Inflammation-independent TL1A-mediated intestinal fibrosis is dependent on the gut microbiome

炎症性肠病 免疫学 结肠炎 纤维化 回肠炎 炎症 成纤维细胞 肿瘤坏死因子α 失调 微生物群 促炎细胞因子 人口 白细胞介素17 肠道菌群 生物 微生物学 克罗恩病 医学 体外 疾病 病理 环境卫生 生物信息学 生物化学
作者
Noam Jacob,Jonathan P. Jacobs,Kotaro Kumagai,Connie Ha,Yoshitake Kanazawa,Venu Lagishetty,Katherine Altmayer,Ariel M. Hamill,Aimee Von Arx,R. Balfour Sartor,Suzanne Devkota,Jonathan Braun,Kathrin S. Michelsen,Stephan R. Targan,David Q. Shih
出处
期刊:Mucosal Immunology [Elsevier BV]
卷期号:11 (5): 1466-1476 被引量:56
标识
DOI:10.1038/s41385-018-0055-y
摘要

Tumor necrosis factor-like cytokine 1A (TL1A, TNFSF15) is implicated in inflammatory bowel disease (IBD), modulating the location and severity of intestinal inflammation and fibrosis. TL1A expression is increased in inflamed gut mucosa and associated with fibrostenosing Crohn's disease. Tl1a-overexpression in mice lead to spontaneous ileitis, and exacerbated induced proximal colitis and fibrosis. IBD is associated with shifts in the gut microbiome, but the effect of differing microbial populations and their interaction with TL1A on fibrosis has not been investigated. We demonstrate that the pro-fibrotic and inflammatory phenotype resulting from Tl1a-overexpression is abrogated in the absence of resident microbiota. To evaluate if this is due to the absence of a unique bacterial population, as opposed to any bacteria per se, we gavaged germ-free (GF) wild-type and Tl1a-transgenic (Tl1a-Tg) mice with stool from specific pathogen free (SPF) mice and a healthy human donor (Hu). Reconstitution with SPF, but not Hu microbiota, resulted in increased intestinal collagen deposition and fibroblast activation in Tl1a-Tg mice. Notably, there was reduced fibroblast migration and activation under GF conditions compared to native conditions. We then identified several candidate organisms that correlated directly with increased fibrosis in reconstituted mice and showed that these organisms directly impact fibroblast function in vitro. Thus, Tl1a-mediated intestinal fibrosis and fibroblast activation are dependent on specific microbial populations.
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