Am J Physiol Cell Physiol AJP: Gastrointestinal and Liver Physiology
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Am J Physiol Cell Physiol (August 20, 2003). doi:10.1152/ajpcell.00386.2002
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Submitted on August 26, 2002
Accepted on August 4, 2003

Purinergic-induced signaling in C11-MDCK cells inhibits the secretory Na-K-Cl cotransporter

Tatyana A Brindikova1, Nathalie Bourcier2, Brian Torres3, Dimitri Pchezhetski4, Michel Gekle5, Georgy V Maximov1, Valerie Montminy6, Paul A Insel3, Sergei N Orlov4, and Paul Isenring6*

1 Biology, MV Lomonosov Moscow State University, Moscow, Russian Federation
2 Medicine, Montreal University, Montreal, Quebec, Canada
3 Pharmacology, University of California, La Jolla, California, USA
4 Medicine, Montreal University, Montreal, Quebec, Canada; Biology, MV Lomonosov Moscow State University, Moscow, Russian Federation
5 Physiology, Wurzburg University, Wurzburg, Quebec, Germany
6 Medicine, Laval University, Quebec, Quebec, Canada

* To whom correspondence should be addressed. E-mail: paul.isenring{at}crhdq.ulaval.ca.

Purinergic inhibition of Na-K-Cl cotransport has been noted in various renal epithelial cells derived from the collecting tubule, including Madin-Darby canine kidney (MDCK) cells. In recent studies, we have observed purinergic inhibition of Na-K-Cl cotransport in C11-MDCK subclones ({alpha}-intercalated-like cells). Interestingly, Na-K-Cl cotransport activity was also detected in C7-MDCK subclones (principal-like cells) but was not affected by ATP. In this investigation, we have transfected human Na-K-Cl cotransporter (huNKCC1) in both C11 and C7 cells to determine whether these differences in NKCC regulation by ATP were due to cell-specific purinoceptor signaling pathways or cell-specific isoforms/splice variants of the transporter. In both cell lines, we found that endogenous as well as huNKCC1-derived cotransport activity was restricted to the basolateral side. In addition, we were able to show that extracellular application of 100 µM ATP or 100 µM UTP abolished NKCC activity in both mock- and huNKCC1-transfected C11 cells but not in mock- and huNKCC1-transfected C7 cells; in C11 cells, intriguingly, this inhibition was not affected by inhibitors of RNA and protein synthesis and occurred even though expression levels of UTP-sensitive P2Y2-, P2Y4-, and P2Y6-purinoceptors were not different from those observed in C7 cells. These results suggest that C11 cells express an undetermined type of UTP-sensitive P2-purinoceptors or a unique P2Y-purinoceptor-triggered signaling cascade that leads to inhibition of NKCC1.




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