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        EMSA Protocol

        互联网

        3924

        Pour Acrylamide Gel:

        1. Assemble Plates, spacers, and clamps. Seal with 1% agarose to prevent leaks.

        2. Pour 5% acrylamide Gel

        Plate size Large Medium

        H2 O 78mL 39mL

        10x TBE 5mL 2.5mL

        30% Polyacrylamide 16.6mL 8.4mL

        10% APS 500uL 250uL

        mix well while minimizing bubble formation. Add 50uL/25uL TEMED. Mix and pour, add combs. Gel will take 30-45 min to polymerize. After polymerization, gel can be wrapped in Saran Wrap and stored at 4o C.

        5x Binding Buffer:

        Composition Recipe for 10mL

        50mM Tris HCl (pH 8.0) 0.5 mL of 1M Tris HCl (pH 8.0)

        750 mM KCl 3mL of 2.5 M KCl

        2.5 mM EDTA 50uL of 0.5 M EDTA (pH 8.0)

        0.5% Triton-X 100 50uL Triton-X 100

        62.5 % glycerol (v/v) 7.87 g glycerol

        1mM DTT add DTT fresh before use

        Binding Reaction:

        1uL of poly-dIdC (1ug/uL in TE)

        2uL of 5x Binding Buffer

        1uL of labeled probe

        1uL cold competitor (if needed)

        0.1uL 100x BSA

        ?? uL Nuclear Extract (5ug protein total)

        Add H2 O to 10uL

        Incubate 30 min room temp. Add antibody for supershift (if needed). Incubate additional 30 min, room temp.

        While binding reaction is incubating, pre-run polyacrylamide gel 150V, 30 min, using 0.5xTBE as running buffer.

        Run samples on acrylamide gel ~2hours 150V

        Dry the Gel (Optional)Dry the Gel (Optional)

        Transfer Gel to Whatman Paper. Cover top of gel with Saran Wrap and dry at 80o C in vacuum dryer 1-2 hour.

        Expose the Gel

        Place gel in cassette with reflection screen. Add film and place in -80o C freezer.

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