Purine nucleoside phosphorylase inhibition is an effective approach for the treatment of chemical hemorrhagic cystitis
Amanda Wolf-Johnston, … , Edwin K. Jackson, Lori A. Birder
Amanda Wolf-Johnston, … , Edwin K. Jackson, Lori A. Birder
Published January 25, 2024
Citation Information: JCI Insight. 2024;9(5):e176103. https://doi.org/10.1172/jci.insight.176103.
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Research Article Inflammation

Purine nucleoside phosphorylase inhibition is an effective approach for the treatment of chemical hemorrhagic cystitis

Abstract

Hemorrhagic cystitis may be induced by infection, radiation therapy, or medications or may be idiopathic. Along with hemorrhagic features, symptoms include urinary urgency and frequency, dysuria (painful urination), and visceral pain. Cystitis-induced visceral pain is one of the most challenging types of pain to treat, and an effective treatment would address a major unmet medical need. We assessed the efficacy of a purine nucleoside phosphorylase inhibitor, 8-aminoguanine (8-AG), for the treatment of hemorrhagic/ulcerative cystitis. Lower urinary tract (LUT) function and structure were assessed in adult Sprague-Dawley rats, treated chronically with cyclophosphamide (CYP; sacrificed day 8) and randomized to daily oral treatment with 8-AG (begun 14 days prior to CYP induction) or its vehicle. CYP-treated rats exhibited multiple abnormalities, including increased urinary frequency and neural mechanosensitivity, reduced bladder levels of inosine, urothelial inflammation/damage, and activation of spinal cord microglia, which is associated with pain hypersensitivity. 8-AG treatment of CYP-treated rats normalized all observed histological, structural, biochemical, and physiological abnormalities. In cystitis 8-AG improved function and reduced both pain and inflammation likely by increasing inosine, a tissue-protective purine metabolite. These findings demonstrate that 8-AG has translational potential for reducing pain and preventing bladder damage in cystitis-associated LUT dysfunctions.

Authors

Amanda Wolf-Johnston, Youko Ikeda, Irina Zabbarova, Anthony J. Kanai, Sheldon Bastacky, Robert Moldwin, Joel N.H. Stern, Edwin K. Jackson, Lori A. Birder

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Figure 2

8-AG attenuates CYP-associated morphological and histological changes to the urinary bladder mucosa.

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8-AG attenuates CYP-associated morphological and histological changes to...
(AF) Representative images (from 4 experiments) show CYP-associated mucosal hemorrhage (B) versus control (A) and damage to the apical urothelial surface (shown at arrows) in CYP-bladder (E) versus control bladder (D). Inset panel (E) depicts reactive epithelial cells with large, multinucleated nuclei in CYP-bladders as compared with control. (G and H) Western immunoblotting revealed decreases in the urothelial umbrella cell proteins cytokeratin 20 (G; n = 11–16 per group) and uroplakin III (H; n = 13–16 per group) in CYP-bladders compared with control rat bladders. Upper insets (G and H) show representative bands from cytokeratin 20 and uroplakin III Western immunoblotting. Densitometry was normalized to total protein staining (loading control [LC]; representative bands shown in lower inset). Representative bands were run on the same blot but were noncontiguous. (C and FH) 8-AG treatment restored the abnormal morphological and histological changes to a control state. (AC) Scale bars: 5 mm. (DF) Scale bars: 50 μm and original magnification 40×. (DF insets) Scale bars: 20 μm and original magnification 100×. Data are presented as means ± SD. Ordinary 1-way ANOVA followed by Tukey’s post hoc multiple comparison test was used to evaluate significance; *P < 0.05, **P < 0.01; ****P < 0.00001.