• Refine Query
  • Source
  • Publication year
  • to
  • Language
  • 3
  • 1
  • 1
  • 1
  • 1
  • Tagged with
  • 10
  • 4
  • 4
  • 4
  • 3
  • 3
  • 3
  • 3
  • 3
  • 3
  • 3
  • 2
  • 2
  • 2
  • 2
  • About
  • The Global ETD Search service is a free service for researchers to find electronic theses and dissertations. This service is provided by the Networked Digital Library of Theses and Dissertations.
    Our metadata is collected from universities around the world. If you manage a university/consortium/country archive and want to be added, details can be found on the NDLTD website.
1

Einfluss von L-alpha-Lysophosphatidylinositol (LPI) auf neuronale Schädigungsprozesse

Kremzow, Stine 04 March 2016 (has links) (PDF)
Die vorliegende Arbeit beinhaltet experimentelle Untersuchungen zur neuroprotektiven Wirkung des körpereigenen Lipids L-alpha-Lysophosphatidylinositol (LPI). Die Vermittlung dieser Wirkung soll durch den zentralnervös exprimierten G-Protein-gekoppelten Rezeptor 55 (GPR55) erfolgen. Als Modelsystem diente die organotypische hippocampale Schnittkultur (OHSC) der Ratte, welche exzitotoxisch mittels N-Methyl-D-Aspartat (NMDA) geschädigt wurde, um Neurodegeneration zu initiieren. Die Inkubation mit LPI nach NMDA-Schädigung reduzierte die Anzahl toter Neurone und die der Mikroglia in der Körnerzellschicht des Gyrus dentatus. Ein Clodronat-induzierter Verlust der Mikroglia und die siRNA-vermittelte Herabregulation von Gpr55 hoben jeweils den neuroprotektiven Effekt von LPI in der OHSC auf. Diese Beobachtungen wiesen auf eine Mikroglia- und GPR55 abhängige Neuroprotektion hin. LPI wirkte zudem synergistisch und verstärkte die (bekannter Maßen) durch Cannabinoide induzierte und über den Cannabinoid Typ 1 Rezeptor vermittelte Neuroprotektion. Ferner wurde Gpr55 mittels qPCR in Mikroglia und Astrozyten nachgewiesen. LPI steuerte außerdem die Expression von Gpr55 in Mikroglia und beeinflusste deren Migrationsverhalten. Die vorliegenden Ergebnisse machen deutlich, dass LPI in einem in vitro Modellsystem zur Untersuchung des sekundären neuronalen Schadens protektiv wirkt und für die Vermittlung dieser Neuroprotektion Mikroglia und GPR55 in Frage kommen.
2

THE ROLE OF GPR55 IN NEURAL STEM CELL PROLIFERATION, DIFFERENTIATION, AND IMMUNE RESPONSES TO CHRONIC, SYSTEMIC INFLAMMATION

