Acetylating Tryptic Peptides Enhances b Ion Intensity in MALDI TOF/TOF: Implications in Peptide Sequencing and Identification of Proteins in an Antarctic Bacterium Pseudomonas Syringae
Author(s) -
Heramb M. Kulkarni,
V. Ramesh,
R. Srinivas,
Medicharla V. Jagannadham
Publication year - 2010
Publication title -
proteomics insights
Language(s) - English
Resource type - Journals
SCImago Journal Rank - 0.337
H-Index - 7
ISSN - 1178-6418
DOI - 10.4137/pri.s3676
Subject(s) - peptide , mass spectrometry , peptide sequence , acetylation , peptide mass fingerprinting , chemistry , bottom up proteomics , pseudomonas , matrix assisted laser desorption/ionization , pseudomonas syringae , signal peptide , biochemistry , mass spectrum , bacteria , computational biology , chromatography , protein mass spectrometry , proteomics , biology , tandem mass spectrometry , genetics , gene , organic chemistry , adsorption , desorption
Several approaches have been described to identify proteins from MALDI MS/MS mass spectra. The sequence of tryptic peptides is determined by database searching or by de novo sequencing. Different algorithms are available to determine peptide sequence using mass spectra. False discovery of peptides is an associated problem with it. A combination of chemical modifications followed by mass spectral analysis helps in overcoming this problem. Acetylating the tryptic peptides of β-galactosidase in methanol is found to increase the b-ion signal intensity in MALDI TOF mass spectrometry. The method of acetylation is extended to the tryptic peptides of the proteins of an Antarctic bacterium Pseudomonas syringae, whose genome sequence is not known. These proteins are identified by searching the available database of the Pseudomonas spp at NCBI using the MS/MS spectra. The sequences of the peptides are validated using the CID mass spectra of the acetylated tryptic peptides.
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