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Renal Division, Department of Medicine, Emory University School of
Medicine, Atlanta, Georgia
Department of Physiology, Emory University School of Medicine, Atlanta,
Georgia
Correspondence to Dr. Jeff M. Sands, Emory University School of Medicine, Renal Division, WMRD Room 338, 1639 Pierce Drive, NE, Atlanta, GA 30322. Phone: 404-727-2435; Fax: 404-727-3425; E-mail: jsands{at}emory.edu
Abstract. In perfused rat liver, there is phloretin-inhibitable urea efflux, but whether it is mediated by the kidney UT-A urea transporter family is unknown. To determine whether cultured HepG2 cells transport urea, thiourea influx was measured. HepG2 cells had a thiourea influx rate of 1739 ± 156 nmol/g protein per min; influx was inhibited 46% by phloretin and 32% by thionicotinamide. Western analysis of HepG2 cell lysate using an antibody to UT-A1, UT-A2, and UT-A4 revealed two protein bands: 49 and 36 kD. The same bands were detected in cultured rat hepatocytes, freshly isolated rat hepatocytes, and in liver from rat, mouse, and chimpanzee. Both bands were present when analyzed by native gel electrophoresis, and deglycosylation of rat liver lysate had no effect on either band. Differential centrifugation of rat liver lysate showed that the 49-kD protein is in the membrane fraction and the 36-kD protein is in the cytoplasm. To determine whether the abundance of these UT-A proteins varies in vivo, rats were made uremic by 5/6 nephrectomy. The 49-kD protein was significantly increased 5.5-fold in livers from uremic rats compared to pair-fed control rats. It is concluded that phloretininhibitable urea flux in liver may occur via a 49-kD protein that is specifically detected by a UT-A antibody. Uremia increases the abundance of this 49-kD UT-A protein in rat liver in vivo.
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R. A. Fenton, G. S. Stewart, B. Carpenter, A. Howorth, E. A. Potter, G. J. Cooper, and C. P. Smith Characterization of mouse urea transporters UT-A1 and UT-A2 Am J Physiol Renal Physiol, October 1, 2002; 283(4): F817 - F825. [Abstract] [Full Text] [PDF] |
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