Hill, Jeremy David January 2018 (has links)
The cannabinoid system exerts functional regulation of neural stem cell (NSC) selfrenewal, proliferation, and differentiation during both homeostatic and pathologic conditions. Recent evidence suggests that cannabinoid signaling is neuroprotective against reduction in NSC proliferation and neurogenesis caused by a multitude of conditions including injury due to HIV-1 associated neurotoxic proteins, neuroinflammation, and stroke. Yet not all effects of cannabinoids or cannabinoid-like compounds on neurogenesis can be attributed to signaling through either of the classical cannabinoid receptors CB1 or CB2. The recently de-orphaned GPR55 is targeted by numerous cannabinoid compounds suggesting GPR55 may be causing these aberrant effects. Activation of GPR55 has shown immune-modulatory effects outside the central nervous system (CNS) and anti-inflammatory actions on microglia, the resident immune cells within the CNS. New evidence has confirmed that both human and murine NSCs express functional levels of GPR55 yet the effects that GPR55 activation has on adult neurogenesis or NSC responses to inflammation has not been elucidated. In the present study we sought to determine the role GPR55 signaling has on NSC proliferation and neurogenesis as well as possible neuroprotective mechanisms within the NSC pool in response to inflammatory insult. Activation of GPR55 increased human NSC proliferation in vitro as assessed by BrdU incorporation and flow cytometry. Neuronal differentiation was also upregulated by signaling through GPR55 under homeostatic conditions in both human and murine NSC samples. Expression of NSC differentiation markers (nestin, sox2, GFAP, S100b, DCX, bIII-tubulin) in vitro was determined by immunohistochemistry, qPCR, and flow cytometry. In vivo, C57BL/6 and GPR55-/- mice were administered the GPR55 agonist O-1602 (4 μg/kg/day) directly into the left hippocampus via stainless steel cannula connected to an osmotic mini-pump for a continuous 14 days. O-1602 treatment increased hippocampal NSC proliferation, survival, and immature neuron formation as compared to vehicle treated animals. These results were determined to be dependent on GPR55 activation as GPR55-/- animals did not show any response to agonist treatment. Interestingly, GPR55-/- mice displayed significantly reduced rates of hippocampal NSC proliferation and neuroblast formation as compared to C57BL/6 animals. Chronic production of inflammatory mediators, such as IL-1b seen in neuroinflammation, to NSCs is known to reduce proliferation rates and attenuate neurogenesis both in vitro and in vivo. Addition of GPR55 agonists to IL-1b (10 ng/mL) treated human and murine NSC samples in vitro protected against reductions in neuron formation as assessed by immunohistochemistry and flow cytometry. Moreover, inflammatory cytokine receptor mRNA expression was down regulated by GPR55 activation in a neuroprotective manner. To determine inflammatory responses in vivo, we treated C57BL/6 and GPR55-/- mice with LPS (0.2 mg/kg/day) continuously for 14 days via osmotic mini-pump. Reductions in NSC survival (as determined by BrdU incorporation), immature neurons, and neuroblast formation due to LPS were attenuated by concurrent direct intrahippocampal administration of the GPR55 agonist, O-1602 (4μg/kg/day) in C57BL/6 mice but not in GPR55-/-mice. Neuroprotection by O-1602 treatment was not found to be microglia dependent as microglia activation was not altered by agonist administration. Molecular analysis of the hippocampal region showed a suppressed ability to regulate immune responses by GPR55-/- animals manifesting in a prolonged inflammatory response (IL-1b, IL-6, TNFa) after chronic, systemic inflammation as compared to C57BL/6 animals. Taken together, these results suggest a neuroprotective role of GPR55 activation on NSCs in vitro and in vivo and that GPR55 provides a novel therapeutic target against negative regulation of hippocampal neurogenesis by inflammatory insult. / Biomedical Sciences
3

Einfluss von L-alpha-Lysophosphatidylinositol (LPI) auf neuronale Schädigungsprozesse: Einfluss von L-alpha-Lysophosphatidylinositol (LPI) aufneuronale Schädigungsprozesse

Kremzow, Stine 31 August 2015 (has links)
Die vorliegende Arbeit beinhaltet experimentelle Untersuchungen zur neuroprotektiven Wirkung des körpereigenen Lipids L-alpha-Lysophosphatidylinositol (LPI). Die Vermittlung dieser Wirkung soll durch den zentralnervös exprimierten G-Protein-gekoppelten Rezeptor 55 (GPR55) erfolgen. Als Modelsystem diente die organotypische hippocampale Schnittkultur (OHSC) der Ratte, welche exzitotoxisch mittels N-Methyl-D-Aspartat (NMDA) geschädigt wurde, um Neurodegeneration zu initiieren. Die Inkubation mit LPI nach NMDA-Schädigung reduzierte die Anzahl toter Neurone und die der Mikroglia in der Körnerzellschicht des Gyrus dentatus. Ein Clodronat-induzierter Verlust der Mikroglia und die siRNA-vermittelte Herabregulation von Gpr55 hoben jeweils den neuroprotektiven Effekt von LPI in der OHSC auf. Diese Beobachtungen wiesen auf eine Mikroglia- und GPR55 abhängige Neuroprotektion hin. LPI wirkte zudem synergistisch und verstärkte die (bekannter Maßen) durch Cannabinoide induzierte und über den Cannabinoid Typ 1 Rezeptor vermittelte Neuroprotektion. Ferner wurde Gpr55 mittels qPCR in Mikroglia und Astrozyten nachgewiesen. LPI steuerte außerdem die Expression von Gpr55 in Mikroglia und beeinflusste deren Migrationsverhalten. Die vorliegenden Ergebnisse machen deutlich, dass LPI in einem in vitro Modellsystem zur Untersuchung des sekundären neuronalen Schadens protektiv wirkt und für die Vermittlung dieser Neuroprotektion Mikroglia und GPR55 in Frage kommen.
4

