IBCN   20355
INSTITUTO DE BIOLOGIA CELULAR Y NEUROCIENCIA "PROFESOR EDUARDO DE ROBERTIS"
Unidad Ejecutora - UE
información general
recursos humanos
líneas de investigación
servicios tecnológicos
proyectos financiados por CONICET
proyectos financiados por otras instituciones
artículos
libros
capítulos de libros
congresos y reuniones científicas
informe técnico
congresos y reuniones científicas
Título:
Deficiency of CB1 receptor produces alterations in dendritic fibers in striatum
Autor/es:
NOVAK LUCIANA; VILLALBA, NERINA; SORIANO DELIA; CALTANA LAURA; MADARNAS CATALINA; BRUSCO ALICIA
Lugar:
BUENOS AIRES
Reunión:
Congreso; IV INTERNATIONAL CONGRESS IN TRASLATIONAL MEDICINE; 2018
Institución organizadora:
FACULTAD DE FARMACIA Y BIOQUIMICA - UBA
Resumen:
INTRODUCTION The cannabinoid receptor type 1 (CB1R) is one of the most abundant G protein-coupled receptors in the Central Nervous System and is presynaptically located in axonal terminals, dendrites and soma. It is widely distributed in the Central Nervous System, both in neurons and glial cells, and has a greater expression in areas such as hippocampus, cerebellum, cerebral cortex, striatum, among others. CB1R is involved in physiological processes such as memory, learning, motor coordination, anxiety and mood. Previous results of ourgroup showed that hippocampal neurons presented less dendritic and axonal arborization and changes in the synaptic structure. AIMS The aim of this work is to evaluate the axonal and dendritic neuronal cytoskeleton in the Striatum in the absence of CB1R, using cnr1 -/- knockout mice (CB1R -/-). EXPERIMENTAL PROCEDURE Sixty-day-old female and male, CD1 CB1R wild type (CB1R+/+) and CB1R knock-out mice (CB1R-/-) were used in this study. CB1R-/- mice were generated by disruption of the cnr1 gene. Animals were fixed by intracardiac perfusion with 4% (w/v) parafolmaldehyde in 0.1M phosphate buffer (PB) pH 7.4 and post-fixed for 4h in the same solution. Coronal sections of the brains were cut with a vibratome (40μm thick) and stored in 50% (v/v) glycerol solution at -20°C until use. Immunohistochemistry was performed with primary antibodies: mouse anti-Syn (1:1000); mouse anti-MAP-2 (1:1000); mouse anti- NF160 (1:1000); mouse anti- NF200 (1:1000). In order to evaluate MAP-2, NF160+ and NF200+ fibers, the total area of the immunolabeled fibers was related to the total area of the corresponding microscopic field (20x primary magnification), rendering a relative area parameter. The intensity of Syn immunoreactivity was evaluated by means of a relative optical density (ROD). RESULTS MAP2 is a protein expressed in neuronal dendrites. We observed significant decrease in female CB1R-/- mice when compared with female CB1R+/+ mice and male CB1R-/- mice (p