Glu-C, an alternative digestive enzyme for the quantitative LC–MS/MS analysis of an IgG-based antibody biotherapeutic

Author:

Hansen Kjetil1,Szarka Szabolcs1,Escoffier Emilie2,Berthet Amandine2,Venet Joris2,Collet-Brose Justine2,Hepburn Sophie3,Wright Michael1,Wheller Robert1,Nelson Robert2,Kay Richard G14

Affiliation:

1. LGC, Newmarket Road, Fordham, Cambridgeshire, CB7 5WW, UK

2. Novimmune SA, 1228 Plan-les-Ouates, Geneva, Switzerland

3. Blood Sciences Department, Ipswich Hospital Hub Laboratory, Ipswich IP4 5PD, UK

4. Present affiliation: Metabolic Research Laboratories, Institute of Metabolic Science, Addenbrooke's Hospital, Hills Road, Cambridge CB2 0QQ, UK

Abstract

Aim: LC–MS/MS bottom-up quantitation of proteins has become increasingly popular with trypsin as the most commonly used protease. However, trypsin does not always yield suitable surrogate peptides. An alternative enzyme, Glu-C, was used to generate surrogate peptides for quantifying a bispecific IgG1 biotherapeutic antibody in preclinical matrices.  Materials and methods: IgG1 was quantified by pellet digestion using an Acquity UPLC coupled  with a Xevo TQ-S mass spectrometer.  Results: Two generic LC–MS/MS methods (heavy and light chain) were developed which afforded acceptable precision and accuracy, and an lower limit of quantitation of 1 μg/ml in three preclinical matrices. A small nonsignificant bias was observed when cynomolgus serum LC–MS/MS results were compared with electrochemiluminescent immunoassay data. Conclusion: Glu-C was successfully used as an alternative digestion enzyme for bottom-up quantitation of an IgG1 in matrices from multiple preclinical species, with good agreement with electrochemiluminescent immunoassay data.

Publisher

Future Science Ltd

Subject

Medical Laboratory Technology,Clinical Biochemistry,General Pharmacology, Toxicology and Pharmaceutics,General Medicine,Analytical Chemistry

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