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        PCR Method to Make Radioactive Probes

        互联网

        939

        Materials

        Hot Probe dNTP Mix:
        25 mM dATP
        25 mM dTTP
        25 mM dGTP
        2.5 mM dCTP

        Hybridization Solution:
        5X SSC
        0.5% (w/v) Blocking Reagent
        0.1% (w/v) N-lauroylsarcosine, Na-salt
        0.02% (w/v) SDS
        50% Formamide

        Blot Wash 1:
        2X SSC
        0.1% SDS

        Blot Wash 2:
        0.1X SSC
        0.1% SDS

        Method

        PCR Reaction
        1. Combine reaction mix on ice:

          16.6 µl 30% Glycerol
          16 µl 100 mM (NH 4 ) 2 SO 4
          6.8 µl 1 M Tris , pH 8.5
          2.5 µl 100 mM MgAc 2
          1 µl 1% Triton X-100
          0.8 µl hot probe dNTP mix
          40 pmols of each primer
          0.5 to 1 µg of template
          0.4 µl Taq polymerase (5 Units/µl)
          ____________________________
          ==> H 2 O to 95 µl
          Then add 5 µl α- 32 P dCTP (3000Ci/mMole)
           
        2. PCR cycle profile:

          94℃ 5 minutes
          _________________
          94℃ 30 sec
          55℃ 30 sec
          72℃ 30 sec
          ==> 10 cycles
          _________________
          72℃ 7 minutes
           
        3. Clean probe on Sephadex G50 spin columns.
        4. Check activity with scintilation counter.
        Southern Hybridization
        1. After transfer, crosslink blot and hybridize for 5 min in hybridization solution at 42℃.
        2. Boil probe for 5 minutes in 10 to 20 ml hyb solution.
        3. Pour off hyb solution from blot and add probe. Incubate overnight at 42℃.
        4. Pour off probe and wash blot 2X 5 minutes in the hyb tube with Blot Wash 1.
        5. Remove blot from bottle and wash 2X 15 minutes at 55℃ with Blot Wash 2.
        6. Check radioactivity associated with corner of blot. If still hot: 15 min 55℃ Blot Wash 2.
        7. Wrap blot in plastic wrap and put down on phosphorimager cassette or film.
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