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首页> 外文期刊>Biomacromolecules >Unravelling the Binding Mechanism of a Poly(cationic) Anthracenyl Fluorescent Probe with High Affinity toward Double-Stranded DNA
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Unravelling the Binding Mechanism of a Poly(cationic) Anthracenyl Fluorescent Probe with High Affinity toward Double-Stranded DNA

机译:揭示对双链DNA具有高亲和力的聚(阳离子)蒽基荧光探针的结合机理

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We report the synthesis, spectroscopy, and the DNA binding properties of a biocompatible, water-soluble, polycationic two-photon absorbing anthracenyl derivative (Ant-PIm) specifically designed for biorelated applications. Detailed insights into the Ant-PIm-DNA binding interaction are provided by using several spectroscopic approaches,. including UV-vis absorption, circular dichroism (CD), Fourier-transform infrared spectroscopy (FTIR), steady-state, and time-resolved fluorescence techniques. Absorption and fluorescence quantitative data analysis show a strong Ant-PIm-duplex interaction with binding constants of K-f = 4.7 +/- 0.2 X 10(5)M(-1), 7.1 +/- 0.3 X 10(5) M-1, and 1.0 +/- 0.1 X 10(6)M(-1) at 298, 304, and 310 K, respectively. Spectral changes observed upon DNA binding provide evidence for a complex formation with off-on fluorescence pattern, which can be related to two consecutive binding equilibria. Results of DNA binders displacement and iodide quenching experimental assays unambiguously point to the groove binding mode of Ant-PIm to the DNA-helicate. Thermodynamic and chemical denaturation studies suggest that long-range interactions of hydrophobic nature regulate the association of Ant-PIm with the biopolymer. The ionic strength dependence of the binding constant shows that electrostatic component has an important contribution to the overall Gibbs free energy. FTIR and CD data provide evidence of partial modification of the B-DNA secondary structure, while the increase in the melting temperature clearly indicates the enhancement of the thermal stability of the duplex. Furthermore, the two-photon absorption cross section spectrum determined using the two photon excited fluorescence (TPEF) technique shows a strong 2PA maximum at 820 nm with a sigma(2) > 800 GM, which emphasizes the advantageous combination of biological and optical properties possessed by this positively charged bioprobe.
机译:我们报告了生物相容性,水溶性,聚阳离子双光子吸收蒽基衍生物(Ant-PIm)的生物相容性,光谱学和DNA结合特性,专为生物相关应用而设计。通过使用几种光谱方法,可以深入了解Ant-PIm-DNA结合相互作用。包括紫外可见吸收,圆二色性(CD),傅立叶变换红外光谱(FTIR),稳态和时间分辨荧光技术。吸收和荧光定量数据分析显示强大的Ant-PIm-双链体相互作用,结合常数Kf = 4.7 +/- 0.2 X 10(5)M(-1),7.1 +/- 0.3 X 10(5)M-1 ,分别在298、304和310 K时为1.0 +/- 0.1 X 10(6)M(-1)。 DNA结合后观察到的光谱变化提供了具有错开荧光模式的复合物形成的证据,这可能与两个连续的结合平衡有关。 DNA结合物置换和碘化物淬灭实验分析的结果明确指出了Ant-PIm与DNA-螺旋产物的沟结合模式。热力学和化学变性研究表明,疏水性的长程相互作用调节了Ant-PIm与生物聚合物的缔合。结合常数对离子强度的依赖性表明,静电成分对总的吉布斯自由能有重要贡献。 FTIR和CD数据提供了B-DNA二级结构部分修饰的证据,而熔融温度的升高清楚地表明了双链体的热稳定性增强。此外,使用双光子激发荧光(TPEF)技术测定的双光子吸收截面光谱显示出在820 nm处的最大2PA最大值,且sigma(2)> 800 GM,这强调了所拥有的生物学和光学性质的有利组合通过这种带正电的生物探针。

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