Latest revision as of 02:13, 4 October 2012

SDS PAGE Gel Electrophoresis

Place gel cartridge in gel box with loading buffer
Load samples
Run the gel
Place gel in DI water for one hour
Remove water, add staining agent (GelCode Blue), leave on rocker overnight
Remove GelCode Blue, add DI water. Refresh DI water every hour until gel bands are visible

4X Loading Buffer

10X Running Buffer

Take protein sample, add Loading Buffer. Boil at 95 degrees Celsius for ten minutes
Remove premade gel cartridge from package, remove comb, rinse wells with DI water
Insert cartridge into gel box, add running buffer to top and bottom wells
Add samples into separate wells, along with a protein ladder.
Run gel at 200V for around one hour

@@ Line 15: / Line 15: @@
 X Loading Buffer
-.0 ml 1M Tris-HCl pH 6.8
+#2.0 ml 1M Tris-HCl pH 6.8
-.8 g SDS
+#0.8 g SDS
-.0 ml 100% glycerol
+#4.0 ml 100% glycerol
-.4 ml 14.7 M β-mercaptoethanol
+#0.4 ml 14.7 M β-mercaptoethanol
-.0 ml 0.5 M EDTA
+#1.0 ml 0.5 M EDTA
-mg bromophenol Blue
+#8 mg bromophenol Blue
 X Running Buffer
-g glycine
+#288 g glycine
-.4 g Tris base
+#60.4 g Tris base
-g SDS
+#20 g SDS
-.8 L H2O
+#1.8 L H2O
 #Take protein sample, add Loading Buffer. Boil at 95 degrees Celsius for ten minutes
@@ Line 34: / Line 38: @@
 #Add samples into separate wells, along with a protein ladder.
 #Run gel at 200V for around one hour
+== Equipment Necessary ==
+#Power Supply
+#SDS-PAGE Gel Box
+#SDS-PAGE Gel Cartridge
+'''&larr; [[Team:Washington/Protocols|Back to Protocols]]'''