Notebook: Protocol
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Western Blot Protocol
Buffers:
RIPA buffer:
Reagent | Final Concentration |
Tris-HCl (pH=7.4) |
25mM |
NaCl |
150mM |
EDTA |
2mM |
EGTA |
2mM |
Triton-X-100 |
1.0% |
Glycerol |
5% |
Phosphate-buffered saline (PBS)
Reagent | Final concentration (1X) |
NaCl |
137mM |
KCl |
2.7mM |
Na2HPO4 |
10mM |
KH2PO4 |
1.8mM |
Adjust pH to 7.2-7.4. Autoclave before use.
293T Cell lysate preparation:
- Carefully aspirate culture media from each well of the 6-well plate.
- Add 1mL PBS to wash each well and remove the wash.
- Add 1mL PBS to each well and resuspend the cell by pipetting up and down multiple times.
- Transfer the 1mL resuspension to a clean EP tube and label well.
- Centrifuge at 4oC at 800g for 10min to spin down the cells and remove the supernatant.
- Add 400ul RIPA buffer to each tube and pipette several times to break the pellet.
- Rock the tube at 4oC overnight to lysis the cell.
SDS-PAGE:
- Proper amount of cell lysate was mixed with 5X loading buffer and boiled for 5 minutes before loading.
- Run the gel at 50V for 5 minutes.
- Invrease the voltage to 100-150V and run for 1-2 hours.
Transfer the protein to PVDF membrane:
- The PVDF membrane was soaked in methonal immediately before use.
- Assemble the transfer sandwich with clip, fiber pad, filter paper, gel and membrane.
- Put the transfer sandwich into transfer buffer and transfer on ice at 100v for 1h.
Blocking:
- Block the membrane with 5% non-fat milk for at room temperature for at least 2h.
Antibody incubation:
- Incubate the membrane with primary antibody at proper dilution in TTBS for 2h or at 4oC overnight.
- Wash the membrane with TTBS: 3x10 minutes.
- Incubate the membrane with secondary antibody conjugated with horse radsih peroxidase at proper dilution in TTBS for 2h.
- Wash the membrane with TTBS: 3x10 minutes.
Horse radish peroxidase(HRP) staining and imaging:
- Incubate the membrane with HRP substrate following manufacturer's instructions.
- Expose to film and develop image.
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