Team:TU Darmstadt/Protocols/Western Blot
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Latest revision as of 20:58, 26 September 2012
Contents |
Western Blot
Materials
Equipment
- Blot chamber (Transblot SD Semi Dry transfer cell)
- plastic bowl
- SDS gel
Chemicals & consumables
- 3% milk powder PBS buffer pH=7.4
- 1.5% milk powder PBS buffer pH=7.4
- 0.05% Tween 20 in PBS pH=7.4
- Antibody (mouse-antimyc)
- antibody (goat-antimouse-AP)
- NBT
- BCIP
- Blotting buffer
- AP buffer
- nitrocellulose membrane (Whatman Nitrocellulose membran)
- filter paper
Procedure
Transfer
- seperate proteins via SDS gel (SDS PAGE)
- put 3 layers of filter paper (drenched in Blotting buffer) on the graphite diode of the apparatus
- cover it with nitrocellulose membrane with the size of your SDS gel
- place SDS gel on top of it (should be wet)
- cover it with 3 layers of filter paper (drenched in Blotting buffer)
- put cathode on top of the apparatus
- transfer of from SDS gel to membrane is performed by adding a constant current of 12 V for 1 h
- afterwards the nitrocellulose membrane, carrying the proteins, is blocked by incubating it in 3% milk powder PBS buffer for 2 h at room temperature or over night at 4°C
Staining
- wash membrane with Tween PBS buffer 3x for 5 min each
- add 1.5% milk powder PBS carrying 1. antibody in 1:1000 concentration
- incubate for at least one hour at RT, keep shaking the whole time
- wash membrane with Tween PBS buffer 3x for 5 min each
- add 1.5% milk powder PBS carrying 2. antibody in 1:10000 concentration
- incubate for at least one hour at RT, keep shaking the whole time
- wash membrane with Tween PBS buffer 3x for 5 min each
- wash membrane with ddH2 once for 5 min
- add AP buffer, 20 µL of NBT and 70 µL of BCIP
- keep shaking for 1 h