Evaluation of immune and chemical precipitation methods for plasma exosome isolation

Tatiana Shtam,Anastasia Malek,Maria Slyusarenko,Roman Kamyshinsky,Vladimir Burdakov,Luiza Garaeva,Nikolay Verlov,Roman Samsonov,Nadezhda Nikiforova,Vladimir Evtushenko,Yana Zabrodskaya,Lidia Zabegina,Andrey Konevega,Girijesh Kumar Patel

doi:10.1371/journal.pone.0242732

Abstract

Exosomes are a type of extracellular vesicles (EVs) secreted by multiple mammalian cell types and involved in intercellular communication. Numerous studies have explored the diagnostic and therapeutic potential of exosomes. The key challenge is the lack of efficient and standard techniques for isolation and downstream analysis of nanovesicles. Conventional isolation methods, such as ultracentrifugation, precipitation, filtration, chromatography, and immune-affinity-based approaches, rely on specific physical properties or on surface biomarkers. However, any of the existing methods has its limitations. Various parameters, such as efficacy, specificity, labor input, cost and scalability, and standardization options, must be considered for the correct choice of appropriate approach. The isolation of exosomes from biological fluids is especially challenged by the complex nature and variability of these liquids. Here, we present a comparison of five protocols for exosome isolation from human plasma: two chemical affinity precipitation methods (lectin-based purification and SubX™ technology), immunoaffinity precipitation, and reference ultracentrifugation-based exosome isolation method in two modifications. An approach for the isolation of exosomes based on the phenomenon of binding and aggregation of these particles via clusters of outer membrane phosphate groups in the presence of SubX™ molecules has been put forward in the present study. The isolated EVs were characterized based upon size, quantity, and protein content.

Highlights

Extracellular vesicles (EVs) are nanoscale size bubble-like membranous structures secreted by most cell types and present in blood, urine, saliva, breast milk and cerebrospinal fluid [1]
An approach to isolating extracellular vesicles (EVs) based on the phenomenon of binding and aggregation of these particles via clusters of outer membrane phosphate groups in the presence of SubXTM reagent (Capital Biosciences, USA) has been put forward in the present study
Since vesicular membrane phospholipids contain multiple phosphate groups, this can lead to the formation of [SubX+EVs] aggregates

Summary

Introduction

Extracellular vesicles (EVs) are nanoscale size bubble-like membranous structures secreted by most cell types and present in blood, urine, saliva, breast milk and cerebrospinal fluid [1]. There are several categories of EVs: apoptotic bodies (500–1000 nm), which are released from cells undergoing apoptosis, microvesicles (100–350 nm), which are released by evagination of the plasma membrane, and exosomes (40–150 nm) [3]. Growing data suggests that exosomes are involved in facilitating oncogenesis by regulating angiogenesis, immunity, and metastasis [7,8,9]. This provides a growing demand for simple, efficient, and affordable techniques to isolate exosomes. The isolation of exosomes with reliable quality and substantial concentration is still a major challenge

Methods

Results

Discussion

Conclusion