Flow cytometric analysis of extracellular vesicle subsets in plasma: impact of swarm by particles of non‐interest |
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| Authors: | S. F. W. M. Libregts G. J. A. Arkesteijn A. Németh E. N. M. Nolte‐’t Hoen M. H. M. Wauben |
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| Affiliation: | 1. Department of Biochemistry & Cell Biology, Faculty of Veterinary Medicine, Utrecht University, Utrecht, the Netherlands;2. Department of Genetics, Cell‐ and Immunobiology, Faculty of Medicine, Semmelweis University, Budapest, Hungary |
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| Abstract: | ![]()
Essentials - Extracellular vesicles (EVs) in biological fluids are promising biomarkers for disease.
- Fluorescence‐based flow cytometric analysis is suitable to detect low abundant EV subsets.
- Particles of non‐interest can induce false‐positive light scatter and fluorescent signals.
- Interference of particles of non‐interest can be monitored by analyzing serial dilutions.
Summary Background Extracellular vesicles (EVs) in plasma are increasingly being recognized as potential biomarkers. EV analysis for diagnostic purposes should be robust and should allow analysis of EV subsets with a wide range of abundance and in a large number of patient samples. Flow cytometry offers possibilities to meet these criteria, as it allows multiparameter analysis of individual EVs. However, analysis of plasma EVs is challenging, because of their size and heterogeneity, and the presence of other submicrometer‐sized particles in plasma that could interfere with EV analysis. Objectives To explore whether fluorescence‐based flow cytometric analysis of EV subsets is suitable when the EVs of interest are present in low abundance in a background of non‐labeled or differently labeled EVs and particles. Methods Fluorescently labeled EVs of interest were spiked at different ratios in full plasma, purified plasma components, or (non‐)fluorescent polystyrene beads, and subsequently analyzed by flow cytometry with fluorescence threshold triggering. Results We found that light scatter detection of low‐abundance or rare EV subsets during fluorescence threshold triggering was severely affected by particles of non‐interest, owing to coincidence and swarming. Importantly, we show that interfering particles labeled with different fluorophores induced false‐positive fluorescent signals on the particles of interest. These unwanted effects could only be discerned and controlled by performing serial dilutions and analyzing light scatter and fluorescence parameters. Conclusions We demonstrate how particles of non‐interest in plasma can impact on the light scatter and fluorescence detection of low‐abundance EVs of interest during fluorescence‐based flow cytometric analysis, and provide a means to prevent erroneous data interpretation. |
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| Keywords: | biomarkers cell‐derived microparticles exosomes extracellular vesicles flow cytometry |
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