 1.355

6.  Cathepsin L Causes Proteolytic Cleavage of Chinese-Hamster-Ovary Cell Expressed Proteins During Processing and Storage: Identification, Characterization, and Mitigation.

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7.  Detection and quantitation of host cell proteins in monoclonal antibody drug products using automated sample preparation and data-independent acquisition LC-MS/MS.

Authors:  Lisa Strasser; Giorgio Oliviero; Craig Jakes; Izabela Zaborowska; Patrick Floris; Meire Ribeiro da Silva; Florian Füssl; Sara Carillo; Jonathan Bones
Journal:  J Pharm Anal       Date:  2021-05-20

8.  Exploring sample preparation and data evaluation strategies for enhanced identification of host cell proteins in drug products of therapeutic antibodies and Fc-fusion proteins.

Authors:  Wolfgang Esser-Skala; Marius Segl; Therese Wohlschlager; Veronika Reisinger; Johann Holzmann; Christian G Huber
Journal:  Anal Bioanal Chem       Date:  2020-07-20       Impact factor: 4.142

  8 in total

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