Protein Quantification by Selective Isolation and Fragmentation of Isotopic Pairs Using FT-ICR MS

Hannah Johnson, Stephen C. C. Wong, Deborah M. Simpson, Robert J. Beynon, Simon J. Gaskell

Research output: Contribution to journalArticlepeer-review

Abstract

Isolation of tryptic peptide ions, along with their differentially labeled analogs derived from an artificial QconCAT protein, is performed using multiple correlated harmonic excitation fields in an FT-ICR cell. Simultaneous fragmentation of the isolated unlabeled and labeled peptide pairs using IRMPD yields specific y-series fragment ions useful for quantification. The mass increment attributed to stable isotope labeling at the C-terminus is maintained in the C-terminal fragment ions, providing multiple measurements of labeled/unlabeled intensity ratios during highly selective detection. The utility of this approach has been demonstrated in the absolute quantification of components of an unfractionated chicken muscle protein mixture. © 2008 American Society for Mass Spectrometry.
Original languageEnglish
Pages (from-to)973-977
Number of pages4
JournalJournal of the American Society for Mass Spectrometry
Volume19
Issue number7
DOIs
Publication statusPublished - Jul 2008

Keywords

  • MULTIPLEXED ABSOLUTE QUANTIFICATION
  • CONCATENATED SIGNATURE PEPTIDES
  • MASS-SPECTROMETRY
  • PROTEOMICS
  • QUANTITATION
  • EXCITATION
  • QCONCAT
  • IONS

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