The GlycoFilter: A Simple and Comprehensive Sample Preparation Platform for Proteomics, N-Glycomics and Glycosylation Site Assignment

Zhou, Hui; Froehlich, John W.; Briscoe, Andrew C.; Lee, Richard S.

doi:10.1074/mcp.m113.027953

Cited by 31 publications

(44 citation statements)

References 45 publications

(59 reference statements)

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“…As a demonstration of the method, the partially occupied glycosylation site of bovine fetuin at Asn-158 was studied [16-17]. As a first step, we verified that no additional PTMs were present on this peptide.…”

Section: Resultsmentioning

confidence: 74%

Absolute Quantitation of Glycosylation Site Occupancy Using Isotopically Labeled Standards and LC-MS

Zhu

Desaire

2014

J. Am. Soc. Mass Spectrom.

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N-linked glycans are required to maintain appropriate biological functions on proteins. Underglycosylation leads to many diseases in plants and animals; therefore, characterizing the extent of glycosylation on proteins is an important step in understanding, diagnosing, and treating diseases. To determine the glycosylation site occupancy, protein N-glycosidase F (PNGase F) is typically used to detach the glycan from the protein, during which the formerly glycosylated asparagine undergoes deamidation to become an aspartic acid. By comparing the abundance of the resulting peptide containing aspartic acid against the one containing non-glycosylated asparagine, the glycosylation site occupancy can be evaluated. However, this approach can give inaccurate results when spontaneous chemical deamidation of the non-glycosylated asparagine occurs. To overcome this limitation, we developed a new method to measure the glycosylation site occupancy that does not rely on converting glycosylated peptides to their deglycosylated forms. Specifically, the overall protein concentration and the non-glycosylated portion of the protein are quantified simultaneously by using heavy isotope-labeled internal standards coupled with LC-MS analysis, and the extent of site occupancy is accurately determined. The efficacy of the method was demonstrated by quantifying the occupancy of a glycosylation site on bovine fetuin. The developed method is the first work that measures the glycosylation site occupancy without using PNGase F, and it can be done in parallel with glycopeptide analysis because the glycan remains intact throughout the workflow.

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Section: Resultsmentioning

confidence: 74%

Absolute Quantitation of Glycosylation Site Occupancy Using Isotopically Labeled Standards and LC-MS

Zhu

Desaire

2014

J. Am. Soc. Mass Spectrom.

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“…If a specific motif was identified in the deglycosylated form and also identified in either of the other two forms, this indicated that that motif was partially glycosylated [8]. When all motifs were compared, evident differences were observed among the results from three search engines (Figure 1a -c).…”

Section: N-glycosylation Consensus Motifs Analysismentioning

confidence: 98%

“…The depletion of albumin in urine was performed according to a published one-step protocol [15], and the protein concentration was measured by the Bradford assay in triplicate. Approximately 250 µg of depleted urinary proteins from each donor were further processed according to the GlycoFilter platform to obtain released N-glycans and tryptic peptides [8], respectively. PNGase F catalyzed de-N-glycosylation was carried out in a H 2 18 O buffer via a 20-min domestic microwave protocol [16].…”

Section: Urine Processingmentioning

confidence: 99%

“…First, the removal of complex and heterogeneous sugar residues enables the detection, characterization, and even quantification of deglycopeptides by standard proteomic methodologies [7]. Second, the stripping off of sugar-moieties allows the detection of both deglycopeptides and their counterpart unmodified (non-glycosylated) peptides simultaneously, which are necessary to identify partially glycosylated sites unambiguously [8]. Third, the sugar residues can be employed to enrich for glycoproteins or glycopeptides using hydrazide-chemistry or lectins [7,9].…”

Section: Introductionmentioning

confidence: 99%

“…Unfortunately, this product is identical to those derived from spontaneous chemical deamidation [11], which may occur in vivo or in vitro. Researchers have shown that performing the enzymatic reaction in an H 2 18 O environment is effective in differentiating enzymatic conversion (Asn to 18 O-Asp, +2.9883 Da) from chemical deamidation [8,9]. Identifying 18 O-incorporated deglycopeptides usually involves searching MS/MS spectra against an appropriate protein database using various search engines such as Mascot [12], ProteinPilot [13], and Sequest [14].…”

Section: Introductionmentioning

confidence: 99%

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