A selective EP4 PGE2 receptor agonist alleviates disease in a new mouse model of X-linked nephrogenic diabetes insipidus
Jian Hua Li, … , Mark A. Knepper, Jürgen Wess
Jian Hua Li, … , Mark A. Knepper, Jürgen Wess
Published September 1, 2009
Citation Information: J Clin Invest. 2009;119(10):3115-3126. https://doi.org/10.1172/JCI39680.
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Research Article Nephrology

A selective EP4 PGE2 receptor agonist alleviates disease in a new mouse model of X-linked nephrogenic diabetes insipidus

Abstract

X-linked nephrogenic diabetes insipidus (XNDI) is a severe kidney disease caused by inactivating mutations in the V2 vasopressin receptor (V2R) gene that result in the loss of renal urine-concentrating ability. At present, no specific pharmacological therapy has been developed for XNDI, primarily due to the lack of suitable animal models. To develop what we believe to be the first viable animal model of XNDI, we generated mice in which the V2R gene could be conditionally deleted during adulthood by administration of 4-OH-tamoxifen. Radioligand-binding studies confirmed the lack of V2R-binding sites in kidneys following 4-OH-tamoxifen treatment, and further analysis indicated that upon V2R deletion, adult mice displayed all characteristic symptoms of XNDI, including polyuria, polydipsia, and resistance to the antidiuretic actions of vasopressin. Gene expression analysis suggested that activation of renal EP4 PGE2 receptors might compensate for the lack of renal V2R activity in XNDI mice. Strikingly, both acute and chronic treatment of the mutant mice with a selective EP4 receptor agonist greatly reduced all major manifestations of XNDI, including changes in renal morphology. These physiological improvements were most likely due to a direct action on EP4 receptors expressed on collecting duct cells. These findings illustrate the usefulness of the newly generated V2R mutant mice for elucidating and testing new strategies for the potential treatment of humans with XNDI.

Authors

Jian Hua Li, Chung-Lin Chou, Bo Li, Oksana Gavrilova, Christoph Eisner, Jürgen Schnermann, Stasia A. Anderson, Chu-Xia Deng, Mark A. Knepper, Jürgen Wess

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Figure 2

Loss of urinary concentrating ability in V2R-KO mice.

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Loss of urinary concentrating ability in V2R-KO mice. (A and B) 24-hour ...
(A and B) 24-hour urine output and water consumption of V2R mutant mice and control littermates. V2Rfl/yEsr1-Cre mice and V2Rfl/y control littermates were injected at the indicated days with a single dose of TMX (0.5 mg i.p./mouse). Daily urine output (A) and water consumption (B) were determined at the indicated days by using metabolic cages. (C and D) Urine osmolality and body weight of V2Rfl/yEsr1-Cre mice and control littermates. (EJ) Urine-concentrating ability of dDAVP. Urine osmolalities were determined immediately before and 1.5–2 hours after a single injection of dDAVP (0.4 μg/kg, i.p.). (E and F) Data obtained with individual V2Rfl/y and V2Rfl/yEsr1-Cre mice that had not been treated with TMX are shown (mouse age, 7 weeks). (G) Summary of the data shown in E and F. (H and I) Data obtained with individual TMX-treated V2Rfl/y mice (controls) and V2Rfl/yEsr1-Cre mice (V2R-KO mice; mouse age, 9 weeks). (J) Summary of data depicted in H and I. Data are shown as mean ± SEM. n = 5–7 per group.**P < 0.01; ***P < 0.001.