Lidstrom: Agarose Gel Electrophoresis

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handy link: gel electrophoresis
- click the gel electrophoresis button on the left

Starting with an empty box

Fill with TBE until it covers the gel holding tray.
Add 40 uL of ethidium bromide if your gels don't already have it mixed into the liquefied agarose.
- If your buffer already has some ethidium bromide but it needs more, 20 uL is probably good.
Load sample
- 1.7 uL of a PCR product is usually plenty
Load ladder
- If using MassRuler, 4 uL is good for skinny lanes.
Run @ 110 V for 20 min and check the gel.
- 40 min is pretty safe for 0.7 - 1% agarose gels

Imaging

Exposures should be < 0.5 seconds to minimize background emissions. If you need longer, you probably should have had more ethidium bromide.

Tips

If you have a voltage source that will stop after a set amount of time, feel free to run your gel as you leave and image it in the morning. Diffusion of bands shouldn't be a big problem unless they are << 500 bp.
- Don't do this if you are going to cut & gel purify the band.

gel sat 16 hours between photos

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