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用于快速分离和按大小特异性富集合成囊泡和细胞外囊泡亚群的光敏纳米探针。

Photosensitive Nanoprobes for Rapid Isolation and Size-Specific Enrichment of Synthetic and Extracellular Vesicle Subpopulations.

作者信息

Weerakkody Jonathan S, Tseng Tiffany, Topper Mackenzie, Thoduvayil Sikha, Radhakrishnan Abhijith, Pincet Frederic, Kyriakides Themis R, Gunasekara Roshan W, Ramakrishnan Sathish

机构信息

Yale Nanobiology Institute, West Haven, CT 06516, USA.

Department of Pathology, Yale University School of Medicine, New Haven, CT 06510, USA.

出版信息

Adv Funct Mater. 2024 Aug 22;34(34). doi: 10.1002/adfm.202400390. Epub 2024 Mar 29.

DOI:10.1002/adfm.202400390
PMID:39372670
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC11452007/
Abstract

The biggest challenge in current isolation methods for lipid bilayer-encapsulated vesicles, such as exosomes, secretory, and synthetic vesicles, lies in the absence of a unified approach that seamlessly delivers high purity, yield, and scalability for large-scale applications. To address this gap, we have developed an innovative method that utilizes photosensitive lipid nanoprobes specifically designed for efficient isolation of vesicles and sorting them into subpopulations based on size. The photosensitive component in the probe undergoes cleavage upon exposure to light, facilitating the release of vesicles in their near-native form. We demonstrate that our method provides superior capability in isolating extracellular vesicles from complex biological media and separating them into size-based subpopulations within 1 hour, achieving more efficiency and purity than ultracentrifugation. Furthermore, this method's cost-effectiveness and rapid enrichment of the vesicles align with demands for large-scale isolation and downstream analyses of nucleic acids and proteins. Our method opens new avenues in exploring, analyzing, and utilizing synthetic and extracellular vesicle subpopulations in various biomedical applications, including diagnostics, therapeutic delivery, and biomarker discovery.

摘要

目前用于脂质双层包裹囊泡(如外泌体、分泌性囊泡和合成囊泡)的分离方法面临的最大挑战在于缺乏一种统一的方法,无法为大规模应用无缝提供高纯度、高产量和可扩展性。为了弥补这一差距,我们开发了一种创新方法,该方法利用专门设计的光敏脂质纳米探针来高效分离囊泡,并根据大小将它们分类为亚群。探针中的光敏成分在光照下会发生裂解,便于以接近天然的形式释放囊泡。我们证明,我们的方法在从复杂生物介质中分离细胞外囊泡并在1小时内将它们分离成基于大小的亚群方面具有卓越能力,比超速离心更高效、更纯净。此外,该方法的成本效益以及对囊泡的快速富集符合大规模分离以及核酸和蛋白质下游分析的要求。我们的方法为探索、分析和利用各种生物医学应用(包括诊断、治疗递送和生物标志物发现)中的合成囊泡和细胞外囊泡亚群开辟了新途径。