S. D. Química Analítica, Facultad de Farmacia, Universidad Complutense de Madrid, 28040 Madrid, Spain.
Anal Bioanal Chem. 2011 Apr;400(2):321-7. doi: 10.1007/s00216-010-4640-5. Epub 2011 Jan 19.
The interaction between DNA and several newly synthesized derivatives of the natural anticancer compound luotonin A has been studied. The results from our work reveal an effective and selective alkaloid/double-stranded DNA (ds-DNA) interaction. In the presence of increasing amounts of ds-DNA, a noticeable fluorescence quenching of the luotonin A derivatives under study was observed. However, this effect did not take place when single-stranded DNA (ss-DNA) was employed. The association constant alkaloids/ds-DNA was calculated by quantitation of such a quenching effect. The influence of other quenchers, namely Co(2+) and Br(-) on the native fluorescence of luotonin A and derivatives was also studied, and a remarkable quenching effect was observed for both ions. We have also investigated how by binding DNA the alkaloids could get protected from the external Co(2+) and Br(-) quenchers. The Stern-Volmer constants (K (SV)) for Co(2+) and Br(-) quenching effect on the studied alkaloids were considerably reduced (10-50%) after incubation of the compounds in the presence of DNA with regard to the K (SV) values in absence of DNA. An increase in the fluorescence anisotropy values of luotonins was also produced only in the presence of ds-DNA but not in the case of ss-DNA. To better characterize the nature of that interaction, viscosimetry assays and ethidium bromide displacement studies were conducted. With regard to DNA reference solutions, the viscosity of solutions containing DNA and luotonin A derivatives was reduced or not significantly increased. It was also observed that the studied compounds were unable to displace the intercalating agent ethidium bromide. All of these results, together with the obtained association constants values (K (ass) = 2.2 × 10(2) - 1.3 × 10(3)), support that neither covalent nor intercalating interactions luotonin A derivatives/ds-DNA are produced, leading to the conclusion that these alkaloids bind ds-DNA through the minor groove. The specific changes in the fluorescence behavior of luotonin A and derivatives distinguishing between ss-DNA and ds-DNA binding, lead us to propose these compounds as attractive turn-off probes to detect DNA hybridization.
已研究了 DNA 与几种天然抗癌化合物洛洛托宁 A 的新合成衍生物之间的相互作用。我们的工作结果揭示了有效的和选择性的生物碱/双链 DNA(ds-DNA)相互作用。在 ds-DNA 量增加的情况下,观察到所研究的洛洛托宁 A 衍生物的荧光显著猝灭。然而,当使用单链 DNA(ss-DNA)时,不会发生这种效应。通过定量这种猝灭效应,计算了生物碱/ds-DNA 的结合常数。还研究了其他猝灭剂,即 Co(2+)和 Br(-)对洛洛托宁 A 和衍生物的天然荧光的影响,并且观察到两种离子都具有显著的猝灭效应。我们还研究了通过与 DNA 结合,生物碱如何免受外部 Co(2+)和 Br(-)猝灭剂的影响。与不存在 DNA 时的 K(SV)值相比,在化合物存在于 DNA 存在下孵育后,Co(2+)和 Br(-)对研究的生物碱的猝灭效应的 Stern-Volmer 常数(K(SV))显着降低(10-50%)。仅在存在 ds-DNA 的情况下,洛洛托宁的荧光各向异性值也增加,而在 ss-DNA 的情况下则没有。为了更好地表征这种相互作用的性质,进行了粘度测定和溴化乙锭置换研究。关于 DNA 参比溶液,含有 DNA 和洛洛托宁 A 衍生物的溶液的粘度降低或没有显着增加。还观察到,研究的化合物无法置换嵌入剂溴化乙锭。所有这些结果,以及获得的结合常数值(K(ass)= 2.2×10(2)-1.3×10(3)),都表明既没有产生洛洛托宁 A 衍生物/ds-DNA 的共价或嵌入相互作用,这导致结论是,这些生物碱通过小沟结合 ds-DNA。洛洛托宁 A 和衍生物的荧光行为的特定变化区分 ss-DNA 和 ds-DNA 结合,使我们提出这些化合物作为有吸引力的关闭探针来检测 DNA 杂交。
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