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        Northern Blotting步骤和试剂配制(Breeden Lab)

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        相关专题
        Northern Blotting技术专题

        I. Electrophoresis

        clean gel box with NaOH and/or SDS, 2 hours to overnight, rinse with water

        prepare Agarose gel solution [1 % Agarose, 1 x MOPS, H2O to 95 % of endvolume]

        microwave until completely dissolved

        cool down to 60-70 °C, add Formaldehyde (37 %) to 0.6 M endconcentration, pour immediately

        allow gel to harden at least 30 min

        prepare running buffer [1 x MOPS, 0.2 M Formaldehyde]

        II. Sample preparation

        use 5-10 µg total RNA per lane (up to 30 µg)

        bring RNA with H2ODEPC to equal volume (5-10 µl), add same vol. loading buffer

        add 0.5 µl EtBr (0.5 µg/µl)

        heat for 5 min @ 90 °C, cool on ice

        III. Gel run

        run gel (8 x 10 cm) in fume hood with 70-100 V (-> 50-70 mA)

        run until BPB is near the gel end (2.5-3.5 h)

        IV. Northern transfer of RNA

        soak gel 3 times 5 min in distilled water (to remove Formaldehyde)

        photogragh gel with ruler beside it

        cut GeneScreen membrane (Nylon, DuPont) to exact gel size

        soak membrane in water for a few seconds

        set up capillary blot with 10 x SSC transfer buffer:

        2 wet Whatman - gel - membrane - 2 wet Whatman - 2 dry Whatman - papertowel - glasplate - weight

        transfer 16-24 h with changes of the papertowel

        mark lanes, remove membrane, wash briefly in 2 x SSC

        place membrane on wet Whatman paper and UV-crosslink damp (auto crosslink setting, 254 nm, Stratagene, Stratalinker)

        bake membrane @ 80 °C for 1-2 h

        V. Hybridization

        prehybridize membrane for 1-4 h @ 42 °C with 5-10 ml prehybridization buffer

        heat radioactive labeled probe for 3 min @ 95 °C, cool on ice

        discard prehybridization buffer, add hybridization buffer and probe, incubate ON @ 42 °C

        wash membrane 1 x 15 min with 2 x SSC @ RT

        wash with 2 x SSC, 0.1 % SDS @ 65 °C until background is low

        wash with 0.1 x SSC, 0.1 x SDS @ 65 °C (optional)

        expose wet membrane under saran wrap (-80 °C)

        important: never let the membrane dry (until the blot is stripped)

        VI. Stripping and re-hybridization

        wash membrane for 30 min to 3 h in strip solution @ 75 - 85 °C until no radioactivity can be detected on the membrane

        membrane can now be air dried and stored @ RT

        for re-hybridization (up to 10 times) follow the hybridization protocol

        Buffers:

        10 x MOPS:

        0.4 M Morpholinopropanesulfonic acid (free acid); 0.1 M Na-acetate-3 x H2O; 10 mM EDTA ; adjust to pH 7.2 with NaOH; store dark in fridge:

        [500 ml: 41.9 g MOPS, 6.8 g NaAc, 10 ml 0.5 M EDTA]

        Loading Buffer:

        1 x MOPS; 18.5 % Formaldehyde; 50 % Formamide; 4 % Ficoll400; Bromophenolblue; store at -20 °C:

        [1 ml: 100 µl 10 x MOPS, 500 µl Formamide, 185 µl Formaldehyde, 40 mg Ficoll400, Bromophenolblue, 215 µl H2O]

        Prehybridization-buffer:

        5 x SSC; 50 % Formamide; 5 x Denhardt"s-solution; 1 % SDS; 100 µg/ml heat-deNature d sheared non- homologous DNA (Salmon sperm DNA or yeast tRNA)

        [100 ml: 25 ml 20 x SSC, 50 ml Formamide, 5 ml 100 x Denhardt"s, 1 g SDS, 1 ml 10 mg/ml DNA]

        Hybridization-buffer:

        Prehybridization buffer with 5 % Dextransulfate (Na-salt, MW 500,000, 50 % stock-solution) and without non-homologous DNA

        100 x Denhardt"s solution:

        [for 500 ml: 10 g Ficoll 400; 10 g polyvinylpyrrolidone MW 360000; 10 g BSA fraction V; H2O]

        store at -20 °C.

        20 x SSC:

        3 M NaCl; 0.3 M Na-citrate

        [1 l: 175.3 g NaCl, 88.2 g NaCitrate]

        Strip-solution:

        5 mM Tris pH 8; 0.2 mM EDTA; 0.05 % Na-pyrophosphate; 0.1 x Denhardt"s solution

        [500 ml: 2.5 ml 1 M Tris, 200 µl 0.5 M EDTA, 5 ml 5 % NaPP, 1 ml 50 x Denhardt"s]

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