MDR1 in taste buds of rat vallate papilla: functional, immunohistochemical, and biochemical evidence

Author:

Jakob Ingrid1,Hauser Ingeborg A.2,Thévenod Frank1,Lindemann Bernd1

Affiliation:

1. Department of Physiology, Saar University, D-66421 Homburg; and

2. Department of Internal Medicine IV, University of Erlangen-Nürnberg, D-90471 Nürnberg, Germany

Abstract

Multidrug resistance P-glycoprotein (MDR1) is a membrane protein of 150–170 kDa that catalyzes the ATP-driven efflux of hydrophobic xenobiotics, including fluorescent dyes, from cells. Expressed in many epithelial tissues and in the endothelia of the blood-brain barrier, the MDR1 protein provides major routes of detoxification. We found that taste cells of the rat vallate papilla (VP; posterior tongue) had only a slow increase in fluorescence due to uptake of the hydrophobic dye calcein acetoxymethyl ester. However, the development of fluorescence was accelerated two- to threefold by substrates and/or inhibitors of MDR1, such as verapamil, tamoxifen, and cyclosporin A, and by addition of the transport-blocking antibody to MDR1, UIC2. Western blots of vallate tissue rich in taste buds with the MDR1-specific monoclonal antibodies C219 and C494 revealed an immunoreactive protein at ∼170 kDa. In contrast, the lingual epithelium surrounding the VP showed a much weaker band with these antibodies. Furthermore, using the antibodies C494 and UIC2 with tissue sections, MDR1-like immunoreactivity was found in taste cells. These results show that MDR1 is present and functional in vallate taste cells of the rat. MDR1-related transport may achieve active elimination of xenobiotics from the sensory cells and thereby protect the peripheral taste organs from potentially harmful molecules contained in an animal’s food.

Publisher

American Physiological Society

Subject

Cell Biology,Physiology

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