Longitudinal Assessment of Pupil Response to Red and Blue Light in Youth Hockey Players

Zulliger, Kristen Marie

09 August 2022

No description available.

Ophthalmology

Optics

Neurosciences

A deep dive into the sablefish (Anoplopoma fimbria) opsin repertoire: insight into melanopsin expression, localization and function in an unlikely demersal model.

Barnes, Hayley

29 September 2022

Light regulates many biological processes through light-sensitive proteins called opsins. Opsins are involved in vision, but they are also expressed in extraretinal tissue, where their roles are far less clear. Fish have large opsin repertoires, derived from a long history of gene duplication and divergence, making them useful models to study opsin diversity and function. I introduce the deep-sea sablefish (Anoplopoma fimbria) as a model for opsin research for three main reasons: i) the availability of a draft genome and transcriptome, simplifying the characterization of this species’ opsin repertoire, ii) the proximity of the only sablefish aquaculture facility in the world, providing exclusive access to a large number of individuals at all developmental stages, iii) the observation that sablefish occupy very different light environments during the course of development, ranging from well-lit shallow waters to the aphotic zone, which provides a light environment context for opsin gene expression data. My survey of the genome showed that sablefish have 36 distinct opsin genes (7 visual and 29 non-visual), even though they spend most of their lives in the dark. The sablefish opsin sequences and repertoire are similar to those of other teleost fish. To test the hypothesis that the sablefish opsin repertoire is being expressed/transcribed during the comparatively brief period of time when this species is exposed to light (the free-swimming larval stage through to the juvenile stage), I quantified the expression of five paralogous genes from a well-studied non-visual opsin family (OPN4’s) in the brain across life stages. Data show statistically stable expression of Opn4m1 and Opn4m3 among life stages, a rough association of Opn4x1 and Opn4m2 expression with age and light environment, and little-to-no expression of Opn4x2. I localized proteins encoded by the most highly expressed class of OPN4 genes in the brain, the Opn4m genes, to the surface of the optic tectum just below a cranial ‘window’; a zone that has been shown to express dozens of opsins in zebrafish (a distant relative, with their ancestor diverging more than 230 million years ago). Thus, in some cases, expression appears to be correlated with light exposure not only temporally, but also spatially. By studying non-visual opsins in sablefish, I have challenged and broadened the current understanding of opsin evolution and function in fish and provided the foundation for future studies to test brain regions for light-sensitivity, perform opsin gene knock-outs, and explore potential light-independent processes. / Graduate / 2023-09-06

Radial glia

Sablefish

Opsin

Melanopsin

Immunohistochemistry

qPCR

Photoreceptors

Gene expression

Deep-sea fish

Novel Roles for Reelin in Retinogeniculate Targeting

Haner, Cheryl

02 August 2010

In the developing visual system, the axon of a pre-synaptic cell must be guided to a post-synaptic partner. Retinal ganglion cells (RGCs) in the eye are an excellent model to study this process. Multiple classes exist that respond to specific types of light input, and these project to different destinations in the brain that process distinct types of information. The RGC axons that navigate to the lateral geniculate nucleus (LGN) do so in a class-specific manner. Axons from RGCs that mediate non-image forming functions innervate the ventral LGN (vLGN) and the intergeniculate leaflet (IGL). Axons from RGCs that process image-forming information bypass these regions to innervate the dorsal LGN (dLGN). The extracellular protein reelin was identified as a potential factor in RGC axonal targeting of the vLGN and IGL, and the reeler mutant mouse used to study the effects of its functional absence. Anterograde labeling of RGCs and their axons with Cholera toxin B (CTB) revealed reduced patterns of retinal innervation to the vLGN and IGL in mutant mice. Moreover, the absence of functional reelin resulted in axons incorrectly growing into inappropriate regions of the thalamus. We identified these misrouted axons as those of the intrinsically photosensitive RGCs (ipRGCS), a class of RGCs known to project to the affected subnuclei. In contrast to defects in ipRGC targeting, no deficits were seen in retinogeniculate or corticothalamic projections in classes of axons that normally target the dLGN. Immunohistochemistry did not reveal any effects of the absence of the functional reelin on the LGN cytoarchitecture, which is unlike many other brain regions altered in the reeler. In summary, results suggest that intact reelin is required for class-specific retinogeniculate targeting to the vLGN and IGL. The defects are likely to be in targeting and not in neuronal positioning.

synaptic targeting

axon guidance

retinal ganglion cell

thalamus

lateral geniculate nucleus

extracellular matrix

melanopsin

Anatomy

Medicine and Health Sciences

Nervous System

Characterisation of non-visual photoreception in humans / Caractérisation de la photoréception non-visuelle chez l'homme

