Vision relies on photoactivation of visual pigments in rod and cone photoreceptor cells of the retina. The human eye structure and the absorption spectra of pigments limit our visual perception of light. Our visual perception is most responsive to stimulating light in the 400-to 720-nm (visible) range. First, we demonstrate by psychophysical experiments that humans can perceive infrared laser emission as visible light. Moreover, we show that mammalian photoreceptors can be directly activated by near infrared light with a sensitivity that paradoxically increases at wavelengths above 900 nm, and display quadratic dependence on laser power, indicating a nonlinear optical process. Biochemical experiments with rhodopsin, cone visual pigments, and a chromophore model compound 11-cis-retinyl-propylamine Schiff base demonstrate the direct isomerization of visual chromophore by a two-photon chromophore isomerization. Indeed, quantum mechanics modeling indicates the feasibility of this mechanism. Together, these findings clearly show that human visual perception of near infrared light occurs by twophoton isomerization of visual pigments.visual pigment | two-photon absorption | rhodopsin | transretinal electrophysiology | multiscale modeling H uman vision is generally believed to be restricted to a visible light range, although >50% of the sun's radiation energy that reaches earth is in the infrared (IR) range (1). Human rod and cone visual pigments with the 11-cis-retinylidene chromophore absorb in the visible range, with absorption monotonically declining from their maxima of 430-560 nm toward longer wavelengths. The spectral sensitivity of human dim light perception matches well with the absorption spectrum of the rod visual pigment, rhodopsin (2, 3). Activation of visual pigments is temperature independent around their absorption peaks (λ max ), but at longer wavelengths, the lower energy photons must be supplemented by heat to achieve chromophore photoisomerization (4). Long wavelength-sensitive visual pigments of vertebrates exhibit maximal absorption at the ∼500-to ∼625-nm range. Pigments with λ max > 700 nm are theoretically possible, but the high noise due to spontaneous thermal activation would render them impractical (5). At human body temperature and with 1,050-nm stimulation, the sensitivity of the peripheral retina to one-photon (1PO) stimulation is less than 10 −12 of its maximum value at 505 nm (4, 6). Indeed, reports about human IR vision can be found in the literature, although they are fragmentary and do not describe the mechanism of this phenomenon.With the invention of radar during World War II, it was immediately questioned if pilots could detect high intensity radiation in the IR range of the spectrum. Wald and colleagues reported that at wavelengths above 800 nm, rod photoreceptors become more sensitive than cones, resulting in perception of IR signals as white light selectively in the peripheral retina (6). They proposed that relative spectral sensitivity declines monotonically toward longer wavele...
Microperimetry is a subjective ophthalmologic test used to assess retinal function at various specific and focal locations of the visual field. Historically, visible light has been described as ranging from 400 to 720 nm. However, we previously demonstrated that infra-red light can initiate visual transduction in rod photoreceptors by a mechanism of two-photon absorption by visual pigments. Here we introduce a newly designed and constructed two-photon microperimeter. We provide for the first time evidence of the presence of a nonlinear process occurring in the human retina based on psychophysical tests using newly developed instrumentation. Since infra-red light penetrates the aged front of the eye better than visible light, it has the potential for improved functional diagnostics in patients with age-related visual disorders.
Two-photon microscopy allows visualization of subcellular structures in the living animal retina. In previously reported experiments it was necessary to apply a contact lens to each subject. Extending this technology to larger animals would require fitting a custom contact lens to each animal and cumbersome placement of the living animal head on microscope stage. Here we demonstrate a new device, periscope, for coupling light energy into mouse eye and capturing emitted fluorescence. Using this periscope we obtained images of the RPE and their subcellular organelles, retinosomes, with larger field of view than previously reported. This periscope provides an interface with a commercial microscope, does not require contact lens and its design could be modified to image retina in larger animals.
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