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Chikungunya virus infection disrupts lymph node lymphatic endothelial cell composition and function via MARCO
Cormac J. Lucas, … , Beth A.J. Tamburini, Thomas E. Morrison
Cormac J. Lucas, … , Beth A.J. Tamburini, Thomas E. Morrison
Published January 9, 2024
Citation Information: JCI Insight. 2024;9(4):e176537. https://doi.org/10.1172/jci.insight.176537.
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Research Article Immunology Virology

Chikungunya virus infection disrupts lymph node lymphatic endothelial cell composition and function via MARCO

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Abstract

Infection with chikungunya virus (CHIKV) causes disruption of draining lymph node (dLN) organization, including paracortical relocalization of B cells, loss of the B cell–T cell border, and lymphocyte depletion that is associated with infiltration of the LN with inflammatory myeloid cells. Here, we found that, during the first 24 hours of infection, CHIKV RNA accumulated in MARCO-expressing lymphatic endothelial cells (LECs) in both the floor and medullary LN sinuses. The accumulation of viral RNA in the LN was associated with a switch to an antiviral and inflammatory gene expression program across LN stromal cells, and this inflammatory response — including recruitment of myeloid cells to the LN — was accelerated by CHIKV-MARCO interactions. As CHIKV infection progressed, both floor and medullary LECs diminished in number, suggesting further functional impairment of the LN by infection. Consistent with this idea, antigen acquisition by LECs, a key function of LN LECs during infection and immunization, was reduced during pathogenic CHIKV infection.

Authors

Cormac J. Lucas, Ryan M. Sheridan, Glennys V. Reynoso, Bennett J. Davenport, Mary K. McCarthy, Aspen Martin, Jay R. Hesselberth, Heather D. Hickman, Beth A.J. Tamburini, Thomas E. Morrison

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Figure 1

CHIKV RNA accumulates in MARCO-expressing floor LECs in the dLN.

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CHIKV RNA accumulates in MARCO-expressing floor LECs in the dLN.
(A–F) W...
(A–F) WT mice were inoculated with PBS (mock, n = 2) or 1 × 103 PFU of CHIKV (n = 2) in the footpad. At 8 hours after infection, the dLN was collected and enzymatically digested into a single-cell suspension. Cells were enriched for CD45– cells and analyzed by scRNA-Seq. (A) UMAP shows CHIKV score, calculated as the fraction of total reads that align to the CHIKV genome for each cell from the CHIKV-enriched libraries. (B) UMAP shows CHIKV+ cells. (C) CHIKV score is shown for CHIKV+ cells for cell types with > 40 total cells and > 3 CHIKV+ cells. P values were calculated using a 1-sided Wilcoxon rank sum test with Bonferroni correction comparing each cell type with all other CHIKV+ cells. Only adjusted P < 0.05 are shown. (D) The fraction of cells identified as CHIKV+ is shown for each cell type in C. P values were calculated using a 1-sided hypergeometric test with Bonferroni correction. Labels show the number of CHIKV+ cells/total cells. Only adjusted P < 0.05 are shown. (E and F) Marco and Madcam1 expression for floor LECs (fLEC). P values were calculated using a 2-sided Wilcoxon rank-sum test with Bonferroni correction. In the box plots, the central lines, the box limits, and the whiskers represent medians, the interquartile range (IQR), and the minimum/maximum values that are not outliers, respectively. Outliers are shown as points and include any values that are more than 1.5× IQR away from the box.

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