Prayag, Abhishek Sokappadu

26 July 2017

Chez l'homme, la lumière influence 1) les rythmes circadiens, 2) le cycle veille-sommeil, et 3) active les fonctions non-visuelles. La rétine qui reçoit et traite l’information lumineuse possède des caractéristiques uniques de sensibilité à la lumière qui dépendent de la longueur d'onde. Elle se compose de photorécepteurs visuels (cônes S-, M-, ou L-) présentant une sensibilité au bleu, vert, et rouge et des photorécepteurs non-visuels (les cellules ganglionnaires à mélanopsine, ipRGCs) sensible à 480nm. Peu d'études ont étudié l'impact de lumières colorées sur les fonctions non-visuelles. De telles études ont utilisées des lumières monochromatiques de longue durée, administrées après les horaires normaux de coucher, avec une pupille dilatée. Cela contraste avec l'exposition à la lumière ambiante. Comment celle-ci influence la dynamique des réponses non-visuelles et est-ce que leur intensité ou leur composition de couleur influe sur les rythmes circadiens n'est toujours pas élucidée.Nous avons étudié les effets d’une lumière polychromatique sur les dynamiques de l'activité corticale (EEG), le réflexe pupillaire, la suppression de la mélatonine, la fréquence cardiaque, la température et les performances neurocomportementales. 28 sujets hommes ont été exposés à 4 stimuli lumineux de 50 min, entre 19-2300 h. Les stimuli avaient une contribution mélanopique différente, mais une densité de photons identique de 10e14 photons/cm²/s. Cela nous a permis de disséquer les contributions relatives des photorécepteurs non-visuels/visuels dans les fonctions non-visuelles. Dans une seconde étude, les photorécepteurs et niveaux de lumière nécessaires pour 1) initier et saturer la suppression de la mélatonine et 2) les plages actives ont été calculés. Ces résultats ont des implications dans notre compréhension des effets d’une exposition à la lumière artificielle sur la veille et le sommeil et les troubles du rythme circadien tels que le syndrome du retard de phase / In humans, light influences 1) circadian rhythms, 2) sleep-wake cycle, and 3)activate non-visual functions. While white bright light studies provide insight on the effect of light per se, the retina consists of visual photoreceptors (S-M-L cones) exhibiting sensitivity in blue, green, red colour range and non-visual photoreceptors (intrinsically photosensitive retinal ganglion cells, ipRGCs) most sensitive at 480nm. Few studies investigated the impact of coloured light corresponding to the different photoreceptors on light-dependent physiology. Such studies employed long duration monochromatic light, administered past normal bedtimes, after pupil dilator application. This contrasts with real-life light exposure. Furthermore, the link between light, non-visual responses and sleep-wake cycle has not been dynamically assessed. How ambient light influences the kinetics of non-visual responses and whether their intensity or colour impacts circadian rhythms is still unclear.We investigated polychromatic light exposure on the kinetics of cortical activity (EEG), pupillary light reflex, melatonin suppression, heart rate, temperature and neurobehavioral performances in humans. In a first study, 28 males were exposed to 4 light pulses of 50 min each from 19-2300 h. Light pulses had different melanopic contribution but identical photon density of 1014 photons/cm²/s. This allowed us to dissect relative contributions of non-visual/visual photoreceptors on light-dependent physiology and wakefulness markers. In a second study, we determined the sensitivity and thresholds of nocturnal melatonin suppression by light and the photoreceptors involved. Light levels needed to 1) initiate suppression, 2) saturation and 3) the active ranges were calculated. These findings have implications in our understanding of artificial light exposure on the sleep-wake cycle and circadian rhythm disorders such as delayed sleep phase disorder

Lumière

Réponses non-visuelles

Mélanopsine

EEG

Mélatonine

Cognition

Circadien

Photoréception

Light

Non-visual responses

Melanopsin

EEG

Melatonin

Cognition

Circadian

Photoreception

612.8

Efeito da luz e endotelina no mecanismo molecular do relógio em melanóforos de Xenopus laevis / Effect of light and endothelin on clock molecular mechanisms in Xenopus laevis melanophores

