Urinary Extracellular Vesicles as a Readily Available Biomarker Source: A Simplified Stratification Method

Author:

Filipović Lidija1ORCID,Spasojević Savković Milica1ORCID,Prodanović Radivoje2ORCID,Matijašević Joković Suzana3,Stevanović Sanja4,Marco Ario de5ORCID,Kosanović Maja6,Brajušković Goran3ORCID,Popović Milica2

Affiliation:

1. Innovative Centre of the Faculty of Chemistry, 11158 Belgrade, Serbia

2. Faculty of Chemistry, University of Belgrade, 11158 Belgrade, Serbia

3. Faculty of Biology, University of Belgrade, 11158 Belgrade, Serbia

4. Center for Chemistry, Institute for Chemistry, Technology, and Metallurgy, National Institute of Republic of Serbia, 11000 Belgrade, Serbia

5. Laboratory for Environmental and Life Sciences, University of Nova Gorica, 5000 Nova Gorica, Slovenia

6. Institute for the Application of Nuclear Energy, INEP, University of Belgrade, 11080 Belgrade, Serbia

Abstract

Urine, a common source of biological markers in biomedical research and clinical diagnosis, has recently generated a new wave of interest. It has recently become a focus of study due to the presence of its content of extracellular vesicles (EVs). These uEVs have been found to reflect physiological and pathological conditions in kidney, urothelial, and prostate tissue and can illustrate further molecular processes, leading to a rapid expansion of research in this field In this work, we present the advantages of an immunoaffinity-based method for uEVs’ isolation with respect to the gold standard purification approach performed by differential ultracentrifugation [in terms of purity and antigen presence. The immunoaffinity method was made feasible by combining specific antibodies with a functionalized polymethacrylate polymer. Flow cytometry indicated a significant fluorescence shift, validating the presence of the markers (CD9, CD63, CD81) and confirming the effectiveness of the isolation method. Microscopy evaluations have shown that the morphology of the vesicles remained intact and corresponded to the expected shapes and dimensions of uEVs. The described protocol is inexpensive, fast, easy to process, has good reproducibility, and can be applied to further biological samples.

Funder

Science Fund of the Republic of Serbia

Publisher

MDPI AG

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