Numbers of Exchangeable Hydrogens from LC–MS Data of Heavy Water Metabolically Labeled Samples

Abstract: Labeling with deuterium oxide (D 2 O) has emerged as one of the preferred approaches for measuring the synthesis of individual proteins in vivo. In these experiments, the synthesis rates of proteins are determined by modeling mass shifts in peptides during the labeling period. This modeling depends on a theoretical maximum enrichment determined by the number of labeling sites (N EH ) of each amino acid in the peptide sequence. Currently, N EH is determined from one set of published values. However, it has been… Show more