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The use of phosphorothioate-modified DNA in restriction enzyme reactions to prepare nicked DNA.

机译:在限制酶反应中使用硫代磷酸酯修饰的DNA制备带切口的DNA。

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摘要

The RF IV form of M13 DNA was synthesized enzymatically in vitro, using the viral (+)strand as template, to contain phosphorothioate-modified internucleotidic linkages of the Rp configuration on the 5' side of every base of a particular type in the newly-synthesized (-)strand. Twenty nine restriction enzymes were then tested for their reactions with the appropriate modified DNA types having a phosphorothioate linkage placed exactly at the cleavage site(s) of these enzymes in the (-)strand. Eleven of the seventeen restriction enzymes tested that had recognition sequences of five bases or more could be used to convert the phosphorothioate DNA entirely into the nicked form, either by simply allowing the reaction to go to completion with excess enzyme (Ava I, Ava II, Ban II, Hind II, Nci I, Pst I or Pvu I) or by stopping the reaction at the appropriate time before the nicked DNA is linearized (Bam HI, Bgl I, Eco RI or Hind III). Only modification of the exact cleavage site in the (-)strand could block linearization by the first class of enzymes. The results presented imply that the restriction enzyme-directed nicking of phosphorothioate M13 DNA occurs exclusively in the (+)strand.
机译:M13 DNA的RF IV形式是通过体外酶促合成的,使用病毒(+)链作为模板,在新近形成的特定类型的每个碱基的5'侧含有Rp构型的硫代磷酸酯修饰的核苷酸间键合。合成(-)链。然后测试了29种限制酶与适当修饰的DNA类型的反应,所述修饰的DNA类型具有恰好位于(-)链中这些酶的切割位点的硫代磷酸酯键。测试的17种限制性酶中识别出5个碱基或以上的限制性酶中的11种可用于将硫代磷酸酯DNA完全转化为带切口的形式,方法是简单地使反应用过量的酶完成(Ava I,Ava II,禁止II,Hind II,Nci I,Pst I或Pvu I)或通过在有切口的DNA线性化之前的适当时间停止反应(Bam HI,Bgl I,Eco RI或Hind III)。只有对(-)链中精确切割位点的修饰,才能阻止第一类酶的线性化。提出的结果暗示,硫代磷酸酯M13 DNA的限制性内切酶导向的切口仅在(+)链中发生。

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