Combining low- and high-energy tandem mass spectra for optimized peptide quantification with isobaric tags

被引:81
|
作者
Dayon, Loic [1 ]
Pasquarello, Carla [2 ]
Hoogland, Christine [3 ]
Sanchez, Jean-Charles [1 ,2 ]
Scherl, Alexander [2 ]
机构
[1] Univ Geneva, Fac Med, Dept Struct Biol & Bioinformat, Biomed Prote Grp, Geneva, Switzerland
[2] Univ Geneva, Fac Med, Prote Core Facil, Geneva, Switzerland
[3] Swiss Inst Bioinformat, Proteome Informat Grp, Geneva, Switzerland
关键词
Quantitation; ESI; iTRAQ; Mass spectrometry; Orbitrap; Proteomics; Tandem mass tags; TMT; COMPLEX PROTEIN MIXTURES; QUANTITATIVE PROTEOMICS; SPECTROMETER; ORBITRAP; EXPRESSION; ACCURACY; STRATEGY; MS/MS; IONS;
D O I
10.1016/j.jprot.2009.10.015
中图分类号
Q5 [生物化学];
学科分类号
071010 ; 081704 ;
摘要
Isobaric tagging, via TMT or iTRAQ is widely used in quantitative proteomics. To date, tandem mass spectrometric analysis of isobarically-labeled peptides with hybrid ion trap-orbitrap (LTQ-OT) instruments has been mainly carried out with higher-energy C-trap dissociation (HCD) or pulsed q dissociation (PQD). HCD provides good fragmentation of the reporter-ions, but peptide sequence-ion recovery is generally poor compared to collision-induced dissociation (CID). Herein, we describe an approach where CID and HCD spectra are combined. The approach ensures efficiently both identification and relative quantification of proteins. Tandem mass tags (TMTs) were used to label digests of human plasma and LC-MS/MS was performed with an LTQ-OT instrument. Different HCD collision energies were tested. The benefits to use CID and HCD with respect to HCD alone were demonstrated in terms of number of identifications, subsequent number of quantifiable proteins, and quantification accuracy. A program was developed to merge the peptide sequence-ion m/z range from CID spectra and the reporter-ion m/z range from HCD spectra, and alternatively to separate both spectral data into different files. As parallel CID in the LTQ almost doesn't affect the analysis duty cycle, the procedure should become a standard for quantitative analyses of proteins with isobaric tagging using LTQ-OT instruments. (C) 2009 Elsevier B.V. All rights reserved.
引用
收藏
页码:769 / 777
页数:9
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