Altered expression profile of transporters in the inner medullary collecting duct of aquaporin-1 knockout mice

doi:10.1152/ajprenal.00121.2004

Altered expression profile of transporters in the inner medullary collecting duct of aquaporin-1 knockout mice

Ryan G. Morris,¹ Shinichi Uchida,² Heddwen Brooks,³ Mark A. Knepper,¹ and Chung-Lin Chou¹

¹Laboratory of Kidney and Electrolyte Metabolism, National Heart, Lung, and Blood Institute, National Institutes of Health, Bethesda, Maryland; ²Department of Nephrology, Graduate School, Tokyo Medical and Dental University, Yushima Bunkyo-Ku, Tokyo, Japan; and ³Department of Physiology University of Arizona, Tuscon, Arizona

Submitted 6 April 2004 ; accepted in final form 3 February 2005

Aquaporin-1 is the major protein responsible for transport ofwater across the epithelia of the proximal tubule and thin descendinglimbs. Rapid water efflux across the thin descending limb isrequired for the normal function of the countercurrent multipliermechanism. Therefore, urinary concentrating capacity is severelyimpaired in aquaporin-1 knockout (AQP1 –/–) mice.Here, we have investigated the long-term consequences of deletionof the AQP1 gene product by profiling abundance changes in transportersexpressed in the inner medullas of AQP1 (–/–) micevs. heterozygotes [AQP1 (+/–)], which have a normal concentratingcapacity. Semiquantitative immunoblotting demonstrated markedsuppression of two proteins strongly expressed in the innermedullary collecting duct (IMCD): UT-A1 (a urea transporter)and AQP4 (a basolateral water channel). Furthermore, the ureapermeability of the IMCD was significantly reduced in AQP1 (–/–)mice. In contrast, there was increased expression of three proteinsnormally expressed at higher levels in the cortical collectingduct (CCD) than in IMCD: AQP3 (another basolateral water channel)and the epithelial sodium channel subunits ${beta}$ -ENaC and ${gamma}$ -ENaC.Changes in expression of these proteins were confirmed by immunocytochemistry.Messenger RNA profiling (real-time RT-PCR) revealed changesin UT-A1, ${beta}$ -ENaC, ${gamma}$ -ENaC, and AQP3 transcript abundance that paralleledthe changes in protein abundance. Thus, from the perspectiveof transport proteins, the IMCDs of AQP1 (–/–) micehave a significantly altered phenotype. To address whether thesechanges are specific to AQP1 (–/–) mice, we profiledIMCD transporter expression in a second knockout model manifestinga concentrating defect, that of ClC-nK1, a chloride channelin the ascending thin limb important for urinary concentration.As in the AQP1 knockout mice, ClC-nK1 (–/–) miceshowed decreased expression of UT-A1 and increased expressionof ${beta}$ -ENaC and ${gamma}$ -ENaC vs. WT controls. In conclusion, the expressionprofile of IMCD transporters is markedly altered in AQP1 –/–mice and this manifestation is related to the associated concentratingdefect.

ClC-nK1; urea

Address for reprint requests and other correspondence: C.-L. Chou, National Institutes of Health, Bldg. 10, Rm. 6N260, 10 Center Dr MSC 1603, Bethesda, MD 20892-1603 (e-mail: chouj{at}nhlbi.nih.gov)

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