Studium signalizace a cytoprotektivního potenciálu kanabinoidních GPR55 receptorů v PC12 buňkách / A study of signaling and cytoprotective potential of cannabinoid GPR55 receptors in PC12 cells

Pavluch, Vojtěch January 2016 (has links)
At the end of the 20th century it was known that cannabinoid drugs interact with two receptors, CB1 and CB2. Subsequent pharmacological studies have confirmed that there are other receptors interacting with cannabinoids. GPR55 is a transmembrane G protein coupled receptor, which together with the receptor GPR18 and GPR119 belong to a group of new cannabinoid receptors and is involved in the function of the endocannabinoid system. In addition to some of cannabinoid substances, it is stimulated primarily phospholipid lysofosfatidylinositolem. LPI-dependent signaling GPR55 plays an important role in the regulation of many physiological and pathological processes, such as pain, inflammation, cell proliferation, or endothelial function. It was found that LPI confers tolerance to ischemic brain damage and has a cytoprotective effect on the pyramidal cells. The aim of the study was to determine whether the application of five ligands induce phosphorylation of protein kinase ERK 1/2, Akt and activate the GTPase RhoA and whether activation of the receptor GPR55 has cytoprotective effect in model cell line PC12, in which hypoxic conditions were simulated by adding CoCl2. For working methods were used SDS-PAGE, Western bloting and colorimetric measurement. Pharmacological studies in recent years have shown...
5

Modulation of Synaptic Plasticity: Endocannabinoids and Novel G-protein Coupled Receptors Expression and Translational Effects in Interneurons

Hurst, Katrina M. 01 July 2017 (has links)
Learning and memory are important processes that occur in the brain. The brain is comprised of neurons that make connections with each other known as synapses. Synaptic plasticity is widely believed to be the physiologic mechanism by which learning and memory occur. Synapses can either be strengthened through a process known as long-term potentiation (LTP) or weakened through long-term depression (LTD). The area of the brain that is most studied for its role in learning and memory is the hippocampus, which has been shown to be involved in memory consolidation. The detection of endocannabinoids and their receptors has opened a whole new field of study in regards to synaptic plasticity. Cannabinoid receptor 1 (CB1) and transient receptor potential vanilloid 1 (TRPV1) are among the commonly studied endocannabinoid receptors found in the central nervous system. In the brain, these receptors' natural ligands, anandamide and 2-arachidonylglycerol (2-AG), are found in abundance. Yet not all forms of observed plasticity are accounted for by just these two receptors, so studies into other G-protein coupled receptors (GPCRs) continues. One GPCR, GPR55 is found in many regions of the brain, as well as lysophosphatidylinositol (LPI), its specific ligand. Here we have researched the role of GPR55 in modulating synaptic plasticity in the hippocampus. Using quantitative reverse transcription PCR and immunohistochemistry, we have found GPR55 to be expressed in the hippocampus with highest expression in pyramidal cells, the main excitatory neurons in the hippocampus. Using field and whole cell electrophysiology, we have investigated its effects on synaptic plasticity, discovering that activation of GPR55 by LPI significantly enhances LTP. In memory behavioral assays there are no significant differences between GPR55 KO mice and wild type littermates, indicating that it may not be involved in endogenous memory processes. However, our electrophysiology data makes GPR55 a potential target for treating memory disorders such as dementia. We have also investigated GPR18 and GPR119 for their potential roles in synaptic plasticity. First, we confirmed their expression in the hippocampus and then investigated the effects of their agonists on plasticity. Another receptor, TRPV1 has been studied to alter plasticity. However, the study of how protein translation and RNA transcription involvement in TRPV1 plasticity in mammals has not been investigated. While translation and transcription are known to be important in many forms of LTP, it is unknown whether these processes are important for TRPV1-induced LTD. We are investigating their necessity via whole cell patching and using translation and transcription inhibitors Anisomycin and Actinomycin D, both previously used in slice electrophysiology.
6

