A Comparative Study of High-Contrast Fluorescence Lifetime Probes for Imaging Amyloid in Tissue

硫黄素 荧光 淀粉样蛋白(真菌学) 生物物理学 化学 荧光寿命成像显微镜 吖啶酮 病理 立体化学 阿尔茨海默病 生物 光学 医学 物理 无机化学 疾病
作者
Felix Gorka,Sam Daly,Colin M. Pearson,Edita Bulovaite,Yu P. Zhang,Anoushka Handa,Seth G. N. Grant,Thomas N. Snaddon,Lisa-Maria Needham,Steven F. Lee
出处
期刊:Journal of Physical Chemistry B [American Chemical Society]
卷期号:125 (50): 13710-13717 被引量:4
标识
DOI:10.1021/acs.jpcb.1c07762
摘要

Optical imaging of protein aggregates in living and post-mortem tissue can often be impeded by unwanted fluorescence, prompting the need for novel methods to extract meaningful signal in complex biological environments. Historically, benzothiazolium derivatives, prominently Thioflavin T, have been the state-of-the-art fluorescent probes for amyloid aggregates, but their optical, structural, and binding properties typically limit them to in vitro applications. This study compares the use of novel uncharged derivative, PAP_1, with parent Thioflavin T as a fluorescence lifetime imaging probe. This is applied specifically to imaging recombinant α-synuclein aggregates doped into brain tissue. Despite the 100-fold lower brightness of PAP_1 compared to that of Thioflavin T, PAP_1 binds to α-synuclein aggregates with an affinity several orders of magnitude greater than Thioflavin T; thus, we observe a specific decrease in the fluorescence lifetime of PAP_1 bound to α-synuclein aggregates, resulting in a separation of >1.4 standard deviations between PAP_1-stained brain tissue background and α-synuclein aggregates that is not observed with Thioflavin T. This enables contrast between highly fluorescent background tissue and amyloid fibrils that is attributed to the greater affinity of PAP_1 for α-synuclein aggregates, avoiding the substantial off-target staining observed with Thioflavin T.
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