Difference between revisions of "Inositol Labeling and Lipid Extraction"
From Bridges Lab Protocols
Davebridges (Talk | contribs) m (→References) |
Davebridges (Talk | contribs) m |
||
Line 34: | Line 34: | ||
PMID 8920990 | PMID 8920990 | ||
PMID 18434594 | PMID 18434594 | ||
+ | [[Category: Cell Culture]] | ||
+ | [[Category: Lipid Analysis]] | ||
+ | [[Category: Inositol Lipids]] |
Latest revision as of 15:44, 7 August 2009
Materials
- Cells in 100 mm culture dishes
- Labelling Media (Inositol Free DMEM with PSG, 10% dialysed serum and 100 uCi inositol per plate
of cells)
- Perchloric acid (640 uL into 10 mL water) keep cold
- 100 mM EDTA (2 mL of 0.5M stock in 10 mL) keep cold
- Water
- Deacylation Mix (3.5 mL Methylamine, 6 mL Methanol, 1.5 mL Butanol, 2.1 mL Water)
- Lipid Extraction Mix (10 mL Butanol, 2 mL Ethyl Ether and 0.5 mL Ethyl Formate)
Protocol
- Label subconfluent cells (60-80% confluence) for 48h in labelling media. If using adipocytes label at 4-6 days post-FBS for 48h
- Check that eppendorf centrifuge is at 4C and that heating block (with right size holes) is at 56C
- Treat cells as required(remove media if necessary)
- Aspirate media and add 1 mL Perchloric acid. Incubate at 4 C for 15 min
- Scrape cells, transfer to eppendorf tubes and spin 10 min at 16 000g at 4 C
- Aspirate supernantant and resuspend cells in 1 mL 100 mM EDTA. Centrifuge again.
- Suspend pellet in 50 uL of water.
- Deacylation
- Add 1 mL Deacylation mix and transfer to glass tube
- Incubate at 56 C for 45 min
- Dry under vacuum
- Resuspend pellet in 0.5 mL water. Vortex 30s
- Centrifuge at room temperature for 2 min
- Extract Lipids:
- Remove supernatant to tube with 0.5 mL Lipid Extraction Mix
- Vortex 15s
- Centrifuge at room temperature for 2 min
- Remove lower phase and repeat steps a-c once
- Remove lower phase to clean tube and dry under vacuum.
- Store dried samples at -20 C