The Putative Cannabinoid Receptor GPR55 Modulates Synaptic Plasticity in the Hippocampus

Badgley, Corinne Marie 14 June 2012 (has links) (PDF)
Endocannabinoids (eCBs) are small molecules that are capable of modulating synaptic plasticity of both excitatory and inhibitory synapses in the brain. While eCBs bind to transient receptor potential vanilloid 1 (TRPV1) and cannabinoid receptor 1 (CB1) in the central nervous system, we recently identified a form of non-CB1, non-TRPV1 mediated long term depression activated by the eCB anandamide at CA1 hippocampal stratum radiatum interneurons. GPR55, an orphan G-protein receptor, has been identified in the hippocampus and is capable of activation by eCBs, making it a good candidate for mediating this non-CB1, non-TRPV1 form of synaptic plasticity. Here we performed whole-cell patch clamp recordings from CA1 stratum radiatum interneurons in rat brain slices to investigate the effect of GPR55 agonist O-1602 on excitatory synapses. We also performed field recordings from CA1 pyramidal cells in rats and GPR55 knockout mice and littermate controls to investigate the effect of GPR55 agonists O-1602 and lysophosphatidylinositol (LPI) on both basal output and electrically induced long-term depression and long-term potentiation in the hippocampus. Application of O-1602 in rats depressed long-term potentiation in CA1 pyramidal cells, and depressed excitatory glutamatergic transmission onto some interneurons. O-1602 had no effect on long-term depression of CA1 pyramidal cells. GPR55 +/+ mice showed an increase in long-term potentiation in the presence of LPI compared to GPR55-/- littermates. GPR55-/-mice had no change in long-term potentiation when exposed to O-1602, though there was an increase in post-tetanic potentiation with O-1602. In order to examine whether GPR55 has a role in formation of spatial memory, GPR55 -/- mice were compared to littermate controls during a Morris water maze behavioral task, with a reversal task after 7 days of training. GPR55-/-mice did not perform in a different manner on either the training task or the reversal, though there may be a trend of difference in training worth investigating further. This study illustrates a novel pathway for synaptic plasticity modulation through GPR55 in the hippocampus, and may therefore provide valuable insight into both the effects of synthetic and endogenous cannabinoids on the brain and the processes underlying learning and memory.
7

