Site-specific protein glycosylation analysis with glycan isomer differentiation

被引:99
作者
Hua, Serenus [5 ]
Nwosu, Charles C. [5 ]
Strum, John S. [5 ]
Seipert, Richard R. [5 ]
An, Hyun Joo [4 ]
Zivkovic, Angela M. [2 ,3 ]
German, J. Bruce [2 ,3 ]
Lebrilla, Carlito B. [1 ,2 ,5 ]
机构
[1] Univ Calif Davis, Dept Biochem & Mol Med, Davis, CA 95616 USA
[2] Univ Calif Davis, Foods Hlth Inst, Davis, CA 95616 USA
[3] Univ Calif Davis, Dept Food Sci & Technol, Davis, CA 95616 USA
[4] Chungnam Natl Univ, Grad Sch Analyt Sci & Technol, Taejon 305764, South Korea
[5] Univ Calif Davis, Dept Chem, Davis, CA 95616 USA
关键词
Site-specific glycosylation; Glycopeptide; Non-specific protease; Isomer; Quantitation; LC/MS; PERFORMANCE LIQUID-CHROMATOGRAPHY; GRAPHITIZED CARBON COLUMN; FLIGHT MASS-SPECTROMETRY; AFFINITY-CHROMATOGRAPHY; NONSPECIFIC PROTEASES; RIBONUCLEASE-B; OLIGOSACCHARIDES; GLYCOPEPTIDES; GLYCOPROTEINS; MS;
D O I
10.1007/s00216-011-5109-x
中图分类号
Q5 [生物化学];
学科分类号
071010 ; 081704 ;
摘要
Glycosylation is one of the most common yet diverse post-translational modifications. Information on glycan heterogeneity and glycosite occupancy is increasingly recognized as crucial to understanding glycoprotein structure and function. Yet, no approach currently exists with which to holistically consider both the proteomic and glycomic aspects of a system. Here, we developed a novel method of comprehensive glycosite profiling using nanoflow liquid chromatography/mass spectrometry (nano-LC/MS) that shows glycan isomer-specific differentiation on specific sites. Glycoproteins were digested by controlled non-specific proteolysis in order to produce informative glycopeptides. High-resolution, isomer-sensitive chromatographic separation of the glycopeptides was achieved using microfluidic chip-based capillaries packed with graphitized carbon. Integrated LC/MS/MS not only confirmed glycopeptide composition but also differentiated glycan and peptide isomers and yielded structural information on both the glycan and peptide moieties. Our analysis identified at least 13 distinct glycans (including isomers) corresponding to five compositions at the single N-glycosylation site on bovine ribonuclease B, 59 distinct glycans at five N-glycosylation sites on bovine lactoferrin, 13 distinct glycans at one N-glycosylation site on four subclasses of human immunoglobulin G, and 20 distinct glycans at five O-glycosylation sites on bovine kappa-casein. Porous graphitized carbon provided effective separation of glycopeptide isomers. The integration of nano-LC with MS and MS/MS of non-specifically cleaved glycopeptides allows quantitative, isomer-sensitive, and site-specific glycoprotein analysis.
引用
收藏
页码:1291 / 1302
页数:12
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