To begin, take 293FT cells cultured in a 10 centimeter dish, and aspirate the media. Wash cells with five milliliters of PBS. Then add one milliliter of trypsin EDTA, and incubate for 3-5 minutes at 37 degrees Celsius to detach cells from the dish.
After incubation, add nine milliliters of complete DMEM to the cells to neutralize the trypsin. Pipette up and down repeatedly to generate a homogenous single cell suspension, and transfer the cells to a 15 milliliter tube. Immediately transfer 20 microliters of cells to a 1.7 milliliter tube, and mix with 20 microliters of trypan blue stain.
Count cells using either an automated cell counter or a hemocytometer. Transfer the appropriate volume of cells to a 50 milliliter tube, and dilute in complete DMEM. Add two milliliters of cell suspension to each well of a six-well plate.
Incubate cells at 37 degrees Celsius and 10%carbon dioxide overnight. Prior to transfection, dilute nanoluciferase CRAF and 1433 zeta halo plasmids, along with a pCDNA3 empty vector in TE buffer. Label a set of sterile 1.7 milliliter tubes.
Add 100 microliters of transfection media to each tube, along with the expression constructs. Now add two microliters of transfection reagent, and vortex gently to mix. Pulse spin the tubes briefly in a microcentrifuge, and then incubate the tubes at around 25 degrees Celsius for 15 minutes to allow transfection complexes to form.
Afterwards, add transfection complexes to cells dropwise, and incubate at 37 degrees Celsius for 16-20 hours to express the halo and nanotagged proteins.
