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Forskolin stimulates phosphorylation and membrane accumulation of UT-A3

UT-A1 is regulated by vasopressin and is localized to the apical membrane and intracellular compartment of inner medullary collecting duct (IMCD) cells. UT-A3 is also expressed in the IMCD and is regulated by forskolin in heterologous systems. The goal of the present study is to investigate mechanis...

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Published in:	American journal of physiology. Renal physiology 2007-10, Vol.293 (4), p.F1308-F1313
Main Authors:	Blount, Mitsi A, Klein, Janet D, Martin, Christopher F, Tchapyjnikov, Dmitry, Sands, Jeff M
Format:	Article
Language:	English
Subjects:	Animals Antidiuretic Agents - pharmacology Cell Membrane - metabolism Cells Colforsin - pharmacology Kidney Medulla - cytology Kidney Medulla - metabolism Kidney Tubules, Collecting - cytology Kidney Tubules, Collecting - metabolism Kidneys Membrane Transport Proteins - metabolism Membranes Phosphorylation - drug effects Proteins Rats Rats, Sprague-Dawley Rodents Studies Urea Transporters Vasopressins - pharmacology
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container_title	American journal of physiology. Renal physiology
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creator	Blount, Mitsi A Klein, Janet D Martin, Christopher F Tchapyjnikov, Dmitry Sands, Jeff M
description	UT-A1 is regulated by vasopressin and is localized to the apical membrane and intracellular compartment of inner medullary collecting duct (IMCD) cells. UT-A3 is also expressed in the IMCD and is regulated by forskolin in heterologous systems. The goal of the present study is to investigate mechanisms by which vasopressin regulates UT-A3 in rat IMCD. In fresh suspensions of rat IMCD, forskolin increases the phosphorylation of UT-A3, similar to UT-A1. Biotinylation studies indicate that UT-A3 is located in the plasma membrane. Forskolin treatment increases the abundance of UT-A3 in the plasma membrane similar to UT-A1. However, these two transporters do not form a complex through a protein-protein interaction, suggesting that transporter function is unique to each protein. While immunohistochemistry localized UT-A3 to the basal and lateral membranes, a majority of the staining was cytosolic. Immunohistochemistry of vasopressin-treated rat kidney sections also localized UT-A3 primarily to the cytosol with basal and lateral membrane staining but also showed some apical membrane staining in some IMCD cells. This suggests that under normal conditions, UT-A3 functions as the basolateral transporter but in a high cAMP environment, the transporter may move from the cytosol to all plasma membranes to increase urea flux in the IMCD. In summary, this study confirms that UT-A3 is located in the inner medullary tip where it is expressed in the basolateral membrane, shows that UT-A3 is a phosphoprotein in rat IMCD that can be trafficked to the plasma membrane independent of UT-A1, and suggests that vasopressin may induce UT-A3 expression in the apical plasma membrane of IMCD.
