| Isolation of Yeast Genomic DNA 酵母基因组DNA提取【Upstate Medical University】 | | 点击: 作者: 来源: 时间: 2007-04-11 本站论坛 |
|  | Amberg Lab ,Upstate Medical University
DNA.html">http://www.upstate.edu/biochem/amberg/protocols/yeast_genomic_DNA.html
- Grow 100 ml culture to about 1x10 to the 8th
- Spin 4 x 15 mls of culture down about 3k x 3 min.
- Resuspend entire pool in about 6 mls ddH2O, aliqoute into 1.5ml microfuge tubes and spin down.
- Aspirate off super and vortex pellet till suspended.
- Add 200ul soln A, add 200ul Phenol/CHCl3 and 0.3g acid washed glass beads.
- Vortex 2 min, add 200ul TEpH8 and spin at max speed for 5 min.
- Transfer super to a new tube and add 1ml 100% EtOH, mix by inversion.
- Spin 2 min, pour off super and recon in 0.4ml TEpH8 30ug/ml RNaseA.
- Incubate 5 min x 37¡C, add 18ul 5M NH4OAc and 1ml 100% EtOH and store at -20¡C for a few hrs.
- Spin down DNA 10 min and recon each pellet in 25-50ul or whatever convenient volume.
- Solution A:
- 200ul neat or 2ml 10% Triton X-100 (2%)
- 1ml 10% SDS (1%)
- 200ul 5M NaCl (0.1M)
- 100ul 1M Tris pH8 (0.01M)
- 20 ul 0.5M EDTA (1mM)
- Water to 10ml
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