JUNB/AP-1 controls IFN-γ during inflammatory liver disease
Martin K. Thomsen, … , Lola Martinez, Erwin F. Wagner
Martin K. Thomsen, … , Lola Martinez, Erwin F. Wagner
Published November 8, 2013
Citation Information: J Clin Invest. 2013;123(12):5258-5268. https://doi.org/10.1172/JCI70405.
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Research Article Hepatology

JUNB/AP-1 controls IFN-γ during inflammatory liver disease

Abstract

Understanding the molecular pathogenesis of inflammatory liver disease is essential to design efficient therapeutic approaches. In hepatocytes, the dimeric transcription factor c-JUN/AP-1 is a major mediator of cell survival during hepatitis, although functions for other JUN proteins in liver disease are less defined. Here, we found that JUNB was specifically expressed in human and murine immune cells during acute liver injury. We analyzed the molecular function of JUNB in experimental models of hepatitis, including administration of concanavalin A (ConA) or α-galactosyl-ceramide, which induce liver inflammation and injury. Mice specifically lacking JUNB in hepatocytes displayed a mild increase in ConA-induced liver damage. However, targeted deletion of Junb in immune cells and hepatocytes protected against hepatitis in experimental models that involved NK/NKT cells. The absence of JUNB in immune cells decreased IFN-γ expression and secretion from NK and NKT cells, leading to reduced STAT1 pathway activation. Systemic IFN-γ treatment or adenovirus-based IRF1 delivery to Junb-deficient mice restored hepatotoxicity, and we demonstrate that Ifng is a direct transcriptional target of JUNB. These findings demonstrate that JUNB/AP-1 promotes cell death during acute hepatitis by regulating IFN-γ production in NK and NKT cells and thus functionally antagonizes the hepatoprotective function of c-JUN/AP-1 in hepatocytes.

Authors

Martin K. Thomsen, Latifa Bakiri, Sebastian C. Hasenfuss, Rainer Hamacher, Lola Martinez, Erwin F. Wagner

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Figure 4

STAT1 pathway is altered in JunbΔli* mice.

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STAT1 pathway is altered in JunbΔli* mice. Control and JunbΔli* mice w...
Control and JunbΔli* mice were treated with ConA and liver samples analyzed. (A) Western blot for phosphorylated and total STAT1, STAT3, STAT5. Vinculin is included to control for equal loading. Quantification is shown (n = 5; *P < 0.05). (B) Liver sections stained for pSTAT1 (brown) after ConA treatment. Arrowheads indicate positive immune cells (red) and hepatocytes (black). n = 5. Immunofluorescence costaining of pSTAT1 (green) and F4/80 (red) is shown in the inset. A representative experiment is shown. Scale bar: 20 μm.