Parallel reaction monitoring using quadrupole-Orbitrap mass spectrometer: Principle and applications

被引:207
|
作者
Bourmaud, Adele [1 ,2 ]
Gallien, Sebastien [1 ]
Domon, Bruno [1 ,2 ]
机构
[1] Luxembourg Inst Hlth, Luxembourg Clin Prote Ctr, L-1445 Strassen, Luxembourg
[2] Univ Luxembourg, Doctoral Sch Syst & Mol Biomed, Esch Sur Alzette, Luxembourg
关键词
High resolution accurate mass; Parallel reaction monitoring; Precise quantification; Targeted proteomics; Technology; TARGETED PROTEOMICS; HIGH-RESOLUTION; YEAST PROTEOME; DYNAMIC-RANGE; QUANTIFICATION; SPECTRA; SRM; PRM; IDENTIFICATION; PLASMA;
D O I
10.1002/pmic.201500543
中图分类号
Q5 [生物化学];
学科分类号
071010 ; 081704 ;
摘要
Targeted mass spectrometry-based approaches are nowadays widely used for quantitative proteomics studies and more recently have been implemented on high resolution/accurate mass (HRAM) instruments resulting in a considerable performance improvement. More specifically, the parallel reaction monitoring technique (PRM) performed on quadrupole-Orbitrap mass spectrometers, leveraging the high resolution and trapping capabilities of the instrument, offers a clear advantage over the conventional selected reaction monitoring (SRM) measurements executed on triple quadrupole instruments. Analyses performed in HRAM mode allow for an improved discrimination between signals derived from analytes and those resulting from matrix interferences translating in the reliable quantification of low abundance components. The purpose of the study defines various implementation schemes of PRM, namely: (i) exploratory experiments assessing the detectability of very large sets of peptides (100-1000), (ii) wide-screen analyses using (crude) internal standards to obtain statistically meaningful (relative) quantitative analyses, and (iii) precise/accurate quantification of a limited number of analytes using calibrated internal standards. Each of the three implementation schemes requires specific acquisition methods with defined parameters to appropriately control the acquisition during the actual peptide elution. This tutorial describes the different PRM approaches and discusses their benefits and limitations in terms of quantification performance and confidence in analyte identification.
引用
收藏
页码:2146 / 2159
页数:14
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