Moraes, Maria Nathália de Carvalho Magalhães

17 December 2014

Os ciclos claro-escuro (CE) são considerados importantes pistas para o ajuste de relógios biológicos. Alças de retroalimentação positiva e negativa de transcrição e tradução de genes de relógio são a base molecular subjacente tanto a relógios centrais como periféricos. A opsina não visual, melanopsina (Opn4), expressa na retina de mamíferos, é considerada o fotopigmento circadiano pois é responsável pelo ajuste do relógio biológico endógeno. Este fotopigmento também está presente nos melanóforos de Xenopus laevis, onde ele foi descrito pela primeira vez, mas seu papel nestas células ainda não está completamente esclarecido. Espécies de vertebrados não mamíferos expressam duas ou mais melanopsinas e, no caso de X. laevis, há dois genes, Opn4m and Opn4x. Melanóforos de X. laevis respondem à luz com dispersão dos grânulos de melanina, a resposta máxima sendo atingida no comprimento de onda correspondente àquele de excitação máxima da melanopsina. Entre vários hormônios, endotelinas também dispersam os melanossomos em melanóforos de Xenopus através de via similar àquela evocada pela luz. Tendo esses fatos em mente, decidimos investigar se a luz e a endotelina modulam a expressão de genes de relógio em melanóforos de Xenopus, usando PCR quantitativo para avaliar os níveis relativos de RNAm de Per1, Per2, Clock e Bmal1. Ciclos CE promoveram alterações temporais na expressão de Per1, Per2 e Bmal1. Pulsos de 10 min de luz azul aumentaram a expressão de Per1 e Per2, diminuíram a expressão de Opn4x, mas não tiveram efeito sobre Opn4m. Ainda mais, diferentes localizações foram mostradas para cada melanopsina: imunorreatividade para OPN4x foi vista principalmente na membrana celular, enquanto OPN4m foi imuno-localizada no núcleo. Estes resultados em conjunto apontam para funções diferenciais das duas melanopsinas neste modelo. A translocação de grânulos de melanina foi maior quando um pulso de luz azul foi aplicado na presença de endotelina ET-3. E os níveis de RNAm de Clock exibiram variação temporal em melanóforos submetidos a CE após tratamento com ET-3 10-9M, enquanto a expressão de Per1 não foi afetada pelo tratamento hormonal. Em adição, ensaios farmacológicos indicaram que as respostas de Per1 e Per2 à luz azul são evocadas através da ativação da via de fosfoinositídeos, com crosstalks com GMPc/proteina quinase G (PKG) para ativar os genes de relógio. Estes dados sugerem a participação de melanopsina na foto-ativação de genes de relógio, e apontam para uma participação menor de endotelina como sincronizador desta linhagem celular. Nossos resultados constituem uma importante contribuição ao campo emergente dos relógios periféricos os quais, em espécies de não mamíferos têm sido mais extensivamente estudados em Drosophila melanogaster e Danio rerio. Dentro deste contexto, nós mostramos que os melanóforos de Xenopus laevis representam um modelo ideal para a compreensão da modulação de ritmos circadianos por luz e hormônios / Light-dark cycles (LD) are considered important cues to entrain biological clocks. Positive and negative feedback loops of clock gene transcription and translation are the molecular basis underlying the mechanism of both central and peripheral clocks. The non-visual opsin, melanopsin (Opn4), expressed in the mammalian retina, is considered a circadian photopigment because it is responsible of entraining the endogenous biological clock. This photopigment is also present in the melanophores of Xenopus laevis, where it was first described, but its role in these cells is not fully understood. Non-mammalian vertebrate species express two or more melanopsins, and in X. laevis there are two melanopsin genes, Opn4m and Opn4x. X. laevis melanophores respond to light with melanin granule dispersion, the maximal response being achieved at the wavelength of melanopsin maximal excitation. Among various hormones, endothelins also disperse melanosomes in Xenopus melanophores through a similar pathway as light does. Therefore, we decided to investigate whether light and endothelin modulate clock gene expression in Xenopus melanophores, using quantitative PCR to evaluate the relative mRNA levels of Per1, Per2, Clock and Bmal1. LD cycles elicited temporal changes in the expression of Per1, Per2 and Bmal1. A 10 min pulse of blue light increased the expression of Per1 and Per2, decreased Opn4x expression, but had no effect on Opn4m. In addition, a different localization was shown for each melanopsin: immunoreactivity for OPN4x was mainly seen in the cell membrane, whereas OPN4m was immunolocalized in the nucleus. These results taken together point to a differential role for each melanopsin in this model. Melanosome translocation was greater when a blue light pulse was applied in the presence of endothelin ET-3. And mRNA levels of Clock exhibited temporal variation in melanophores under LD cycles after 10-9 M ET-3 treatment, whereas Per1 expression was not affected by the hormone treatment. In addition, pharmacological assays indicated that Per1 and Per2 responses to blue light are evoked through the activation of the phosphoinositide pathway, which crosstalks with cGMP/protein kinase G (PKG) to activate the clock genes. These data suggest the participation of melanopsin in the photo-activation of clock genes and point to a minor role of endothelin as synchronizer for this cell line. Our results add an important contribution to the emerging field of peripheral clocks, which in non-mammalian species have been mostly studied in Drosophila melanogaster and Danio rerio. Within this context, we show that Xenopus laevis melanophores represent an ideal model to understanding circadian rhythms modulation by light and hormone

