Acetate Incorporation into Lipid
Materials
- Cells plated in 12 well dishes
- Low Glucose Starvation Media (5 mM Glucose, 0.5% FBS)
- Acetate Incorporation Media (Low Glucose Starvation Media + 2 mM Acetate and 10 uCi/mL 14C Acetic Acid)
- PBS at 4C
- [2-14C] Acetic Acid. Perkin Elmer Cat# NEC085H001MC
Protocol
- Turn radioactive tissue culture incubator on at 37C, make sure to turn on the CO2 as well.
- Starve cells in Low Glucose Starvation Media for >3h.
- Prepare Acetate Incorporation Media Make at least enough for one extra well, using 50 uL/well for a 12 well dish. If monitoring lipogenesis in a line other than adipocytes, increase the hot glucose to 50 uCi per mL.
- Pretreat cells with inhibitors if required.
- Add 100 nM insulin as required.
- Add 50 uL of Hot Acetate Solution to each well.
- Place in the radioactive tissue culture incubator for 60-120 minutes.
- Save 3 x 5 uL of the Acetate Incorporation Media to count total radioactivity.
- After 60 min wash cells 3x with 1 mL of PBS.
- Resuspend cells in 1 mL of PBS.
- Transfer 900 uL of resuspended cells 2.1 mL of PBS and 3 mL of non-aqueous betaflour scintillant and vortex. Set aside to let separate
- Do a bradford assay on 50 uL of lysed cells for protein normalization.
- Add 200 uL of glycogen solution to cells and vortex.
- The next day, move the lipid portion to a fresh vial and count.
Adapted from Matt Brady's protocol.