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Proinflammatory macrophages transporting gut-derived bacterial DNA drive autoimmune arthritis in spondyloarthropathy
Benjamin Cai, … , Anne-Sophie Bergot, Ranjeny Thomas
Benjamin Cai, … , Anne-Sophie Bergot, Ranjeny Thomas
Published July 31, 2025
Citation Information: JCI Insight. 2025;10(17):e188028. https://doi.org/10.1172/jci.insight.188028.
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Research Article Inflammation

Proinflammatory macrophages transporting gut-derived bacterial DNA drive autoimmune arthritis in spondyloarthropathy

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Abstract

Spondyloarthritis (SpA) is an inflammatory arthritis of the spine and joints associated with intestinal inflammation, in which it is hypothesized that innate immune exposure to enteroinvasive species is followed by self-/bacterial peptide presentation. However, the mechanisms underlying loss of tolerance to gut bacteria in genetically at-risk individuals are unclear. Curdlan-treated (β-1,3-glucan, dectin-1 ligand–treated) ZAP-70W163C (SKG) mice develop autoimmune arthritis and ileitis associated with Gram-negative fecal dysbiosis. Using gnotobiotic mice, we show that curdlan-treated SKG mice monoassociated with Parabacteroides goldsteinii or Lactobacillus murinus developed ileitis, arthritis, and enthesitis, while BALB/c mice were tolerant. Gnotobiotic SKG ileum upregulated Il23a and ER stress genes and lost goblet cells. Whereas bacterial DNA colocalized with neutrophils and inflammatory macrophages in SKG lamina propria, periarticular bone marrow, entheses, and spleen, in BALB/c mice, bacterial DNA colocalized with resident macrophages in lamina propria and spleen. Human psoriatic-arthritis synovial tissue also contained cell-associated perivascular bacterial DNA. Curdlan-treated SKG spleen/bone marrow macrophages transferred severe arthritis and expanded Th17 cells in naive SKG recipients, while BALB/c or germ-free SKG macrophages transferred mild arthritis and regulated Th17 cells. Thus, bacterial DNA and myeloid cells in the gut and their subsequent traffic regulate or enforce T cell pathogenicity in SpA.

Authors

Benjamin Cai, Rabina Giri, Amy J. Cameron, M. Arifur Rahman, Annabelle Small, Christopher Altmann, Yenkai Lim, Linda M. Rehaume, Mark Morrison, Mihir D. Wechalekar, Jakob Begun, Anne-Sophie Bergot, Ranjeny Thomas

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Figure 6

Curdlan promotes P. goldsteinii and L. murinus penetration through the ileal mucosa.

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Curdlan promotes P. goldsteinii and L. murinus penetration through the i...
GF-SKG and GF-BALB/c mice remained GF or were monocolonized with P.g. or L.m. 4 weeks prior to curdlan i.p. at day 0. Some mice were treated with anti–IL-23p19 at day –1. At 1 week after curdlan, ileum tissues were imaged for bacterial translocation from lumen to villi using FISH with EUB338 probe on Carnoy-fixed tissues. (A) Experiment design for Figures 6 and 7. (B) Log of the count of bacteria per villi area at week 1 after curdlan. Data show mean ± SEM of the log values with each data point representing 1 ROI. (C) Ratio of L.m. or P.g. bacteria counts in BALB/c and SKG mice treated with or without curdlan. Data show mean ± SEM of the log values, with each data point representing 1 ROI. Two-way ANOVA (B) and 1-tailed t test (C) with **P < 0.01 and ****P < 0.0001.

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