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用于组织中淀粉样蛋白成像的高对比度荧光寿命探针的比较研究。

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

机构信息

Yusuf Hamied Department of Chemistry, University of Cambridge, Cambridge CB2 1EW, U.K.

Department of Physics, Philipps-University Marburg, Marburg 35032, Germany.

出版信息

J Phys Chem B. 2021 Dec 23;125(50):13710-13717. doi: 10.1021/acs.jpcb.1c07762. Epub 2021 Dec 9.

Abstract

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 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.

摘要

活组织和尸检组织中蛋白质聚集体的光学成像通常会受到不想要的荧光的阻碍,这促使人们需要新的方法来从复杂的生物环境中提取有意义的信号。从历史上看,苯并噻唑盐衍生物,特别是噻唑黄素 T,一直是淀粉样蛋白聚集体的最先进的荧光探针,但它们的光学、结构和结合特性通常将其应用限制在某些方面。本研究比较了新型非荷正电衍生物 PAP_1 与母体噻唑黄素 T 作为荧光寿命成像探针的用途。这特别应用于对掺杂在脑组织中的重组α-突触核蛋白聚集体进行成像。尽管 PAP_1 的亮度比噻唑黄素 T 低 100 倍,但 PAP_1 与α-突触核蛋白聚集体的结合亲和力要高出几个数量级;因此,我们观察到与 PAP_1 结合的α-突触核蛋白聚集体的荧光寿命特异性降低,导致 PAP_1 染色的脑组织背景与α-突触核蛋白聚集体之间的分离超过 1.4 个标准差,而噻唑黄素 T 则观察不到这种分离。这使得高度荧光背景组织与淀粉样纤维之间产生了对比,这归因于 PAP_1 与α-突触核蛋白聚集体的亲和力更强,从而避免了噻唑黄素 T 观察到的大量非靶标染色。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/8f5e/7615715/42abf3e0e7fb/EMS194355-f001.jpg

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