1.Xenopus laevis

2.Melanopsina

3.Genes do relógio

4.Endotelina

5.Relógio periférico

Clock genes

Endothelin

Melanopsin

Peripheral clock

Xenopus laevis

Efeito da luz e endotelina no mecanismo molecular do relógio em melanóforos de Xenopus laevis / Effect of light and endothelin on clock molecular mechanisms in Xenopus laevis melanophores

Maria Nathália de Carvalho Magalhães Moraes

17 December 2014

Os ciclos claro-escuro (CE) são considerados importantes pistas para o ajuste de relógios biológicos. Alças de retroalimentação positiva e negativa de transcrição e tradução de genes de relógio são a base molecular subjacente tanto a relógios centrais como periféricos. A opsina não visual, melanopsina (Opn4), expressa na retina de mamíferos, é considerada o fotopigmento circadiano pois é responsável pelo ajuste do relógio biológico endógeno. Este fotopigmento também está presente nos melanóforos de Xenopus laevis, onde ele foi descrito pela primeira vez, mas seu papel nestas células ainda não está completamente esclarecido. Espécies de vertebrados não mamíferos expressam duas ou mais melanopsinas e, no caso de X. laevis, há dois genes, Opn4m and Opn4x. Melanóforos de X. laevis respondem à luz com dispersão dos grânulos de melanina, a resposta máxima sendo atingida no comprimento de onda correspondente àquele de excitação máxima da melanopsina. Entre vários hormônios, endotelinas também dispersam os melanossomos em melanóforos de Xenopus através de via similar àquela evocada pela luz. Tendo esses fatos em mente, decidimos investigar se a luz e a endotelina modulam a expressão de genes de relógio em melanóforos de Xenopus, usando PCR quantitativo para avaliar os níveis relativos de RNAm de Per1, Per2, Clock e Bmal1. Ciclos CE promoveram alterações temporais na expressão de Per1, Per2 e Bmal1. Pulsos de 10 min de luz azul aumentaram a expressão de Per1 e Per2, diminuíram a expressão de Opn4x, mas não tiveram efeito sobre Opn4m. Ainda mais, diferentes localizações foram mostradas para cada melanopsina: imunorreatividade para OPN4x foi vista principalmente na membrana celular, enquanto OPN4m foi imuno-localizada no núcleo. Estes resultados em conjunto apontam para funções diferenciais das duas melanopsinas neste modelo. A translocação de grânulos de melanina foi maior quando um pulso de luz azul foi aplicado na presença de endotelina ET-3. E os níveis de RNAm de Clock exibiram variação temporal em melanóforos submetidos a CE após tratamento com ET-3 10-9M, enquanto a expressão de Per1 não foi afetada pelo tratamento hormonal. Em adição, ensaios farmacológicos indicaram que as respostas de Per1 e Per2 à luz azul são evocadas através da ativação da via de fosfoinositídeos, com crosstalks com GMPc/proteina quinase G (PKG) para ativar os genes de relógio. Estes dados sugerem a participação de melanopsina na foto-ativação de genes de relógio, e apontam para uma participação menor de endotelina como sincronizador desta linhagem celular. Nossos resultados constituem uma importante contribuição ao campo emergente dos relógios periféricos os quais, em espécies de não mamíferos têm sido mais extensivamente estudados em Drosophila melanogaster e Danio rerio. Dentro deste contexto, nós mostramos que os melanóforos de Xenopus laevis representam um modelo ideal para a compreensão da modulação de ritmos circadianos por luz e hormônios / Light-dark cycles (LD) are considered important cues to entrain biological clocks. Positive and negative feedback loops of clock gene transcription and translation are the molecular basis underlying the mechanism of both central and peripheral clocks. The non-visual opsin, melanopsin (Opn4), expressed in the mammalian retina, is considered a circadian photopigment because it is responsible of entraining the endogenous biological clock. This photopigment is also present in the melanophores of Xenopus laevis, where it was first described, but its role in these cells is not fully understood. Non-mammalian vertebrate species express two or more melanopsins, and in X. laevis there are two melanopsin genes, Opn4m and Opn4x. X. laevis melanophores respond to light with melanin granule dispersion, the maximal response being achieved at the wavelength of melanopsin maximal excitation. Among various hormones, endothelins also disperse melanosomes in Xenopus melanophores through a similar pathway as light does. Therefore, we decided to investigate whether light and endothelin modulate clock gene expression in Xenopus melanophores, using quantitative PCR to evaluate the relative mRNA levels of Per1, Per2, Clock and Bmal1. LD cycles elicited temporal changes in the expression of Per1, Per2 and Bmal1. A 10 min pulse of blue light increased the expression of Per1 and Per2, decreased Opn4x expression, but had no effect on Opn4m. In addition, a different localization was shown for each melanopsin: immunoreactivity for OPN4x was mainly seen in the cell membrane, whereas OPN4m was immunolocalized in the nucleus. These results taken together point to a differential role for each melanopsin in this model. Melanosome translocation was greater when a blue light pulse was applied in the presence of endothelin ET-3. And mRNA levels of Clock exhibited temporal variation in melanophores under LD cycles after 10-9 M ET-3 treatment, whereas Per1 expression was not affected by the hormone treatment. In addition, pharmacological assays indicated that Per1 and Per2 responses to blue light are evoked through the activation of the phosphoinositide pathway, which crosstalks with cGMP/protein kinase G (PKG) to activate the clock genes. These data suggest the participation of melanopsin in the photo-activation of clock genes and point to a minor role of endothelin as synchronizer for this cell line. Our results add an important contribution to the emerging field of peripheral clocks, which in non-mammalian species have been mostly studied in Drosophila melanogaster and Danio rerio. Within this context, we show that Xenopus laevis melanophores represent an ideal model to understanding circadian rhythms modulation by light and hormone

