p40 homodimers bridge ischemic tissue inflammation and heterologous alloimmunity in mice via IL-15 transpresentation
Hidetoshi Tsuda, … , Anna Valujskikh, Robert L. Fairchild
Hidetoshi Tsuda, … , Anna Valujskikh, Robert L. Fairchild
Published January 25, 2024
Citation Information: J Clin Invest. 2024;134(6):e172760. https://doi.org/10.1172/JCI172760.
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Research Article

p40 homodimers bridge ischemic tissue inflammation and heterologous alloimmunity in mice via IL-15 transpresentation

Abstract

Virus-induced memory T cells often express functional cross-reactivity, or heterologous immunity, to other viruses and to allogeneic MHC molecules that is an important component of pathogenic responses to allogeneic transplants. During immune responses, antigen-reactive naive and central memory T cells proliferate in secondary lymphoid organs to achieve sufficient cell numbers to effectively respond, whereas effector memory T cell proliferation occurs directly within the peripheral inflammatory microenvironment. Mechanisms driving heterologous memory T cell proliferation and effector function expression within peripheral tissues remain poorly understood. Here, we dissected proliferation of heterologous donor-reactive memory CD8+ T cells and their effector functions following infiltration into heart allografts with low or high intensities of ischemic inflammation. Proliferation within both ischemic conditions required p40 homodimer–induced IL-15 transpresentation by graft DCs, but expression of effector functions mediating acute allograft injury occurred only in high-ischemic allografts. Transcriptional responses of heterologous donor-reactive memory CD8+ T cells were distinct from donor antigen–primed memory CD8+ T cells during early activation in allografts and at graft rejection. Overall, the results provide insights into mechanisms driving heterologous effector memory CD8+ T cell proliferation and the separation between proliferation and effector function that is dependent on the intensity of inflammation within the tissue microenvironment.

Authors

Hidetoshi Tsuda, Karen S. Keslar, William M. Baldwin III, Peter S. Heeger, Anna Valujskikh, Robert L. Fairchild

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Figure 6

Endogenous memory CD8+ T cell proliferation within the allograft subjected to prolonged CIS requires IL-15 transpresentation.

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Endogenous memory CD8+ T cell proliferation within the allograft subject...
(A) Groups of BALB/c mice (n = 4–6 per group) received cardiac allografts subjected to 8 hours of CIS from either C57BL/6 mice or B6.129X1-IL15ratm1Ama/J mice and were injected with 100 μg BrdU i.p. on days 0 and 1. On day 2 after transplant, allografts were harvested and digested, and aliquots of single-cell suspensions were stained with antibody and analyzed by flow cytometry to quantitate the infiltration and proliferation of memory CD4+ and CD8+ T cells. *P < 0.05 as determined by the Mann-Whitney nonparametric test. (B) Allografts were harvested 48 hours after transplant, and total RNA was isolated from heart graft homogenates from each recipient and analyzed by quantitative reverse transcriptase PCR for expression of the indicated inflammatory mediator gene. Data indicate relative RNA expression of each test mediator versus expression in hearts from non-transplanted C57BL/6 mice. *P < 0.05 vs. RNA expression of C57BL/6 allografts subjected to 8 hours of CIS, as determined by the Mann-Whitney nonparametric test. (C) Survival of C57BL/6 or B6.129X1-IL15ratm1Ama/J allografts subjected to 8 hours of CIS in BALB/c recipients conditioned with 250 mg CTLA-4Ig i.p. on days 0 and 1. Graft survival was monitored daily by abdominal palpation, and rejection was confirmed visually by laparotomy. **P < 0.01 vs. survival of C57BL/6 allografts in CTLA-4–treated BALB/c recipients, as determined by the log-rank (Mantel-Cox) test.