| Literature DB >> 26573365 |
Martin Pabst1, Iva Benešová1,2, Stephan R Fagerer1, Mathias Jacobsen1, Klaus Eyer1, Gregor Schmidt3, Robert Steinhoff1, Jasmin Krismer1, Fabian Wahl4, Jan Preisler2,5, Renato Zenobi1.
Abstract
We introduce a stable isotope labeling approach for glycopeptides that allows a specific glycosylation site in a protein to be quantitatively evaluated using mass spectrometry. Succinic anhydride is used to specifically label primary amino groups of the peptide portion of the glycopeptides. The heavy form (D4(13)C4) provides an 8 Da mass increment over the light natural form (H4(12)C4), allowing simultaneous analysis and direct comparison of two glycopeptide profiles in a single MS scan. We have optimized a protocol for an in-solution trypsin digestion, a one-pot labeling procedure, and a post-labeling solid-phase extraction to obtain purified and labeled glycopeptides. We provide the first demonstration of this approach by comparing IgG1 Fc glycopeptides from polyclonal IgG samples with respect to their galactosylation and sialylation patterns using MALDI MS and LC-ESI-MS.Entities:
Keywords: IgG; LC−ESI−MS; MALDI MS; glycopeptides; stable isotope labeling
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Year: 2015 PMID: 26573365 DOI: 10.1021/acs.jproteome.5b00899
Source DB: PubMed Journal: J Proteome Res ISSN: 1535-3893 Impact factor: 4.466