Contribution du récepteur GPR55 à la synaptogenèse

Germain, Philippe 04 1900 (has links)
Les connections synaptiques entre les cellules nerveuses (appelées synapses) sont essentielles à l’établissement de l’architecture du système nerveux. La modification de ces synapses est un des mécanismes par lequel l’apprentissage et la mémoire fonctionnent. On sait depuis plusieurs années déjà que la consommation de cannabis exerce une profonde influence sur l’apprentissage et la mémoire, et que sa consommation chez la femme durant la grossesse ou l’allaitement peut causer des déficits cognitifs chez l’enfant qui perdureront à l’âge adulte. Pour le moment, on ne sait toujours pas si ces effets sont médiés par les récepteurs aux cannabinoïdes classiques (CB1 et CB2) ou par d’autres récepteurs tel le GPR55. Des études récentes du laboratoire du Pr. Bouchard ont démontré un rôle important du système endocannabinoïde dans le développement du système nerveux notamment par la présence du récepteur GPR55 et son implication dans la modulation du guidage et de la croissance des axones durant les périodes foetale et périnatale. Comme certaines molécules et mécanismes cellulaires impliqués dans ces processus peuvent aussi jouer un rôle dans la formation de synapses (synaptogenèse), l’objectif de la présente étude est de déterminer la contribution du GPR55 dans la formation de contacts synaptiques. À partir de cortex d’embryons de souris, nous avons cultivé puis traité des neurones corticaux soit avec un agoniste sélectif de GPR55 (O-1602) ou son antagoniste sélectif (ML-193), soit avec un phytocannabinoïde (cannabidiol) pendant 24 heures au 9e jour in vitro. En immunocytochimie, les neurones traités avec le ML-193 ont démontré une réduction significative du nombre de contacts synaptiques et une augmentation significative avec l’O-1602 et le cannabidiol. Ces changements anatomiques sont corrélés avec des modifications de l’expression des protéines synaptiques GluR1 et synaptophysine au niveau du cortex. En plus de fournir d’importantes informations sur le développement du système nerveux, les résultats de cette étude contribuent à l’amélioration de nos connaissances sur les anomalies du développement induites par la consommation périnatale de cannabis. / Functional connections between nerve cells (called synapses) are essential to establish the architecture of the nervous system. The modification of synapses is thought to be one of the mechanisms by which learning and memory occur. It has been known for decades that cannabis consumption has a profound influence on learning and memory, and that maternal marijuana smoking during perinatal period causes cognitive deficits that last in the adulthood of the offspring. For the moment, we do not know if these effects are mediated by the classic CB1 and CB2 cannabinoid receptors or by other receptors such as GPR55. Recent studies by Pr. Bouchard have demonstrated an important role for the endocannabinoid system in the development of the nervous system, including the presence of GPR55 and its involvement in axon growth and target innervation during the fetal and early postnatal periods. As certain molecules and cellular mechanisms involved in these processes may also regulate synapse formation (synaptogenesis), the objective of the present study is to determine the contribution of GPR55 in the formation of new synaptic contacts. Primary cortical neurons isolated from embryonic mice were cultivated and then treated either with a selective agonist of GPR55 (O-1602) or his selective antagonist (ML-193), or with a phytocannabinoid (cannabidiol) for 24h at the ninth day in vitro (DIV9). In immunocytochemistry, neurons treated with ML-193 have shown a decrease in synaptic density, while the treatment with O-1602 or cannabidiol increased it. These anatomical changes were correlated with changes in the expression of synaptic proteins GluR1 and synaptophysin. Results from this study provide important insight on the development of the nervous system and contribute to improving our knowledge on developmental abnormalities induced by perinatal cannabis use.
8

