Fibroblastic reticular cells mitigate acute GvHD via MHCII-dependent maintenance of regulatory T cells
Haroon Shaikh, … , Jochen Huehn, Andreas Beilhack
Haroon Shaikh, … , Jochen Huehn, Andreas Beilhack
Published October 13, 2022
Citation Information: JCI Insight. 2022;7(22):e154250. https://doi.org/10.1172/jci.insight.154250.
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Research Article Hematology Transplantation

Fibroblastic reticular cells mitigate acute GvHD via MHCII-dependent maintenance of regulatory T cells

Abstract

Acute graft versus host disease (aGvHD) is a life-threatening complication of allogeneic hematopoietic cell transplantation (allo-HCT) inflicted by alloreactive T cells primed in secondary lymphoid organs (SLOs) and subsequent damage to aGvHD target tissues. In recent years, Treg transfer and/or expansion has emerged as a promising therapy to modulate aGvHD. However, cellular niches essential for fostering Tregs to prevent aGvHD have not been explored. Here, we tested whether and to what extent MHC class II (MHCII) expressed on Ccl19+ fibroblastic reticular cells (FRCs) shape the donor CD4+ T cell response during aGvHD. Animals lacking MHCII expression on Ccl19-Cre–expressing FRCs (MHCIIΔCcl19) showed aberrant CD4+ T cell activation in the effector phase, resulting in exacerbated aGvHD that was associated with significantly reduced expansion of Foxp3+ Tregs and invariant NK T (iNKT) cells. Skewed Treg maintenance in MHCIIΔCcl19 mice resulted in loss of protection from aGvHD provided by adoptively transferred donor Tregs. In contrast, although FRCs upregulated costimulatory surface receptors, and although they degraded and processed exogenous antigens after myeloablative irradiation, FRCs were dispensable to activate alloreactive CD4+ T cells in 2 mouse models of aGvHD. In summary, these data reveal an immunoprotective, MHCII-mediated function of FRC niches in secondary lymphoid organs (SLOs) after allo-HCT and highlight a framework of cellular and molecular interactions that regulate CD4+ T cell alloimmunity.

Authors

Haroon Shaikh, Joern Pezoldt, Zeinab Mokhtari, Juan Gamboa Vargas, Duc-Dung Le, Josefina Peña Mosca, Estibaliz Arellano Viera, Michael A.G. Kern, Caroline Graf, Niklas Beyersdorf, Manfred B. Lutz, Angela Riedel, Maike Büttner-Herold, Alma Zernecke, Hermann Einsele, Antoine-Emmanuel Saliba, Burkhard Ludewig, Jochen Huehn, Andreas Beilhack

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Figure 1

scRNA-Seq reveals differential expression of MHCII-mediated antigen presentation in the SCs subset of LNs.

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scRNA-Seq reveals differential expression of MHCII-mediated antigen pres...
Single-cell suspension from mLNs and pLNs were sorted for CD45CD24 cells and subjected to scRNA-Seq. Endothelial cells were identified as Pecam+ and were excluded from further downstream analysis. Data shown are pooled from 2 mLNs (sample 1, 2,247 cells; sample 2, 1,339 cells) and 2 pLNs (sample 1, 2,935 cells; sample 2, 2,757 cells) data sets. (A) UMAP plot of merged mLNs SCs and pLNs SCs showing cluster segregation. (B) Expression of subset defining DEGs across SCs on UMAP plot. (C) Heatmap of expression of genes involved in expression of MHCII-mediated antigen presentation genes on 15 identified clusters of SCs. (D) Expression of CIITA pI and pIV on DCs and FRCs evaluated by qPCR. Data are from 1 experiment, and 1 data point represents 1 mouse. Two-tailed unpaired Student’s t test was used; data are shown as mean± SD. ***P < 0.001. (E) Expression of autophagy on 15 identified clusters of SCs. mLNs, mesenteric lymph nodes; pLNs, peripheral lymph nodes, pLNs; stromal cells, SCs; DEGs, differentially expressed gene; UMAP, Uniform manifold approximation and projection for dimension reduction.