Enrichment of Astrocyte-Derived Extracellular Vesicles from Human Plasma

星形胶质细胞 细胞外小泡 纳米粒子跟踪分析 细胞生物学 微泡 胞外囊泡 细胞外 化学 生物 神经科学 生物化学 中枢神经系统 小RNA 基因
作者
Natalia Valle‐Tamayo,Rocío Pérez‐González,Gemma Chiva‐Blanch,Olivia Belbin,Sara Serrano‐Requena,Sònia Sirisi,Alba Cervantes González,Oriol Giró,Érika Sánchez‐Aced,Oriol Dols‐Icardo,Daniel Alcolea,María Carmona‐Iragui,Amanda Jiménez,Alberto Lleó,Juan Fortea,M. Florencia Iulita
出处
期刊:Journal of Visualized Experiments [MyJoVE Corporation]
卷期号: (186) 被引量:7
标识
DOI:10.3791/64107
摘要

Extracellular vesicles (EVs) are biological nanoparticles secreted by all cells for cellular communication and waste elimination. They participate in a vast range of functions by acting on and transferring their cargos to other cells in physiological and pathological conditions. Given their presence in biofluids, EVs represent an excellent resource for studying disease processes and can be considered a liquid biopsy for biomarker discovery. An attractive aspect of EV analysis is that they can be selected based on markers of their cell of origin, thus reflecting the environment of a specific tissue in their cargo. However, one of the major handicaps related to EV isolation methods is the lack of methodological consensuses and standardized protocols. Astrocytes are glial cells with essential roles in the brain. In neurodegenerative diseases, astrocyte reactivity may lead to altered EV cargo and aberrant cellular communication, facilitating/enhancing disease progression. Thus, analysis of astrocyte EVs may lead to the discovery of biomarkers and potential disease targets. This protocol describes a 2-step method of enrichment of astrocyte-derived EVs (ADEVs) from human plasma. First, EVs are enriched from defibrinated plasma via polymer-based precipitation. This is followed by enrichment of ADEVs through ACSA-1-based immunocapture with magnetic micro-beads, where resuspended EVs are loaded onto a column placed in a magnetic field. Magnetically labeled ACSA-1+ EVs are retained within the column, while other EVs flow through. Once the column is removed from the magnet, ADEVs are eluted and are ready for storage and analysis. To validate the enrichment of astrocyte markers, glial fibrillary acidic protein (GFAP), or other specific astrocytic markers of intracellular origin, can be measured in the eluate and compared with the flow-through. This protocol proposes an easy, time-efficient method to enrich ADEVs from plasma that can be used as a platform to examine astrocyte-relevant markers.
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