Les impacts du récepteur GPR55 sur les fonctions visuelles

Bachand, Ismaël 12 1900 (has links)
Il est connu que le cannabis, par son action sur le système endocannabinoïde, affecte de multiples paramètres de la vision. Les fonctions de GPR55, un récepteur associé au système endocannabinoïde, ont moins été étudiées que celles des récepteurs cannabinoïdes les plus importants, CB1 et CB2. Nous savons cependant que GPR55 est présent dans la rétine de la souris et qu’il module la croissance et le guidage axonal des cellules ganglionnaires rétiniennes durant le développement. Le but de cette étude est d’étudier les effets de GPR55 sur la vision en utilisant un modèle de souris avec une délétion du gène Gpr55. Des électrorétinographies (ERG) plein champ scotopique et photopique ont été effectuées dans le but d’étudier le rôle du récepteur sur les fonctions rétiniennes. Nous avons trouvé que les souris Gpr55-/- ont, en ERG scotopique, une amplitude réduite de l’onde-b et des potentiels oscillatoires qui ont aussi une latence plus longue. Chez ces animaux, l’onde-a photopique a aussi une amplitude plus basse. Par la suite, pour vérifier les conséquences des déficits de fonction rétinienne sur les fonctions visuelles, le modèle de réflexe optomoteur a été utilisé sur des souris knock-out ou avec des injections systémiques d’un antagoniste et d’un agoniste de GPR55. L’absence de GPR55 retarde le développement de l’acuité visuelle, mais la délétion de Gpr55 ou l’action pharmacologique sur le récepteur ne change pas l’acuité visuelle chez les adultes. La délétion de Gpr55 et l’administration d’un antagoniste du récepteur diminuent la sensibilité au contraste. Ces observations suggèrent que GPR55 peut modifier l'activité des cônes, des cellules bipolaires et des cellules de la rétine interne avec des conséquences comportementales. / The observations on how cannabis affects multiple properties of vision have fostered the interest in the study of the functions of cannabinoid receptors CB1 and CB2 in the visual system. However, other non-classical cannabinoid receptors are thought to be involved in mediating the actions of cannabinoid ligands in the eye. One of these candidate receptors is GPR55, a receptor that modulates the growth and axonal guidance of retinal ganglion cells during development in mice. The purpose of this study was to investigate the effects of the deletion of the Gpr55 gene and the pharmacological modulation of GPR55 on retinal function and visual behavior. Full-field scotopic and photopic electroretinography (ERG) were used to functionally assess the state of the retina. Recordings obtained from Gpr55-/- mice revealed a diminution of the scotopic b-wave and the photopic a-wave responses. These animals also had reduced and delayed oscillatory potentials. The optomotor reflex method was used to evaluate the consequences of Gpr55 deletion on visual acuity and contrast sensitivity. The absence of GPR55 delayed the developmental trajectory of visual acuity in Gpr55 knockout mice without affecting the maximum visual acuity reached in adulthood. Pharmacological manipulation of GPR55 in adult wild-type mice did not alter visual acuity. Both the deletion of Gpr55 and the administration of a receptor antagonist decreased contrast sensitivity while an agonist of GPR55 increased contrast sensitivity. These observations suggest that GPR55 can modify the activity of cones, bipolar cells, and cells in the inner retina with behavioral consequences.
9

