(A) Infrared eye fundus image and (B) optical coherence tomography (OCT) image of the eye injected intravitreally with AAV2-7m8-PR1.7-Jaws-GFP (n = 1, 1 × 10¹¹ vg and n = 1, 1 × 10¹⁰ vg). (C) Eye fundus fluorescence image 2 months after injection shows Jaws-GFP expression in the fovea. Inset magnification (B and C): ×1.5. (D) Half foveal flatmount showing efficient and specific foveal transduction using AAV2-7m8-PR1.7-Jaws-GFP. Scale bar: 50 μm. Arrow, foveola; red rectangle, close-up to the foveola shown in retinal sections in E; scale bar: 20 μm. (F–K) Characteristics of the cone photoreceptor light responses triggered by optogenetic stimulation of Jaws in living macaque retinas (n = 4 cells). (F) Superimposed infrared and epifluorescence images showing strong Jaws-GFP fluorescence in the foveal cones of patched explants. (G) Infrared image of the same tissue. Patch electrode (black dotted line) is shown in contact with a Jaws-GFP⁺ cone cell body highlighted in cyan. ONL, outer nuclear layer; IS, inner segments; OS, outer segments. (H and I) Whole-cell patch clamp recordings of Jaws-GFP–expressing macaque cones. Jaws-induced photocurrents as a function of light intensity. Orange light stimulation ranged from 1 × 10¹⁴ to 3 × 10¹⁷ photons cm^–2·s^–1. (J) Jaws-induced photocurrents as a function of stimulation wavelength in intravitreally injected macaque eye. Stimuli were applied from 400–650 nm, separated by 25-nm steps, at an intensity equal to 8 × 10¹⁶ photons cm^–2·s^–1. Maximal responses were obtained at 575 nm. (K) Jaws-GFP–expressing cones recorded in current-clamp configuration in current zero mode (with their resting membrane potential indicated in gray), displaying light-elicited hyperpolarizations followed by short depolarizations. AAV, adeno-associated virus; PR1.7, promoter of 1.7 kilobases in length, based on the human red opsin gene enhancer and promoter sequences.