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Schlagwörter:
Hordeum vulgare; Protein microarray technology; Kinase assay; Casein kinase; CK2small alpha, Greek; Phosphorylation of target proteins; Substrates
Zusammenfassung:
We have successfully established a novel protein microarray-based kinase assay, which we applied to identify target proteins of the barley protein kinase CK2small alpha, Greek. As a source of recombinant barley proteins we cloned cDNAs specific for filial tissues of developing barley seeds into an E. coli expression vector. By using robot technology, 21,500 library clones were arrayed in microtiter plates and gridded onto high-density filters. Protein expressing clones were detected using an anti-RGS-His6 antibody and rearrayed into a sublibrary of 4100 clones. All of these clones were sequenced from the 5′-end and the sequences were analysed by homology searches against protein databases. Based on these results we selected 768 clones expressing different barley proteins for protein purification. The purified proteins were robotically arrayed onto FASTTM slides. The generated protein microarrays were incubated with an expression library-derived barley CK2small alpha, Greek in the presence of [small gamma, Greek-33P]ATP, and signals were detected by X-ray film or phosphor imager. We were able to demonstrate the power of the protein microarray technology by identification of 21 potential targets out of 768 proteins including such well-known substrates of CK2small alpha, Greek as high mobility group proteins and calreticulin.