Myofibroblast dedifferentiation proceeds via distinct transcriptomic and phenotypic transitions
Sean M. Fortier, … , Giovanni Ligresti, Marc Peters-Golden
Sean M. Fortier, … , Giovanni Ligresti, Marc Peters-Golden
Published February 9, 2021
Citation Information: JCI Insight. 2021;6(6):e144799. https://doi.org/10.1172/jci.insight.144799.
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Research Article Cell biology Pulmonology

Myofibroblast dedifferentiation proceeds via distinct transcriptomic and phenotypic transitions

Abstract

Myofibroblasts are the major cellular source of collagen, and their accumulation — via differentiation from fibroblasts and resistance to apoptosis — is a hallmark of tissue fibrosis. Clearance of myofibroblasts by dedifferentiation and restoration of apoptosis sensitivity has the potential to reverse fibrosis. Prostaglandin E2 (PGE2) and mitogens such as FGF2 have each been shown to dedifferentiate myofibroblasts, but — to our knowledge — the resultant cellular phenotypes have neither been comprehensively characterized or compared. Here, we show that PGE2 elicited dedifferentiation of human lung myofibroblasts via cAMP/PKA, while FGF2 utilized MEK/ERK. The 2 mediators yielded transitional cells with distinct transcriptomes, with FGF2 promoting but PGE2 inhibiting proliferation and survival. The gene expression pattern in fibroblasts isolated from the lungs of mice undergoing resolution of experimental fibrosis resembled that of myofibroblasts treated with PGE2 in vitro. We conclude that myofibroblast dedifferentiation can proceed via distinct programs exemplified by treatment with PGE2 and FGF2, with dedifferentiation occurring in vivo most closely resembling the former.

Authors

Sean M. Fortier, Loka R. Penke, Dana King, Tho X. Pham, Giovanni Ligresti, Marc Peters-Golden

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Figure 6

Myofibroblasts treated with PGE2 and FGF2 separately or in combination produce distinct cellular morphologies and fibrosis-associated gene expression patterns.

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Myofibroblasts treated with PGE2 and FGF2 separately or in combination p...
CCL210 fibroblasts were differentiated to myofibroblasts with TGF-β (2 ng/mL) and treated with PGE2 (1 μM), FGF2 (50 ng/mL), or both. (A) Cells were stained with the membrane dye PKH26 (2 μM) and examined by fluorescence microscopy 5 days after treatment. (B) Kinetics of ACTA2 in untreated, PGE2-, FGF2-, and PGE2 + FGF2–treated myofibroblasts. Fibroblasts were treated with TGF-β for 48 hours, followed by treatment and harvesting for mRNA at the indicated time points. (C) Immunofluorescence microscopy and representative Western blot for αSMA in untreated and PGE2 + FGF2–treated myofibroblasts evaluated at 5 days. The histogram depicts mean densitometry values. (D) qPCR analysis of the fibrosis-associated genes ACTA2, COL1A1, FN1, CTGF, VASP, and NOX4 after 24 hours of PGE2 ± FGF2 compared with untreated myofibroblast control. Relative fold changes of indicated genes measured by qPCR are normalized to GAPDH. Data are presented as mean ± SEM; data points represent replicate samples from 3 experiments. Lines indicate conditions being compared. *Statistical significance compared with untreated myofibroblast; +Statistical significance compared with untreated, PGE2-, and FGF2-treated myofibroblasts. *P < 0.05 and +P < 0.05. Performed 2-way ANOVA for B, paired 2-tailed t test for C, and 1-way ANOVA for D. Diff, differentiation; De-diff, dedifferentiation.