Live-cell imaging of human liver fibrosis using hepatic micro-organoids
Yuan Guan, … , Annika Enejder, Gary Peltz
Yuan Guan, … , Annika Enejder, Gary Peltz
Published December 10, 2024
Citation Information: JCI Insight. 2025;10(2):e187099. https://doi.org/10.1172/jci.insight.187099.
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Research Article Hepatology

Live-cell imaging of human liver fibrosis using hepatic micro-organoids

Abstract

Due to the limitations of available in vitro systems and animal models, we lack a detailed understanding of the pathogenetic mechanisms of and have minimal treatment options for liver fibrosis. Therefore, we engineered a live-cell imaging system that assessed fibrosis in a human multilineage hepatic organoid in a microwell (i.e., microHOs). Transcriptomic analysis revealed that TGFB converted mesenchymal cells in microHOs into myofibroblast-like cells resembling those in fibrotic human liver tissue. When pro-fibrotic intracellular signaling pathways were examined, the antifibrotic effect of receptor-specific tyrosine kinase inhibitors was limited to the fibrosis induced by the corresponding growth factor, which indicates their antifibrotic efficacy would be limited to fibrotic diseases solely mediated by that growth factor. Based upon transcriptomic and transcription factor activation analyses in microHOs, glycogen synthase kinase 3β and p38 MAPK inhibitors were identified as potential new broad-spectrum therapies for liver fibrosis. Other new therapies could subsequently be identified using the microHO system.

Authors

Yuan Guan, Zhuoqing Fang, Angelina Hu, Sarah Roberts, Meiyue Wang, Wenlong Ren, Patrik K. Johansson, Sarah C. Heilshorn, Annika Enejder, Gary Peltz

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Figure 8

Antifibrotic drugs inhibit fibrosis in microHOs produced from iPSCs of different genetic backgrounds.

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Antifibrotic drugs inhibit fibrosis in microHOs produced from iPSCs of d...
microHOs produced from iPSC lines generated from 2 donors (C1, C2) (10) were treated with no addition (NC), TGFB (T) (50 ng/mL), or TGFB and 1 of the following drugs on day 13: TGFBR inhibitor (10 μM SB431542), GSK3β inhibitor (3 μM CHIR), or p38 inhibitor (10 μM SB202190). The microHOs were analyzed by trichrome staining on day 21. (A) Images of trichrome-stained, TGFB-treated microHOs show a marked increase in collagen-rich connective tissue (blue-stained regions) relative to control (NC) microHOs, which only had a thin layer of connective tissue. The TGFB-induced increased in collagen was markedly inhibited by addition of the TGFBR, GSK3β, or p38 inhibitors. The scale bar: 50 μm. (B) Box plots show the area in microHOs that received indicated treatments (n = 6–9 per group) occupied by collagen (collagen fraction). The means for each group were compared using a 1-way ANOVA and Tukey’s posttest: ****, P < 0.0001 (for T vs. NC or T vs. T+drug).