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Mycobacterial hypersensitivity pneumonitis requires TLR9–MyD88 in lung CD11b+ CD11c+ cells
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Mycobacteria are among the most common causes of hypersensitivity pneumonitis (HP), but controversy persists with regard to the involvement of the infectious potency of the organism in mycobacterial HP (hot tub lung). This study aimed to establish a mouse model of hot tub lung to clarify its pathophysiology.Mice were exposed intranasally to formalin-killedMycobacterium aviumfrom a patient with hot tub lung (HP strain) or chronic pulmonary infection (non-HP strain), and bronchoalveolar lavage fluids and lung tissues were evaluated for allergic inflammation.DeadM. aviumHP strain, but not non-HP strain, elicited marked HP-like pulmonary inflammation in wild-type mice. Although the inflammation was induced in mice lacking CD4 or CD8, the induction of HP-like responses was prevented in mice lacking myeloid differentiation factor (MyD)88 or Toll-like receptor (TLR)9. Cultured lung CD11c+ cells responded toM. aviumin a TLR9-dependent manner, and reconstitution of TLR9-/- mice with lung CD11c+ cells from wild-type mice restored the inflammatory responses. Further investigation revealed that pulmonary exposure toM. aviumHP strain increased the number of lung CD11b+ CD11c+ cells (dendritic cells) through TLR9 signalling.Our results provide evidence that hot tub lung developsviathe mycobacterial engagement of TLR9–MyD88 signalling in lung CD11b+ dendritic cells independent of the mycobacterial infectious capacity.
European Respiratory Society (ERS)
Title: Mycobacterial hypersensitivity pneumonitis requires TLR9–MyD88 in lung CD11b+ CD11c+ cells
Description:
Mycobacteria are among the most common causes of hypersensitivity pneumonitis (HP), but controversy persists with regard to the involvement of the infectious potency of the organism in mycobacterial HP (hot tub lung).
This study aimed to establish a mouse model of hot tub lung to clarify its pathophysiology.
Mice were exposed intranasally to formalin-killedMycobacterium aviumfrom a patient with hot tub lung (HP strain) or chronic pulmonary infection (non-HP strain), and bronchoalveolar lavage fluids and lung tissues were evaluated for allergic inflammation.
DeadM.
aviumHP strain, but not non-HP strain, elicited marked HP-like pulmonary inflammation in wild-type mice.
Although the inflammation was induced in mice lacking CD4 or CD8, the induction of HP-like responses was prevented in mice lacking myeloid differentiation factor (MyD)88 or Toll-like receptor (TLR)9.
Cultured lung CD11c+ cells responded toM.
aviumin a TLR9-dependent manner, and reconstitution of TLR9-/- mice with lung CD11c+ cells from wild-type mice restored the inflammatory responses.
Further investigation revealed that pulmonary exposure toM.
aviumHP strain increased the number of lung CD11b+ CD11c+ cells (dendritic cells) through TLR9 signalling.
Our results provide evidence that hot tub lung developsviathe mycobacterial engagement of TLR9–MyD88 signalling in lung CD11b+ dendritic cells independent of the mycobacterial infectious capacity.
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