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Journal home Advance online publication Current issue Archive Press releases Supplements Focuses Conferences Guide to authors Online submission Permissions For referees Free online issue Contact the journal Subscribe Advertising work@npg naturereprints About this site For librarians   NPG Resources Bioentrepreneur Nature Reviews Drug Discovery Nature Nature Medicine Nature Genetics Nature Reviews Genetics Nature Methods Nature Chemical Biology news@nature.com Clinical Pharmacology & Therapeutics Nature Conferences NPG Subject areas Biotechnology Cancer Chemistry Clinical Medicine Dentistry Development Drug Discovery Earth Sciences Evolution & Ecology Genetics Immunology Materials Science Medical Research Microbiology Molecular Cell Biology Neuroscience Pharmacology Physics Browse all publications Technical Report Nature Biotechnology  20, 301 - 305 (2002) doi:10.1038/nbt0302-301 Phosphoproteome analysis by mass spectrometry and its application to Saccharomyces cerevisiae Scott B. Ficarro1, Mark L. McCleland2, P. Todd Stukenberg2, Daniel J. Burke2, Mark M. Ross4, Jeffrey Shabanowitz1, Donald F. Hunt1, 3 & Forest M. White4 1  Department of Chemistry, University of Virginia, Charlottesville, VA 22901. 2  Departments of Biochemistry and Molecular Genetics, University of Virginia, Charlottesville, VA 22908. 3  Pathology, Health Sciences Center, University of Virginia, Charlottesville, VA 22908. 4  MDS Proteomics, Charlottesville, VA 22901. Correspondence should be addressed to Forest M. White fwhite@mdsp.comProtein kinases are coded by more than 2,000 genes and thus constitute the largest single enzyme family in the human genome. Most cellular processes are in fact regulated by the reversible phosphorylation of proteins on serine, threonine, and tyrosine residues1. At least 30% of all proteins are thought to contain covalently bound phosphate. Despite the importance and widespread occurrence of this modification, identification of sites of protein phosphorylation is still a challenge, even when performed on highly purified protein2. Reported here is methodology that should make it possible to characterize most, if not all, phosphoproteins from a whole-cell lysate in a single experiment. Proteins are digested with trypsin and the resulting peptides are then converted to methyl esters, enriched for phosphopeptides by immobilized metal-affinity chromatography (IMAC)3, 4, and analyzed by nanoflow HPLC/electrospray ionization mass spectrometry. More than 1,000 phosphopeptides were detected when the methodology was applied to the analysis of a whole-cell lysate from Saccharomyces cerevisiae. A total of 216 peptide sequences defining 383 sites of phosphorylation were determined. Of these, 60 were singly phosphorylated, 145 doubly phosphorylated, and 11 triply phosphorylated. Comparison with the literature revealed that 18 of these sites were previously identified, including the doubly phosphorylated motif pTXpY derived from the activation loop of two mitogen-activated protein (MAP) kinases. We note that the methodology can easily be extended to display and quantify differential expression of phosphoproteins in two different cell systems, and therefore demonstrates an approach for "phosphoprofiling" as a measure of cellular states. MORE ARTICLES LIKE THIS These links to content published by NPG are automatically generated REFERENCE Mass Spectrometry: Analysis of Two-dimensional Protein Gels Nature Encyclopaedia of Life Sciences REVIEWS Proteomics: the first decade and beyond Nature Genetics Review (01 Mar 2003) RESEARCH De novo peptide sequencing and quantitative profiling of complex protein mixtures using mass-coded abundance tagging Nature Biotechnology Research (01 Feb 2002) Golgi targeting of ARF-like GTPase Arl3p requires its N-acetylation and the integral membrane protein Sys1p Nature Cell Biology Article (01 May 2004) A systematic approach to the analysis of protein phosphorylation Nature Biotechnology Research (01 Apr 2001)  See all 52 matches for Research  Top Abstract Previous | Next Table of contents Full text Download PDF Send to a friend Save this link Open Innovation Challenges Efficient Chromosome Doubling: Plant Cell Division Deadline: Jul 15 2009 Reward: $20,000 USD The Seeker is looking for an efficient chromosome doubling method in plants and in particular, metho... Corrosion Inhibitor Deadline: Aug 19 2009 Reward: $10,000 USD The Seeker is looking for inhibitors of corrosion. This Challenge requires only a written descripti... More Challenges Powered by: nature jobs Scientist, Recombinant Protein Expression Novo Nordisk Foundation Center for Protein Research, University of Copenhagen Copenhagen 2200 Denmark Faculty Position in Biochemistry University of Tuebingen Tuebingen 72076 Germany More science jobs Post a job for free Competing financial interests Figures & Tables Export citation Search buyers guide:   ADVERTISEMENT

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