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Site-1 protease–derived soluble (pro)renin receptor targets vasopressin receptor 2 to enhance urine concentrating capability
Fei Wang, Chuanming Xu, Renfei Luo, Kexin Peng, Nirupama Ramkumar, Shiying Xie, Xiaohan Lu, Long Zhao, Chang-Jiang Zuo, Donald E. Kohan, Tianxin Yang
Fei Wang, Chuanming Xu, Renfei Luo, Kexin Peng, Nirupama Ramkumar, Shiying Xie, Xiaohan Lu, Long Zhao, Chang-Jiang Zuo, Donald E. Kohan, Tianxin Yang
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Research Article Nephrology

Site-1 protease–derived soluble (pro)renin receptor targets vasopressin receptor 2 to enhance urine concentrating capability

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Abstract

The antidiuretic hormone vasopressin (AVP), acting through its type 2 receptor (V2R) in the collecting duct (CD), critically controls urine concentrating capability. Here, we report that site-1 protease–derived (S1P-derived) soluble (pro)renin receptor (sPRR) participates in regulation of fluid homeostasis via targeting V2R. In cultured inner medullary collecting duct (IMCD) cells, AVP-induced V2R expression was blunted by a PRR antagonist, PRO20; a PRR-neutralizing antibody; or a S1P inhibitor, PF-429242. In parallel, sPRR release was increased by AVP and reduced by PF-429242. Administration of histidine-tagged sPRR, sPRR-His, stimulated V2R expression and also reversed the inhibitory effect of PF-429242 on the expression induced by AVP. PF-429242 treatment in C57/BL6 mice impaired urine concentrating capability, which was rescued by sPRR-His. This observation was recapitulated in mice with renal tubule–specific deletion of S1P. During the pharmacological or genetic manipulation of S1P alone or in combination with sPRR-His, the changes in urine concentration were paralleled with renal expression of V2R and aquaporin-2 (AQP2). Together, these results support that S1P-derived sPRR exerts a key role in determining renal V2R expression and, thus, urine concentrating capability.

Authors

Fei Wang, Chuanming Xu, Renfei Luo, Kexin Peng, Nirupama Ramkumar, Shiying Xie, Xiaohan Lu, Long Zhao, Chang-Jiang Zuo, Donald E. Kohan, Tianxin Yang

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Figure 5

Validation of inducible renal tubule–specific deletion of S1P.

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Validation of inducible renal tubule–specific deletion of S1P.
(A) Schem...
(A) Schematic illustration of the PCR strategy to detect the floxed and recombined alleles by using primers P1 × P2 and P1 × P3, respectively. (B) PCR amplification using P1 × P2 to detect the floxed allele from various organs of S1Pfl/fl-Cre+ and S1Pfl/fl-Cre– mice following doxycycline treatment. WT denotes C57/BL6 mouse. This amplification resulted in a 434-bp product from the floxed allele and a 380-bp product from WT allele. (C) PCR amplification using P1 × P3 to detect the recombined allele from various organs of S1Pfl/fl-Cre+ following doxycycline treatment. The recombined allele was detected as an 1800-bp product. (D) Confirmation of renal S1P deletion at protein level. Immunoblotting analysis of renal S1P protein expression in mice with the indicated genotypes following the same doxycycline treatment.

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