Difference between revisions of "Glucose Uptake Assay"

Revision as of 21:03, 11 July 2012

2-Deoxyglucose (cold): Sigma D-6134. Dissolve 32.8mg/mL (200 mM) in KRBH Buffer
0.5% BSA in KRBH Buffer
Radioactive ¹⁴C-2-deoxyglucose
Hot 2-DG. Need 50 uL per well, prepare 1 mL KRBH/BSA, 1 uL cold 2-DG and 50 uL radioactive 2-DG. count 3X5 ul of hot 2DG.

Starve cells >3h in 0.5% FBS
Prepare insulin in KRBH/BSA (0.6uL (100nM) insulin/mL, needing 0.5 mL per well)
Wash cells 2x with warm PBS -/-
Add 450 uL KRBH/BSA with or without insulin to wells. Typically do triplicate measurements
Wait 30 min
Add 50 uL hot 2-DG solution per well and start timer
After 5 min add 50 uL cold 2-DG
Wash cells 3x1mL with cold PBS
Add 500 uL PBS per well
Scrape cells with an upside down p200 tip
Add 400 uL cells to 5 mL aqueous scintillation fluid, vortex and count on program 3
Do a bradford assay on 50 uL of cells (use PBS as blank)

@@ Line 3: / Line 3: @@
 *0.5% BSA in [[KRBH Buffer]]
 *Radioactive <sup>14</sup>C-2-deoxyglucose
-*Hot 2-DG.  Need 50 uL per well, prepare 1 mL KRBH/BSA, 1 uL cold 2-DG and 50 uL radioactive 2-DG
+*Hot 2-DG.  Need 50 uL per well, prepare 1 mL KRBH/BSA, 1 uL cold 2-DG and 50 uL radioactive 2-DG. count 3X5 ul of hot 2DG.
 ==Protocol==
 #Starve cells >3h in 0.5% FBS
-#Prepare insulin in KRBH/BSA (0.6uL insulin/mL, needing 0.5 mL per well)
+#Prepare insulin in KRBH/BSA (0.6uL (100nM) insulin/mL, needing 0.5 mL per well)
 #Wash cells 2x with warm PBS -/-
 #Add 450 uL KRBH/BSA with or without insulin to wells.  Typically do triplicate measurements
@@ Line 17: / Line 17: @@
 #Scrape cells with an upside down p200 tip
 #Add 400 uL cells to 5 mL aqueous scintillation fluid, vortex and count on program 3
-#Do a bradford assay on 20 uL of cells (use PBS as blank)
+#Do a bradford assay on 50 uL of cells (use PBS as blank)
 ==Analysis==