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首页> 外文期刊>Cytometry, Part A: the journal of the International Society for Analytical Cytology >Techniques to improve detection and analysis of extracellular vesicles using flow cytometry
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Techniques to improve detection and analysis of extracellular vesicles using flow cytometry

机译:利用流式细胞仪改善细胞外囊泡检测和分析的技术

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Extracellular vesicles (EVs) range in size from 50 nm to 1 mu m. Flow cytometry (FCM) is the most commonly used method for analyzing EVs; however, accurate characterization of EVs remains challenging due to their small size and lack of discrete positive populations. Here we report the use of optimization techniques that are especially well-suited for analyzing EVs from a high volume of clinical samples. Utilizing a two pronged approach that included 1) pre-filtration of antibodies to remove aggregates, followed by 2) detergent lysis of a replicate sample to account for remaining false positive events, we were able to effectively limit false positive non-EV events. In addition, we show that lysed samples are a useful alternative to isotypes for setting gates to exclude background fluorescence. To reduce background, we developed an approach using filters to wash samples post-staining thus providing a faster alternative to ultracentrifugation and sucrose gradient fractionation. In conclusion, use of these optimized techniques enhances the accuracy and efficiency of EV detection using FCM. (c) 2015 International Society for Advancement of Cytometry
机译:细胞外囊泡(EVs)的大小范围为50 nm至1μm。流式细胞仪(FCM)是最常用的分析电动汽车的方法。然而,由于电动汽车体积小且缺乏离散的阳性种群,因此准确鉴定电动汽车仍然具有挑战性。在这里,我们报告了最适合用于分析大量临床样品中电动汽车的优化技术的使用。利用两种方法,包括1)抗体的预过滤以去除聚集物,然后2)重复样品的去污剂裂解以解决剩余的假阳性事件,我们能够有效地限制假阳性的非EV事件。此外,我们显示裂解样品是同种型的有用替代品,可用于设置门以排除背景荧光。为了减少背景,我们开发了一种使用过滤器在染色后洗涤样品的方法,从而提供了超速离心和蔗糖梯度分级分离的更快选择。总之,使用这些优化技术可以提高使用FCM进行EV检测的准确性和效率。 (c)2015国际细胞计数学会

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