Simplified protocol for flow cytometry analysis of fluorescently labeled exosomes and microvesicles using dedicated flow cytometer

Flow cytometry is a powerful method, which is widely used for high-throughput quantitative and qualitative analysis of cells. However, its straightforward applicability for extracellular vesicles (EVs) and mainly exosomes is hampered by several challenges, reflecting mostly the small size of these v...

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Autores principales: Pospichalova, Vendula, Svoboda, Jan, Dave, Zankruti, Kotrbova, Anna, Kaiser, Karol, Klemova, Dobromila, Ilkovics, Ladislav, Hampl, Ales, Crha, Igor, Jandakova, Eva, Minar, Lubos, Weinberger, Vit, Bryja, Vitezslav
Formato: Online Artículo Texto
Lenguaje:English
Publicado: Co-Action Publishing 2015
Materias:
Technical Report
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC4382613/
https://www.ncbi.nlm.nih.gov/pubmed/25833224
http://dx.doi.org/10.3402/jev.v4.25530
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author Pospichalova, Vendula
Svoboda, Jan
Dave, Zankruti
Kotrbova, Anna
Kaiser, Karol
Klemova, Dobromila
Ilkovics, Ladislav
Hampl, Ales
Crha, Igor
Jandakova, Eva
Minar, Lubos
Weinberger, Vit
Bryja, Vitezslav
author_facet Pospichalova, Vendula
Svoboda, Jan
Dave, Zankruti
Kotrbova, Anna
Kaiser, Karol
Klemova, Dobromila
Ilkovics, Ladislav
Hampl, Ales
Crha, Igor
Jandakova, Eva
Minar, Lubos
Weinberger, Vit
Bryja, Vitezslav
author_sort Pospichalova, Vendula
collection PubMed
description Flow cytometry is a powerful method, which is widely used for high-throughput quantitative and qualitative analysis of cells. However, its straightforward applicability for extracellular vesicles (EVs) and mainly exosomes is hampered by several challenges, reflecting mostly the small size of these vesicles (exosomes: ~80–200 nm, microvesicles: ~200–1,000 nm), their polydispersity, and low refractive index. The current best and most widely used protocol for beads-free flow cytometry of exosomes uses ultracentrifugation (UC) coupled with floatation in sucrose gradient for their isolation, labeling with lipophilic dye PKH67 and antibodies, and an optimized version of commercial high-end cytometer for analysis. However, this approach requires an experienced flow cytometer operator capable of manual hardware adjustments and calibration of the cytometer. Here, we provide a novel and fast approach for quantification and characterization of both exosomes and microvesicles isolated from cell culture media as well as from more complex human samples (ascites of ovarian cancer patients) suitable for multiuser labs by using a flow cytometer especially designed for small particles, which can be used without adjustments prior to data acquisition. EVs can be fluorescently labeled with protein-(Carboxyfluoresceinsuccinimidyl ester, CFSE) and/or lipid- (FM) specific dyes, without the necessity of removing the unbound fluorescent dye by UC, which further facilitates and speeds up the characterization of microvesicles and exosomes using flow cytometry. In addition, double labeling with protein- and lipid-specific dyes enables separation of EVs from common contaminants of EV preparations, such as protein aggregates or micelles formed by unbound lipophilic styryl dyes, thus not leading to overestimation of EV numbers. Moreover, our protocol is compatible with antibody labeling using fluorescently conjugated primary antibodies. The presented methodology opens the possibility for routine quantification and characterization of EVs from various sources. Finally, it has the potential to bring a desired level of control into routine experiments and non-specialized labs, thanks to its simple bead-based standardization.
