Literature DB >> 12872225

Quantitative analysis of protein phosphorylation status and protein kinase activity on microarrays using a novel fluorescent phosphorylation sensor dye.

Karen Martin1, Thomas H Steinberg, Laurie A Cooley, Kyle R Gee, Joseph M Beechem, Wayne F Patton.   

Abstract

Ultrasensitive detection of minute amounts of phosphorylated proteins and peptides is a key requirement for unraveling many of the most important signal transduction pathways in mammalian systems. Protein microarrays are potentially useful tools for sensitive screening of global protein expression and post-translational modifications, such as phosphorylation. However, the analysis of signaling pathways has been hampered by a lack of reagents capable of conveniently detecting the targets of protein kinases. Historically, phosphorylation detection methods have relied upon either radioisotopes ((gamma-(32)P)ATP(gamma-(33)P)ATP labeling) or phosphoamino acid-selective antibodies. Both of these methods suffer from relatively well-known shortcomings. In this study, a small molecule fluorophore phosphosensor technology is described, referred to as Pro-Q Diamond dye, which is capable of ultrasensitive global detection and quantitation of phosphorylated amino acid residues in peptides and proteins displayed on microarrays. The utility of the fluorescent Pro-Q Diamond phosphosensor dye technology is demonstrated using phosphoproteins and phosphopeptides as well as with protein kinase reactions performed in miniaturized microarray assay format. Instead of applying a phosphoamino acid-selective antibody labeled with a fluorescent or enzymatic tag for detection, a small, fluorescent probe is employed as a universal sensor of phosphorylation status. The detection limit for phosphoproteins on a variety of different commercially available protein array substrates was found to be 312-625 fg, depending upon the number of phosphate residues. Characterization of the enzymatic phosphorylation of immobilized peptide targets with Pro-Q Diamond dye readily permits differentiation between specific and non-specific peptide labeling at picogram to subpicogram levels of detection sensitivity.

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Year:  2003        PMID: 12872225     DOI: 10.1002/pmic.200300445

Source DB:  PubMed          Journal:  Proteomics        ISSN: 1615-9853            Impact factor:   3.984


  18 in total

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Journal:  J Proteome Res       Date:  2008-05-30       Impact factor: 4.466

Review 4.  Deciphering enzyme function using peptide arrays.

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Journal:  Mol Biotechnol       Date:  2011-11       Impact factor: 2.695

5.  Optimizing thiophosphorylation in the presence of competing phosphorylation with MALDI-TOF-MS detection.

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Journal:  J Proteome Res       Date:  2005 Sep-Oct       Impact factor: 4.466

6.  Requirement of the cytosolic interaction between PATHOGENESIS-RELATED PROTEIN10 and LEUCINE-RICH REPEAT PROTEIN1 for cell death and defense signaling in pepper.

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Review 8.  Analytical challenges translating mass spectrometry-based phosphoproteomics from discovery to clinical applications.

Authors:  Anton B Iliuk; Justine V Arrington; Weiguo Andy Tao
Journal:  Electrophoresis       Date:  2014-07-10       Impact factor: 3.535

9.  Multiplexed Imaging of Protein Phosphorylation on Membranes Based on Ti(IV) Functionalized Nanopolymers.

Authors:  Anton Iliuk; Li Li; Michael Melesse; Mark C Hall; W Andy Tao
Journal:  Chembiochem       Date:  2016-04-01       Impact factor: 3.164

10.  O-GlcNAcylation is involved in the transcriptional activity of EWS-FLI1 in Ewing's sarcoma.

Authors:  R Bachmaier; D N T Aryee; G Jug; M Kauer; M Kreppel; K A Lee; H Kovar
Journal:  Oncogene       Date:  2009-01-19       Impact factor: 9.867

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