Large extracellular vesicles derived from human regulatory macrophages (L-EV(Mreg)) attenuate CD3/CD28-induced T-cell activation in vitro

ABSTRACT: Macrophages belong to the innate immune system, and we have recently shown that in vitro differentiated human regulatory macrophages (Mreg) release large extracellular vesicles (L-EV(Mreg)) with an average size of 7.5 μm which regulate wound healing and angiogenesis in vitro. The aim of th...

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Detalles Bibliográficos
Autores principales: Albrecht, Martin, Hummitzsch, Lars, Rusch, Rene, Eimer, Christine, Rusch, Melanie, Heß, Katharina, Steinfath, Markus, Cremer, Jochen, Fändrich, Fred, Berndt, Rouven, Zitta, Karina
Formato: Online Artículo Texto
Lenguaje:English
Publicado: Springer Berlin Heidelberg 2023
Materias:
Original Article
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC10663190/
https://www.ncbi.nlm.nih.gov/pubmed/37725101
http://dx.doi.org/10.1007/s00109-023-02374-9
Descripción
Sumario:ABSTRACT: Macrophages belong to the innate immune system, and we have recently shown that in vitro differentiated human regulatory macrophages (Mreg) release large extracellular vesicles (L-EV(Mreg)) with an average size of 7.5 μm which regulate wound healing and angiogenesis in vitro. The aim of this study was to investigate whether L-EV(Mreg) also affect the CD3/CD28-mediated activation of T-cells. Mreg were differentiated using blood monocytes and L-EV(Mreg) were isolated from culture supernatants by differential centrifugation. Activation of human T-cells was induced by CD3/CD28-coated beads in the absence or presence of Mreg or different concentrations of L-EV(Mreg). Inhibition of T-cell activation was quantified by flow cytometry and antibodies directed against the T-cell marker granzyme B. Phosphatidylserine (PS) exposure on the surface of Mreg and L-EV(Mreg) was analyzed by fluorescence microscopy. Incubation of human lymphocytes with CD3/CD28 beads resulted in an increase of cell size, cell granularity, and number of granzyme B–positive cells (P < 0.05) which is indicative of T-cell activation. The presence of Mreg (0.5 × 10(6) Mreg/ml) led to a reduction of T-cell activation (number of granzyme B–positive cells; P < 0.001), and a similar but less pronounced effect was also observed when incubating activated T-cells with L-EV(Mreg) (P < 0.05 for 3.2 × 10(6) L-EV(Mreg)/ml). A differential analysis of the effects of Mreg and L-EV(Mreg) on CD4(+) and CD8(+) T-cells showed an inhibition of CD4(+) T-cells by Mreg (P < 0.01) and L-EV(Mreg) (P < 0.05 for 1.6 × 10(6) L-EV(Mreg)/ml; P < 0.01 for 3.2 × 10(6) L-EV(Mreg)/ml). A moderate inhibition of CD8(+) T-cells was observed by Mreg (P < 0.05) and by L-EV(Mreg) (P < 0.01 for 1.6 × 10(6) L-EV(Mreg)/ml and 3.2 × 10(6) L-EV(Mreg)/ml). PS was restricted to confined regions of the Mreg surface, while L-EV(Mreg) showed strong signals for PS in the exoplasmic leaflet. L-EV(Mreg) attenuate CD3/CD28-mediated activation of CD4(+) and CD8(+) T-cells. L-EV(Mreg) may have clinical relevance, particularly in the treatment of diseases associated with increased T-cell activity. KEY MESSAGES: Mreg release large extracellular vesicles (L-EV(Mreg)) with an average size of 7.5 µm. L-EV(Mreg) exhibit phosphatidylserine positivity. L-EV(Mreg) suppress CD4(+) and CD8(+) T-cells. L-EV(Mreg) hold clinical potential in T-cell-related diseases.

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