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        Human RNA Extraction protocol(哈佛RNA提取方法)

        互联网

        2236

        REAGENTS

        Guanadinium Thiocyanate

        1.0 M Sodium Citrate pH 7.0

        10% Sarcosyl

        2-mercaptoethanol

        water saturated phenol pH 4.0-7.0

        Na2EDTA MOPS (free acid)

        2.0 M Sodium Acetate pH 4.0

        Formaldehyde

        Formamide

        10% SDS

        49:1 Chloroform:Isoamyl Alcohol

        SOLUTIONS

        filter sterilize through 0.2 μm filter

        NOTE: Solution D may be made ahead of time and stored at room temp for one month,but the 2-mercaptoethanol must be added immediately before use.

        PROTOCOL

        1) Aspirate off media

        2) Lyse cells in Solution D

        T-150 = 4 ml Solution D

        Transfer to pre-chilled 30 ml Oakridge centrifuge tube; make sure there is enough space for additions below.

        3) Sequentially add:

        a) 0.1 volume 2.0 M NaOAc - mix well

        b) 1 volume phenol - mix well

        c) 0.2 volume chlorofom/isoamyl alcohol

        4) Vortex 10 sec

        5) Incubate on ice for 15 min

        6) Centrifuge 10,000 x g, 20 min, 4 ℃

        7) Transfer aqueous phase to a new 50 ml conical

        8) Precipitate with 1 volume isopropanol, >1 hour, -20 ℃

        9) Centrifuge in 50 ml conical tube, 3,000 x g, 1 hour, 4 ℃

        alternatively, spin in oakridge tubes 10,000 x g, 20 min, 4 ℃

        10) Dissolve pellet in 0.3 ml Solution D; transfer to microfuge tube

        11) Precipitate with 1 volume isopropanol, >1 hour, -20 ℃

        12) Centrifuge 15 min, 4 ℃

        13) Wash pellet with 75% ethanol

        14) Drundefined, dissolve in H2undefined~E_heat_to_65__℃for 10 min to completely dissolve.

        Chomczynske, P. and Sacchi, N. Analytical Biochem. 1987. 162:156-159

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