Microscale Thermophoresis to Study Protein-Lipid Interactions in Solution
Microscale Thermophoresis to Study Protein-Lipid Interactions in Solution
Trascrizione
Before beginning an analysis, turn on the power switch on the back of the MST device, and open the control software. Confirm that the computer is attached to the device and in "Connected" status, and set the MSTBefore to 3 seconds, the MST to 30 seconds, and the FluorescenceRecovery to after 1 second.
For each capillary tube, enter the name of the target ligand, the name of the ligand analyte, the concentration of the target, and the highest titration concentration using the autofill titration ratio. Select a range of MST powers and enter the values for each power to test for the most robust binding fit.
To prepare labeled MST samples, dilute a Vam7-octahistidine solution to a 200-nanomolar concentration and an NTA-Atto 647 dye to a 100-nanomolar concentration, both in PBS. Mix the Vam7-octahistidine and the NTA-Atto 647 dye at a 1 to 1 volumetric ratio, and allow the mixture to sit at room temperature, protected from light, for 30 minutes. At the end of the incubation, centrifuge the dye and protein mixture, and store the solution at 4 degrees Celsius for up to a few hours before use. Then, prepare the sample. Take dye to ligand and expose the analyte.
For MicroScale Thermophoresis of the sample, open the device and slide the capillary rack out. Load the sample capillaries into the rack with the highest concentration at position 1, and select the red channel in the control software. Then, load the rack in the instrument. Then, select a range of MST power and start the CapScan+MST measurement and evaluate the shift response.