Abstract
Mass spectrometry-based multiple reaction monitoring (MRM) quantitation of proteins can dramatically impact the discovery and quantitation of biomarkers via rapid, targeted, multiplexed protein expression profiling of clinical samples. A mixture of 45 peptide standards, easily adaptable to common plasma proteomics work flows, was created to permit absolute quantitation of 45 endogenous proteins in human plasma trypsin digests. All experiments were performed on simple tryptic digests of human EDTA-plasma without prior affinity depletion or enrichment. Stable isotope-labeled standard peptides were added immediately following tryptic digestion because addition of stable isotope-labeled standard peptides prior to trypsin digestion was found to generate elevated and unpredictable results. Proteotypic tryptic peptides containing isotopically coded amino acids ([(13)C(6)]Arg or [(13)C(6)]Lys) were synthesized for all 45 proteins. Peptide purity was assessed by capillary zone electrophoresis, and the peptide quantity was determined by amino acid analysis. For maximum sensitivity and specificity, instrumental parameters were empirically determined to generate the most abundant precursor ions and y ion fragments. Concentrations of individual peptide standards in the mixture were optimized to approximate endogenous concentrations of analytes and to ensure the maximum linear dynamic range of the MRM assays. Excellent linear responses (r > 0.99) were obtained for 43 of the 45 proteins with attomole level limits of quantitation (<20% coefficient of variation) for 27 of the 45 proteins. Analytical precision for 44 of the 45 assays varied by <10%. LC-MRM/MS analyses performed on 3 different days on different batches of plasma trypsin digests resulted in coefficients of variation of <20% for 42 of the 45 assays. Concentrations for 39 of the 45 proteins are within a factor of 2 of reported literature values. This mixture of internal standards has many uses and can be applied to the characterization of trypsin digestion kinetics and plasma protein expression profiling because 31 of the 45 proteins are putative biomarkers of cardiovascular disease.
Highlights
Mass spectrometry-based multiple reaction monitoring (MRM) quantitation of proteins can dramatically impact the discovery and quantitation of biomarkers via rapid, targeted, multiplexed protein expression profiling of clinical samples
1) The peptide amino acid sequence must be unique to the target protein and contain no missed cleavage sites, 2) the peptide should be reproducibly observed in proteolytic digests, and 3) the peptide should not contain amino acids that are susceptible to chemical modification (Cys and Met)
When working with a species for which the genome has been sequenced and widely studied, as it has been for Homo sapiens, publicly accessible MS/MS spectra databases such as the Global Proteome Machine and Peptide Atlas are useful for determining which tryptic peptides of proteins are frequently observed by MS/MS analysis [21, 22]
Summary
Reagents and Chemicals—All reagents were American Chemical Society (ACS) grade or higher. MRM Q1/Q3 Ion Pair Selection by Nanoinfusion—Isotopically labeled peptides were diluted to 1 pmol/l (1 mM) in 30% acetonitrile, 0.1% formic acid for infusion at a flow rate of 300 nl/min using a Harvard PicoPlus 11 syringe pump (Harvard Apparatus, Holliston, MA). For quantitation of unknown samples, a concentration-balanced mixture of 45 isotopically labeled internal standard peptides (0.1% (v/v) formic acid) was added to each plasma digest at a ratio of 1 volume of SIS peptide mixture to 4 volumes of acidified plasma trypsin digest. This came to 50 l of SIS peptide mixture added per 1-l equivalent of neat plasma. Raw data files for these analyses are available from the ProteomeCommons Tranche network (http://www.proteomecommons. org/data-downloader.jsp?fileNameϭO3Hbto5xoHSurD7i5FYQMe6IKix jYxsB8ao8W/gpnNmIxQX2hNxoHXJORjyDg9s5x1mVmmϩ7ϩJ33b8F aEUBB7MuoGMAAAAAAAAAUXAϭϭ) using hash codes
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