1.Xenopus laevis

2.Melanopsina

3.Genes do relógio

4.Endotelina

5.Relógio periférico

Clock genes

Endothelin

Melanopsin

Peripheral clock

Xenopus laevis

The melanopsin-dependent direct non-circadian effects of light : a third principal mechanism for the regulation of sleep and wake / Effets directs non-circadiens de la lumière médiés par la mélanopsine : un troisième mécanisme majeur de régulation du sommeil et de l'éveil

Hubbard, Jeffrey

05 October 2012

Entre 15 et 30% de la population souffrent de troubles du sommeil, ce qui représente un enjeu majeur de santé publique et souligne la nécessité de mieux comprendre les mécanismes de régulation du sommeil. La régulation du sommeil est décrite comme un modèle à 2-processus comprenant un mécanisme circadien et homéostatique. La lumière exerce un effet sur le sommeil de deux manières distinctes: indirectement en resynchronisant l'horloge, et directement par des mécanismes qui restent mal compris. Cet effet direct est médié par des cellules spécialisées de la rétine intrinsèquement photosensibles et contenant un photopigment la mélanopsine (Opn4) mais aussi par les cônes et bâtonnets qui transfèrent l'information à ces cellules. Pour comprendre la façon dont ces effets directs influencent le sommeil et la veille, nous avons caractérisé des souris Opn4-/- et des souris sans horloge fonctionnelle (Syn10cre/creBmal1fl/-), ainsi qu’un rongeur diurne, Arvicanthis ansorgei. Les objectifs de cette étude étaient les suivants: (1) identifier les voies neuronales sous-tendant les effets directs de la lumière médiés par la mélanopsine ; (2) valider ces effets chez un rongeur diurne; (3) établir une relation entre lumière, Opn4 et homéostasie du sommeil. Ce travail a permis (1) de mettre en évidence que les effets directs de la lumière représente un troisième mécanisme majeur de régulation du sommeil permettant même de maintenir un rythme veille sommeil en l’absence d’horloge centrale (2) de démontrer que ces effets sont inversés entre espèces diurnes et nocturnes; (3) de démontrer que la mélanopsine et la lumière sont fortement liées à la modulation de l’homéostasie du sommeil. / Between 15-30% of the general population is affected by sleep disorders, representing a major public health challenge, and as such a need to better understand the regulatory mechanisms of sleep and waking. This has been previously described as a 2-process model; both a circadian and homeostatic process. Light exerts an effect on sleep and wake in two distinct ways: indirectly, through the resynchronization of the clock, and directly via mechanisms that remain poorly understood. This direct effect is primarily a result of interaction with specialized cells in the retina which are intrinsically photosensitive containing the photopigment melanopsin (Opn4) in addition to rods and cones, which to a lesser extent pass information through these cells. To understand the way in which these direct effects influence sleep and waking we characterized mice lacking Opn4, and a second group possessing a functionally disabled clock (Syn10cre/creBmal1fl/-), as well as a diurnal rodent, arvicanthis ansorgei. The aims of this study were to: (1) identify the possible neural pathways to the hypothalamus transmitting the Opn4-mediated direct effects of light; (2) validate these effects in a diurnal rodent; (3) demonstrate a biological link between light, Opn4, and sleep homeostasis. This work has provided (1) strong evidence for a third regulatory mechanism of sleep and waking (direct effects of light) that is able to maintain a sleep wake rhythm in the absence of central clock (2) an inversion of this mechanism between nocturnal and diurnal species; (3) demonstration that Opn4 and light are strongly related to the modulation of homeostatic sleep process.

