Running SDS-PAGE: Difference between revisions
From Powers Wiki
No edit summary |
No edit summary |
||
Line 4: | Line 4: | ||
[[Category:Protein expression]] | [[Category:Protein expression]] | ||
[[File:SDS_PAGE.pdf|SDS PAGE]] | [[:File:SDS_PAGE.pdf|SDS PAGE]] | ||
See also [[SDS-PAGE_Protocol | SDS-PAGE Protocol]] | See also [[SDS-PAGE_Protocol | SDS-PAGE Protocol]] |
Revision as of 22:00, 13 November 2021
See also SDS-PAGE Protocol
Running SDS-PAGE
- Make ready the samples to run
- Make ready the sample running buffer
- Make ready the gel
- Have the SDS-PAGE apparatus
- Place the the gel in the SDS-PAGE stand
- Place the stand with the gel in the SDS-PAGE apparatus bath
- fill the space between the gels with running buffer
- Take off the combs of the gel (take it out gently)
- Load the sample to each well
- Do not use the wells at the left and right end of the gel
- fill the SDS-PAGE apparatus bath with running buffer to the bottom of the gel
- Place the cover of the SDS-PAGE
- N.B Make sure the correct plug is connected to the correct electrode (red goes to red and black goes to black)
- Plug the cables to the SDS-PAGE apparatus power source
- Turn of the SDS-PAGE power source
- Set to constant voltage
- Use 200 V
- Press the Run button to start the electrophoresis
- The voltage increases to 200 V from 0 V
- For 4% staking gel and 12.5 % separating gel the current reaches 50-60 mA and the power 10 -12 W
- The current the the power decreases in time but not reach zero (if it reaches zero see the troubleshoot)
- For the state type of gel it takes 35 - 40 min
Troubleshoot
- The power drops to zero
- really old buffer
- the space in between the gels is not filled with buffer to the top