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Interaction of novel benzanthrone derivative with amyloid lysozyme

机译:新型苯并蒽醌衍生物与淀粉样溶菌酶的相互作用

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摘要

A novel benzanthrone derivative AM18 was investigated with respect to its photophysical properties when bound to native, oligomeric and fibrillar hen egg white lysozyme. As shown by fluorimetric titration AM18 is more sensitive to pathogenic protein aggregates than Thioflavin T, however has no ability to differentiate between mature and immature lysozyme fibrils. The recovered affinity and fluorescence response of the novel probe to amyloid protein appeared to be similar to those of recently developed amyloid lysozyme-sensitive dyes like e. g. Nile Red and cyanine dye 7515. Despite the high increase of the probe emission in the presence of amyloid lysozyme compared to its fluorescence in buffer, the minimal amount that could be detected by 1 μM AM18 was 10 times lower for amyloid-native protein solutions due to high affinity of the dye for lysozyme monomers. In general, because of high quantum yields and “signal-to-noise” ratios in the presence of pathogenic protein aggregates AM18 appeared to be an effective tool for amyloid detection and characterization in vitro, being however unable to detect pathogenic protein aggregates in vivo like e.g. recently reported p-FTAA because of the sensitivity to lipids. Compared to previously reported AM3 a novel dye showed 2-fold lower “signal-to- noise” ratio in the presence of fibrillar lysozyme, and 2 fold lower blue shift of emission maximum. This tendency was explained in terms of decreased charge transfer from the donor to acceptor groupes of AM18 compared to AM3. Finally, as concluded from the comparison of AM18 and previously studied benzanthrone derivatives, the 5 nm – red edge excitation shift of AM18 is indicative of its possible binding to fibril “deep cavities”, containing no water. High anisotropy values of amyloid-bound dye led us to conclusion that the enhanced fluorescence of the probe is associated with the decrease of the rotational motion of the amino-substitute about the benzanthrone unit. This is a sign of AM18 behaviour as a molecular rotor.
机译:研究了新型苯并蒽醌衍生物AM18与天然,寡聚和原纤维鸡蛋清溶菌酶结合后的光物理性质。如荧光滴定所示,AM18比硫黄素T对致病性蛋白质聚集体更敏感,但是没有能力区分成熟和未成熟的溶菌酶原纤维。新型探针对淀粉样蛋白的亲和力和荧光响应的恢复似乎与最近开发的淀粉样溶菌酶敏感染料(如e。)相似。 G。 Nile Red和花青染料7515。尽管与在缓冲液中的荧光相比,在存在淀粉样蛋白溶菌酶的情况下探针发射增加了很多,但对于淀粉样蛋白天然蛋白溶液,通过1μMAM18可以检测到的最小量要低10倍染料对溶菌酶单体的高亲和力。通常,由于在致病蛋白聚集体的存在下高量子产率和“信噪比”,AM18似乎是体外淀粉样蛋白检测和表征的有效工具,但是无法像在体内那样检测致病蛋白聚集体例如最近由于对脂质的敏感性而报道了p-FTAA。与以前报道的AM3相比,新型染料在原纤溶菌酶的存在下显示出低2倍的“信噪比”和最大发射蓝移低2倍。这种趋势的解释是,与AM3相比,从AM18的供体到受体的电荷转移减少。最后,从对AM18和以前研究过的苯并蒽酮衍生物的比较得出的结论是,AM18在5 nm-红边的激发位移表明它可能与不含水的原纤维“深腔”结合。淀粉样蛋白结合染料的高各向异性值使我们得出结论,即探针荧光增强与氨基取代基绕苯并蒽酮单元旋转运动的降低有关。这是AM18作为分子转子的行为的标志。

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