Multimode chromatography-based techniques for high purity isolation of extracellular vesicles from human blood plasma

Alan J. Zimmerman, Getulio Pereira de Oliveira Jr., Xianyi Su, Jacqueline Wood, Zhengxin Fu, Brandy Pinckney, John Tigges, Ionita Ghiran, Alexander R. Ivanov
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Abstract

Extracellular vesicles (EVs) play a pivotal role in various biological pathways, such as immune responses and the progression of diseases, including cancer. However, it is challenging to isolate EVs at high purity from blood plasma and other biofluids due to their low abundance compared to more predominant biomolecular species such as lipoprotein particles and free protein complexes. Ultracentrifugation-based EV isolation, the current gold standard technique, cannot overcome this challenge due to the similar biophysical characteristics of such species. We developed several novel approaches to enrich EVs from plasma while depleting contaminating molecular species using multimode chromatography-based strategies. On average, we identified 716 ± 68 and 1054 ± 35 protein groups in EV isolates from 100 µL of plasma using multimode chromatography- and ultracentrifugation-based techniques, respectively. The developed methods resulted in similar EV isolates purity, providing significant advantages in simplicity, throughput, scalability, and applicability for various downstream analytical and potential clinical applications.

Abstract Image

从人血浆中高纯度分离细胞外囊泡的多模式色谱技术
细胞外囊泡(EVs)在免疫反应和疾病(包括癌症)进展等各种生物通路中发挥着关键作用。然而,与脂蛋白颗粒和游离蛋白复合物等更主要的生物分子物种相比,EVs的丰度较低,因此从血浆和其他生物流体中分离出高纯度的EVs具有挑战性。基于超速离心的 EV 分离是目前的黄金标准技术,但由于这些物种具有相似的生物物理特征,因此无法克服这一挑战。我们开发了几种新方法,利用基于多模式色谱的策略从血浆中富集EV,同时清除污染的分子物种。使用基于多模式色谱和超速离心的技术,我们从 100 µL 血浆中分离出的 EV 平均分别鉴定出 716 ± 68 和 1054 ± 35 个蛋白质组。所开发的方法可获得相似的 EV 分离物纯度,在简便性、通量、可扩展性和适用性方面具有显著优势,可用于各种下游分析和潜在的临床应用。
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