Abstract

The mammalian kidney has a substantial capacity to excrete an alkaline load. For example, rodents given isotonic NaHCO3 in their drinking water develop only a mild metabolic alkalosis despite this huge base load. The kidney's ability to excrete large alkaline loads occurs in part through active HCO3- secretion in the cortical collecting duct (CCD) mediated by apical anion exchange in the B intercalated cell. While apical anion exchange has been characterized functionally in the CCD, the gene product, which mediates this transport process has remained an area of controversy. However the work of our laboratory and that of our collaborators has demonstrated that pendrin, an anion exchanger, localizes to the apical membrane of non-A intercalated cells in rat, human and mouse. Moreover, our laboratory has demonstrated that pendrin mediates secretion of HCO3- in the mouse CCD. Whether this transporter represents the putative apical anion exchanger remains to be tested fully. Development of knockout mice has greatly facilitated the study of the renal physiology of pendrin in vivo. Because there are no specific inhibitors of either pendrin or apical anion exchange available, knockout mice can be exploited as a biological inhibitor and used to test transport characteristics of pendrin in kidney in vitro. Moreover, balance studies using these animals will allow us to determine if these pendrin-deficient mice have a defect in excretion of an alkaline load. Thus, the present proposal will test if pendrin represents the putative anion exchanger of the CCD. Moreover, these studies will contribute to our understanding of the physiological role of this transporter. To answer these questions our laboratory and that of our collaborators will employ balance studies, tubules perfused in vitro, real-time quantitative RT-PCR, immunogold cytochemistry and immunohistochemistry studies in wild type and pendrin-deficient mice.
The Specific Aims of the project are: 1. To determine the transport characteristics of pendrin in native renal tissue, 2. To determine if pendrin is upregulated in kidney during metabolic alkalosis, 3. To determine the renal phenotype of pendrin and 4. To determine the localization of pendrin in kidney. These studies will contribute to our understanding of how the mammalian kidney excretes an alkaline load.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Institute of Diabetes and Digestive and Kidney Diseases (NIDDK)
Type
Research Project (R01)
Project #
5R01DK052935-07
Application #
6621959
Study Section
General Medicine B Study Section (GMB)
Program Officer
Ketchum, Christian J
Project Start
1997-08-01
Project End
2006-07-31
Budget Start
2003-08-01
Budget End
2004-07-31
Support Year
7
Fiscal Year
2003
Total Cost
$290,702
Indirect Cost

  Institution

Name
Emory University
Department
Internal Medicine/Medicine
Type
Schools of Medicine
DUNS #
066469933
City
Atlanta
State
GA
Country
United States
Zip Code
30322

  Publications

Pech, Vladimir; Thumova, Monika; Kim, Young Hee et al. (2012) ENaC inhibition stimulates Cl- secretion in the mouse cortical collecting duct through an NKCC1-dependent mechanism. Am J Physiol Renal Physiol 303:F45-55
Verlander, Jill W; Hong, Seongun; Pech, Vladimir et al. (2011) Angiotensin II acts through the angiotensin 1a receptor to upregulate pendrin. Am J Physiol Renal Physiol 301:F1314-25
Wall, Susan M; Pech, Vladimir (2010) Pendrin and sodium channels: relevance to hypertension. J Nephrol 23 Suppl 16:S118-23
Leviel, Françoise; Hübner, Christian A; Houillier, Pascal et al. (2010) The Na+-dependent chloride-bicarbonate exchanger SLC4A8 mediates an electroneutral Na+ reabsorption process in the renal cortical collecting ducts of mice. J Clin Invest 120:1627-35
Pech, Vladimir; Pham, Truyen D; Hong, Seongun et al. (2010) Pendrin modulates ENaC function by changing luminal HCO3-. J Am Soc Nephrol 21:1928-41
Pech, Vladimir; Kim, Young Hee; Weinstein, Alan M et al. (2007) Angiotensin II increases chloride absorption in the cortical collecting duct in mice through a pendrin-dependent mechanism. Am J Physiol Renal Physiol 292:F914-20
Verlander, Jill W; Kim, Young Hee; Shin, Wonkyong et al. (2006) Dietary Cl(-) restriction upregulates pendrin expression within the apical plasma membrane of type B intercalated cells. Am J Physiol Renal Physiol 291:F833-9
Jabba, Sairam V; Oelke, Alisha; Singh, Ruchira et al. (2006) Macrophage invasion contributes to degeneration of stria vascularis in Pendred syndrome mouse model. BMC Med 4:37
Wall, Susan M (2006) The renal physiology of pendrin (SLC26A4) and its role in hypertension. Novartis Found Symp 273:231-9; discussion 239-43, 261-4
Kim, Young-Hee; Verlander, Jill W; Matthews, Sharon W et al. (2005) Intercalated cell H+/OH- transporter expression is reduced in Slc26a4 null mice. Am J Physiol Renal Physiol 289:F1262-72

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