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      Loss of cone function without degeneration in a novel Gnat2 knock-out mouse

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          Abstract

          Rods and cones mediate visual perception over 9 log units of light intensities, with both photoreceptor types contributing to a middle 3-log unit range that comprises most night-time conditions. Rod function in this mesopic range has been difficult to isolate and study in vivo because of the paucity of mutants that abolish cone signaling without causing photoreceptor degeneration. Here we describe a novel Gnat2 knockout mouse line ( Gnat2 −/− ) ideal for dissecting rod and cone function. In this line, loss of Gnat2 expression abolished cone phototransduction, yet there was no loss of cones, disruption of the photoreceptor mosaic, nor change in general retinal morphology up to at least 9 months of age. Retinal microglia and Müller glia, which are highly sensitive to neuronal pathophysiology, were distributed normally with morphologies indistinguishable between Gnat2 −/− and wildtype adult mice. ERG recordings demonstrated complete loss of cone-driven a-waves in Gnat2 −/− mice; comparison to WT controls revealed that rods of both strains continue to function at light intensities exceeding 10 4 photoisomerizations rod −1 s −1. We conclude that the Gnat2 −/− mouse is a preferred model for functional studies of rod pathways in the retina when degeneration could be an experimental confound.

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          Analyzing real-time PCR data by the comparative CT method

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            Connexin36 is essential for transmission of rod-mediated visual signals in the mammalian retina.

            To examine the functions of electrical synapses in the transmission of signals from rod photoreceptors to ganglion cells, we generated connexin36 knockout mice. Reporter expression indicated that connexin36 was present in multiple retinal neurons including rod photoreceptors, cone bipolar cells, and AII amacrine cells. Disruption of electrical synapses between adjacent AIIs and between AIIs and ON cone bipolars was demonstrated by intracellular injection of Neurobiotin. In addition, extracellular recording in the knockout revealed the complete elimination of rod-mediated, on-center responses at the ganglion cell level. These data represent direct proof that electrical synapses are critical for the propagation of rod signals across the mammalian retina, and they demonstrate the existence of multiple rod pathways, each of which is dependent on electrical synapses.
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              Phototransduction in transgenic mice after targeted deletion of the rod transducin alpha -subunit.

              Retinal photoreceptors use the heterotrimeric G protein transducin to couple rhodopsin to a biochemical cascade that underlies the electrical photoresponse. Several isoforms of each transducin subunit are present in the retina. Although rods and cones seem to contain distinct transducin subunits, it is not known whether phototransduction in a given cell type depends strictly on a single form of each subunit. To approach this question, we have deleted the gene for the rod transducin alpha-subunit in mice. In hemizygous knockout mice, there was a small reduction in retinal transducin alpha-subunit content but retinal morphology and the physiology of single rods were largely normal. In homozygous knockout mice, a mild retinal degeneration occurred with age. Rod-driven components were absent from the electroretinogram, whereas cone-driven components were retained. Every photoreceptor examined by single-cell recording failed to respond to flashes, with one exception. The solitary responsive cell was insensitive, as expected for a cone, but had a rod-like spectral sensitivity and flash response kinetics that were slow, even for rods. These results indicate that most if not all rods use a single transducin type in phototransduction.
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                Author and article information

                Journal
                0370707
                3647
                Exp Eye Res
                Exp. Eye Res.
                Experimental eye research
                0014-4835
                1096-0007
                28 May 2018
                05 March 2018
                June 2018
                05 June 2018
                : 171
                : 111-118
                Affiliations
                [a ]Center for Neuroscience, University of California Davis, Davis, CA 95616, USA
                [b ]Department of Cell Biology and Human Anatomy, University of California Davis, Davis, CA 95616, USA
                [c ]EyePod Small Animal Ocular Imaging Laboratory, University of California Davis, Davis, CA 95616, USA
                [d ]Department of Ophthalmology & Vision Science, University of California Davis, Davis, CA 95616, USA
                [e ]Department of Ophthalmology, Medical College of Wisconsin, Milwaukee, WI 53226, USA
                Author notes
                [* ]Corresponding author. Department of Ophthalmology & Vision Science, University of California Davis, Davis, CA 95616, USA. meburns@ 123456ucdavis.edu (M.E. Burns)
                Article
                NIHMS971060
                10.1016/j.exer.2018.02.024
                5987249
                29518352
                f9cf5c3c-e770-4322-85f3-ed2ddcf3d049

                This is an open access article under the CC BY-NC-ND license ( http://creativecommons.org/licenses/BY-NC-ND/4.0/).

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                Categories
                Article

                Vision sciences
                g-protein,photoreceptor,retina,phototransduction
                Vision sciences
                g-protein, photoreceptor, retina, phototransduction

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