Detection of the interactions of tumour derived extracellular vesicles with immune cells is dependent on EV-labelling methods

Luisa Loconte; Davinia Arguedas; Rojbin El; Alix Zhou; Anna Chipont; Lea Guyonnet; Coralie Guerin; Ester Piovesana; José Luis Vázquez-Ibar; Alain Joliot; Clotilde Théry; Lorena Martín-Jaular

doi:10.1002/jev2.12384

Detection of the interactions of tumour derived extracellular vesicles with immune cells is dependent on EV-labelling methods

J Extracell Vesicles. 2023 Dec;12(12):e12384. doi: 10.1002/jev2.12384.

Authors

Luisa Loconte^{1

2}, Davinia Arguedas¹, Rojbin El¹, Alix Zhou^{1

3}, Anna Chipont⁴, Lea Guyonnet⁴, Coralie Guerin^{3

4}, Ester Piovesana¹, José Luis Vázquez-Ibar⁵, Alain Joliot¹, Clotilde Théry^{1

3}, Lorena Martín-Jaular^{1

3}

Affiliations

¹ Institut Curie, PSL University, Inserm U932, Immunity and Cancer, Paris, France.
² Istituto Pasteur Italia-Fondazione Cenci Bolognetti, Department of Molecular Medicine, Sapienza' University of Rome, Rome, Italy.
³ Institut Curie centre de recherche, CurieCoretech Extracellular Vesicles, Paris, France.
⁴ Institut Curie centre de recherche, CurieCoretech Cytometry Platform, Paris, France.
⁵ Université Paris-Saclay, CEA, CNRS, Institute for Integrative Biology of the Cell (I2BC), Gif-sur-Yvette, France.

Abstract

Cell-cell communication within the complex tumour microenvironment is critical to cancer progression. Tumor-derived extracellular vesicles (TD-EVs) are key players in this process. They can interact with immune cells and modulate their activity, either suppressing or activating the immune system. Deciphering the interactions between TD-EVs and immune cells is essential to understand immune modulation by cancer cells. Fluorescent labelling of TD-EVs is a method of choice to study such interaction. This work aims to determine the impact of EV labelling methods on the detection by imaging flow cytometry and multicolour spectral flow cytometry of EV interaction and capture by the different immune cell types within human Peripheral Blood Mononuclear Cells (PBMCs). EVs released by the triple-negative breast carcinoma cell line MDA-MB-231 were labelled either with the lipophilic dye MemGlow-488 (MG-488), Carboxyfluorescein diacetate, succinimidyl ester (CFDA-SE) or through ectopic expression of a MyrPalm-superFolderGFP reporter (mp-sfGFP), which incorporates into EVs during their biogenesis. Our results show that these labelling strategies, although analysed with the same techniques, led to diverging results. While MG-488-labelled EVs incorporate in all cell types, CFSE-labelled EVs are restricted to a minor subset of cells and mp-sfGFP-labelled EVs are mainly detected in CD14+ monocytes which are the main uptakers of EVs and other particles, regardless of the labelling method. Furthermore, our results show that the method used for EV labelling influences the detection of the different types of EV interactions with the recipient cells. Specifically, MG-488, CFSE and mp-sfGFP result in observation suggesting, respectively, transient EV-PM interaction that results in dye transfer, EV content delivery, and capture of intact EVs. Consequently, the type of EV labelling method has to be considered as they can provide complementary information on various types of EV-cell interaction and EV fate.

Keywords: extracellular vesicles; immune cells; labelling; uptake.

Publication types

Research Support, Non-U.S. Gov't

MeSH terms

Cell Line
Extracellular Vesicles* / metabolism
Humans
Leukocytes, Mononuclear
Succinimides / metabolism

Substances

5-(6)-carboxyfluorescein diacetate succinimidyl ester
Succinimides

Grants and funding

UH3 CA241694/CA/NCI NIH HHS/United States