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

被引:0
|
作者
Lisa Strasser [1 ]
Giorgio Oliviero [1 ]
Craig Jakes [1 ,2 ]
Izabela Zaborowska [1 ]
Patrick Floris [1 ]
Meire Ribeiro da Silva [1 ]
Florian Füssl [1 ]
Sara Carillo [1 ]
Jonathan Bones [1 ,2 ]
机构
[1] Characterization and Comparability Laboratory,NIBRT-National Institute for Bioprocessing Research and Training
[2] School of Chemical and Bioprocess Engineering,University College Dublin
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中图分类号
R392 [医学免疫学];
学科分类号
100102 ;
摘要
Ensuring the removal of host cell proteins(HCPs) during downstream processing of recombinant proteins such as monoclonal antibodies(m Abs) remains a challenge. Since residual HCPs might affect product stability or safety, constant monitoring is required to demonstrate their removal to be below the regulatory accepted level of 100 ng/mg. The current standard analytical approach for this procedure is based on ELISA; however, this approach only measures the overall HCP content. Therefore, the use of orthogonal methods, such as liquid chromatography-mass spectrometry(LC-MS), has been established,as it facilitates the quantitation of total HCPs as well as the identification and quantitation of the individual HCPs present. In the present study, a workflow for HCP detection and quantitation using an automated magnetic bead-based sample preparation, in combination with a data-independent acquisition(DIA) LC-MS analysis, was established. Employing the same instrumental setup commonly used for peptide mapping analysis of m Abs allows for its quick and easy implementation into pre-existing workflows, avoiding the need for dedicated instrumentation or personnel. Thereby, quantitation of HCPs over a broad dynamic range was enabled to allow monitoring of problematic HCPs or to track changes upon altered bioprocessing conditions.
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页码:726 / 731
页数:6
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