Characterization of Variable Regions of Monoclonal Antibodies by Top-Down Mass Spectrometry

26 June 2007

journal article
Published by American Chemical Society (ACS) in Analytical Chemistry

Vol. 79 (15), 5723-5729
https://doi.org/10.1021/ac070483q

Abstract

A technique for rapid characterization of variable regions of monoclonal antibodies (mAb) is described. Several intact mAbs were analyzed on a Thermo-Fisher LTQ-Orbitrap high-resolution mass spectrometer (MS) by in-source fragmentation. In-source fragmentation has the unique advantage of fragmenting all charge states of a protein at the same time and, thus, greatly improves the sensitivity of the fragment ions over a true MS/MS experiment, where a single charge state is isolated and fragmented. In addition, immediate fragmentation of the protein before tertiary structure formation may also facilitate protein fragmentation. This technique has been proved very useful for top-down analysis of large proteins. In-source fragmentation of mAbs generated a series of fragment ions. In addition to some small b and y ions from the light chain and heavy chain in the low m/z region, a series of b ions corresponding to N-terminal 106−120 residues of both heavy chain and light chain were observed. The cleavage sites for these b ions happen to be near the linker regions between the variable domains and the constant domains of these antibodies. These b ions, therefore, correspond to the entire variable region of each chain. Similar results were obtained for all mAbs analyzed, including both immunoglobulin G₁ and G₂ molecules. To further characterize the variable regions, these b ions were isolated and fragmented by collision-induced dissociation in the linear trap, followed by mass analysis in the orbitrap. Large number of product ions was observed from these b ions. Many of these product ions are internal fragments between the two disulfide-linked cysteine residues. To demonstrate the capability of the technique, several mAbs were force-oxidized by treating with tert-butyl hydroperoxide, followed by mass spectrometric analysis. In-source fragmentation and MS/MS of the variable region b ions clearly identified the locations of the oxidized methionine.

Keywords

This publication has 11 references indexed in Scilit:

Top-down Protein Sequencing and MS3 on a Hybrid Linear Quadrupole Ion Trap-Orbitrap Mass Spectrometer
Molecular & Cellular Proteomics, 2006
Formation of Pyroglutamic Acid from N-Terminal Glutamic Acid in Immunoglobulin Gamma Antibodies
Analytical Chemistry, 2006
Stepwise Deamidation of Ribonuclease A at Five Sites Determined by Top Down Mass Spectrometry
Biochemistry, 2005
Consecutive Ion Activation for Top Down Mass Spectrometry: Improved Protein Sequencing by Nozzle−Skimmer Dissociation
Analytical Chemistry, 2005
Peer Reviewed: Top-Down Proteomics
Published by American Chemical Society (ACS) ,2004
Proteomics by FTICR mass spectrometry: Top down and bottom up
Mass Spectrometry Reviews, 2004
Matrix-assisted laser desorption/ionization mass spectrometry for the evaluation of the C-terminal lysine distribution of a recombinant monoclonal antibody
Rapid Communications in Mass Spectrometry, 2004
A top down approach to protein structural studies using chemical cross‐linking and Fourier transform mass spectrometry
Rapid Communications in Mass Spectrometry, 2002
Top Down versus Bottom Up Protein Characterization by Tandem High-Resolution Mass Spectrometry
Journal of the American Chemical Society, 1999
Nondependence of diffusion-controlled peak dispersion on diffusion coefficient and ionic mobility in capillary zone electrophoresis without electroosmotic flow
Analytical Chemistry, 1991

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