Quantitative Analysis of Complex Peptide Mixtures Using FTMS and Differential Mass Spectrometry

Label-free LC-MS profiling is a powerful quantitative proteomic method to study relative peptide abundances between two or more biological samples. Here we demonstrate the use of a previously described comparative LC-MS method, differential mass spectrometry (dMS), to analyze high-resolution Fourier...

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Veröffentlicht in:Journal of the American Society for Mass Spectrometry 2007-02, Vol.18 (2), p.226-233
Hauptverfasser: Meng, Fanyu, Wiener, Matthew C., Sachs, Jeffrey R., Burns, Chrissina, Verma, Priyanka, Paweletz, Cloud P., Mazur, Matthew T., Deyanova, Ekaterina G., Yates, Nathan A., Hendrickson, Ronald C.
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Sprache:eng
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Zusammenfassung:Label-free LC-MS profiling is a powerful quantitative proteomic method to study relative peptide abundances between two or more biological samples. Here we demonstrate the use of a previously described comparative LC-MS method, differential mass spectrometry (dMS), to analyze high-resolution Fourier transform mass spectrometry (FTMS) data for detection and quantification of known peptide differences between two sets of complex mixtures. Six standard peptides were spiked into a processed plasma background at fixed ratios from 1.25:1 to 4:1 to make two sets of samples. The resulting mixtures were analyzed by microcapillary LC-FTMS and dMS. dMS successfully identified five out of the six peptides as statistically significant differences ( p ≤ 0.005). In this experiment, the smallest fold change reliably detected by our method was 1.5:1, and the errors of estimated ratios of concentrations were less than 20% for peptides spiked at 1.5:1 to 4:1. We conclude that LC-FTMS coupled with dMS is a useful label-free quantitative MS method that can be used to detect subtle yet statistically significant peptide differences in complex protein mixtures, including plasma samples.
ISSN:1044-0305
1879-1123
DOI:10.1016/j.jasms.2006.09.014