Tailoring the Amphiphilicity of Fluorescent Protein Chromophores to Detect Intracellular Proteome Aggregation in Diverse Biological Samples

化学 蛋白质组 硫黄素 蛋白质聚集 细胞内 荧光 生物化学 发色团 绿色荧光蛋白 人类蛋白质组计划 生物物理学 蛋白质折叠 细胞外 蛋白质组学 生物 物理 基因 病理 有机化学 医学 量子力学 阿尔茨海默病 疾病
作者
Mengdie Wang,Zhenduo Zhang,Biao Jing,Xuepeng Dong,Kun Guo,Jintai Deng,Zhiming Wang,Wang Wan,Wenhan Jin,Zhenming Gao,Yu Liu
出处
期刊:Analytical Chemistry [American Chemical Society]
卷期号:95 (31): 11751-11760 被引量:3
标识
DOI:10.1021/acs.analchem.3c01903
摘要

The formation of amorphous misfolded and aggregated proteins is a hallmark of proteome stress in diseased cells. Given its lack of defined targeting sites, the rational design of intracellular proteome aggregation sensors has been challenging. Herein, we modulate the amphiphilicity of fluorescent protein chromophores to enable selective detection of aggregated proteins in different biological samples, including recombinant proteins, stressed live cells, intoxicated mouse liver tissue, and human hepatocellular carcinoma tissue. By tuning the number of hydroxyl groups, we optimize the selectivity of fluorescent protein chromophores toward aggregated proteins in these biological samples. In recombinant protein applications, the most hydrophobic P0 (cLogP = 5.28) offers the highest fold change (FC = 31.6), sensitivity (LLOD = 0.1 μM), and brightness (Φ = 0.20) upon binding to aggregated proteins. In contrast, P4 of balanced amphiphilicity (cLogP = 2.32) is required for selective detection of proteome stresses in live cells. In mouse and human liver histology tissues, hydrophobic P1 exhibits the best performance in staining the aggregated proteome. Overall, the amphiphilicity of fluorescent chromophores governs the sensor's performance by matching the diverse nature of different biological samples. Together with common extracellular amyloid sensors (e.g., Thioflavin T), these sensors developed herein for intracellular amorphous aggregation complement the toolbox to study protein aggregation.
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