Chikungunya virus infection disrupts lymph node lymphatic endothelial cell composition and function via MARCO
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
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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Research Article Immunology Virology

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

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 2

WT CHIKV infection disrupts LEC marker expression and elicits infiltration of LN sinuses.

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WT CHIKV infection disrupts LEC marker expression and elicits infiltrati...
(AD) WT mice were mock inoculated (n = 3) or inoculated in the footpad with 1 × 103 PFU CHIKV 181/25 (n = 5) or WT CHIKV (n = 5), and the dLN was collected at 48 hours after infection. (A) LN sections stained for B220 (B cells, blue) and Lyve1 (LECs, white). Scale bar: 200 μm. (B) LN sections stained for B220 (B cells, blue) and MARCO (red). Scale bar: 200 μm. (C) Higher-magnification images of subcapsular and medullary sinus regions in LNs stained for B220 (B cells, blue), Lyve1 (floor and medullary LECs, white), CD36 (ceiling LECs, green), and MARCO (red). Scale bar: 50 μm. (D) LNs stained for B220 (B cells, blue), ERTR-7 (fibroblasts, white), nuclei (red), and CD11b (myeloid cells, green). Scale bar: 200 μm (left), 50 μm (right). Images are representative of 3–5 dLNs per group (2 independent experiments).