[No authors listed]
We present a robust and general method for the identification and relative quantification of phosphorylation sites in complex protein mixtures. It is based on a new chemical derivatization strategy using a dendrimer as a soluble polymer support and tandem mass spectrometry (MS/MS). In a single step, phosphorylated peptides are covalently conjugated to a dendrimer in a reaction catalyzed by carbodiimide and imidazole. Modified phosphopeptides are released from the dendrimer via acid hydrolysis and analyzed by MS/MS. When coupled with an initial antiphosphotyrosine protein immunoprecipitation step and stable-isotope labeling, in a single experiment, we identified all known tyrosine phosphorylation sites within the immunoreceptor tyrosine-based activation motifs (ITAM) of the T-cell receptor (TCR) CD3 chains, and previously unknown phosphorylation sites on total 97 tyrosine phosphoproteins and their interacting partners in human T cells. The dynamic changes in phosphorylation were quantified in these proteins.
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G3BP1, ABCA10, SEC24B, ANP32B, PTGES3, C11orf58, C1QTNF4, PLD4, DBN1, DDX3X, DHX8, DMD, DOK1, AGO4, EMD, WBP2, TMEM50A, C1orf43, SPATA31A7, PTPN18, SIT1, DBNL, HCLS1, HNRNPD, HSP90AB1, HTR6, ILF3, IRAK1, STMN1, LASP1, LCP2, ABLIM1, LPP, MBD1, MYH9, NDUFS4, NEU1, PCBP2, PBRM1, CDV3, ERBIN, MAPK1, TRIM39, CASKIN2, NCOA5, PTPN11, PXN, REV3L, RPLP1, GMCL1P1, CAPRIN2, TDO2, TERT, TIA1, TP53BP1, TRIO, EIF4H, YES1, ZAP70, LBH, SETD3, TMTC4, PKP4, YBX3, UNK, CBL, ADAM23, DOK2, ZNF598, CD3D, CD3E, CD3G, CD247, MFHAS1, CD28, LPXN, ARHGEF6, BAG3, KDM4A, UBAP2L
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