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通过纳米流式细胞术对单个细胞外囊泡跨膜蛋白进行表征

Single Extracellular Vesicle Transmembrane Protein Characterization by Nano-Flow Cytometry.

作者信息

Lees Rebecca, Tempest Robert, Law Alice, Aubert Dimitri, Davies Owen G, Williams Soraya, Peake Nick, Peacock Ben

机构信息

NanoFCM Co., Ltd.

School of Sport, Exercise and Health Sciences, Loughborough University.

出版信息

J Vis Exp. 2022 Jul 26(185). doi: 10.3791/64020.

DOI:10.3791/64020
PMID:35969098
Abstract

Single particle characterization has become increasingly relevant for research into extracellular vesicles, progressing from bulk analysis techniques and first-generation particle analysis to comprehensive multi-parameter measurements such as nano-flow cytometry (nFCM). nFCM is a form of flow cytometry that utilizes instrumentation specifically designed for nano-particle analysis, allowing for thousands of EVs to be characterized per minute both with and without the use of staining techniques. High resolution side scatter (SS) detection allows for size and concentration to be determined for all biological particles larger than 45 nm, while simultaneous fluorescence (FL) detection identifies the presence of labeled markers and targets of interest. Labeled subpopulations can then be described in quantitative units of particles/mL or as a percentage of the total particles identified by side scatter. Here, EVs derived from conditioned cell culture media (CCM) are labeled with both a lipid dye, to identify particles with a membrane, and antibodies specific for CD9, CD63, and CD81 as common EV markers. Measurements of comparison material, a concentration standard and a size standard of silica nanospheres, as well as labeled sample material are analyzed in a 1-minute analysis. The software is then used to measure the concentration and size distribution profile of all particles, independent of labeling, before determining the particles that are positive for each of the labels. Simultaneous SS and FL detection can be utilized flexibly with many different EV sources and labeling targets, both external and internal, describing EV samples in a comprehensive and quantitative manner.

摘要

单颗粒表征在细胞外囊泡研究中变得越来越重要,已从整体分析技术和第一代颗粒分析发展到诸如纳米流式细胞术(nFCM)等全面的多参数测量。nFCM是流式细胞术的一种形式,它利用专门为纳米颗粒分析设计的仪器,无论是否使用染色技术,每分钟都能对数千个细胞外囊泡进行表征。高分辨率侧向散射(SS)检测可确定所有大于45 nm的生物颗粒的大小和浓度,同时荧光(FL)检测可识别标记物和感兴趣靶标的存在。然后可以用颗粒数/毫升的定量单位或作为侧向散射识别的总颗粒的百分比来描述标记的亚群。在此,源自条件细胞培养基(CCM)的细胞外囊泡用脂质染料标记以识别有膜的颗粒,并用针对CD9、CD63和CD81的抗体作为常见的细胞外囊泡标记物。在1分钟的分析中对比较材料、二氧化硅纳米球的浓度标准和大小标准以及标记的样品材料进行测量。然后使用该软件测量所有颗粒的浓度和大小分布概况,而不考虑标记情况,然后确定每个标记呈阳性的颗粒。同时进行的SS和FL检测可灵活用于许多不同的细胞外囊泡来源以及外部和内部的标记靶标,以全面和定量的方式描述细胞外囊泡样品。

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