4.6 Article

Xenorecognition and costimulation of porcine endothelium-derived extracellular vesicles in initiating human porcine-specific T cell immune responses

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AMERICAN JOURNAL OF TRANSPLANTATION
卷 23, 期 7, 页码 904-919

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ELSEVIER SCIENCE INC
DOI: 10.1016/j.ajt.2023.04.006

关键词

xenotransplantation; porcine endothelial cells; extracellular vesicles; swine leukocyte antigen; xenorecognition; xeno-costimulation

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Porcine vascular endothelial cells release extracellular vesicles expressing SLA-I, which can directly initiate T cell-mediated immune responses through xenorecognition and costimulation, suggesting a potential role in xenograft rejection.
Porcine vascular endothelial cells (PECs) form a mechanistic centerpiece of xenograft rejection. Here, we determined that resting PECs release swine leukocyte antigen class I (SLA-I) but not swine leukocyte antigen class-II DR (SLA-DR) expressing extracellular vesi-cles (EVs) and investigated whether these EVs proficiently initiate xenoreactive T cell re-sponses via direct xenorecognition and costimulation. Human T cells acquired SLA-I thorn EVs with or without direct contact to PECs, and these EVs colocalized with T cell receptors. Although interferon gamma-activated PECs released SLA-DR thorn EVs, the binding of SLA-DR thorn EVs to T cells was sparse. Human T cells demonstrated low levels of proliferation without direct contact to PECs, but marked T cell proliferation was induced following exposure to EVs. EV-induced proliferation proceeded independent of monocytes/macrophages, suggesting that EVs delivered both a T cell receptor signal and costimulation. Costimulation blockade targeting B7, CD40L, or CD11a significantly reduced T cell proliferation to PEC-derived EVs. These findings indicate that endothelial-derived EVs can directly initiate T cell-mediated im-mune responses, and suggest that inhibiting the release of SLA-I EVs from organ xenografts has the potential to modify the xenograft rejection. We propose a secondary-direct pathway for T cell activation via xenoantigen recognition/costimulation by endothelial-derived EVs.

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