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A TGF-β1/LEF1/β-catenin/JLP network motif regulates autophagy and tubule injury in renal fibrosis
Chen Li, Meng Zhang, Maoqing Tian, Zeyu Tang, Yuying Hu, Yuyu Long, Xiaofei Wang, Liwen Qiao, Jiefei Zeng, Yujuan Wang, Xinghua Chen, Cheng Chen, Xiaoyan Li, Lu Zhang, Huiming Wang
Chen Li, Meng Zhang, Maoqing Tian, Zeyu Tang, Yuying Hu, Yuyu Long, Xiaofei Wang, Liwen Qiao, Jiefei Zeng, Yujuan Wang, Xinghua Chen, Cheng Chen, Xiaoyan Li, Lu Zhang, Huiming Wang
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Research Article Cell biology Nephrology

A TGF-β1/LEF1/β-catenin/JLP network motif regulates autophagy and tubule injury in renal fibrosis

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Abstract

Sustained injury to renal tubular epithelial cells (TECs), driven by excessive autophagy, is a critical mechanism underlying kidney fibrosis. Our previous work identified JLP — a TEC-expressed scaffolding protein — as an endogenous antifibrotic factor that counteracts TGF-β1–induced autophagy and fibrogenesis. However, the mechanism underlying JLP downregulation in renal fibrosis remains unclear. Here, we delineated a TGF-β1/LEF1/β-catenin/JLP axis that governs TEC autophagy through a dichotomous regulatory circuit. Under physiological conditions, low levels of β-catenin and LEF1 with minimal nuclear localization permitted normal JLP expression, which in turn maintained autophagy in check. In contrast, during renal injury, TGF-β1 promoted the expression and nuclear translocation of β-catenin and LEF1, which together suppressed JLP transcription. This loss of JLP-mediated inhibition led to unchecked autophagy and exacerbated fibrotic damage. Analyses of kidney tissues from patients with CKD, murine fibrotic kidneys, and cultured HK-2 cells confirmed consistent JLP downregulation accompanied by upregulation and nuclear accumulation of LEF1 and β-catenin. Therapeutic intervention using the β-catenin/LEF1 inhibitor iCRT3 or LEF1-targeted silencing in murine fibrosis models restored JLP expression, attenuated TEC autophagy, and ameliorated renal fibrosis. These findings revealed an autoregulatory circuit controlling TEC autophagy and fibrogenesis, and supported LEF1 and β-catenin as potential therapeutic targets in CKD.

Authors

Chen Li, Meng Zhang, Maoqing Tian, Zeyu Tang, Yuying Hu, Yuyu Long, Xiaofei Wang, Liwen Qiao, Jiefei Zeng, Yujuan Wang, Xinghua Chen, Cheng Chen, Xiaoyan Li, Lu Zhang, Huiming Wang

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Figure 5

Renal tubule–specific Lef1 deficiency ameliorates renal fibrosis.

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Renal tubule–specific Lef1 deficiency ameliorates renal fibrosis.
(A) Gr...
(A) Gross appearance of kidneys from the indicated groups. (B) Photomicrographs exhibiting the H&E staining of kidney sections from the indicated groups. Scale bar: 2 mm. (C) Schematic diagram indicating the region of the kidney (renal cortex, highlighted area) used for histological and molecular analyses. (D) H&E, Masson’s trichrome, and Sirius red staining of kidney tissues from the indicated group. Tubular damage score was quantified from staining; the percentage of tubulointerstitial fibrosis was quantified from Masson’s trichrome– or Sirius red–stained kidney sections using ImageJ (n = 6 mice per group). Scale bars: 50 μm. (E) Immunohistochemical staining of fibronectin, collagen I, JLP, and LEF1 in kidney tissues with quantitative analysis (n = 6 mice per group). Scale bars: 50 μm. (F and G) Western blot analysis and densitometric analysis of LEF1, JLP, fibronectin, and collagen I normalized to GAPDH (n = 6 mice per group). (H) Relative mRNA levels in kidney tissues in the 4 groups were calculated by normalization to GAPDH mRNA (n = 6 mice per group). (I) Representative TEM images of renal tubular cells from indicated groups. Scale bars: 2 μm and 1 μm (enlarged insets). (J) Quantification of results in I. The number of autophagosomes was counted per field. Statistical analyses were performed on data from 5 independent experiments, with counts of more than 30 fields (n = 6 mice per group). (K and L) Immunofluorescence of LC3 (green) and DAPI (blue) in kidney sections from indicated groups. L shows quantification of results in K (n = 6 mice per group). Scale bars: 50 μm and 20 μm (enlarged insets). (M and N) Immunoblot analysis of LC3, Beclin-1, and p62 in sham or UUO mouse kidneys from Lef1cKO and Lef1fl/fl littermate mice (n = 6 mice per group). Statistical analysis was performed using 1-way ANOVA followed by Tukey’s multiple-comparison test (D, E, G, H, J, L, and N). Data are mean ± SD.

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