Isolation and Enrichment of Extracellular Vesicles with Double‐Positive Membrane Protein for Subsequent Biological Studies

Author:

Liu Chunchen12,Lin Huixian12,Yu Haiyang12,Mai Xueying12,Pan Weilun12,Guo Jingyun3,Liao Tong12,Feng Junjie12,Zhang Ye12,Situ Bo12,Zheng Lei12ORCID,Li Bo12

Affiliation:

1. Department of Laboratory Medicine Nanfang Hospital Southern Medical University Guangzhou 510515 China

2. Guangdong Engineering and Technology Research Center for Rapid Diagnostic Biosensors Nanfang Hospital Southern Medical University Guangzhou 510515 China

3. Breast Center Department of General Surgery Nanfang Hospital Southern Medical University Guangzhou 510515 China

Abstract

AbstractThe isolation and enrichment of specific extracellular vesicle (EV) subpopulations are essential in the context of precision medicine. However, the current methods predominantly rely on a single‐positive marker and are susceptible to interference from soluble proteins or impurities. This limitation represents a significant obstacle to the widespread application of EVs in biological research. Herein, a novel approach that utilizes proximity ligation assay (PLA) and DNA–RNA hybridization are proposed to facilitate the binding of two proteins on the EV membrane in advance enabling the isolation and enrichment of intact EVs with double‐positive membrane proteins followed by using functionalized magnetic beads for capture and enzymatic cleavage for isolated EVs release. The isolated subpopulations of EVs can be further utilized for cellular uptake studies, high‐throughput small RNA sequencing, and breast cancer diagnosis. Hence, developing and implementing a specialized system for isolating and enriching a specific subpopulation of EVs can enhance basic and clinical research in this field.

Funder

National Science Fund for Distinguished Young Scholars

National Basic Research Program of China

National Natural Science Foundation of China

Publisher

Wiley

Subject

Pharmaceutical Science,Biomedical Engineering,Biomaterials

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