I use HEK293 cell lines and trying to transfection D3R.
My protocol is 2.5 microgram DNA is added to 100 microliter serum free media, then added 18 microliter frozen polyethylimine (PEI) and vortex it several time. Incubated for 15min. Then added 900 microliter serum free media to it. Then this DNA solution is transfer into 100 cm cell culture dish which contains 9 ml serum media. Then 4hour incubation. After 4 hours change this serum media to 9 ml serum media.
But this process show extremely low numbers of surface receptor. Can any one give me a proper way.