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Factors affecting the ultraviolet laser desorption of proteins
Author(s) -
Beavis Ronald C.,
Chait Brian T.,
Standing K. G.
Publication year - 1989
Publication title -
rapid communications in mass spectrometry
Language(s) - English
Resource type - Journals
SCImago Journal Rank - 0.528
H-Index - 136
eISSN - 1097-0231
pISSN - 0951-4198
DOI - 10.1002/rcm.1290030708
Subject(s) - chemistry , adduct , ion , desorption , mass spectrometry , mass spectrum , ultraviolet , molecule , laser , analytical chemistry (journal) , matrix (chemical analysis) , resolution (logic) , chromatography , optics , organic chemistry , adsorption , physics , artificial intelligence , computer science
The production of high‐mass quasimolecular ions from proteins by matrix‐assisted ultraviolet laser desorption is described. A simple time‐of‐fight system using a Q‐switched frequency‐quadrupled Nd‐YAG laser to desorb protein molecules is shown to have a mass range of up to 116 000 u by the observation of intact, singly charged quasimolecular ions from 700 fmol of β‐galactosidase subunit (mol.wt = 116 336 Da). Both positive‐ and negative‐ion spectra of proteins are shown. Four new matrix materials, with properties as good as or better than nicotinic acid, are described. A mass resolution of approximately 500 (full width at half maximum definition) is demonstrated for proteins with mol.wt < 20 000 Da. Product species, formed by fast photochemical reactions in the matrix, are observed to form adduct ions with protein molecules. These adduct ions are a significant cause of the observed broadness of protein quasimolecular ion peaks. The practical physical considerations in detection of large‐mass quasimolecular ions from laser desorption, such as detector overloading, are discussed.