Revision as of 11:40, 30 May 2012

Wageningen UR

SDS-polyacrylamide and native gel electrophoresis

running gel

polymerization:

Add 4 ul TEMED to the running gel mix, mix and pipet the gel into the slides until the green edge.
Add a layer of iso-propanol on top of the polymerizing gel to equalize.

Stacking gel

When the running gel has fully polymerized, remove the remaing iso-propanol with a tissue
Prepare stacking gel mix in a small beaker for 2 gels:

Add 2 ul TEMED to the stacking gel mix, mix and pipet the gel onto the running gel.
Place comb
After the stacking gel has fully polymerized, the gels can be stored at 4 degree Celcius in a box with wet tissues.

Sample preparation

Protein denaturation for SDS-PAGE:

Dependent on the protein concentration, typically 15 ul of sample are transferred to a 1.5 ml tube
Pipet 5 ul of SDS-PAGE loading buffer 5X in the caps of the tubes
Spin tubes briefly
Heat samples and a protein marker in a thermobloch 10' at 99 degree Celcius
Spin down samples briefly

@@ Line 41: / Line 41: @@
 <li>Place comb</li>
 <li>After the stacking gel has fully polymerized, the gels can be stored at 4 degree Celcius in a box with wet tissues.</li>
+</ol>
+'''Sample preparation'''
+Protein denaturation for SDS-PAGE:
+<ol>
+<li>Dependent on the protein concentration, typically 15 ul of sample are transferred to a 1.5 ml tube</li>
+<li>Pipet 5 ul of SDS-PAGE loading buffer 5X in the caps of the tubes</li>
+<li>Spin tubes briefly</li>
+<li>Heat samples and a protein marker in a thermobloch 10' at 99  degree Celcius</li>
+<li>Spin down samples briefly</li>
 </ol>