首页> 美国卫生研究院文献>Biochemical Journal >Interaction of the type I methyltransferase M.EcoR124I with modified DNA substrates: sequence discrimination and base flipping.
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Interaction of the type I methyltransferase M.EcoR124I with modified DNA substrates: sequence discrimination and base flipping.

机译:I型甲基转移酶M.EcoR124I与修饰的DNA底物的相互作用:序列区分和碱基翻转。

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摘要

We have analysed the DNA-protein contacts made between the type I DNA methyltransferase M.EcoR124I and its recognition sequence. The effects of base modifications have been probed by measuring the affinity of M.EcoR124I for the modified sequences relative to that for the wild-type sequence by using gel-retardation competition assays. These results, along with those from methylation interference footprinting and photo-affinity cross-linking have identified the location of potential DNA contacts within the DNA recognition site. Substitution of 6-thioguanosine for each of the three specific guanines in the recognition sequence leads to a large (10-20-fold) decrease in the strength of DNA binding, indicating the importance of hydrogen-bonding interactions in the major groove of DNA. In contrast, replacement of either (or both) of the adenines at the target site for methylation by the enzyme, to produce either a base pair mismatch or loss of the base, leads to a marked increase in DNA-binding affinity. The results strongly support the proposal that type I methyltransferases employ a base-flipping mechanism to methylate their target base.
机译:我们已经分析了I型DNA甲基转移酶M.EcoR124I及其识别序列之间的DNA-蛋白质接触。已经通过使用凝胶延迟竞争测定法测量M.EcoR124I相对于野生型序列的亲和力,来测量M.EcoR124I对修饰的序列的亲和力,从而探究了碱基修饰的作用。这些结果,以及来自甲基化干扰足迹和光亲和性交联的结果,已经确定了DNA识别位点内潜在DNA接触的位置。对于识别序列中的三个特定鸟嘌呤中的每一个,用6-硫代鸟嘌呤取代会导致DNA结合强度大幅下降(10-20倍),这表明在DNA大槽中氢键相互作用的重要性。相反,在靶位点上用于酶的甲基化取代腺嘌呤中的一个(或两个),以产生碱基对错配或碱基丢失,导致DNA结合亲和力显着增加。结果强烈支持I型甲基转移酶采用碱基翻转机制将其目标碱基甲基化的提议。

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