Lidstrom: Agarose Gel Electrophoresis

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

Imaging

Imaging systems

We have two imaging systems:

(1) ______ on the island

(2) Across from the SDS-PAGE gel pouring room

Login info is taped to the monitor
Software = GeneSnap
- Manual

Instructions:

Click the green circle on the top left. This turns the camera on
Set the filter button (button = red/blue/green circles within a circle) to EtBr/UV
Turn on the light by selecting transillumination (not Et. Br) from the drop-down menu
Select a time. 500 ms works.
the buttons below the circle (now red) are:
1. aperture (exposure time; donut-looking button)
2. zoom (magnifying glass)
3. focus (eyeball)
Click the red circle to take the picture
There are buttons to invert the colors (yin-yang) and sharpen (knife).

Imaging tips

Use an ethidium bromide alternative such as MidoriGreen
- 0.5uL mixed into 1 gel volume works.
- If adding to gel directly, 3uL (or less??) can be added to the opposite end of the gel as the DNA.
Exposures should be < 0.5 seconds to minimize background emissions. If you need longer, you probably should have had more ethidium bromide or other DNA dye.

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

You don't need much DNA. 50 ng should be plenty.

75 and 150 ng DNA on a 0.7% agarose gel

TBE buffer can be re-used for months.
- This is nice, because you shouldn't dump ethidium bromide containing solution down the drain.
- Janet usually uses it heavily for 4+ months before replacing it.
- Always add DI water to replace evaporated water, not TBE buffer
Agarose gels can be "drained" and re-used several times.
- Don't use a previously used gel for DNA you will cut and purify for cloning/sequencing.
- Drain with 100V for ~90 min.

OLD: Ethidium bromide instructions

If 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

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