Abstract

In response to RFA-RM-04-020, """"""""Molecular Libraries Screening Instrumentation"""""""", we propose to develop a highly integrated hardware and software platform that performs highly multiplexed high throughput assays for signaling protein activation in extracts from cells treated with individual compounds. Current high throughput screening methods offer powerful tools to discover novel modulators of cell signaling in large libraries of small molecules by detecting the chemical modification of substrates by kinases, phosphatase, proteases and other signaling enzymes. This approach has proven its value in discovering inhibitors of oncogenic tyrosine kinases, leading to clinically important drugs such as Imatinib to target Bcr-Abl in CML and c-kit in GIST, Gefitinib to target EGFR in small cell lung cancer and a number of investigational kinase antagonists such as SU11248 to target Flt3 in AML. However, the state-of-the-art in molecular library screening falls short in identifying molecules that may be agonists or antagonists of specific signaling pathways but that are not necessarily targeted at a particular signaling protein. In prior work, we have developed sensitive assays using immunologic and MALDI-TOF detection of the phosphorylation of immobilized peptides and proteins that accurately report Bcr-Abl activity and inhibition in whole cell extracts from Ph+ leukemia cell lines. Here, we will extend this work and use our established copolymerization methodology to immobilize multiple tyrosine kinase substrate and isotope-coded control peptides in an acrylamide copolymer via photo-cleavable linkers. Peptides that display high specificity for individual tyrosine kinases or specific classes will be selected and validated in this format. Cell extracts will be applied to these surfaces in an array format where each spot corresponds to cells treated with a single library compound. After incubation, the surface will be washed, and the peptides released by UV photo-cleavage. MALDI-TOF analysis of each spot will lead to a spectrum of test and control peptides associated with each compound. These spectra will be normalized and compared with reference spectra to detect statistically significant changes in one or more signaling pathways. Compounds that appear to activate or inhibit one or more tyrosine kinases present in the cell extracts will be flagged for further analysis.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Human Genome Research Institute (NHGRI)
Type
Research Project (R01)
Project #
5R01HG003864-02
Application #
7125566
Study Section
Special Emphasis Panel (ZEB1-OSR-C (O1))
Program Officer
Ozenberger, Bradley
Project Start
2005-09-23
Project End
2009-07-31
Budget Start
2006-08-01
Budget End
2007-07-31
Support Year
2
Fiscal Year
2006
Total Cost
$596,274
Indirect Cost

  Institution

Name
University of Chicago
Department
Genetics
Type
Schools of Medicine
DUNS #
005421136
City
Chicago
State
IL
Country
United States
Zip Code
60637

  Publications

Labay, Edwardine; Efimova, Elena V; Quarshie, Benjamin K et al. (2011) Ionizing radiation-induced foci persistence screen to discover enhancers of accelerated senescence. Int J High Throughput Screen 2:1-13
Zhou, Guangchang; Sylvester, Juliesta E; Wu, Ding et al. (2011) A magnetic bead-based protein kinase assay with dual detection techniques. Anal Biochem 408:5-11
Wu, Ding; Sylvester, Juliesta E; Parker, Laurie L et al. (2010) Peptide reporters of kinase activity in whole cell lysates. Biopolymers 94:475-86
Sylvester, Juliesta E; Kron, Stephen J (2010) A bead-based activity screen for small-molecule inhibitors of signal transduction in chronic myelogenous leukemia cells. Mol Cancer Ther 9:1469-81
Mand, Michael R; Wu, Ding; Veach, Darren R et al. (2010) Cell treatment and lysis in 96-well filter-bottom plates for screening Bcr-Abl activity and inhibition in whole-cell extracts. J Biomol Screen 15:434-40
Zhou, Guangchang; Yan, Xiaoliang; Wu, Ding et al. (2010) Photocleavable peptide-conjugated magnetic beads for protein kinase assays by MALDI-TOF MS. Bioconjug Chem 21:1917-24
Volchenboum, Samuel L; Kristjansdottir, Kolbrun; Wolfgeher, Donald et al. (2009) Rapid validation of Mascot search results via stable isotope labeling, pair picking, and deconvolution of fragmentation patterns. Mol Cell Proteomics 8:2011-22
Parker, Laurie; Engel-Hall, Aaron; Drew, Kevin et al. (2008) Investigating quantitation of phosphorylation using MALDI-TOF mass spectrometry. J Mass Spectrom 43:518-27
Kristjansdottir, Kolbrun; Wolfgeher, Donald; Lucius, Nick et al. (2008) Phosphoprotein profiling by PA-GeLC-MS/MS. J Proteome Res 7:2812-24
Wu, Ding; Mand, Michael R; Veach, Darren R et al. (2008) A solid-phase Bcr-Abl kinase assay in 96-well hydrogel plates. Anal Biochem 375:18-26

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