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spelling pubmed-43826132015-04-08 Simplified protocol for flow cytometry analysis of fluorescently labeled exosomes and microvesicles using dedicated flow cytometer Pospichalova, Vendula Svoboda, Jan Dave, Zankruti Kotrbova, Anna Kaiser, Karol Klemova, Dobromila Ilkovics, Ladislav Hampl, Ales Crha, Igor Jandakova, Eva Minar, Lubos Weinberger, Vit Bryja, Vitezslav J Extracell Vesicles Technical Report Flow cytometry is a powerful method, which is widely used for high-throughput quantitative and qualitative analysis of cells. However, its straightforward applicability for extracellular vesicles (EVs) and mainly exosomes is hampered by several challenges, reflecting mostly the small size of these vesicles (exosomes: ~80–200 nm, microvesicles: ~200–1,000 nm), their polydispersity, and low refractive index. The current best and most widely used protocol for beads-free flow cytometry of exosomes uses ultracentrifugation (UC) coupled with floatation in sucrose gradient for their isolation, labeling with lipophilic dye PKH67 and antibodies, and an optimized version of commercial high-end cytometer for analysis. However, this approach requires an experienced flow cytometer operator capable of manual hardware adjustments and calibration of the cytometer. Here, we provide a novel and fast approach for quantification and characterization of both exosomes and microvesicles isolated from cell culture media as well as from more complex human samples (ascites of ovarian cancer patients) suitable for multiuser labs by using a flow cytometer especially designed for small particles, which can be used without adjustments prior to data acquisition. EVs can be fluorescently labeled with protein-(Carboxyfluoresceinsuccinimidyl ester, CFSE) and/or lipid- (FM) specific dyes, without the necessity of removing the unbound fluorescent dye by UC, which further facilitates and speeds up the characterization of microvesicles and exosomes using flow cytometry. In addition, double labeling with protein- and lipid-specific dyes enables separation of EVs from common contaminants of EV preparations, such as protein aggregates or micelles formed by unbound lipophilic styryl dyes, thus not leading to overestimation of EV numbers. Moreover, our protocol is compatible with antibody labeling using fluorescently conjugated primary antibodies. The presented methodology opens the possibility for routine quantification and characterization of EVs from various sources. Finally, it has the potential to bring a desired level of control into routine experiments and non-specialized labs, thanks to its simple bead-based standardization. Co-Action Publishing 2015-03-31 /pmc/articles/PMC4382613/ /pubmed/25833224 http://dx.doi.org/10.3402/jev.v4.25530 Text en © 2015 Vendula Pospichalova et al. http://creativecommons.org/licenses/by-nc/4.0/ This is an Open Access article distributed under the terms of the Creative Commons Attribution-NonCommercial 4.0 International License, permitting all non-commercial use, distribution, and reproduction in any medium, provided the original work is properly cited.
spellingShingle Technical Report
Pospichalova, Vendula
Svoboda, Jan
Dave, Zankruti
Kotrbova, Anna
Kaiser, Karol
Klemova, Dobromila
Ilkovics, Ladislav
Hampl, Ales
Crha, Igor
Jandakova, Eva
Minar, Lubos
Weinberger, Vit
Bryja, Vitezslav
Simplified protocol for flow cytometry analysis of fluorescently labeled exosomes and microvesicles using dedicated flow cytometer
title Simplified protocol for flow cytometry analysis of fluorescently labeled exosomes and microvesicles using dedicated flow cytometer
title_full Simplified protocol for flow cytometry analysis of fluorescently labeled exosomes and microvesicles using dedicated flow cytometer
title_fullStr Simplified protocol for flow cytometry analysis of fluorescently labeled exosomes and microvesicles using dedicated flow cytometer
title_full_unstemmed Simplified protocol for flow cytometry analysis of fluorescently labeled exosomes and microvesicles using dedicated flow cytometer
title_short Simplified protocol for flow cytometry analysis of fluorescently labeled exosomes and microvesicles using dedicated flow cytometer
title_sort simplified protocol for flow cytometry analysis of fluorescently labeled exosomes and microvesicles using dedicated flow cytometer
topic Technical Report
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC4382613/
https://www.ncbi.nlm.nih.gov/pubmed/25833224
http://dx.doi.org/10.3402/jev.v4.25530
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