Polyacrylamide gel electrophoresis: Difference between revisions
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Referenced from the main protocol, any comments about the protocol should be made here; i.e. how it was developed. Any comments added should be signed (by adding <nowiki>*'''~~~~''':</nowiki> in front) and explained. Links to FAQs/tips provided by other sources such as the manufacturer or other websites would be best made here.<br> | Referenced from the main protocol, any comments about the protocol should be made here; i.e. how it was developed. Any comments added should be signed (by adding <nowiki>*'''~~~~''':</nowiki> in front) and explained. Links to FAQs/tips provided by other sources such as the manufacturer or other websites would be best made here.<br> | ||
Anecdotal observations that might be of use to others can also be posted here; e.g. 'my cells were still floating'.<br> | Anecdotal observations that might be of use to others can also be posted here; e.g. 'my cells were still floating'.<br> | ||
Revision as of 13:44, 17 June 2009
This procedure is useful for the separation of small pieces of DNA, small quantities of DNA, or applications where higher resolution than can be achieved with agarose gel electrophoresis is needed. Because it is very difficult to remove DNA from polyacrylamide gel, it is advised that this protocol should only be used for diagnostic purposes and not for size separation of useful fragments.
Materials
Reagents
- 29:1 Acrylamide Solution
- 10X TBE buffer
- Ammonium Persulfate
- TEMED
- DNA solution
- SYBR green
- Bromophenol Blue
Equipment
- Vertical electrophoresis chamber
- Glass plates w/ spacers (which fit the chamber)
- Casting holder
- Pipettors
Procedure
1. Place Glass plates in casting apparatus
2. Add together the following to make 5ml of gel (0.75mm spacers)
- 500µl 10X TBE solution
- 35µl Ammonium Persulfate (10%w/v)
- X mL 29:1 acrylamide solution (See the table under "notes" to determine the desired acrylamide concentration)
- Y mL water (To make 5 mL)
- 2µl TEMED
- 500µl 10X TBE solution
3. Pipet the acrylamide solution between the casting plates using a 5ml pipetor
4. Insert comb into the top of the gel and allow it to cure vertically for approximately 30 minutes
5. Combine the following for all DNA samples including the ladder
- 10μL DNA solution
- 1μL SYBR green (100X Dilution in DMSO)
- 1μL Bromophenol Blue
- 10μL DNA solution
6. Insert the gel into the electrophoresis chamber allong with the buffer dam
- Make sure both the gel and the buffer dam seal
- The wells on the gel should face the inside
7. Add 1X TBE to the space between the gel and tue buffer dam until the TBE fills the wells in the gel
- No TBE should leak into the space outside of this chamber
8. Add 1X TBE to the outer chamber to the specified fill level.
8. Add DNA mix to wells.
9. Apply 80 volts and run for approximately 60 minutes
Notes
Referenced from the main protocol, any comments about the protocol should be made here; i.e. how it was developed. Any comments added should be signed (by adding *'''~~~~''': in front) and explained. Links to FAQs/tips provided by other sources such as the manufacturer or other websites would be best made here.
Anecdotal observations that might be of use to others can also be posted here; e.g. 'my cells were still floating'.
It might also be good to add an image to show the workflow and timescales for experiment planning.
Acknowledgments
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References
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Specific Protocols
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Discussion
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