首页> 外文期刊>Nucleic Acids Research >The use of diaminopurine to investigate structural properties of nucleic acids and molecular recognition between ligands and DNA.
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The use of diaminopurine to investigate structural properties of nucleic acids and molecular recognition between ligands and DNA.

机译:使用二氨基嘌呤来研究核酸的结构特性以及配体与DNA之间的分子识别。

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摘要

2,6-Diaminopurine (DAP) is an analogue of adenine which can be converted to nucleotides that serve as substrates for incorporation into nucleic acids by polymerases in place of (d)AMP. It pairs with thymidine (or uracil), engaging in three hydrogen bonds of the Watson-Crick type. The result of DAP incorporation is to add considerable stability to the double helix and to impart other structural features, such as an altered groove width and disruption of the normal spine of hydration. DNA containing DAP may or may not be recognized by restriction endonucleases; RNA containing DAP may not engage in normal splicing. The DAP.T pair affects the local flexibility of DNA and impedes the interaction with helix bending proteins. By providing a non-canonical hydrogen bond donor in the minor groove and/or blocking access to the floor of that groove it strongly affects interactions with small molecules such as antibiotics and anticancer drugs. Examples which illustrate altered recognition of nucleotide sequences in DAP-containing DNA are presented: changed sites of cutting by bleomycin, photocleavage by uranyl nitrate and footprinting with mithramycin. Using DNA in which both A-->DAP and G-->Inosine substitutions have been made it is possible to assess precisely the role of the purine 2-amino group in ligand-DNA recognition.
机译:2,6-二氨基嘌呤(DAP)是腺嘌呤的类似物,可以将其转化为核苷酸,用作通过聚合酶代替(d)AMP掺入核酸的底物。它与胸苷(或尿嘧啶)配对,并参与了Watson-Crick型的三个氢键。 DAP掺入的结果是为双螺旋增加了相当大的稳定性,并赋予了其他结构特征,例如改变的凹槽宽度和破坏正常的水合作用。限制性内切核酸酶可能会或可能不会识别出含有DAP的DNA。含有DAP的RNA可能无法正常剪接。 DAP.T对影响DNA的局部柔性并阻碍与螺旋弯曲蛋白的相互作用。通过在小凹槽中提供非规范的氢键供体和/或阻止进入该凹槽的底部,它会严重影响与小分子(如抗生素和抗癌药)的相互作用。举例说明了在含DAP的DNA中核苷酸序列的识别变化:显示了由博来霉素切割的位点,由硝酸铀酰进行的光切割以及与光神霉素产生的足迹的改变。使用已完成A-> DAP和G->肌苷取代的DNA,可以精确评估嘌呤2-氨基在配体-DNA识别中的作用。

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