Autocrine lysophosphatidic acid signaling activates β-catenin and promotes lung allograft fibrosis
Pengxiu Cao, … , Eric R. Fearon, Vibha N. Lama
Pengxiu Cao, … , Eric R. Fearon, Vibha N. Lama
Published February 27, 2017
Citation Information: J Clin Invest. 2017;127(4):1517-1530. https://doi.org/10.1172/JCI88896.
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Research Article Cell biology Transplantation

Autocrine lysophosphatidic acid signaling activates β-catenin and promotes lung allograft fibrosis

Abstract

Tissue fibrosis is the primary cause of long-term graft failure after organ transplantation. In lung allografts, progressive terminal airway fibrosis leads to an irreversible decline in lung function termed bronchiolitis obliterans syndrome (BOS). Here, we have identified an autocrine pathway linking nuclear factor of activated T cells 2 (NFAT1), autotaxin (ATX), lysophosphatidic acid (LPA), and β-catenin that contributes to progression of fibrosis in lung allografts. Mesenchymal cells (MCs) derived from fibrotic lung allografts (BOS MCs) demonstrated constitutive nuclear β-catenin expression that was dependent on autocrine ATX secretion and LPA signaling. We found that NFAT1 upstream of ATX regulated expression of ATX as well as β-catenin. Silencing NFAT1 in BOS MCs suppressed ATX expression, and sustained overexpression of NFAT1 increased ATX expression and activity in non-fibrotic MCs. LPA signaling induced NFAT1 nuclear translocation, suggesting that autocrine LPA synthesis promotes NFAT1 transcriptional activation and ATX secretion in a positive feedback loop. In an in vivo mouse orthotopic lung transplant model of BOS, antagonism of the LPA receptor (LPA1) or ATX inhibition decreased allograft fibrosis and was associated with lower active β-catenin and dephosphorylated NFAT1 expression. Lung allografts from β-catenin reporter mice demonstrated reduced β-catenin transcriptional activation in the presence of LPA1 antagonist, confirming an in vivo role for LPA signaling in β-catenin activation.

Authors

Pengxiu Cao, Yoshiro Aoki, Linda Badri, Natalie M. Walker, Casey M. Manning, Amir Lagstein, Eric R. Fearon, Vibha N. Lama

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Figure 3

Increased ATX expression and activity in BOS MCs.

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Increased ATX expression and activity in BOS MCs. (A) Basal ATX expressi...
(A) Basal ATX expression in BOS and non-BOS MCs was measured by immunoblotting in whole cell lysates. Mean ± SEM (n = 7/group) with unpaired t test. (B) ATX expression in cell supernatant (24-hour collection) was quantitated by ELISA. Mean ± SEM (n = 12/group) with unpaired t test. (C) Cell supernatant collected after 72 hours of incubation from BOS and non-BOS MCs was concentrated, and ATX activity was assayed using the fluorogenic phospholipid ATX substrate FS-3 (n = 4 for BOS MCs and 5 for non-BOS MCs with ANOVA). Data were repeated in 3 independent experiments. Mean ± SEM. **P < 0.01, ****P < 0.0001. (D). Serial sections from lung allografts of patients with BOS collected at autopsy were analyzed by immunohistochemistry for ATX or α-SMA and counterstained with hematoxylin. Two separate areas with completely obliterated airways are shown in the top and bottom panels. Arrows indicated the obliterated bronchi. Scale bars: 80 μm for ×100 images and 200 μm for ×40 images.