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通过红外光谱和荧光研究平行链DNA的结构与药物相互作用。

Structure and drug interactions of parallel-stranded DNA studied by infrared spectroscopy and fluorescence.

作者信息

Fritzsche H, Akhebat A, Taillandier E, Rippe K, Jovin T M

机构信息

Institute of Molecular Biology, Friedrich Schiller University Jena, Germany.

出版信息

Nucleic Acids Res. 1993 Nov 11;21(22):5085-91. doi: 10.1093/nar/21.22.5085.

Abstract

The infrared spectra of three different 25-mer parallel-stranded DNAs (ps-DNA) have been studied. We have used ps-DNAs containing either exclusively dA x dT base pairs or substitution with four dG x dC base pairs and have them compared with their antiparallel-stranded (aps) reference duplexes in a conventional B-DNA conformation. Significant differences have been found in the region of the thymine C = O stretching vibrations. The parallel-stranded duplexes showed characteristic marker bands for the C2 = O2 and C4 = O4 carbonyl stretching vibrations of thymine at 1685 cm-1 and 1668 cm-1, respectively, as compared to values of 1696 cm-1 and 1663 cm-1 for the antiparallel-stranded reference duplexes. The results confirm previous studies indicating that the secondary structure in parallel-stranded DNA is established by reversed Watson--Crick base pairing of dA x dT with hydrogen bonds between N6H...O2 and N1...HN3. The duplex structure of the ps-DNA is much more sensitive to dehydration than that of the aps-DNA. Interaction with three drugs known to bind in the minor groove of aps-DNA--netropsin, distamycin A and Hoechst 33258--induces shifts of the C = O stretching vibrations of ps-DNA even at low ratio of drug per DNA base pair. These results suggest a conformational change of the ps-DNA to optimize the DNA-drug interaction. As demonstrated by excimer fluorescence of strands labeled with pyrene at the 5'-end, the drugs induce dissociation of the ps-DNA duplex with subsequent formation of imperfectly matched aps-DNA to allow the more favorable drug binding to aps-DNA. Similarly, attempts to form a triple helix of the type d(T)n.d(A)n.d(T)n with ps-DNA failed and resulted in the dissociation of the ps-DNA duplex and reformation of a triple helix based upon an aps-DNA duplex core d(T)10.d(A)10.

摘要

对三种不同的25聚体平行链DNA(ps-DNA)的红外光谱进行了研究。我们使用了仅包含dA×dT碱基对或被四个dG×dC碱基对取代的ps-DNA,并将它们与处于传统B-DNA构象的反平行链(aps)参考双链体进行比较。在胸腺嘧啶C=O伸缩振动区域发现了显著差异。与反平行链参考双链体的1696 cm-1和1663 cm-1的值相比,平行链双链体分别在1685 cm-1和1668 cm-1处显示出胸腺嘧啶C2=O2和C4=O4羰基伸缩振动的特征标记带。结果证实了先前的研究,表明平行链DNA中的二级结构是通过dA×dT的反向沃森-克里克碱基配对以及N6H...O2和N1...HN3之间的氢键建立的。ps-DNA的双链体结构比aps-DNA的双链体结构对脱水更敏感。与已知结合在aps-DNA小沟中的三种药物——纺锤菌素、偏端霉素A和Hoechst 33258——相互作用,即使在药物与DNA碱基对的比例较低时,也会诱导ps-DNA的C=O伸缩振动发生位移。这些结果表明ps-DNA发生了构象变化以优化DNA-药物相互作用。如通过在5'-端用芘标记的链段的准分子荧光所证明的,这些药物诱导ps-DNA双链体解离,随后形成不完全匹配的aps-DNA以允许药物更有利地结合到aps-DNA上。同样,尝试用ps-DNA形成d(T)n.d(A)n.d(T)n类型的三链螺旋失败了,并导致ps-DNA双链体解离,基于aps-DNA双链体核心d(T)10.d(A)10重新形成三链螺旋。

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