Sommeil

Mélanopsine

Rythme Circadien

Neurobiologie

Homéostasie du sommeil

Opn4

Photoreception

Neuroscience

Sleep disorders

Melanopsin

Circadian process

Homeostatic process

Neurobiology

Opn4

Photopigment

612.8

612.02

Non visual photoreception in humans : circadian consequences of spectral modulations of light / Photoréception non-visuelle chez l’Homme : effets de la modulation du spectre lumineux sur le système circadien

Najjar, Raymond

02 July 2012

Chez les mammifères dont l’Homme, les rythmes circadiens physiologiques et comportementaux sont régulés par l’horloge centrale, localisée dans les noyaux suprachiasmatiques de l’hypothalamus. Possédant une période endogène proche mais pas exactement de 24 heures, cette horloge est constamment synchronisée à la période terrestre par le cycle lumière-obscurité perçu au niveau de l’oeil. Cette synchronisation entraîne l’expression de rythmes appropriés (hormonaux, veille-sommeil, température corporelle, etc.). Les hypothèses de ma thèse sont : 1- une exposition chronique à un spectre lumineux appauvri en longueurs d’ondes courtes, causée par l’opacification du cristallin chez le sujet âgé ou par l’exposition chronique à des lumières artificielles blanches, est à l’origine d’une altération de la réponse du système circadien à la lumière ; 2- une exposition chronique à un spectre lumineux enrichi en longueurs d’ondes courtes chez le sujet jeune, améliore la synchronisation du système circadien, la vigilance, les performances cognitives et la qualité du sommeil. L’objectif de ma thèse est d‘évaluer ces hypothèses selon deux approches : 1. Une approche physiologique : chez le sujet âgé sain, le brunissement physiologique du cristallin oculaire conduit à une filtration des longueurs d’ondes courtes du spectre lumineux. Cette approche inclus la mise au point et la validation d’un système de mesure de transmittance du cristallin in vivo. Ce système est nécessaire pour quantifier la qualité spectrale de la lumière atteignant la rétine. 2. Une approche artificielle : chez des sujets jeunes exposés de manière chronique (63 jours) à des lumières ambiantes blanches ou enrichies en longueurs d’ondes courtes / Physiological and behavioral circadian rhythms in mammals and humans are under the control of a central clock located in the suprachiasmatic nuclei of the hypothalamus. This endogenous clock has a period close to but not exactly 24 hours and therefore needs to be constantly entrained to the 24-h period of the earth, by the light-dark cycle. Light is perceived through the eyes and implicates all the retina’s photoreceptors (rods, cones, melanopsin ganglion cells (ipRGCs)). A properly entrained circadian system leads to an appropriate rhythmic expression of many physiological functions (hormonal secretion, sleep/wake cycles, core body temperature …). My project’s hypotheses are: 1- a chronic exposure to blue deprived light, as occurring in the aged due to lens filtration or under standard indoor lighting, leads to a decreased nonvisual sensitivity to light.; 2- exposure to blue enriched white light in the young subjects enhances non-visual responses to light such as, entrainment of the circadian system, vigilance, mood, sleep quality and cognitive performance. The aim of my thesis is to evaluate these hypotheses using two approaches : 1. A physiological approach: In the aged subject, in whom the ocular crystalline lens specifically filters short wavelength lights, known to be crucial for circadian entrainment. This approach includes the development and clinical validation of a scotopic heterochromatic flicker photometry technique to assess lens transmittance in vivo. This technique is essential to evaluate individual light spectra reaching the retina. 2. An artificial approach: In young subjects chronically exposed (63 days in the Concordia base, Antarctica) solely to standard white or blue enriched white light

Système circadien

Vieillissement

Lumière

Densité du cristallin

Non-visuel

Psychophysique

Mélatonine

Mélanopsine

Circadian system

Aging

Light exposure

Lens density

Non-visual

Psychophysics

Melatonin

Melanopsin

571.77

Impact de la rétinopathie diabétique sur le fonctionnement et l’entraînement par la lumière des horloges centrale et rétinienne / .

