Trypsin is the primary mechanism by which the 18O isotopic label is lost in quantitative proteomic studies

Publisher Website

1 December 2006

journal article
Published by Elsevier in Analytical Biochemistry

Vol. 359 (1), 26-34
https://doi.org/10.1016/j.ab.2006.08.036

Abstract

No abstract available

Keywords

This publication has 26 references indexed in Scilit:

Proteolytic ¹⁸O Labeling by Peptidyl-Lys Metalloendopeptidase for Comparative Proteomics
Journal of Proteome Research, 2005
Quantitative Proteomic Analysis by Accurate Mass Retention Time Pairs
Analytical Chemistry, 2005
Quantitative Profiling of the Detergent-Resistant Membrane Proteome of Iota-b Toxin Induced Vero Cells
Journal of Proteome Research, 2005
Stable-Isotope Dimethyl Labeling for Quantitative Proteomics
Analytical Chemistry, 2003
Quantitation of Neuropeptides in Cpe^f^at/Cpe^f^atMice Using Differential Isotopic Tags and Mass Spectrometry
Analytical Chemistry, 2002
¹⁸O Labeling: a tool for proteomics
Rapid Communications in Mass Spectrometry, 2001
High Throughput Proteome-Wide Precision Measurements of Protein Expression Using Mass Spectrometry
Journal of the American Chemical Society, 1999
Protease‐catalyzed incorporation of ¹⁸O into peptide fragments and its application for protein sequencing by electrospray and matrix‐assisted laser desorption/ionization mass spectrometry
Electrophoresis, 1996
Preparation of stable isotope-incorporated peptide internal standards for field desorption mass spectrometry quantification of peptides in biologic tissue
Journal of Mass Spectrometry, 1983
INACTIVATION OF CRYSTALLINE TRYPSIN
The Journal of general physiology, 1934

Cited by 18 articles