Among the more remarkable computational feats performed by neurons is the extraction of information from light. In the eye, retinal neural circuits process images. One of the fundamental challenges for eyes is to maintain constancy of neural product over ambient illuminations ranging from starlight to the brightest noontime sun. To cover this range separate classes of photoreceptors have evolved, rods for nocturnal vision, and cones for diurnal vision. Each in turn is served by dedicated sets of interneurons forming intra-retinal rod and cone networks. Mammals such as cats, rabbits, rats and mice provide satisfactory models for rod system circuitry. In primates, color vision is a characteristic of cones and their associated interneurons. Common laboratory mammals have a poorly developed color vision and a low density of cones. The zebrafish model provides a cone dominated retina, rich in color vision, and with the opportunity to study cone networks. The zebrafish is advantageous for ease of genetic manipulations and for extensive libraries of mutants and transgenics. It is for these reasons that, over the past decade, this lab and others have worked to develop zebrafish as a model for electrophysiological and anatomical studies of visual system circuitry. Membrane receptors for neurotransmitters are a vital component of neural circuits. In retina the receptor expression pattern is often a unique signature for different neural types, and these receptor signatures dictate unique functional properties. The initial research focus was neurotransmitter responses of individual zebrafish retinal neurons, either dissociated or in retinal slice. For the former, the method was fluorescent voltage probe recording. For the latter patch electrode recording was used. Glutamatergic actions on cone bipolar cells revealed a variety of mechanisms, including metabotropic receptors, AMPA-kainate receptors, and transporter-associated chloride channels. The distribution of GABA transporters, and a variety of ionotropic GABA receptors on neural types was later uncovered. There appear to be at least three GABA receptor types on bipolar cells, a GABA-A receptor and both picrotoxin sensitive and insensitive GABA-C receptors. Some bipolar cells express a GABA transporter, a marker for GABAergic neurotransmission. Zebrafish horizontal cells lack GABA receptors, but a subset transport GABA and are GABAergic. As seen in voltage-probe techniques, GABA transporter signals are very large, and may serve as a GABA sensor mechanism. During this research phase, in parallel with studies of neurotransmitter receptors, a morphological library of horizontal, bipolar, and amacrine cell types was developed, both through patch microelectrode staining, and through 'diolistic'staining, each technique in retinal slice. The current research phase examines neural light responses and transgenic labeling. A flattened, perfused eyecup preparation provides microelectrode access to horizontal cell and amacrine cell light responses. Cell bodies, dendrites and axons of horizontal cells were revealed in wet epifluorescence microscopy following microelectrode injection of alexafluor 594. Spectral studies reveal 6 chromatic types, including trichromatic UV color opponent cells, with dominant UV cone signals being opposed by blue and green cone signals, but reinforced by red cone signals. The morphology of UV trichromatic cells is characterized by long axons and wide dendritic fields, similar to anatomical H3 types. A UV color-opponent physiology has not been reported in horizontal cells of other species. Tetrachromatic responses were also seen. These were depolarized by UV, hyperpolarized by far blue, depolarized by blue-green, and hyperpolarized by yellow or red. As the spectral responses of horizontal cells contain so many different cone signals, the 570nm-peaking red cones, the 480nm-peaking green cones, the 410nm-peaking blue cones, and the 362nm-peaking UV cones, a model was devised to infer the signal composition. This consists of the sum of four saturable Hill functions, one for each cone spectral type. It is a three-dimensional response-wavelength-irradiance function. The model quantifies the stimulus color calculations that horizontal cells, or other zebrafish retinal neurons perform. Studies of amacrine types revealed four temporal patterns: 1) A red-cone dominated depolarizing transient at ON and at OFF. 2) Sustained depolarization. 3) A hyperpolarizing or biphasic ON response followed by a transient OFF depolarization. 4) Color opponent responses with response sign determined by wavelength. The dendritic stratification pattern of each physiological type was reconstructed from image stacks of microelectrode injected cells in Neurolucida (MBF Bioscience). Each physiological type reveals a unique branching: Type 1 cells are almost exclusively bistratified, though with several patterns of bistratification;type 2 cells are monostratified near the middle, or just below the middle of the inner plexiform layer;type 3 cells are monstratified in the distal IPL, near amacrine cells (sublamina a);type 4 cells are monostratified in the proximal inner plexiform layer, near ganglion cells (sublamina b). Amacrine cell dendritic fields range from 150 to 300 microns. Some are radially symmetric. Others branch profusely only to one side of the cell body. Still others have one or more axon-like processes extending away from a central dendritic arbor. The responses of types 1, 2 and 3 are dominated by red cones. The color opponent patterns in type 4 are various, but include UV tetraphasic types. Recently it has become possible to study the color properties of larval ganglion cells. The most common type is UV triphasic, similar to H3 horizontal cells. It is excited by red and UV stimuli, but inhibited in the mid-spectral range. Altogether zebrafish lives up to the expectation of rich processing networks for cone signals. The current research phase examines the labeling of retinal neurons through forward transgenic insertions of reporter genes. These lines were noted for larval eye fluorescence in other labs. We determine the neural types leading to eye fluorescence. One line of interest is GE4a developed in the Fumihito Ono Lab, NIAAA. In addition to populations of amacrine and ganglion cells, there is label in a select horizontal cell type, perhaps H2. The gene insertion is in a non-coding region of chromosome 14. y245 is a Gal4:UAS line developed in the Harry Burgess lab, NICHD. Red and green cones label brightly, as does a sparse Muller cell population. More faintly marked are amacrine and ganglion cells. The transgene insertion mutates the Musashi1 promoter on chromosome 8. The mutation is associated with a slow retinal degeneration of UV cones, reduced sensitivity, and aberrant spectral pattern, seen in the isolated cone responses of both larvae and adults.

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2014
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Torvund, M M; Ma, T S; Connaughton, V P et al. (2017) Cone signals in monostratified and bistratified amacrine cells of adult zebrafish retina. J Comp Neurol 525:2800-2801
Torvund, M M; Ma, T S; Connaughton, V P et al. (2017) Cone signals in monostratified and bistratified amacrine cells of adult zebrafish retina. J Comp Neurol 525:1532-1557
Lewis, Alaron; Wilson, Neil; Stearns, George et al. (2011) Celsr3 is required for normal development of GABA circuits in the inner retina. PLoS Genet 7:e1002239
Connaughton, Victoria P; Nelson, Ralph (2010) Spectral responses in zebrafish horizontal cells include a tetraphasic response and a novel UV-dominated triphasic response. J Neurophysiol :
Nelson, Ralph F; Singla, Nirmish (2009) A spectral model for signal elements isolated from zebrafish photopic electroretinogram. Vis Neurosci 26:349-63
Nelson, Ralph; Bender, Anna M; Connaughton, Victoria P (2008) Transporter-mediated GABA responses in horizontal and bipolar cells of zebrafish retina. Vis Neurosci 25:155-65
Connaughton, Victoria P; Nelson, Ralph; Bender, Anna M (2008) Electrophysiological evidence of GABAA and GABAC receptors on zebrafish retinal bipolar cells. Vis Neurosci 25:139-53
Pflug, Renate; Nelson, Ralph; Huber, Sonja et al. (2008) Modulation of horizontal cell function by dopaminergic ligands in mammalian retina. Vision Res 48:1383-90