SOX2 regulates foregut squamous epithelial homeostasis and is lost during Barrett’s esophagus development
Ramon U. Jin, Yuanwei Xu, T. Mamie Lih, Yang-Zhe Huang, Toni M. Nittolo, Blake E. Sells, Olivia M. Dres, Jean S. Wang, Qing K. Li, Hui Zhang, Jason C. Mills
Ramon U. Jin, Yuanwei Xu, T. Mamie Lih, Yang-Zhe Huang, Toni M. Nittolo, Blake E. Sells, Olivia M. Dres, Jean S. Wang, Qing K. Li, Hui Zhang, Jason C. Mills
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Research Article Development Gastroenterology

SOX2 regulates foregut squamous epithelial homeostasis and is lost during Barrett’s esophagus development

Abstract

Esophageal adenocarcinoma is increasingly prevalent and is thought to arise from Barrett’s esophagus (BE), a metaplastic condition in which chronic acid and bile reflux transforms the esophageal squamous epithelium into a gastric-intestinal glandular mucosa. The molecular determinants driving this metaplasia are poorly understood. We developed a human BE organoid biobank that recapitulates BE’s molecular heterogeneity. Bulk and single-cell transcriptomics, supported by patient tissue analysis, revealed that BE differentiation reflects a balance between SOX2 (foregut/esophageal) and CDX2 (hindgut/intestinal) transcription factors. Using squamous-specific inducible Sox2-KO (Krt5CreER/+ Sox2Δ/Δ ROSA26tdTomato/+) mice, we observed increased basal proliferation, reduced squamous differentiation, and expanded metaplastic glands at the squamocolumnar junction, some tracing back to Krt5-expressing cells. CUT&RUN analysis showed SOX2 bound and promoted differentiation-associated targets (e.g., Krt13) and repressed proliferation-associated targets (e.g., Mki67). Thus, SOX2 is critical for foregut squamous epithelial differentiation, and its decreased expression is likely an initiating step in progression to BE and then to esophageal adenocarcinoma.

Authors

Ramon U. Jin, Yuanwei Xu, T. Mamie Lih, Yang-Zhe Huang, Toni M. Nittolo, Blake E. Sells, Olivia M. Dres, Jean S. Wang, Qing K. Li, Hui Zhang, Jason C. Mills

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Figure 6

Sox2 loss induces columnar expansion at the squamocolumnar junction.

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Sox2 loss induces columnar expansion at the squamocolumnar junction. (A...
(A) H&E, Alcian blue, and immunofluorescence for SOX2 (green) and cytokeratin 7 (CK7; red) staining of WT control and Sox2Δ/Δ forestomachs. Insets: magnified squamocolumnar junctions and glandular structures. Untreated (top), 1-month DOC-treated (middle), and more than 6-month DOC-treated (bottom). (B) Quantification of squamocolumnar junction areas (μm2, mean ± SEM) by CK7. Each point = average area from 3–7 squamocolumnar regions per mouse. Two-way ANOVA with Šidák’s post hoc test for genotype and treatment effects with P values indicated. (C) Alcian blue, tdTomato (brown), and Das-1 (red) staining in 1-month DOC-treated forestomachs. Insets highlight glandular changes at squamocolumnar junctions. Scale bars: 100 μm. Images are representative of at least 3 independent experiments. (D) Spatial proteomics from FFPE gastric strip tissue using on-site tissue protein labeling. Blue circles indicate 0.6 mm targeted regions. Mass spectrometry detected 4,862 peptide-spectrum matches (PSMs), 2,081 TMT-labeled peptides, and 814 proteins. (E) Comparative proteomics revealed 32 decreased and 782 increased proteins in Sox2Δ/Δ versus control squamocolumnar junctions. Top: GO analysis showed decreased proteins were enriched for Cell Differentiation and Development; increased proteins were enriched for Metabolism and Biosynthesis. Bottom: top 10 enriched proteins per group shown, based on Human Protein Atlas expression in squamous tissues (red) or stomach/intestines (green). (F) Gene set enrichment analysis using Human Protein Atlas tissue-specific genes/proteins for 36 tissues. Top decreased: squamous tissues (e.g., skin, vagina, and esophagus; esophagus shown). Top increased: stomach shown. Top 10 enriched/depleted tissue sets shown with normalized enrichment scores and P values.