Lahouaoui, Hasna

17 December 2014

La rétinopathie diabétique est une cause majeure de cécité et de malvoyance qui affecte jusqu'à 90% des patients atteints de diabète. Le Maroc n’échappe pas à cette pathologie, qui est connue pour altérer le fonctionnement du système visuel et pourrait conduire également à des désordres chronobiologiques, aussi bien chez l’Homme que chez des modèles animaux. Ces altérations pourraient être liées aux dégénérescences neuronales des systèmes de photoréception classique (cône et bâtonnet) et des cellules ganglionnaires à mélanopsine, impliqués dans la régulation et l’entraînement par la lumière du système circadien. Cependant, à l’heure actuelle, peu d’études ont analysé précisément l’impact de la rétinopathie diabétique sur le système circadien. L’objectif de notre travail est d’analyser au cours de la rétinopathie diabétique (1) l’atteinte des cônes, des bâtonnets et des cellules ganglionnaires à mélanopsine, (2) le fonctionnement endogène moléculaire et la réponse à la lumière des horloges centrale et rétinienne et (3) la réponse comportementale du système circadien à la lumière. Notre stratégie est basée sur l’utilisation d’un modèle murin, chez lequel le diabète est induit expérimentalement par l’administration d’un agent chimique la streptozotocine (STZ), toxique pour les cellules β pancréatiques. Des approches morphométriques, moléculaires et comportementales ont été utilisées. Nos résultats montrent que le diabète induit des changements morphologiques des cellules ganglionnaires à mélanopsine tels que des gonflements des somas et des varicosités au niveau des dendrites avec une préservation du nombre total de ces cellules. Ceci est associé à une diminution de l’induction par la lumière du gène c-fos et des gènes de l’horloge Per1 et Per2 au niveau du SCN et à l’absence de cette induction au niveau rétinien au stade 12 semaines après l’induction du diabète. La machinerie moléculaire des horloges rétinienne et centrale évaluée par l’analyse de l’expression circadienne des gènes de l’horloge et des gènes contrôlés par les gènes de l’horloge montre que certains gènes de l’horloge clés pour chaque tissu sont altérés. A l’échelle comportementale, les souris STZ (souris diabétiques) montrent une réduction de l’amplitude du rythme de leur activité locomotrice totale et une diminution de la sensibilité à la lumière aux faibles intensités. Après une avance de phase du cycle 12L/12D, ces animaux présentent également une diminution de la vitesse de resynchronisation au nouveau cycle lumineux imposé par rapport aux animaux témoins. Ces nouvelles données montrent que le diabète de type 1 altère les réponses du système circadien à la lumière d’un point de vue moléculaire et comportemental et suggèrent que les patients diabétiques peuvent présenter des troubles circadiens particulièrement lorsqu’ils sont soumis aux challenges chronobiologiques / Diabetic retinopathy is a major cause of blindness and is commonly viewed as a vascular complication of type 1 diabetes. However, this kind of diabetes causes visual dysfunction before the onset of clinically visible microvascular changes, associated with diabetic retinopathy. Several histopathological studies in diabetic patients and in chemically-induced or genetic rodent models of diabetes indicate that photoreceptors and retinal ganglion cells (RGCs) are affected by diabetes with apoptotic degeneration. There is increasing evidence that melanopsin-expressing ganglion cells that are crucial for the regulation of a range of non-visual functions including the photic synchronization of circadian rhythms are altered in retinal pathologies. The link between diabetes and circadian rhythms has only been addressed in a relatively limited number of studies. Using a streptozotocin-induced (STZ) model of diabetes, we investigated the impact of diabetic retinopathy on non-visual functions by analyzing the morphology of melanopsin ganglion cells and light-induced c-fos and Period 1-2 clock genes in the central (SCN) and the retina clocks. The effect of this pathology on the endogenous circadian function of clock and controlled clock genes was assessed in the SCN and the retina at 12 weeks post-diabetes. Behaviorally, the ability of STZdiabetic mice to entrain to light was challenged by the exposure of animals to 1) successive light/dark (LD) cycle of decreasing or increasing light intensities during the light phase and 2) 6-hr advance of the LD cycle. Our results show that diabetes induces morphological changes of melanopsin-expressing ganglion cells including soma swelling and dendritic varicosities with no reduction in their total number, associated with decreased c-fos and clock genes induction by light in the SCN and also in the retina at 12 weeks post-onset of diabetes. In addition, the circadian expression of major clock genes was altered in the central and retinal clocks, suggesting that RD affects the endogenous molecular machinery and the light response of these two clocks. Moreover, STZ-diabetic mice exhibited a reduction of overall locomotor activity, a decrease of circadian sensitivity to light at low intensities, and a delay in the time to re-entrain after a phase advance of the LD cycle. These novel findings demonstrate that diabetes alters clock genes and behavioral responses of the circadian timing system to light and suggest that diabetic patients may show an increased propensity for circadian disturbances, in particular when they are exposed to chronobiological challenges

