Notch controls urothelial integrity in the mouse bladder
Varvara Paraskevopoulou, … , Ioannis S. Pateras, Apostolos Klinakis
Varvara Paraskevopoulou, … , Ioannis S. Pateras, Apostolos Klinakis
Published February 13, 2020
Citation Information: JCI Insight. 2020;5(3):e133232. https://doi.org/10.1172/jci.insight.133232.
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Research Article Cell biology

Notch controls urothelial integrity in the mouse bladder

Abstract

The Notch signaling pathway mediates cell-cell communication regulating cell differentiation and proliferation and cell fate decisions in various tissues. In the urinary bladder, Notch acts as a tumor suppressor in mice, while mutations in Notch pathway components have been identified in human bladder cancer as well. Here we report that the genetic inactivation of Notch in mice leads to downregulation of cell-cell and cell-ECM interaction components, including proteins previously implicated in interstitial cystitis/bladder pain syndrome (IC/BPS), structural defects and mucosal sloughing, inflammation, and leaky urine-blood barrier. Molecular profiling of ailing mouse bladders showed similarities with IC/BPS patient tissue, which also presented low Notch pathway activity as indicated by reduced expression of canonical Notch targets. Urothelial integrity was reconstituted upon exogenous reactivation of the Notch pathway, implying a direct involvement of Notch. Despite damage and inflammation, urothelial cells failed to proliferate, uncovering a possible role for α4 integrin in urothelial homeostasis. Our data uncover a broad role for Notch in bladder homeostasis involving urothelial cell crosstalk with the microenvironment.

Authors

Varvara Paraskevopoulou, Vangelis Bonis, Vasilis S. Dionellis, Nikolaos Paschalidis, Pelagia Melissa, Evangelia Chavdoula, Eleni Vasilaki, Ioannis S. Pateras, Apostolos Klinakis

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Figure 2

Notch inactivation leads to bladder inflammation.

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Notch inactivation leads to bladder inflammation. (A) Immunofluorescence...
(A) Immunofluorescence on bladder sections from WT and Krt5CreERT2 Ncstnfl/fl or Krt5CreERT2 RBPJfl/fl mice with antibodies against KRT5 and the leukocyte marker CD45. Arrowheads in WT mice indicate positive stromal cells. Scale bars: 100 μm. DAPI was used as nuclear counterstain. (B) Analysis of mass cytometry data on leukocytic populations of bladder tissue from WT and Krt5CreERT2 Ncstnfl/fl mice (n = 10 in each group). Scatter dot plots from normalized data showing expression of CD45, CD3, CD4, CD8, B220, and CD11b. CD3 marks all T cells, CD4 detects helper T cells, CD8 is expressed in cytotoxic T cells, B220 is expressed in B cells, and CD11b is a common myeloid marker. Representative of 3 experiments. (C) Toluidine blue staining on WT and Notch-deficient mice of indicated genotypes marking mast cells. Arrowheads depict positive stromal mast cells that stain red/purple (metachromasia). Scale bars: 100 μm, 25 μm (insets). Scatter dot plot indicates toluidine blue–stained cells per 10 high-power fields (HPFs, original magnification, ×400) (y axis) per bladder analyzed from each group. Data presented are mean ± SEM. Number of mice analyzed: 4, 9, 7, 6, and 3, respectively, for the 5 groups shown. *P < 0.05. Student’s t test was used and P values were corrected for multiple testing using the Benjamini-Hochberg method.