Protein complex heterogeneity and topology revealed by electron capture charge reduction and surface induced dissociation

Author:

Shaw Jared B.ORCID,Harvey Sophie R.ORCID,Du ChenORCID,Xu ZhixinORCID,Edgington Regina M.,Olmedillas EduardoORCID,Saphire Erica OllmannORCID,Wysocki Vicki H.ORCID

Abstract

ABSTRACTWe illustrate the utility of native mass spectrometry (nMS) combined with a fast, tunable gas-phase charge reduction, electron capture charge reduction (ECCR), for the characterization of protein complex topology and glycoprotein heterogeneity. ECCR efficiently reduces the charge states of tetradecameric GroEL, illustrating Orbitrapm/zmeasurements to greater than 100,000m/z. For pentameric C-reactive protein and tetradecameric GroEL, our novel device combining ECCR with surface induced dissociation (SID) reduces the charge states and yields more topologically informative fragmentation. This is the first demonstration that ECCR yields more native-like SID fragmentation. ECCR also significantly improved mass and glycan heterogeneity measurements of heavily glycosylated SARS-CoV-2 spike protein trimer and thyroglobulin dimer. Protein glycosylation is important for structural and functional properties and plays essential roles in many biological processes. The immense heterogeneity in glycosylation sites and glycan structure poses significant analytical challenges that hinder a mechanistic understanding of the biological role of glycosylation. Without ECCR, average mass determination of glycoprotein complexes is available only through charge detection mass spectrometry or mass photometry. With narrowm/zselection windows followed by ECCR, multiple glycoformm/zvalues are apparent, providing quick global glycoform profiling and providing a future path for glycan localization on individual intact glycoforms.

Publisher

Cold Spring Harbor Laboratory

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