Macrophage migration inhibitory factor promotes cyst growth in polycystic kidney disease
Li Chen, … , Jared J. Grantham, Xiaogang Li
Li Chen, … , Jared J. Grantham, Xiaogang Li
Published May 11, 2015
Citation Information: J Clin Invest. 2015;125(6):2399-2412. https://doi.org/10.1172/JCI80467.
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Research Article Nephrology

Macrophage migration inhibitory factor promotes cyst growth in polycystic kidney disease

Abstract

Autosomal dominant polycystic kidney disease (ADPKD) is characterized by renal cyst formation, inflammation, and fibrosis. Macrophages infiltrate cystic kidneys, but the role of these and other inflammatory factors in disease progression are poorly understood. Here, we identified macrophage migration inhibitory factor (MIF) as an important regulator of cyst growth in ADPKD. MIF was upregulated in cyst-lining epithelial cells in polycystin-1–deficient murine kidneys and accumulated in cyst fluid of human ADPKD kidneys. MIF promoted cystic epithelial cell proliferation by activating ERK, mTOR, and Rb/E2F pathways and by increasing glucose uptake and ATP production, which inhibited AMP-activated protein kinase signaling. MIF also regulated cystic renal epithelial cell apoptosis through p53-dependent signaling. In polycystin-1–deficient mice, MIF was required for recruitment and retention of renal macrophages, which promoted cyst expansion, and Mif deletion or pharmacologic inhibition delayed cyst growth in multiple murine ADPKD models. MIF-dependent macrophage recruitment was associated with upregulation of monocyte chemotactic protein 1 (MCP-1) and inflammatory cytokine TNF-α. TNF-α induced MIF expression, and MIF subsequently exacerbated TNF-α expression in renal epithelial cells, suggesting a positive feedback loop between TNF-α and MIF during cyst development. Our study indicates MIF is a central and upstream regulator of ADPKD pathogenesis and provides a rationale for further exploration of MIF as a therapeutic target for ADPKD.

Authors

Li Chen, Xia Zhou, Lucy X. Fan, Ying Yao, Katherine I. Swenson-Fields, Mihaela Gadjeva, Darren P. Wallace, Dorien J.M. Peters, Alan Yu, Jared J. Grantham, Xiaogang Li

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Figure 4

MIF and Pkd1 double KO delayed renal cyst formation.

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MIF and Pkd1 double KO delayed renal cyst formation. (A) Histologic exam...
(A) Histologic examination of PN7 kidneys from Pkd1fl/fl Ksp-Cre Mif+/+ (Mif+/+) and Pkd1fl/fl Ksp-Cre Mif–/– (Mif–/–) neonates. Scale bar: 1 mm. (B) Cystic index was significantly decreased in PN7 kidneys from Mif–/– neonates (n = 6) compared with Mif+/+ neonates (n = 10) (P < 0.05). Shown is mean ± SEM of all sections quantified for each condition. (C) KW/BW ratios from PN7 Mif–/– neonates were dramatically reduced compared with PN7 Mif+/+ neonates. Shown is mean ± SEM. P < 0.05. (D) BUN levels of PN7 Mif+/+ and Mif–/– neonates. Shown is mean ± SEM. P < 0.05. (E) Cell proliferation was decreased in Mif–/– neonate kidneys compared with Mif+/+ kidneys, as detected with PCNA staining. On average, the percentage of PCNA-positive nuclei in cyst-lining epithelial cells was calculated from 1,000 nuclei per mouse-kidney section, and only strongly stained nuclei were considered as PCNA-positive. Shown is mean ± SEM. P < 0.001. Scale bars: 50 μm. Arrows indicate the PCNA-positive cells. (F) KO of Mif induced cyst-lining epithelial cell apoptosis in Pkd1fl/fl Ksp-Cre mouse kidneys, as detected by TUNEL assay. P < 0.05. Scale bars: 100 μm. Statistical analysis was performed using an unpaired 2-tailed Student’s t test.