Characterization and Long-Term Maintenance of Rat Taste Cells in Culture

doi:10.1093/chemse/bjj030

Chemical Senses Advance Access originally published online on February 1, 2006
Chemical Senses 2006 31(3):279-290; doi:10.1093/chemse/bjj030

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Characterization and Long-Term Maintenance of Rat Taste Cells in Culture

Hakan Ozdener¹, Karen K. Yee¹, Jie Cao¹, Joseph G. Brand¹^,2^,3, John H. Teeter¹ and Nancy E. Rawson¹

¹ Monell Chemical Senses Center, Philadelphia, PA 19104, USA, ² Department of Biochemistry, School of Dental Medicine, University of Pennsylvania, Philadelphia, PA 19104, USA and ³ Veterans Affairs Medical Center, Philadelphia, PA 19104, USA

Correspondence to be sent to: Hakan Ozdener, Monell Chemical Senses Center, Philadelphia, PA 19104-3308, USA. e-mail: hozdener{at}monell.org

Taste cells have a limited life span and are replaced from abasal cell population, although the specific factors involvedin this process are not well known. Short- and long-term culturesof other sensory cells have facilitated efforts to understandthe signals involved in proliferation, differentiation, andsenescence, yet few studies have reported successful primaryculture protocols for taste cells. Furthermore, no studies havedemonstrated both proliferation and differentiation in vitro.In this study, we have developed an in vitro culture systemto maintain and utilize rat primary taste cells for more than2 months without losing key molecular and biochemical features.Gustducin, phospholipase C-ß₂ (PLC-ß₂),T1R3, and T2R5 mRNA were detected in the cultured cells by reversetranscriptase–polymerase chain reaction. Western blotanalysis demonstrated gustducin and PLC-ß₂ expressionin the same samples, which was confirmed by immunocytochemistry.Labeling with bromo-2-deoxyuridine (BrdU) demonstrated proliferation,and a subset of BrdU-labeled cells were also immunoreactivefor either gustducin or PLC-ß₂, indicating differentiationof newly generated cells in vitro. Cultured cells also exhibitedincreases in intracellular calcium in response to several tastestimuli. These results indicate that taste cells from adultrats can be generated and maintained under the described conditionsfor at least 2 months. This system will enable further studiesof the processes involved in proliferation, differentiation,and function of mammalian taste receptor cells in an in vitropreparation.

Key words: culture, gustducin, imaging, proliferation, taste receptor

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