Combined thioflavin T–Congo red fluorescence assay for amyloid fibril detection

硫黄素 荧光 化学 刚果红 苯并噻唑 纤维 淀粉样蛋白(真菌学) 淀粉样变性 淀粉样疾病 吸光度 增色性 生物物理学 淀粉样纤维 生物化学 色谱法 淀粉样β DNA 病理 有机化学 生物 医学 无机化学 物理 疾病 量子力学 吸附 阿尔茨海默病
作者
Mykhailo Girych,Galyna Gorbenko,Ivan Maliyov,Valeriya Trusova,Chiharu Mizuguchi,Hiroyuki Saito,Paavo K.J. Kinnunen
出处
期刊:Methods and Applications in Fluorescence [IOP Publishing]
卷期号:4 (3): 034010-034010 被引量:52
标识
DOI:10.1088/2050-6120/4/3/034010
摘要

Fluorescence represents one of the most powerful tools for the detection and structural characterization of the pathogenic protein aggregates, amyloid fibrils. The traditional approaches to the identification and quantification of amyloid fibrils are based on monitoring the fluorescence changes of the benzothiazole dye thioflavin T (ThT) and absorbance changes of the azo dye Congo red (CR). In routine screening it is usually sufficient to perform only the ThT and CR assays, but both of them, when used separately, could give false results. Moreover, fibrillization kinetics can be measured only by ThT fluorescence, while the characteristic absorption spectra and birefringence of CR represent more rigid criteria for the presence of amyloid fibrils. Therefore, it seemed reasonable to use both these dyes simultaneously, combining the advantages of each technique. To this end, we undertook a detailed analysis of the fluorescence spectral behavior of these unique amyloid tracers upon their binding to amyloid fibrils from lysozyme, insulin and an N-terminal fragment of apolipoprotein A-I with Iowa mutation. The fluorescence measurements revealed several criteria for distinguishing between fibrillar and monomeric protein states: (i) a common drastic increase in ThT fluorescence intensity; (ii) a sharp decrease in ThT fluorescence upon addition of CR; (iii) an appearance of the maximum at 535-540 nm in the CR excitation spectra; (iv) increase in CR fluorescence intensity at 610 nm. Based on these findings we designed a novel combined ThT-CR fluorescence assay for amyloid identification. Such an approach not only strengthens the reliability of the ThT assay, but also provides new opportunities for structural characterization of amyloid fibrils.
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