Rétinopathie diabétique

STZ

Système circadien

Horloge

Rétine

SCN

Photorécepteurs

Mélanopsine

Diabetic retinopathy

STZ

Melanopsin

SCN

Retina

Clock genes

Locomotor activity

Light intensity

570

Mechanisms of clock gene modulation by UVA radiation and visible light in normal (Melan-a) and transformed (B16-F10) melanocytes / Mecanismos de modulação de genes de relógio por radiação UVA e luz visível em melanócitos normais (Melan-a) e transformados (melanoma B16-F10)

Assis, Leonardo Vinícius Monteiro de

22 February 2019

The skin has a system that can detect light in a fashion similar to the retina. Although its presence was initially reported almost 20 years ago, only in 2011 functional studies started to be reported. The biological clock of the skin has also been reported in the beginning of the century, but its function and relevance still remain unexplored. Thus, this Ph.D. project was designed to explore the functionality of both systems in melanocytes, and whether the disruption of these systems is associated with the development of melanoma cancer. Using in vitro, in vivo, and bioinformatics approaches, we have shown that: 1) the biological clock of malignant melanocytes is more responsive to visible light, UVA radiation, estradiol, and temperature compared to normal cells; 2) UVA radiation is detected by melanopsin (OPN4) and rhodopsin (OPN2), which triggers a cGMP related cascade that leads to immediate pigment darkening (IPD) in normal and malignant melanocytes; 3) in addition to detecting UVA radiation, OPN4 also senses thermal energy, which activates the biological clock of both normal and malignant melanocytes; 4) regarding the biological clock, we have provided several layers of evidence that proves that in melanoma a chronodisruption scenario is established compared to healthy skin and/or normal pigment cells; 5) in vivo tumor samples display a low amplitude circadian rhythm of clock gene expression and an ultradian oscillatory profile in melanin content; 6) a non-metastatic melanoma leads to a systemic chronodisruption, which we suggest that could favor the metastatic process; 7) in human melanoma, we demonstrated the role of BMAL1 as a prognostic marker and a putative marker of immune therapy success. Taken altogether, these results significantly contributed to the literature as it brought to light new and interesting targets and processes, which will be explored in future projects / A pele possui um sistema que pode detectar luz de forma análoga à retina. Embora a presença deste sistema tenha sido inicialmente descrita quase há 20 anos, apenas no ano de 2011 estudos funcionais começaram a ser relatados. Sabe-se que o relógio biológico da pele também foi identificado no início do século, mas sua função e relevância ainda continuam pouco exploradas. Diante deste cenário, este projeto de doutorado foi desenhado para investigar a funcionalidade de ambos os sistemas em melanócitos e se perturbação dos mesmos estaria associada com o desenvolvimento de melanoma. Através do uso de abordagens in vitro, in vivo e de bioinformática, nós demonstramos que: 1) o relógio biológico de melanócitos malignos é mais responsivo à luz visível, radiação UVA, estradiol e temperatura comparado ao de células normais; 2) a radiação UVA é detectada por melanopsina (OPN4) e rodopsina (OPN2), que ativam uma via de sinalização dependente de GMPc, levando ao processo de pigmentação imediata (IPD) em melanócitos normais e malignos; 3) além de detecção de radiação UVA, a OPN4 também detecta energia térmica que, por sua vez, ativa o relógio biológico de melanócitos normais e malignos; 4) relativo ao relógio biológico, provamos por diferentes abordagens que, no melanoma, um cenário de cronoruputura está estabelecido em comparação a pele saudável e/ou melanócitos; 5) tumores in vivo apresentam um ritmo circadiano de baixa amplitude na expressão dos genes de relógio e um ritmo ultradiano oscilatório no conteúdo de melanina; 6) um melanoma não metastático leva a um quadro sistêmico de cronoruptura, o qual sugerimos favorecer o processo de metástase; 7) em melanoma humano, demonstramos o papel do gene BMAL11 como marcador de prognóstico e um possível indicador de sucesso de imunoterapias. Portanto, este projeto contribuiu de forma significante para a literatura científica uma vez que trouxe à luz novos e interessantes alvos terapêuticos e processos, os quais serão explorados em projetos futuros

Clock genes

Genes de relógio

Malignant melanocyte

Melanócito maligno

Melanocyte

Melanoma

Melanoma

Melanopsin

Melanopsina

Mus musculus

Rhodopsin

Rodopsina

Temperatura

Temperature

Ultraviolet A (UVA) radiation

Visible light