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Drug-tubulin interactions interrogated by transient absorption spectroscopy

机译:瞬态吸收光谱法研究药物与微管蛋白的相互作用

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Colchicine (COL) is a bioactive molecule with antitumor properties. When COL binds to tubulin (TU), it inhibits microtubule assembly dynamics. We have investigated COL-TU interactions using laser flash photolysis (LFP) technique and performing fully flexible molecular dynamics simulations. Excitation of COL at 355 nm in aqueous medium did not lead to any transient absorption spectrum. By contrast, in the presence of TU a transient peaking at lambda(max) ca. 420 nm was registered and assigned as triplet excited COL complexed with TU ((COL)-C-3*@TU). In aerated medium, the lifetime was tau ca. 160 mu s and the quantum yield was 0.138. Likewise, when the bicyclic COL analog MTC was submitted to LFP in the presence of TU, (MTC)-M-3@TU* was detected with a lifetime of ca. 62 ms and a quantum yield of 0.296, Aqueous solutions of MTC did not produce any signal in the microsecond timescale. The triplet energy of MTC was obtained by means of emission measurements and found to be ca. 200 kJ mol(-1), a value that matches with that previously reported for COL (188 kJ mol(-1)). Molecular dynamic simulations, both with the ground and triplet excited state, reveal a strong interaction between COL and TU to give stabilized complexes with restricted mobility inside the protein binding site. These results demonstrate that LFP is a useful methodology to study the binding of COL derivatives to TU and open a new way to evaluate the interactions of non-fluorescent anticancer drugs with this protein.
机译:秋水仙碱(COL)是一种具有抗肿瘤特性的生物活性分子。当COL结合微管蛋白(TU)时,它会抑制微管组装动力学。我们已经研究了使用激光闪光光解(LFP)技术并执行完全灵活的分子动力学模拟的COL-TU相互作用。在水性介质中在355 nm处激发COL不会导致任何瞬态吸收光谱。相比之下,在TU的存在下,在lambda(max)ca处出现一个瞬时峰值。记录420 nm,并指定为与TU((COL)-C-3 * @ TU)络合的三重激发COL。在充气介质中,寿命约为tauca。 160μs,量子产率为0.138。同样,当在TU存在的情况下将双环COL类似物MTC提交给LFP时,检测到(MTC)-M-3 @ TU *的寿命约为。 62毫秒,量子产率为0.296,MTC水溶液在微秒时间范围内未产生任何信号。通过发射测量获得了MTC的三重态能量,大约为。 200 kJ mol(-1),该值与先前报告的COL(188 kJ mol(-1))相匹配。具有基态和三线态激发态的分子动力学模拟显示,COL和TU之间有很强的相互作用,从而在蛋白质结合位点内提供了受限制的迁移率的稳定复合物。这些结果表明,LFP是研究COL衍生物与TU结合的有用方法,并为评估非荧光抗癌药与该蛋白的相互作用开辟了新途径。

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