Single-cell transcriptome mapping identifies a local, innate B cell population driving chronic rejection after lung transplantation
Natalia F. Smirnova, Kent Riemondy, Marta Bueno, Susan Collins, Pavan Suresh, Xingan Wang, Kapil N. Patel, Carlyne Cool, Melanie Königshoff, Nirmal S. Sharma, Oliver Eickelberg
Natalia F. Smirnova, Kent Riemondy, Marta Bueno, Susan Collins, Pavan Suresh, Xingan Wang, Kapil N. Patel, Carlyne Cool, Melanie Königshoff, Nirmal S. Sharma, Oliver Eickelberg
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Resource and Technical Advance Pulmonology Transplantation

Single-cell transcriptome mapping identifies a local, innate B cell population driving chronic rejection after lung transplantation

Abstract

Bronchiolitis obliterans syndrome (BOS) is the main reason for poor outcomes after lung transplantation (LTx). We and others have recently identified B cells as major contributors to BOS after LTx. The extent of B cell heterogeneity and the relative contributions of B cell subpopulations to BOS, however, remain unclear. Here, we provide a comprehensive analysis of cell population changes and their gene expression patterns during chronic rejection after orthotopic LTx in mice. Of 11 major cell types, Mzb1-expressing plasma cells (PCs) were the most prominently increased population in BOS lungs. These findings were validated in 2 different cohorts of human BOS after LTx. A Bhlhe41, Cxcr3, and Itgb1 triple-positive B cell subset, also expressing classical markers of the innate-like B-1 B cell population, served as the progenitor pool for Mzb1+ PCs. This subset accounted for the increase in IgG2c production within BOS lung grafts. A genetic lack of Igs decreased BOS severity after LTx. In summary, we provide a detailed analysis of cell population changes during BOS. IgG+ PCs and their progenitors — an innate B cell subpopulation — are the major source of local Ab production and a significant contributor to BOS after LTx.

Authors

Natalia F. Smirnova, Kent Riemondy, Marta Bueno, Susan Collins, Pavan Suresh, Xingan Wang, Kapil N. Patel, Carlyne Cool, Melanie Königshoff, Nirmal S. Sharma, Oliver Eickelberg

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Figure 6

Functional characterization of the cluster-1 B cell subset.

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Functional characterization of the cluster-1 B cell subset. (A) Gene exp...
(A) Gene expression patterns projected onto UMAP plots of Mzb1, Bhlhe41, Itgb1, and Cxcr3 in the B and PC subclusters from control (B6→B6) and BOS (HLA→B6) lung grafts. (B) Gene expression patterns projected onto UMAP plots of Ig isotypes in the B and PC subclusters from control (B6→B6) and BOS (HLA→B6) lung grafts. (C) Quantification of Ig isotypes in the conditioned media from CD19+CXCR3+ITGBB1+ and CD19CXCR3ITGB1 cells sorted from HLA→B6 and B6→B6 mouse lung grafts 1 month after LTx, stimulated by LPS (1 μg/mL). Data are presented as mean ± SEM and analyzed with a 2-way ANOVA test followed by a Tukey’s multiple comparisons test. (D) Quantification of Ig isotypes in the BALF samples collected from the lung grafts of HLA→B6 and B6→B6 mice 1 month after LTx. Data are presented as mean ± SEM and analyzed with a 2-way ANOVA test followed by a Tukey’s multiple comparisons test. ***P < 0.001, ****P < 0.0001. DN, double negative CXCR3ITGB1; DP, CXCR3+ITGB1+.