---+ Ethanol_precipitation ---++ Precipitating out salts from DNA samples *Materials* * 3M Sodium Acetate buffer, pH 5.2 (store at 4°C) * Cold 100% Ethanol (-20°C) * Cold 70% Ethanol in sterile dH2O (-20°C) * DNA sample * 4°C Microcentrifuge (or normal microcentrifuge in cold room). All centrifuges should be on "soft" (no brake) setting. *Procedure* 1 Transfer DNA to a container where it fills one fourth the total volume (a 500ul tube should have no more that 125ul of DNA solution, for example. 1 Add one tenth volume of Sodium Acetate buffer to equalize ion concentrations. 1 Add at least two volumes of cold 100% ethanol; let stand in -20°C freezer for at least one hour. 1 Remove as much supernatant as possible with a 1ml micropipet; reventrifuge, then remove the rest with a 200ul pipet. 1 Add 200i; of cold 70% ethanol; centrifuge for 5 minutes at 4°C. 1 Remove supernatant with a 200ul pipet; evaporate remaining ethanol in a 37°C water bath or heat block. 1 Resuspend pellet in 50ul of water or TE buffer. -- Main.LindseyWolf - 02 Dec 2011
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Topic revision: r1 - 2011-12-03 - LindseyWolf