Glycogen Determination from Tissues
From Bridges Lab Protocols
Materials and Buffers
- Screw Capped Vials
- 30% KOH, prepared fresh
- 1M Sodium Sulfate
- Ethanol
- 50 mM Sodium Acetate, pH 4.8
- Amyloglucosidease
- Glucose quantification kit (Wako Autokit Glucose Buffer Solution cat # 439-9091)
- Glucose standard solution (500 mg/dL; Wako)
Protocol
- Weight out 30-90 mg tissue into screw cap vial and record weights.
- Add 300 uL 30% KOH and place on 95C heat block for 30 min with occasional mixing.
- Cool and then add 100 uL Sodium Sulfate and 800 uL Ethanol.
- Boil for 5 min.
- Centrifuge at 13 000 RPM for 5 min.
- Resuspend pellet in 200 uL water then add 400 uL ethanol. Boil 5 min, spin 5 min and Repeat wash steps twice more.
- Dry pellet
- Resuspend pellet in 200 uL of 50 mM Sodium Acetate, pH 4.8
- Add 0.3 mg/mL amyloglucosidase and place at 37C for 3h
- Quantify glucose using kit:
- Add 1-5 uL glucose standard for standard curve
- Add 10 uL digested glycogen
- Mix and incubate at 37C for 5 min
- Measure absorbance at 505 nm
- Calculate glycogen levels as umoles glucose released per g tissue (should be ~10)
Reference: