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IL-13 and calpain-14 suppress the expression of SPINK7 by regulating OVOL1 in eosinophilic esophagitis
Nurit P. Azouz, Andrea M. Klingler, Sierra S. Beach, Kalen Rossey, Mark Rochman, Misu Paul, Julie M. Caldwell, Michael Brusilovsky, Alexander T. Dwyer, Xiaoting Chen, Daniel Miller, Carmy Forney, Leah C. Kottyan, Matthew T. Weirauch, Marc E. Rothenberg
Nurit P. Azouz, Andrea M. Klingler, Sierra S. Beach, Kalen Rossey, Mark Rochman, Misu Paul, Julie M. Caldwell, Michael Brusilovsky, Alexander T. Dwyer, Xiaoting Chen, Daniel Miller, Carmy Forney, Leah C. Kottyan, Matthew T. Weirauch, Marc E. Rothenberg
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Research Article Gastroenterology Immunology Inflammation

IL-13 and calpain-14 suppress the expression of SPINK7 by regulating OVOL1 in eosinophilic esophagitis

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Abstract

Eosinophilic esophagitis (EoE) is a type 2 allergic disease characterized by esophageal inflammation and epithelial cell dysfunction. The acquired loss of the anti–serine protease of kazal type 7 (anti-SPINK7) in the squamous epithelium of the esophagus has a causal role in EoE pathogenesis. However, there is a limited understanding of the factors that regulate its expression and responsiveness to inflammatory stimuli. Herein, we have identified the transcription factor, ovo like transcriptional repressor 1 (OVOL1), as an esophageal selective gene product that regulates SPINK7 promoter activity. Overexpression of OVOL1 increased SPINK7 expression, whereas its depletion decreased SPINK7 expression, impaired epithelial barrier, and increased production of the proatopy cytokine thymic stromal lymphopoietin (TSLP). Stimulation with IL-13 abrogated the nuclear translocation of OVOL1 and promoted enhanced degradation of OVOL1 protein. This effect of IL-13 was dependent on the esophageal specific cysteine protease calpain-14 at least in part. Analysis of human esophageal biopsies demonstrated that the expression of esophageal OVOL1 correlated with SPINK7 transcript expression and was lost as a function of EoE disease activity. In summary, our study identifies key regulatory mechanisms in EoE pathogenesis, demonstrating that OVOL1 promotes SPINK7 transcription, whereas IL-13 suppresses this pathway in EoE.

Authors

Nurit P. Azouz, Andrea M. Klingler, Sierra S. Beach, Kalen Rossey, Mark Rochman, Misu Paul, Julie M. Caldwell, Michael Brusilovsky, Alexander T. Dwyer, Xiaoting Chen, Daniel Miller, Carmy Forney, Leah C. Kottyan, Matthew T. Weirauch, Marc E. Rothenberg

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Figure 6

Posttranslational modification of OVOL1 induced by IL-13.

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Posttranslational modification of OVOL1 induced by IL-13.
(A) Western bl...
(A) Western blot analysis of OVOL1, DSG1, and GAPDH expression in differentiated EPC2 cells that were either left untreated (UT) or stimulated with IL-13 (100 ng/mL) for 48 hours. The graphs on the right show quantification of OVOL1 and DSG1 relative to GAPDH with or without IL-13 treatment from paired UT/IL-13 samples from 6 independent experiments. P values were calculated by paired Student’s t test. (B) qPCR analysis of OVOL1 and DSG1 mRNA expression in differentiated EPC2 cells that were either left untreated or stimulated with IL-13 (100 ng/mL) for 48 hours; expression is normalized to GAPDH. P values were calculated by paired Student’s t test. (C) Western blot analysis of OVOL1 and calpain 14 expression in differentiated EPC2 cells with inducible expression of CAPN14 expression. CAPN14 is fused to a flag tag and is induced by doxycycline (Dox) treatment. (D and E) qPCR analysis of OVOL1 (D) and SPINK7 (E) in differentiated EPC2 with inducible expression of CAPN14 expression of CAPN14; expression is normalized to GAPDH. P values were calculated by unpaired Student’s t test. (F) Western blot analysis of OVOL1 in GFP-overexpressing or CAPN14-GFP–overexpressing cells with or without IL-13 treatment. GAPDH was used as a loading control. Anti-GFP was used for detection of GFP and CAPN14-GFP. (G) Western blot analysis of recombinant human OVOL1-GST (60 ng) that was either left untreated or incubated with nonnuclear protein fractions (C) or nuclear protein fractions (N) for the indicated times. The graph on the right is a quantification of OVOL1 band intensity (OD) shown from the left. UT, untreated.

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