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Cellular effectors mediating Th17-dependent clearance of pneumococcal colonization in mice
Zhe Zhang, … , Thomas B. Clarke, Jeffrey N. Weiser
Zhe Zhang, … , Thomas B. Clarke, Jeffrey N. Weiser
Published June 8, 2009
Citation Information: J Clin Invest. 2009;119(7):1899-1909. https://doi.org/10.1172/JCI36731.
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Research Article Infectious disease

Cellular effectors mediating Th17-dependent clearance of pneumococcal colonization in mice

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Abstract

Microbial colonization of mucosal surfaces may be an initial event in the progression to disease, and it is often a transient process. For the extracellular pathogen Streptococcus pneumoniae studied in a mouse model, nasopharyngeal carriage is eliminated over a period of weeks and requires cellular rather than humoral immunity. Here, we demonstrate that primary infection led to TLR2-dependent recruitment of monocyte/macrophages into the upper airway lumen, where they engulfed pneumococci. Pharmacologic depletion of luminal monocyte/macrophages by intranasal instillation of liposomal clodronate diminished pneumococcal clearance. Efficient clearance of colonization required TLR2 signaling to generate a population of pneumococcal-specific IL-17–expressing CD4+ T cells. Depletion of either IL-17A or CD4+ T cells was sufficient to block the recruitment of monocyte/macrophages that allowed for effective late pneumococcal clearance. In contrast with naive mice, previously colonized mice showed enhanced early clearance that correlated with a more robust influx of luminal neutrophils. As for primary colonization, these cellular responses required Th17 immunity. Our findings demonstrate that monocyte/macrophages and neutrophils recruited to the mucosal surface are key effectors in clearing primary and secondary bacterial colonization, respectively.

Authors

Zhe Zhang, Thomas B. Clarke, Jeffrey N. Weiser

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Figure 3

Macrophages in the lumen of the upper respiratory tract engulf colonizing pneumococci.

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Macrophages in the lumen of the upper respiratory tract engulf colonizin...
(A) MOMA-2 mAb staining–positive (red) mononuclear cells associated with pneumococci stained with type 23F antiserum (green). Left panel shows a representative z-section confocal image. Cytospin preparations were from mice inoculated with P1121 for 7 days. Scale bar: 5 μm. Right panel shows representative view of a cytospin preparation from mice inoculated with P1121 for 3 days. Pneumococci were observed to be associated with monocytes/macrophages but not neutrophils. Original magnification, ×200. (B) P1121 stained with type 23F antiserum (green) colocalized with LAMP-1–positive (red) intracellular lysosomal compartments as shown in the overlay (yellow). Mononuclear cells were identified by DAPI staining of the nucleus (blue). Cytospin preparations were from mice inoculated with P1121 for 7 days. Original magnification, ×600.

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