Pepperberg plot: Modeling flash response saturation in retinal rods of mouse

Giovanni Caruso; Colin Klaus; Heidi E Hamm; Vsevolod V Gurevich; Paolo Bisegna; Daniele Andreucci; Emmanuele DiBenedetto; Clint L Makino

doi:10.3389/fnmol.2022.1054449

Pepperberg plot: Modeling flash response saturation in retinal rods of mouse

Front Mol Neurosci. 2023 Jan 13:15:1054449. doi: 10.3389/fnmol.2022.1054449. eCollection 2022.

Authors

Giovanni Caruso¹, Colin Klaus², Heidi E Hamm³, Vsevolod V Gurevich³, Paolo Bisegna⁴, Daniele Andreucci⁵, Emmanuele DiBenedetto⁶, Clint L Makino⁷

Affiliations

¹ Italian National Research Council, Istituto di Scienze del Patrimonio Culturale, Rome, Italy.
² The College of Public Health Division of Biostatistics and The Mathematical Biosciences Institute, The Ohio State University, Columbus, OH, United States.
³ Department of Pharmacology, Vanderbilt University Medical Center, Nashville, TN, United States.
⁴ Department of Civil Engineering and Computer Science, University of Rome Tor Vergata, Rome, Italy.
⁵ Department of Basic and Applied Sciences for Engineering, Sapienza University of Rome, Rome, Italy.
⁶ Department of Mathematics, Vanderbilt University, Nashville, TN, United States.
⁷ Department of Physiology & Biophysics, Boston University Chobanian & Avedisian School of Medicine, Boston, MA, United States.

Abstract

Retinal rods evolved to be able to detect single photons. Despite their exquisite sensitivity, rods operate over many log units of light intensity. Several processes inside photoreceptor cells make this incredible light adaptation possible. Here, we added to our previously developed, fully space resolved biophysical model of rod phototransduction, some of the mechanisms that play significant roles in shaping the rod response under high illumination levels: the function of RGS9 in shutting off G protein transducin, and calcium dependences of the phosphorylation rates of activated rhodopsin, of the binding of cGMP to the light-regulated ion channel, and of two membrane guanylate cyclase activities. A well stirred version of this model captured the responses to bright, saturating flashes in WT and mutant mouse rods and was used to explain "Pepperberg plots," that graph the time during which the response is saturated against the natural logarithm of flash strength for bright flashes. At the lower end of the range, saturation time increases linearly with the natural logarithm of flash strength. The slope of the relation (τ_D) is dictated by the time constant of the rate-limiting (slowest) step in the shutoff of the phototransduction cascade, which is the hydrolysis of GTP by transducin. We characterized mathematically the X-intercept ( $Φ o$ ) which is the number of photoisomerizations that just saturates the rod response. It has been observed that for flash strengths exceeding a few thousand photoisomerizations, the curves depart from linearity. Modeling showed that the "upward bend" for very bright flash intensities could be explained by the dynamics of RGS9 complex and further predicted that there would be a plateau at flash strengths giving rise to more than ~10⁷ photoisomerizations due to activation of all available PDE. The model accurately described alterations in saturation behavior of mutant murine rods resulting from transgenic perturbations of the cascade targeting membrane guanylate cyclase activity, and expression levels of GRK, RGS9, and PDE. Experimental results from rods expressing a mutant light-regulated channel purported to lack calmodulin regulation deviated from model predictions, suggesting that there were other factors at play.

Keywords: CNG channel; G protein; GRK; PDE; RGS9; cyclic GMP; membrane guanylate cyclase; visual transduction.

Abstract

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