doi_str_mv	10.1152/ajprenal.00197.2007
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UT-A3 is also expressed in the IMCD and is regulated by forskolin in heterologous systems. The goal of the present study is to investigate mechanisms by which vasopressin regulates UT-A3 in rat IMCD. In fresh suspensions of rat IMCD, forskolin increases the phosphorylation of UT-A3, similar to UT-A1. Biotinylation studies indicate that UT-A3 is located in the plasma membrane. Forskolin treatment increases the abundance of UT-A3 in the plasma membrane similar to UT-A1. However, these two transporters do not form a complex through a protein-protein interaction, suggesting that transporter function is unique to each protein. While immunohistochemistry localized UT-A3 to the basal and lateral membranes, a majority of the staining was cytosolic. Immunohistochemistry of vasopressin-treated rat kidney sections also localized UT-A3 primarily to the cytosol with basal and lateral membrane staining but also showed some apical membrane staining in some IMCD cells. This suggests that under normal conditions, UT-A3 functions as the basolateral transporter but in a high cAMP environment, the transporter may move from the cytosol to all plasma membranes to increase urea flux in the IMCD. In summary, this study confirms that UT-A3 is located in the inner medullary tip where it is expressed in the basolateral membrane, shows that UT-A3 is a phosphoprotein in rat IMCD that can be trafficked to the plasma membrane independent of UT-A1, and suggests that vasopressin may induce UT-A3 expression in the apical plasma membrane of IMCD.</description><identifier>ISSN: 1931-857X</identifier><identifier>EISSN: 1522-1466</identifier><identifier>DOI: 10.1152/ajprenal.00197.2007</identifier><identifier>PMID: 17686955</identifier><language>eng</language><publisher>United States: American Physiological Society</publisher><subject>Animals ; Antidiuretic Agents - pharmacology ; Cell Membrane - metabolism ; Cells ; Colforsin - pharmacology ; Kidney Medulla - cytology ; Kidney Medulla - metabolism ; Kidney Tubules, Collecting - cytology ; Kidney Tubules, Collecting - metabolism ; Kidneys ; Membrane Transport Proteins - metabolism ; Membranes ; Phosphorylation - drug effects ; Proteins ; Rats ; Rats, Sprague-Dawley ; Rodents ; Studies ; Urea Transporters ; Vasopressins - pharmacology</subject><ispartof>American journal of physiology. 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Renal physiology</title><addtitle>Am J Physiol Renal Physiol</addtitle><description>UT-A1 is regulated by vasopressin and is localized to the apical membrane and intracellular compartment of inner medullary collecting duct (IMCD) cells. UT-A3 is also expressed in the IMCD and is regulated by forskolin in heterologous systems. The goal of the present study is to investigate mechanisms by which vasopressin regulates UT-A3 in rat IMCD. In fresh suspensions of rat IMCD, forskolin increases the phosphorylation of UT-A3, similar to UT-A1. Biotinylation studies indicate that UT-A3 is located in the plasma membrane. Forskolin treatment increases the abundance of UT-A3 in the plasma membrane similar to UT-A1. However, these two transporters do not form a complex through a protein-protein interaction, suggesting that transporter function is unique to each protein. While immunohistochemistry localized UT-A3 to the basal and lateral membranes, a majority of the staining was cytosolic. Immunohistochemistry of vasopressin-treated rat kidney sections also localized UT-A3 primarily to the cytosol with basal and lateral membrane staining but also showed some apical membrane staining in some IMCD cells. This suggests that under normal conditions, UT-A3 functions as the basolateral transporter but in a high cAMP environment, the transporter may move from the cytosol to all plasma membranes to increase urea flux in the IMCD. 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This suggests that under normal conditions, UT-A3 functions as the basolateral transporter but in a high cAMP environment, the transporter may move from the cytosol to all plasma membranes to increase urea flux in the IMCD. In summary, this study confirms that UT-A3 is located in the inner medullary tip where it is expressed in the basolateral membrane, shows that UT-A3 is a phosphoprotein in rat IMCD that can be trafficked to the plasma membrane independent of UT-A1, and suggests that vasopressin may induce UT-A3 expression in the apical plasma membrane of IMCD.</abstract><cop>United States</cop><pub>American Physiological Society</pub><pmid>17686955</pmid><doi>10.1152/ajprenal.00197.2007</doi></addata></record>
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subjects	Animals Antidiuretic Agents - pharmacology Cell Membrane - metabolism Cells Colforsin - pharmacology Kidney Medulla - cytology Kidney Medulla - metabolism Kidney Tubules, Collecting - cytology Kidney Tubules, Collecting - metabolism Kidneys Membrane Transport Proteins - metabolism Membranes Phosphorylation - drug effects Proteins Rats Rats, Sprague-Dawley Rodents Studies Urea Transporters Vasopressins - pharmacology
title	Forskolin stimulates phosphorylation and membrane accumulation of UT-A3
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