Contribution du récepteur GPR55 dans la formation des contacts synaptiques

Lacomme, Lucile 08 1900 (has links)
La synaptogenèse est un processus biologique aboutissant à la mise en place d’un réseau de connexions neuronales, par la genèse de synapses. La mise en place de ce réseau de connexions est essentielle au développement du système nerveux central (SNC) et de ses fonctions. Tout comme les autres étapes du développement du SNC, la synaptogenèse est régulée par une multitude de signaux cellulaires, et le système endocannabinoïde en fait partie. Les dérivés du cannabis tel que le Δ-9-tétrahydrocannabinol (THC) et le cannabidiol (CBD) sont capables de traverser la barrière placentaire et de se retrouver dans le lait maternel. Par leur interaction avec le SNC, entre autres, ces phytocannabinoïdes sont capables d’influencer son développement. Le récepteur couplé à une protéine G 55 (GPR55) est catégorisé comme récepteur atypique du système endocannabinoïde, et il est capable d’être antagonisé par le CBD. Il a été prouvé par de précédentes études qu’il est lui aussi impliqué dans le développement du SNC, notamment dans le guidage et la croissance des axones durant les périodes fœtale et périnatale. Dans la littérature, il est souvent rapporté que les signaux impliqués dans le guidage axonal le sont aussi dans la synaptogenèse. C’est pourquoi le présent mémoire vise à examiner le rôle du récepteur GPR55 et l’effet de sa modulation par le CBD dans la formation de contacts synaptiques. Le modèle utilisé pour cette étude est la culture de neurones corticaux issus d’embryons de souris de génotypes gpr55+/+ et gpr55-/-. Pour comprendre le rôle physiologique de GPR55 dans la synaptogenèse nous avons étudié l’effet de la délétion du récepteur GPR55 à deux temps, Day In Vitro (DIV) 9-10 au début de la synaptogenèse, et à DIV14-15 un temps plus avancé. Ensuite pour comprendre comment le CBD est capable d’influencer la formation de contacts synaptiques de manière dépendante ou non de GPR55, les cultures de neurones corticaux de chaque génotype ont été exposées à DIV9 pour 24h à différentes concentrations du CBD (0,3uM ou 0,6uM ou 1uM). Les effets sur la formation de contacts synaptiques ont été étudiés en immunocytochimie, en immunobuvardage et en électrophysiologie de type patch clamp. Les résultats montrent que la délétion de GPR55 entraine à DIV14-15 une augmentation de la densité des contacts synaptiques, mais une réduction de leur aire et de l’expression de la synaptophysine, en affectant l’activité synaptique. L’exposition au CBD 0,6uM et 1uM entrainent de manière dépendante ou partiellement dépendante à GPR55, une augmentation de la densité des contacts synaptiques sans affecter leur aire, l’expression de protéines synaptiques ainsi que l’activité synaptique. La fréquence de décharge des neurones est diminuée de manière dépendante de GPR55 après l’exposition au CBD 1uM. Ces résultats suggèrent que GPR55 pourrait être un signal important pour l’arrêt de la formation de nouvelles synapses et un signal d’induction pour la maturation des synapses existantes. / Synaptogenesis is a biological process that leads to the establishment of a network of neuronal connections through the genesis of synapses. The formation of this network of connections is essential for the development of the central nervous system (CNS) and its functions. Like other stages of CNS development, synaptogenesis is regulated by multiple cellular signals, and the endocannabinoid system is part of it. Cannabis derivatives such as Δ-9-tetrahydrocannabinol (THC) and cannabidiol (CBD) can cross the placental barrier and be present in breast milk. Through their interaction with the endocannabinoid system, among others, these phytocannabinoids can influence CNS development. The G protein-coupled receptor 55 (GPR55) is categorized as an atypical receptor of the endocannabinoid system, and it can be antagonized by CBD. Previous studies have shown that GPR55 is also involved in CNS development, particularly in the guidance and growth of axons during fetal and perinatal periods. It is often reported in the literature that the signals involved in axonal guidance are also involved in synaptogenesis. Therefore, this study investigates the role of the GPR55 receptor and the effect of its modulation by CBD in the formation of synaptic contacts. The model used for this study consists of cortical neuron cultures from mouse embryos gpr55+/+ and gpr55-/- . To understand the physiological role of GPR55 in synaptogenesis, we studied the effect of gpr55 deletion at two-time points: Day In Vitro (DIV) 9- 10 at the beginning of synaptogenesis, and DIV14-15 at a later time point. Then, to understand how CBD can influence the formation of synaptic contacts, whether dependent or independent of GPR55, cortical neuron cultures of each genotype were exposed to different concentrations of CBD (0.3µM or 0.6µM or 1µM) at DIV9 for 24 hours. The effects on the formation of synaptic contacts were studied through immunocytochemistry, western blot, and patch clamp electrophysiology. The results show that gpr55 deletion leads to an increase in synaptic contact density at DIV14-15 but a reduction in their area and synaptophysin expression, by affecting synaptic activity. Exposure to 0.6µM and 1µM CBD results in a GPR55-dependent or partially dependent increase in synaptic contact density without affecting their area, expression of synaptic proteins, and synaptic activity. The firing frequency of neurons is decreased in a GPR55- dependent manner after exposure to 1µM CBD. These results suggest that GPR55 could be an important signal for stopping the formation of new synapses and an induction signal for the maturation of existing synapses.
10

Rôle des récepteurs aux protéines G (GPR55, GPR91 et GPR99) dans la croissance et le guidage axonal au cours du développement du système visuel

Cherif, Hosni 09 1900 (has links)
No description available.

Page generated in 0.0335 seconds