Arf6 exacerbates allergic asthma through cell-to-cell transmission of ASC inflammasomes
SangJoon Lee, Akari Ishitsuka, Takahiro Kuroki, Yu-Hsien Lin, Akira Shibuya, Tsunaki Hongu, Yuji Funakoshi, Yasunori Kanaho, Kyosuke Nagata, Atsushi Kawaguchi
SangJoon Lee, Akari Ishitsuka, Takahiro Kuroki, Yu-Hsien Lin, Akira Shibuya, Tsunaki Hongu, Yuji Funakoshi, Yasunori Kanaho, Kyosuke Nagata, Atsushi Kawaguchi
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Research Article Inflammation

Arf6 exacerbates allergic asthma through cell-to-cell transmission of ASC inflammasomes

Abstract

Asthma is a chronic inflammatory disease of the airways associated with excess production of Th2 cytokines and lung eosinophil accumulation. This inflammatory response persists in spite of steroid administration that blocks autocrine/paracrine loops of inflammatory cytokines, and the detailed mechanisms underlying asthma exacerbation remain unclear. Here, we show that asthma exacerbation is triggered by airway macrophages through a prion-like cell-to-cell transmission of extracellular particulates, including ASC protein, that assemble inflammasomes and mediate IL-1β production. OVA-induced allergic asthma and associated IL-1β production were alleviated in mice with small GTPase Arf6-deficient macrophages. The extracellular ASC specks were slightly engulfed by Arf6–/– macrophages, and the IL-1β production was reduced in Arf6–/– macrophages compared with that in WT macrophages. Furthermore, pharmacological inhibition of the Arf6 guanine nucleotide exchange factor suppressed asthma-like allergic inflammation in OVA-challenged WT mice. Collectively, the Arf6-dependent intercellular transmission of extracellular ASC specks contributes to the amplification of allergic inflammation and subsequent asthma exacerbation.

Authors

SangJoon Lee, Akari Ishitsuka, Takahiro Kuroki, Yu-Hsien Lin, Akira Shibuya, Tsunaki Hongu, Yuji Funakoshi, Yasunori Kanaho, Kyosuke Nagata, Atsushi Kawaguchi

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Figure 5

Engulfment of extracellular ASC specks is mediated by Arf6 for allergen-independent IL-1β production.

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Engulfment of extracellular ASC specks is mediated by Arf6 for allergen-...
(A–C) WT and Arf6–/– macrophages were stained with Alexa Fluor 568 phalloidin (red) at 6 hours after treatment with 1 × 104 particles of purified GFP-ASC specks (scale bar: 10 μm [top 3 rows]; 5 μm [bottom]) (A). Arrowheads indicate ASC specks. in, intracellular; ex, extracellular. Data are representative of 3 independent experiments. Two different fields are shown in each sample. The vertical section images from Z-stack series were reconstructed. Scale bar: 10 μm. (B). Dotted lines indicate the position of the reconstituted vertical plane. The number of cells showing intracellular ASC specks was counted (C) (n > 100; mean ± SD from 5 independent experiments). ***P < 0.001, 2-tailed Student’s t test. (D) At 6 hours after treatment of purified GFP-ASC specks, the amount of IL-1β secretion in WT or Arf6–/– macrophages was examined by ELISA. ***P < 0.001, 2-tailed Student’s t test. Mean ± SD from 3 independent experiments.