普氏粪杆菌 A2-165 在 GuMI 人体肠道微生理系统中代谢宿主和培养基衍生的化学物质并诱导结肠上皮细胞的转录变化

Microbiome research reports Pub Date : 2024-05-21 DOI:10.20517/mrr.2024.14

Yu-Ja Huang, Caroline A. Lewis, Charles W. Wright, Kirsten Schneider, John Kemmitt, David L. Trumper, David T Breault, Omer Yilmaz, L. Griffith, Jianbo Zhang

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引用次数: 0

摘要

目的：最近，人们建立了一个GuMI肠道微生理系统，将不耐受氧气的普氏粪杆菌（F. prausnitzii ）A2-165与源自原发性人类结肠上皮细胞的器官组织进行共培养。本研究旨在检验这种 GuMI 系统是否适用于不同健康状况的供体，并利用代谢组学揭示肠道微生物在调节肠腔中宿主和饮食衍生分子中的作用。研究方法从憩室炎患者、溃疡性结肠炎患者和克罗恩病患者的未发炎区域生成结肠单层有机体，然后将其整合到 GuMI 系统中与 F. prausnitzii A2-165 共培养 2-4 天。收集根尖培养基用于代谢组学分析。在不含细菌的传统静态培养、不含细菌的 GuMI 和含 F. prausnitzii 的 GuMI 三种条件下，对 169 种极性化学物质进行了靶向代谢组学分析。使用跨上皮阻力测量了单层膜的屏障功能。结果：GuMI 成功地将源自患者的单层膜与表皮生长因子共培养了 4 天，细菌生长活跃。引入气流和氧气梯度可显著增强屏障功能，而暴露于F. prausnitzii可轻微增强屏障功能。靶向代谢组学筛选了 169 种化合物，检测到 76 种代谢物，其中 70 种在至少两种条件下有明显差异。F.prausnitzii能明显调节顶端核苷、核碱基和氨基酸的水平。进一步分析表明，F. prausnitzii 能改变结肠上皮细胞中 260 个转录因子基因的 mRNA 水平。结论GuMI仿生系统可以维持F. prausnitzii与来自不同供体的结肠上皮细胞的共培养。结合代谢组学，我们发现了在与人类结肠上皮细胞的共培养过程中，F. prausnitzii对细胞外化学物质和结肠上皮细胞转录的调节作用，这可能反映了其在体内肠腔中的功能。

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Faecalibacterium prausnitzii A2-165 metabolizes host- and media-derived chemicals and induces transcriptional changes in colonic epithelium in GuMI human gut microphysiological system

Aim: Recently, a GuMI gut microphysiological system has been established to coculture oxygen-intolerant Faecalibacterium prausnitzii (F. prausnitzii ) A2-165 with organoids-derived primary human colonic epithelium. This study aims to test if this GuMI system applies to different donors with different healthy states and uses metabolomics to reveal the role of gut microbes in modulating host- and diet-derived molecules in the gut lumen. Methods: Organoids-derived colonic monolayers were generated from an uninflamed region of diverticulitis, ulcerative colitis, and Crohn’s disease patients and then integrated into the GuMI system to coculture with F. prausnitzii A2-165 for 2 to 4 days. Apical media was collected for metabolomic analysis. Targeted metabolomics was performed to profile 169 polar chemicals under three conditions: conventional static culture without bacteria, GuMI without bacteria, and GuMI with F. prausnitzii . The barrier function of monolayers was measured using transepithelial resistance. Results: GuMI successfully cocultured patient-derived monolayers and F. prausnitzii for up to 4 days, with active bacterial growth. Introducing flow and oxygen gradient significantly increases the barrier function, while exposure to F. prausnitzii slightly increases the barrier function. Targeted metabolomics screened 169 compounds and detected 76 metabolites, of which 70 significantly differed between at least two conditions. F. prausnitzii significantly modulates the levels of nucleosides, nucleobases, and amino acids on the apical side. Further analysis suggests that F. prausnitzii changes the mRNA level of 260 transcription factor genes in colonic epithelial cells. Conclusion: The GuMI physiomimetic system can maintain the coculture of F. prausnitzii and colonic epithelium from different donors. Together with metabolomics, we identified the modulation of F. prausnitzii in extracellular chemicals and colonic epithelial cell transcription in coculture with human colonic epithelium, which may reflect its function in gut lumen in vivo .

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Microbiome research reports

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1.80

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