| Assay Method Information | |
| | In Vitro Effect Assay |
| Description: | Table 5: The experimental procedure referred to the Z′-LYTE Screening Protocol and Assay Conditions provided by ThermoFisher Scientific. C-1. Material Preparation3-fold serial dilution was performed on the test compound stock solution (1 mM) prepared in 100% DMSO was for 10 times for ready to use to determine the IC50 of the test compound on YSK-4. Peptide/Kinase Mixture was pre-diluted with Kinase Buffer to 2× working concentration. ATP solution was pre-diluted with Kinase Buffer (50 mM HEPES pH 7.5, 0.01% BRIJ-35, 10 mM MgCl2, 1 mM EGTA) to 4× working concentration. The development reagent solution is Novel PKC Lipid Mix, which contains 2 mg/mL Phosphatidyl Serine, 0.2 mg/mL DAG in 20 mM HEPES, pH 7.4 and 0.3% CHAPS, and was pre-diluted 10 fold with development buffer.C-2. Analytical Method. 1. 100 nL of the above diluted test compound and 2.4 μL of kinase buffer were added to a black 384-well plate (Corning, Cat. NO. 4514), then add 5 μL of the peptide/kinase mixture mentioned above was added thereto, and after that 2.5 μL of ATP solution was added thereto, and the culture plate was shaken for 30 seconds.2. Next, the culture plate was placed at room temperature and incubated for 60 minutes.3. After that 5 μL of the development reagent solution was added and the culture plate was shaken for 30 seconds in the dark, and then the data was read and analyzed with a fluorescence plate reader. In addition, for the kinase, the following control group was prepared and placed on the same culture plate as the kinase:</p><p id="p-0248" num="0244">(1) 0% Phosphorylation Control (100% Inhibition Control). The maximum Emission Ratio is established by the 0% Phosphorylation Control (100% Inhibition Control), which contains no ATP and therefore exhibits no kinase activity. This control yields 100% cleaved peptide in the Development Reaction.(2) 100% Phosphorylation Control A synthetically phosphorylated peptide of the same sequence as the peptide substrate is used as the 100% Phosphorylation Control. This control yields a very low percentage of cleaved peptide in the Development Reaction.The Phosphorylation percent achieved in a specific reaction well (Experimental group) was calculated based on the 0% Phosphorylation Control and 100% Phosphorylation Control. The Z′-LYTE substrate used in the binding analysis reaction for Z′-LYTE Screening Kinase was Ser/Thr 07 peptide, and ATP reaction concentration was 5 μM (Km of YSK4). |
| Affinity data for this assay | |
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