4.5 Article

Distribution of the Cannabinoid Receptor Type 1 in the Brain of the Genetically Audiogenic Seizure-Prone Hamster GASH/Sal

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出版社

FRONTIERS MEDIA SA
DOI: 10.3389/fnbeh.2021.613798

关键词

cannabinoid receptors; GASH; Sal; epilepsy; gene expression; immunohistochemistry

资金

  1. RiverForce Partners Inc. [Art. 83. 2019/00106/001]
  2. Instituto de Salud Carlos III (ISCIII)
  3. European Union FEDER funds [PI19/01364]

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The study found that CB1R is widely distributed in many nuclei of the central nervous system in epileptic animal models, with practically identical expression patterns between the GASH/Sal model and control group, although with slightly weaker immunostaining intensity in certain regions, especially in brain areas associated with epileptic networks. The research provides an anatomical basis for further investigation of CB1R in acute and kindling audiogenic seizure protocols in the GASH/Sal model, as well as exploring CB1R activation through exogenously administered cannabinoid compounds.
The endocannabinoid system modulates epileptic seizures by regulating neuronal excitability. It has become clear that agonist activation of central type I cannabinoid receptors (CB1R) reduces epileptogenesis in pre-clinical animal models of epilepsy. The audiogenic seizure-prone hamster GASH/Sal is a reliable experimental model of generalized tonic-clonic seizures in response to intense sound stimulation. However, no studies hitherto had investigated CB1R in the GASH/Sal. Although the distribution of CB1R has been extensively studied in mammalian brains, their distribution in the Syrian golden hamster brain also remains unknown. The objective of this research is to determine by immunohistochemistry the differential distribution of CB1R in the brains of GASH/Sal animals under seizure-free conditions, by comparing the results with wild-type Syrian hamsters as controls. CB1R in the GASH/Sal showed a wide distribution in many nuclei of the central nervous system. These patterns of CB1R-immunolabeling are practically identical between the GASH/Sal model and control animals, varying in the intensity of immunostaining in certain regions, being slightly weaker in the GASH/Sal than in the control, mainly in brain regions associated with epileptic networks. The RT-qPCR analysis confirms these results. In summary, our study provides an anatomical basis for further investigating CB1R in acute and kindling audiogenic seizure protocols in the GASH/Sal model as well as exploring CB1R activation via exogenously administered cannabinoid compounds.

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