Multiple myeloma phosphotyrosine proteomic profile associated with FGFR3 expression, ligand activation, and drug inhibition
- Jonathan R. St-Germaina,b,
- Paul Taylora,c,
- Jiefei Tonga,c,
- Lily L. Jina,b,
- Ana Nikolica,c,
- Ian I. Stewartd,
- Robert M. Ewingd,e,
- Moyez Dharseed,
- Zhihua Lic,f,
- Suzanne Trudelc,f and
- Michael F. Morana,b,c,g,1
- aMolecular Structure and Function Program, Hospital for Sick Children, University of Toronto, Toronto, ON, Canada M5G 1X8;
- bDepartment of Molecular Genetics, University of Toronto, Toronto, ON, Canada M5S 1A8;
- cMcLaughlin Centre for Molecular Medicine and
- gBanting and Best Department of Medical Research, University of Toronto, Toronto, ON, Canada M5G 1L7;
- dInfochromics Inc., Toronto, ON, Canada M5G 1L7;
- eCenter for Proteomics and Bioinformatics, School of Medicine, Case Western Reserve University, Cleveland, OH 44106; and
- fHematology-Oncology, Princess Margaret Hospital, Toronto, ON, Canada M5G 1X8
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Communicated by Tony Pawson, Samuel Lunenfeld Research Institute, Toronto, ON, Canada, September 28, 2009 (received for review July 24, 2008)
Abstract
Signaling by growth factor receptor tyrosine kinases is manifest through networks of proteins that are substrates and/or bind to the activated receptors. FGF receptor-3 (FGFR3) is a drug target in a subset of human multiple myelomas (MM) and is mutationally activated in some cervical and colon and many bladder cancers and in certain skeletal dysplasias. To define the FGFR3 network in multiple myeloma, mass spectrometry was used to identify and quantify phosphotyrosine (pY) sites modulated by FGFR3 activation and inhibition in myeloma-derived KMS11 cells. Label-free quantification of peptide ion currents indicated the activation of FGFR3 by phosphorylation of tandem tyrosines in the kinase domain activation loop when cellular pY phosphatases were inhibited by pervanadate. Among the 175 proteins that accumulated pY in response to pervanadate was a subset of 52 including FGFR3 that contained a total of 61 pY sites that were sensitive to inhibition by the FGFR3 inhibitor PD173074. The FGFR3 isoform containing the tandem pY motif in its activation loop was targeted by PD173074. Forty of the drug-sensitive pY sites, including two located within the 35-residue cytoplasmic domain of the transmembrane growth factor binding proteoglycan (and multiple myeloma biomarker) Syndecan-1/CD138, were also stimulated in cells treated with the ligand FGF1, providing additional validation of their link to FGFR3. The identification of these overlapping sets of co-modulated tyrosine phosphorylations presents an outline of an FGFR3 network in the MM model and demonstrates the potential for pharmacodynamic monitoring by label-free quantitative phospho-proteomics.
Footnotes
- 1To whom correspondence should be addressed. E-mail: m.moran{at}utoronto.ca
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Author contributions: M.F.M. designed research; J.R.S., P.T., and J.T. performed research; L.L.J., A.N., I.I.S., R.M.E., M.D., Z.L., S.T., and M.F.M. contributed new reagents/analytic tools; J.R.S., P.T., J.T., L.L.J., I.I.S., R.M.E., M.D., S.T., and M.F.M. analyzed data; and J.R.S. and M.F.M. wrote the paper.
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The authors declare no conflict of interest.
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Data deposition: Data described in this study are freely available through the Human Proteinpedia portal (humanproteinpedia.org), Tranche (proteomecommons.org/tranche), PRIDE (ebi.ac.uk/pride), and GPMDB (thegpm.org).
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This article contains supporting information online at www.pnas.org/cgi/content/full/0910957106/DCSupplemental.
