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  • 實驗方法> DNA實驗技術> DNA基礎知識>Quick?DNA?Plasmid?Prep.

    Quick?DNA?Plasmid?Prep.

    關鍵詞: quick dna plasmid來源: 互聯網
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    Quick DNA Plasmid Prep.

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    This is a very fast mini-prep protocol which is suitable for sequence analysis and restriction digests. Although the yield is higher than Protocol D.1, there is considerable chromosomal DNA, RNA and protein contamination.

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    Solutions

    Sucrose/Tris

    25% sucrose 25 g sucrose

    50 mM Tris pH 8.0 5 ml 1M Tris pH 8.0

    up to 100 ml with Q

    store at room temperature

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    Triton Lysing Mix

    5% Triton X-100 5 ml Triton X-100

    5% sucrose 5 g sucrose

    50 mM Tris pH 7.5 5 ml 1M Tris pH 7.5

    50 mM EDTA 10 ml 0.5 M EDTA pH 8.0

    up to 100 ml with Q

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    store at room temperature

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    2.5 M KOAc

    2.5 M postassium acetate 24.5 g potassium acetate

    pH to 4.8 with glaicial acetic acid

    up to 100 ml with Q

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    store at room temperature

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    Procedure

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    ? Pellet 1.5 ml of an overnight culture in an eppendorf tube by spinning at14K. Resuspend in 15 ml Sucrose/Tris.

    Prepare Lysozyme Mixture (10mg/ml (Sigma #L6876) in Sucrose/Tris)

    Prepare boiling water bath

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    ? Add 100 ml Triton Lysing Mix and briefly vortex on half speed. Add 10 ml Lysozyme Mixture, invert, and incubate at room temperature for 5'.

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    ? Boil for 4' and spin at 14K for 15' in the cold room.

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    ? Remove the pellet with a toothpick and add 12 ml 2.5 M KOAc and 100 ml isopropanol; incubate at -80o for 10'.

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    ? Spin 10' and wash the pellet with 80% EtOH.

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    ? Dry and resuspend in 30 ml Q.

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    I use 5 ml for a standard digest (RNaseA is required), and 13.5 ml for sequencing (Protocol S.1).

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