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  • 實驗方法> DNA實驗技術> DNA基礎知識>DNA片段的Fill-in標記

    DNA片段的Fill-in標記

    關鍵詞: DNA Fill-in 標記來源: 互聯網

    ?

    This protocol was designed to generate directionally end-labeled probes for DNaseI footprinting but it can be used for any application that requires end-labeled DNA probes.

    Solutions

    10 mM dNTP Stocks

    Thaw100 mM stocks (NEB or Boehringer Mannheim) on ice and dilute 10-fold in Q.

    store small (10-20 ml) aliquotes at -80 degrees and thaw on ice just prior to use

    ?

    10 X Klenow Buffer

    0.5 M Tris 7.5 500 ml 1 M Tris 7.5

    0.1 M MgCl2 100 ml 1 M MgCl2

    10 mM DTT 100 ml 0.1 M DTT

    0.5 mg/ml BSA 50 ml 10 mg/ml BSA

    250 ml Q

    store at -20° in 50 ml aliquotes

    ?

    dNTP Mix

    21 ml Q

    3 ml each of 3 cold dNTP's (10 mM stocks, see above)

    Note: leave out the dNTP which will be used for labeling of the chosen restriction site (i.e. a-32P-dATP with EcoRI Labeling).

    Procedure

    ? Digest 2 mg of CsCl purified plasmid DNA (Protocol C.1) with the restriction endonuclease corresponding to the end to be labeled. phenol/chloroform extract and EtOH ppt.

    ? Resuspend the pellet in 19 ml Q, then add:

    25 ml dNTP mix

    5 ml 10X Klenow Buffer

    5 ml a 32P dNTP

    1 ml Klenow

    Incubate at room temperature for 30'.

    ? Phenol/chloroform extract and EtOH ppt. Resuspend in 16 ml Q and digest with the second enzyme for 30' at 37 degrees.

    ? Gel purify by running out the restriction digest (5 minutes 100 mA) on a 1% minigel and spin purifying (Protocol D.5).

    ? Resuspend the purified fragment in 100 ml Q.

    ? Count 1 ml by spotting onto Whattman 3mm filter paper and counting for 1 min. I get 20,000-50,000 cpm for restriction fragments and 200,000-400,000 cpm for double stranded oligos. Anything less than 15,000 for restriction fragments should be trashed.

    ? Probes labeled using this protocol are usually good for 1-2 weeks but the best results are obtained when the probe is used within the first few days after labeling.

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