DNA Isolation from Tails

NaOH extraction (quick "dirty" DNA preparation). Reference: Truett GE et al. 2000. Biotechniques 29(1):52-54
Cut 2 mm of tail and place into an Eppendorf tube or 96-well plate
Add 75ul 25 mM NaOH / 0.2 mM EDTA (Alkaline Lysis Reagent)
Place in thermocycler or heat block at 95ºC for 1 hour, then reduce the temperature to 15°C until ready to proceed to the next step
Add 7 5ul of 40 mM Tris HCl (pH 5.5)
Centrifuge at 4000 rpm for 3 minutes
Take an aliquot for PCR (use 2 ul undiluted, or 2 ul of a 1:100 dilution/reaction)

Alkaline Lysis Reagent

To 25 ml water, add:

62.5 µl of 10 N NaOH (final concentration is 25 mM.)
10.0 µl of 0.5 M disodium EDTA (final concentration is 0.2 mM, pH should be about 12 but should not have to be adjusted.)

Make fresh every one to two months. Keep solution at room temperature.

Neutralization Reagent

Make 1M Tris: 121.14 g Tris base, pH to 7.0 with HCl à 1 L final volume; autoclave

Add 4 ml Tris to ~80 ml water. pH to 5.5 à Make up to 100 ml final volume (40 mM final [ ])

Genotyping

1. Make up reaction mix

2. Make up assay mixture

3. Add master mix (10 ul) to each assay (10 ul) for a total volume of 20 ul

4. Run appropriate PCR program

5. Prepare agarose gels

6) Load 20 ul of the PCR reactions directly into agarose gels.

7) Run gels at a constant 120 volts. Will take approximately 30 to 40 minutes for large gels.

8) Photograph using AlphaImager Gel Imager

Protocols