Microvesicles released from activated CD4+ T cells alter microvascular endothelial cell function

Daria Vdovenko; Carolina Balbi; Dario Di Silvestre; Giulia Passignani; Yustina M Puspitasari; Martina Zarak-Crnkovic; Pierluigi Mauri; Giovanni G Camici; Thomas F Lüscher; Urs Eriksson; Giuseppe Vassalli

doi:10.1111/eci.13769

Microvesicles released from activated CD4⁺ T cells alter microvascular endothelial cell function

Eur J Clin Invest. 2022 Jun;52(6):e13769. doi: 10.1111/eci.13769. Epub 2022 Mar 31.

Authors

Daria Vdovenko¹, Carolina Balbi^{1

2

3}, Dario Di Silvestre⁴, Giulia Passignani⁴, Yustina M Puspitasari¹, Martina Zarak-Crnkovic¹, Pierluigi Mauri⁴, Giovanni G Camici¹, Thomas F Lüscher^{1

5}, Urs Eriksson^{1

6}, Giuseppe Vassalli^{1

2

3

7}

Affiliations

¹ Center for Molecular Cardiology, University of Zurich, Schlieren, Switzerland.
² Laboratory of Cellular and Molecular Cardiology, Istituto Cardiocentro Ticino-EOC, Lugano, Switzerland.
³ Laboratories for Translational Research-EOC, Bellinzona, Switzerland.
⁴ Proteomics and Metabolomic Lab, ITB-CNR, Segrate, Italy.
⁵ Royal Brompton & Harefield Hospital, Imperial College, London, UK.
⁶ Department of Medicine, GZO - Zurich Regional Health Center, Wetzikon, Switzerland.
⁷ Department of Biomedicine, Università della Svizzera Italiana (USI), Lugano, Switzerland.

Abstract

Background: Microvesicles are vesicles shed by plasma membranes following cell activation and apoptosis. The role of lymphocyte-derived microvesicles in endothelial function remains poorly understood.

Methods: CD4⁺ T cells isolated from peripheral blood of healthy human donors were stimulated using anti-CD3/anti-CD28-coated beads. Proteomic profiling of microvesicles was performed using linear discriminant analysis (LDA) from activated T cells (MV.Act) and nonactivated T cells (MV.NAct). In addition, data processing analysis was performed using MaxQUANT workflow. Differentially expressed proteins found in MV.Act or MV.NAct samples with identification frequency = 100%, which were selected by both LDA (p < .01) and MaxQUANT (p < .01) workflows, were defined as "high-confidence" differentially expressed proteins. Functional effects of MV.Act on human primary microvascular endothelial cells were analysed.

Results: T cells released large amounts of microvesicles upon stimulation. Proteomic profiling of microvesicles using LDA identified 2279 proteins (n = 2110 and n = 851 proteins in MV.Act and MV.NAct, respectively). Protein-protein interaction network models reconstructed from both differentially expressed proteins (n = 594; LDA p ≤ .01) and "high-confidence" differentially expressed proteins (n = 98; p ≤ .01) revealed that MV.Act were enriched with proteins related to immune responses, protein translation, cytoskeleton organisation and TNFα-induced apoptosis. For instance, MV.Act were highly enriched with IFN-γ, a key proinflammatory pathway related to effector CD4⁺ T cells. Endothelial cell incubation with MV.Act induced superoxide generation, apoptosis, endothelial wound healing impairment and endothelial monolayer barrier disruption.

Conclusions: T cell receptor-mediated activation of CD4⁺ T cells stimulates the release of microvesicles enriched with proteins involved in immune responses, inflammation and apoptosis. T cell-derived microvesicles alter microvascular endothelial function and barrier permeability, potentially promoting tissue inflammation.

Keywords: T cells; endothelial cell; extracellular vesicle; microvesicle; proteomics.

MeSH terms

CD4-Positive T-Lymphocytes
Cell-Derived Microparticles* / metabolism
Endothelial Cells* / metabolism
Humans
Inflammation / metabolism
Proteomics
T-Lymphocytes

Abstract

MeSH terms

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