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Mice that exclusively express TLR4 on endothelial cells can efficiently clear a lethal systemic Gram-negative bacterial infection
Graciela Andonegui, … , Stephen M. Robbins, Paul Kubes
Graciela Andonegui, … , Stephen M. Robbins, Paul Kubes
Published June 15, 2009
Citation Information: J Clin Invest. 2009;119(7):1921-1930. https://doi.org/10.1172/JCI36411.
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Research Article Immunology

Mice that exclusively express TLR4 on endothelial cells can efficiently clear a lethal systemic Gram-negative bacterial infection

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Abstract

Recognition of LPS by TLR4 on immune sentinel cells such as macrophages is thought to be key to the recruitment of neutrophils to sites of infection with Gram-negative bacteria. To explore whether endothelial TLR4 plays a role in this process, we engineered and imaged mice that expressed TLR4 exclusively on endothelium (known herein as EndotheliumTLR4 mice). Local administration of LPS into tissue induced comparable neutrophil recruitment in EndotheliumTLR4 and wild-type mice. Following systemic LPS or intraperitoneal E. coli administration, most neutrophils were sequestered in the lungs of wild-type mice and did not accumulate at primary sites of infection. In contrast, EndotheliumTLR4 mice showed reduced pulmonary capillary neutrophil sequestration over the first 24 hours; as a result, they mobilized neutrophils to primary sites of infection, cleared bacteria, and resisted a dose of E. coli that killed 50% of wild-type mice in the first 48 hours. In fact, the only defect we detected in EndotheliumTLR4 mice was a failure to accumulate neutrophils in the lungs following intratracheal administration of LPS; this response required TLR4 on bone marrow–derived immune cells. Therefore, endothelial TLR4 functions as the primary intravascular sentinel system for detection of bacteria, whereas bone marrow–derived immune cells are critical for pathogen detection at barrier sites. Nonendothelial TLR4 contributes to failure to accumulate neutrophils at primary infection sites in a disseminated systemic infection.

Authors

Graciela Andonegui, Hong Zhou, Daniel Bullard, Margaret M. Kelly, Sarah C. Mullaly, Braedon McDonald, Elizabeth M. Long, Stephen M. Robbins, Paul Kubes

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Figure 3

Effect of intratracheal LPS on neutrophil sequestration into the lungs.

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Effect of intratracheal LPS on neutrophil sequestration into the lungs.
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Mice were treated with LPS (intratracheal aerosol) for 24 hours, and the lungs were prepared for histology (esterase staining). Intratracheal aerosol of LPS was administered to (A) wild-type and (C) EndotheliumTLR4 mice or saline was administered to (B) wild-type mice. (B) Representative sections show alveolar spaces and capillaries mainly devoid of neutrophils in the saline-treated lungs, (A) while many alveolar spaces contain neutrophils (arrows), with some neutrophils still within capillaries (arrowheads), in the LPS-treated wild-type mice. (C) In contrast, LPS treatment in EndotheliumTLR4 mice resulted in very few neutrophils collecting in the pulmonary capillaries or alveolar spaces. (D) BAL was performed, and number of neutrophils was quantified. Data are expressed as the mean ± SEM (n = 3 to 8 mice in each group). ND, not detectable. Original magnification, ×400 (A–C). In B, the black line represents 100 μm. *P < 0.001 versus saline-treated mice.

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ISSN: 0021-9738 (print), 1558-8238 (online)

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