Molecular characterization of dopamine D2 receptor isoforms tagged with green fluorescent protein |
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Authors: | Keyvan Sedaghat Marie-France Nantel Simon Ginsberg Véronique Lalonde Mario Tiberi |
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Affiliation: | (1) Moses and Rose Loeb Research Centre (Neuroscience Program), Ottawa Health Research Institute, 725 Parkdale Ave., KIY 4E9 Ottawa, ON, Canada;(2) Departments of Medicine/Cellular and Molecular Medicine/Psychiatry, University of Ottawa, Ottawa, ON, Canada |
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Abstract: | In this study, a cleavable signal peptide fused to the enhanced green fluorescent protein (EGFP) was tagged to the extracellular N-terminus of the human dopamine D2 receptor short and long isoforms (D2S and D2L). Ligand-binding properties of EGFP-tagged receptors were essentially unchanged in comparison to their respective wild-type receptors. The dopamine-mediated activation of both EGFP-D2 isoforms generated a robust inhibition of adenylyl cyclase type 5 in intact cells. In addition, the receptor density of EGFP-D2S and EGFP-D2L in transfected human embryonic kidney 293 (HEK293) cells was not altered when compared to cells transfected with the untagged D2S and D2L. However, the receptor densities of untagged and EGFP-tagged D2L were significantly lower in comparison to those measured with D2S constructs. Moreover, the receptor density of EGFP-D2S and EGFP-D2L was differentially upregulated in cells treated with antipsychotic drugs. As assessed by confocal microscopy, both EGFP-D2 isoforms were present on the cell surface. Notably, in contrast to the predominant plasma membrane localization of EGFP-D2S, EGFP-D2L was visualized both on the plasma membrane and intracellularly before dopamine exposure. Importantly, EGFP-D2S and EGFP-D2L are robustly internalized after dopamine treatment. Overall, our data suggest a differential intracellular sorting of D2S and D2L. |
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Keywords: | Dopamine D2 receptors enhanced green fluorescent protein amino terminus ligand binding G protein coupling adenylyl cyclase type 5 |
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