Extracellular vesicles from seminal plasma interact with T cells in vitro and drive their differentiation into regulatory T‐cells-Reference-Cited by-同舟云学术

Extracellular vesicles from seminal plasma interact with T cells in vitro and drive their differentiation into regulatory T‐cells

Published:2024-07 Issue:7 Volume:13 Page:
ISSN:2001-3078
Container-title:Journal of Extracellular Vesicles
language:en
Short-container-title:J of Extracellular Vesicle

Author:

Zhang Xiaogang¹^ORCID,Greve Patrick F.²,Minh Thi Tran Ngoc¹³,Wubbolts Richard¹,Demir Ayşe Y.⁴,Zaal Esther A.¹³,Berkers Celia R.¹³,Boes Marianne²,Stoorvogel Willem¹^ORCID

Affiliation:

1. Department of Biomolecular Health Sciences Faculty of Veterinary Science Utrecht University Utrecht The Netherlands

2. Department of Pediatrics and Center for Translational Immunology University Medical Center Utrecht Utrecht University Utrecht The Netherlands

3. Biomolecular Mass Spectrometry and Proteomics, Bijvoet Center for Biomolecular Research and Utrecht Institute of Pharmaceutical Sciences Utrecht University Utrecht The Netherlands

4. Department of Clinical Chemistry and Hematology Meander Medical Centre Amersfoort The Netherlands

Abstract

AbstractSeminal plasma induces immune tolerance towards paternal allogenic antigens within the female reproductive tract and during foetal development. Recent evidence suggests a role for extracellular vesicles in seminal plasma (spEVs). We isolated spEVs from seminal plasma that was donated by vasectomized men, thereby excluding any contributions from the testis or epididymis. Previous analysis demonstrated that such isolated spEVs originate mainly from the prostate. Here we observed that when isolated fluorescently labelled spEVs were mixed with peripheral blood mononuclear cells, they were endocytosed predominantly by monocytes, and to a lesser extent also by T‐cells. In a mixed lymphocyte reaction, T‐cell proliferation was inhibited by spEVs. A direct effect of spEVs on T‐cells was demonstrated when isolated T cells were activated by anti‐CD3/CD28 coated beads. Again, spEVs interfered with T cell proliferation, as well as with the expression of CD25 and the release of IFN‐γ, TNF, and IL‐2. Moreover, spEVs stimulated the expression of Foxp3 and IL‐10 by CD4+CD25+CD127‐ T cells, indicating differentiation into regulatory T‐cells (Tregs). Prior treatment of spEVs with proteinase K revoked their effects on T‐cells, indicating a requirement for surface‐exposed spEV proteins. The adenosine A2A receptor‐specific antagonist CPI‐444 also reduced effects of spEVs on T‐cells, consistent with the notion that the development of Tregs and their immune suppressive functions are under the influence of adenosine‐A2A receptor signalling. We found that adenosine is highly enriched in spEVs and propose that spEVs are targeted to and endocytosed by T‐cells, after which they may release their adenosine content into the lumen of endosomes, thus allowing endosome‐localized A2A receptor signalling in spEVs targeted T‐cells. Collectively, these data support the idea that spEVs can prime T cells directly for differentiation into Tregs.

Funder

China Scholarship Council

Publisher

Wiley

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