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        DNA probes are prepared using a modification of the method of Feinberg and Vogelstein

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        1061

        DNA probes are prepared using a modification of the method of Feinberg and Vogelstein, (1983).

        You will need:

        Nuclease-free BSA
        [a-32P]-dCTP (Amersham or DuPont)
        Klenow DNA Polymerase (New England Biolabs or Pharmacia)
        500mM EDTA, pH 8
        dNTP solutions (separate solutions of 100mM dATP, dGTP, dCTP and dTTP in TE, pH 7.0
        Solution O (1.25M Tris.Cl, 125mM MgCl2 , pH 8.0)
        Solution A (1ml solution O, 18ul b-mercaptoethanol, 5ul of each dNTP solution
        Solution B (2M HEPES, pH 6.6)
        Solution C (Random hexanucleotides at 90 OD260 nm/ml)
        Sterile, nano-pure water

        1) Digest plasmid DNA with the appropriate restriction enzyme,fractionate electrophoretically, and purify by the NaI/glass method (see Gene-Klene Protocol). Resuspend in sterile,distilled H2 O at approximately 2ng/ul.

        2) Boil DNA at 100°C or 10 minutes.

        3) Snap chill in an ice/water bath and hold on ice prior to use.

        4) Carry out labelling reactions at room temperature by the addition, to a sterile Eppendorf tube, of the following reagents in the stated order:-

        5ul OLB buffer (see below)
        1ul 10mg/ml nuclease free BSA
        17.5ul (25ng) DNA fragment
        370KBq [a-32P]-dCTP (1ul of a 370KBq/ul stock)
        0.5ul Klenow fragment of E. coli DNA polymerase (0.5-1 unit)
        OLB buffer is made by mixing solutions A, B and C in the ratio 10: 25: 15, respectively.

        5) Allow reactions to continue for at least 5 hours.

        6) Terminate reactions by the addition of 1ul 0.5M EDTA, 74ul sterile, distilled H2 O and 5 minutes incubation at 100°C.

        The specific activity and the percentage incorporation of 32P-dCTP into the probe should be determined by TCA precipitation of 1ml probe and scintillation counting.

         

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