Multiplex Substrate Profiling by Mass Spectrometry for Kinases as a Method for Revealing Quantitative Substrate Motifs

被引:12
|
作者
Meyer, Nicole O. [1 ]
O'Donoghue, Anthony J. [1 ,3 ]
Schulze-Gahmen, Ursula [2 ]
Ravalin, Matthew [1 ]
Moss, Steven M. [1 ]
Winter, Michael B. [1 ]
Knudsen, Giselle M. [1 ]
Craik, Charles S. [1 ]
机构
[1] Univ Calif San Francisco, Dept Pharmaceut Chem, San Francisco, CA 94158 USA
[2] Univ Calif Berkeley, Dept Mol & Cell Biol, Berkeley, CA 94720 USA
[3] Univ Calif San Diego, Skaggs Sch Pharm & Pharmaceut Sci, San Diego, CA 92103 USA
关键词
RNA-POLYMERASE-II; CELL NUCLEAR ANTIGEN; TYROSINE KINASE; MICROARRAY DATA; SPECIFICITY; IDENTIFICATION; PHOSPHORYLATION; ASSAY; TRANSCRIPTION; CYCLE;
D O I
10.1021/acs.analchem.6b05002
中图分类号
O65 [分析化学];
学科分类号
070302 ; 081704 ;
摘要
The more than 500 protein kinases comprising the human kinome catalyze hundreds of thousands of phosphorylation events to regulate a diversity of cellular functions; however, the extended substrate specificity is still unknown for many of these kinases. We report here a method for quantitatively describing kinase substrate specificity using an unbiased peptide library-based approach with direct measurement of phosphorylation by tandem liquid chromatography-tandem mass spectrometry (LC MS/MS) peptide sequencing (multiplex substrate profiling by mass spectrometry, MSP-MS). This method can be deployed with as low as 10 nM enzyme to determine activity against S/T/Y-containing peptides; additionally, label-free quantitation is used to ascertain catalytic efficiency values for individual peptide substrates in the multiplex assay. Using this approach we developed quantitative motifs for a selection of kinases from each branch of the kinome, with and without known substrates, highlighting the applicability of the method. The sensitivity of this approach is evidenced by its ability to detect phosphorylation events from nanogram quantities of immunoprecipitated material, which allows for wider applicability of this method. To increase the information content of the quantitative kinase motifs, a sublibrary approach was used to expand the testable sequence space within a peptide library of approximately 100 members for CDK1, CDK7, and CDK9. Kinetic analysis of the HIV-1 Tat (transactivator of transcription)-positive transcription elongation factor b (P-TEFb) interaction allowed for localization of the P-TEFb phosphorylation site as well as characterization of the stimulatory effect of Tat on P-TEFb catalytic efficiency.
引用
收藏
页码:4550 / 4558
页数:9
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