Cloning and characterization of RGS9-2: A striatal-enriched alternatively spliced product of the RGS9 gene

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Abstract

Regulators of G-protein signaling (RGS) proteins act as GTPase- activating protein (GAPs) for α subunits of heterotrimeric G-proteins. Previous in situ hybridization analysis of mRNAs encoding RGS3-RGS11 revealed region-specific expression patterns in rat brain. RGS9 showed a particularly striking pattern of almost exclusive enrichment in striatum. In a parallel study, RGS9 cDNA, here referred to as RGS9-1, was cloned from retinal cDNA libraries, and the encoded protein was identified as a GAP for transducin (Gα(t)) in rod outer segments. In the present study we identify a novel splice variant of RGS9, RGS9-2, cloned from a mouse forebrain cDNA library, which encodes a striatal-specific isoform of the protein. RGS9-2 is 191 amino acids longer than the retinal isoform, has a unique 3' untranslated region, and is highly enriched in striatum, with much lower levels seen in other brain regions and no expression detectable in retina. Immunohistochemistry showed that RGS9-2 protein is restricted to striatal neuropil and absent in striatal terminal fields. The functional activity of RGS9-2 is supported by the finding that it, but not RGS9-1, dampens the G(i/o)-coupled μ-opioid receptor response in vitro. Characterization of a bacterial artificial chromosome genomic clone of ~200 kb indicates that these isoforms represent alternatively spliced mRNAs from a single gene and that the RGS domain, conserved among all known RGS members, is encoded over three distinct exons. The distinct C-terminal domains of RGS9-2 and RGS9-1 presumably contribute to unique regulatory properties in the neural and retinal cells in which these proteins are selectively expressed.

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Rahman, Z., Gold, S. J., Potenza, M. N., Cowan, C. W., Ni, Y. G., He, W., … Nestler, E. J. (1999). Cloning and characterization of RGS9-2: A striatal-enriched alternatively spliced product of the RGS9 gene. Journal of Neuroscience, 19(6), 2016–2026. https://doi.org/10.1523/jneurosci.19-06-02016.1999

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