18O-Labelling of N-glycosylation sites to improve the identification of gel-separated glycoproteins using peptide mass mapping and database searching

Type: Application

Scientific Paper

Number: Technology

L00:3:1100

MALDI-TOF

Year Products

1999

Reflex

  Author
 

Kuster, B., Mann, M.(*)
Protein Interaction Lab., Univ. Southern Denmark, Campusvej 55, 5230 Odense M, Denmark

  Reference
 

Anal. Chem. 71(7) 1999 1431-1440

 

Abstract

 

Glycosylated proteins are in-gel deglycosylated with PNGase F in H 2

18O-contg. medium in order to label

partially (50%) the glycosylated Asn residues prior to tryptic digestion and peptide mass mapping by MALDI

MS with database searching. Peptides extd. from the gel pieces and present in the in-gel proteolysis supernatant

mixt. are also analyzed by nano-electrospray (ESP) MS/MS. For MALDI, a satd. matrix soln. in acetone is

mixed 4:1 (v/v) with nitrocellulose in 50% acetone-isopropanol and prepd. by the fast evapn. method. A drop of

10% formic acid is deposited and 0.3-0.5 μl of the digest supernatant is added and allowed to dry.

MS1: modified Bruker Reflex, MALDI, TOF, pos. mode, N2 laser, 337 nm.

Infusion: desalted peptides in 5% formic acid.

MS2: Perkin-Elmer Sciex QqTOF prototype, nano-ESP, pos. mode, CAD: N2, 20-60 eV.

Due to isotope labelling, more peptides are detected by MALDI MS to give better database search specificity.

Detection of a labelled peptide helps partial sequencing because N-linked carbohydrates are attached solely to

Asn residues that form part of the NXS/T sequence. This increases search specificity 100-fold. For all proteins

studied (bovine fetuin, human α1-acid glycoprotein, HIVrgp120) glycosylation sites are identified by MALDI

MS when 10 pmol glycoprotein is subjected to SDS-PAGE. ESP MS/MS may be used to verify glycosylation

site assignment and give detailed sequence information by peptide sequencing of the labelled peptides. An

example is given with a peptide from fetuin.

 

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