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Enhancing Protein Sequencing through the C-Terminal Labeling Strategy: Resolving Isobaric Ambiguities by Electron-Transfer/Higher Energy Collision Dissociation (EThcD). | LitMetric

AI Article Synopsis

  • The study discusses a new labeling strategy for improving peptide detection in mass spectrometry by modifying peptides at their C-terminal and specific amino acids (Aspartic and Glutamic acid) with arginine methyl ester (R-met).
  • This modification enhances peptide fragmentation and helps distinguish isobaric ambiguities, which can complicate protein sequencing.
  • The approach is tested across various proteins and proteases, demonstrating its effectiveness in producing clearer mass spectrometry results, particularly when focusing on charge states of +2 or higher for better fragmentation.

Article Abstract

protein sequencing via a bottom-up approach requires various proteases to produce overlapping peptides. However, peptides generated by proteases other than trypsin, LysC, and ArgC often yield C-terminal fragments with suboptimal ionization in positive mode mass spectrometry (MS). This study introduces a novel peptide labeling strategy that involves modifying peptides at the C-terminal and at the carboxyl groups of Aspartic and Glutamic acid with arginine methyl ester (R-met) to improve peptide fragmentation and resolve isobaric ambiguities encountered during sequencing. An amidation reaction is used with coupling reagents to conjugate R-met to the peptide's C-terminal end, introducing a functional group that enhances the detectability of C-terminal peptide fragment ions by mass spectrometry. Subsequently, selecting a charge state of +2 or higher can facilitate optimal fragmentation of the derivatized peptides using electron-transfer/higher energy collision dissociation (EThcD), thereby generating essential w-ions to resolve common isobaric ambiguities. Demonstrating this strategy across diverse protein types, including albumin and antibodies and using different proteases for digestion, highlights the unique characteristics of combining the proposed amidation reaction with the specific proteases tested.

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Source
http://dx.doi.org/10.1021/acs.analchem.4c03459DOI Listing

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