| Preparation of Salmon Sperm DNA | 点击: 作者:51protocol收集 来源: 时间: 2007-03-28 本站论坛
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Preparation of Salmon Sperm DNA
Denatured Salmon Sperm DNA is used in prehybridization and hybridization solutions to reduce background signal. The Salmon Sperm DNA (Sigma No. D-1626) is first "denatured" in large volumes and then again immediately before it is used. Two methods ( Sonication or NaOH/boiling SS DNA) are prevail. NaOH/boiling SS DNA is available in this lab.
NaOH/boiling of SS DNA
- Add 1.0 g salmon sperm DNA to 100 ml 0.4 NaOH in a 250 ml Erlenmyer flask: (If 250-ml centrifuge bottles are necessary, ask Dr. M.D. Thomas to use his centrifuge and 250 ml centrifuge bottles). Dissolve by placing on a rotator or stir plate overnight at room temperature.
- Place in a boiling water bath for 45 min to shear the DNA. Chill on ice.
- Neutralize with glacial acetic acid to pH 7.0.
- After transfer 50 ml PPT, and centrifuge tubes (2000 rpm, 10 min) to remove debris. Pour DNA solution into another 250 ml Erlenmyer flask.
- Add two volume of 95 % EtOH, and place at -20 C for 1 hr.
- Transfer to PPT, and centrifuge tubes again (2000 rpm, 10 min).
- Rinse pellet with 70 % EtOH, invert to the tube to drain for 1-2 min, if desired, vacuum dry 5 min, dissolve in 50 ml TE.
- Determine DNA quantity by determining the fluorescent density or measuring the absorbance of the solution at 260 nm and dilute to 10 mg/ml.
- Store at -20 C.
NaOH denaturation of SS DNA immediately before use
- Remove the appropriate amount of previously NaOH/boiled SS DNA after thawing.
- Add 1/10 volume of 1 N NaOH, voltex and let sit for 10 min for room temperature.
- Neutralize the base with 1/10 volume of 1.8 M Tris-HCl and 0.2 M Tris- Base sequentially. Vortex and let sit at room temperature for 10 min.
- Add prehybridization or hybridization solution and mix in a stir plate.
* If you want to access to 250 ml centrifuge bottles and the centrifuge, ask.
* Sonicator is accessible, if desired to denature SS DNA by a sonicator.
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