Stable isotope labeling based on relative peptide/protein abundance measurements is commonly applied for quantitative proteomics. Recently, trypsin-catalyzed oxygen-18 labeling has grown in popularity due to its simplicity, cost-effectiveness, and its ability to universally label peptides with high sample recovery. In (18)O labeling, both C-terminal carboxyl group atoms of tryptic peptides can be enzymatically exchanged with (18)O, thus providing the labeled peptide with a 4 Da mass shift from the (16)O-labeled sample. Peptide (18)O labeling is ideally suited for generating a labeled "universal" reference sample used for obtaining accurate and reproducible quantitative measurements across large number of samples in quantitative discovery proteomics.
Revised: July 20, 2011 |
Published: July 1, 2011
Citation
Qian W., B.O. Petritis, C.D. Nicora, and R.D. Smith. 2011.Trypsin-catalyzed oxygen-18 labeling for quantitative proteomics. In Gel-Free Proteomics, Methods and Protocols: Methods in Molecular Biology, edited by K Gevaert and J Vandekerckhove. 43-54. Totowa, New Jersey:Humana Press Inc.PNNL-SA-78931.