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Your search keyword '"Voigt, Anja"' showing total 6 results
Start Over Author "Voigt, Anja" Publisher oxford university press / usa
6 results on '"Voigt, Anja"'

1. Cre-Mediated Recombination in Tas2r131 Cells--A Unique Way to Explore Bitter Taste Receptor Function Inside and Outside of the Taste System.

Author

Voigt, Anja, Hübner, Sandra, Döring, Linda, Perlach, Nathalie, Hermans-Borgmeyer, Irm, Boehm, Ulrich, and Meyerhof, Wolfgang

Subjects
*TASTE receptors, *G protein coupled receptors, *GENETIC recombination, *GENE expression, *CELL populations
Abstract

The type 2 taste receptors (Tas2rs) comprise a large family of G protein-coupled receptors that recognize compounds bitter to humans and aversive to vertebrates. Tas2rs are expressed in both gustatory and nongustatory tissues, however, identification and functional analyses of T2Rexpressing cells have been difficult in most tissues. To overcome these limitations and to be able to manipulate Tas2r-expressing cells in vivo, we used gene-targeting to generate a Tas2r131-specific Cre knock-in mouse strain. We then employed a binary genetic approach to characterize Cremediated recombination in these animals and to investigate Tas2r131 expression during postnatal development. We demonstrate that a Cre-activated fluorescent reporter reliably visualizes Tas2r131- cells in gustatory tissue. We show that the onset of Tas2r131 as well as of a-Gustducin expression is initiated at different developmental stages depending on the type of taste bud. Furthermore, the number of Tas2r131- and a-Gustducin-expressing cells increased during postnatal development. Our results demonstrate that the Tas2r131-expressing cells constitute a subpopulation of a-Gustducin positive cells at all stages. We detected Tas2r131-expressing cells in several nongustatory tissues including lung, trachea, ovary, ganglia, and brain. Thus, the Tas2r131-Cre strain will help to dissect the functional role of Tas2r131 cells in both gustatory and nongustatory tissues in the future. [ABSTRACT FROM AUTHOR]

Published
2015
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2. A Binary Genetic Approach to Characterize TRPM5 Cells in Mice.

Author

Kusumakshi, Soumya, Voigt, Anja, Hübner, Sandra, Hermans-Borgmeyer, Irm, Ortalli, Ana, Pyrski, Martina, Dörr, Janka, Zufall, Frank, Flockerzi, Veit, Meyerhof, Wolfgang, Montmayeur, Jean-Pierre, and Boehm, Ulrich

Subjects
*TRP channels, *TASTE perception, *LABORATORY mice, *ALLELES, *FUNGIFORM papilla
Abstract

Transient receptor potential channel subfamily M member 5 (TRPM5) is an important downstream signaling component in a subset of taste receptor cells making it a potential target for taste modulation. Interestingly, TRPM5 has been detected in extra-oral tissues; however, the function of extra-gustatory TRPM5-expressing cells is less well understood. To facilitate visualization and manipulation of TRPM5-expressing cells in mice, we generated a Cre knock-in TRPM5 allele by homologous recombination. We then used the novel TRPM5-IRES-Cre mouse strain to report TRPM5 expression by activating a ΤGFP transgene. To conirm faithful coexpression of ΤGFP and TRPM5 we generated and validated a new anti-TRPM5 antiserum enabling us to analyze acute TRPM5 protein expression. ΤGFP cells were found in taste bud cells of the vallate, foliate, and fungiform papillae as well as in the palate. We also detected TRPM5 expression in several other tissues such as in the septal organ of Masera. Interestingly, in the olfactory epithelium of adult mice acute TRPM5 expression was detected in only one (short microvillar cells) of two cell populations previously reported to express TRPM5. The TRPM5-IC mouse strain described here represents a novel genetic tool and will facilitate the study and tissue-speciic manipulation of TRPM5-expressing cells in vivo. [ABSTRACT FROM AUTHOR]

Published
2015
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3. Genetic Labeling of Tas1r1 and Tas2r131 Taste Receptor Cells in Mice.

Author

Voigt, Anja, Hübner, Sandra, Lossow, Kristina, Hermans-Borgmeyer, Irm, Boehm, Ulrich, and Meyerhof, Wolfgang

Subjects
*TASTE buds, *TASTE receptors, *UMAMI (Taste), *CELL populations, *FUNGIFORM papilla
Abstract

Characterization of the peripheral taste system relies on the identification and visualization of the different taste bud cell types. So far, genetic strategies to label taste receptor cells are limited to sweet, sour, and salty detecting cells. To visualize Tas1r1 umami and Tas2r131 bitter sensing cells, we generated animals in which the Tas1r1 and Tas2r131 open reading frames are replaced by expression cassettes containing the fluorescent proteins mCherry or hrGFP, respectively. These animals enabled us to visualize and quantify the entire oral Tas1r1 and Tas2r131 cell populations. Tas1r1-mCherry cells were predominantly detected in fungiform papillae, whereas Tas2r131-hrGFP cells, which are ~4-fold more abundant, were mainly present in foliate and vallate papillae. In the palate, both cell types were similarly distributed. Mice carrying both recombinant alleles demonstrated completely segregated Tas1r1 and Tas2r131 cell populations. Only ~50% of the entire bitter cell population expressed hrGFP, indicating that bitter taste receptor cells express a subset of the bitter receptor repertoire. In extragustatory tissues, mCherry fluorescence was observed in testis and hrGFP fluorescence in testis, thymus, vomeronasal organ, and respiratory epithelium, suggesting that only few extraoral sites express Tas2r131 and Tas1r1 receptors at levels comparable to taste tissue. [ABSTRACT FROM AUTHOR]

Published
2012
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