Quick Isolation of DNA from Agarose Gels
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Hancock Laboratory Methods. Department of Microbiology and Immunology,
University of British Columbia, British Columbia, Canada http://www.cmdr.ubc.ca/bobh/showmethod.php?methodid=67
METHOD:
1.Run gel as normal in 1X TBE.
2.Visualize band under LONG wave UV.
3.Cut band out with razor blade.
4.Place excised agarose slice in an Eppendorf tube, which has a hole in its bottom (by inserting a hot needle), and which has a small amount of siliconized glass wool covering the opening.
5.Place this tube inside another Eppendorf tube.
6.Spin tubes either at 1/2 maximum speed for 15 minutes or, if not possible, full speed for 5 minutes.
7.Phenol/chloroform the resulting liquid.
8.Repeat with 1/10 volume 3 M NaAc 2x volume EtOH.
