MAP kinase pathway activation is measured by ERK1/2 phosphorylation

Rafael Rivas-Santisteban; Alejandro Lillo; Jaume Lillo; Joan-Biel Rebassa; Joan S. Contestí; Carlos A. Saura; Rafael Franco; Gemma Navarro

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MAP kinase pathway activation is measured by ERK1/2 phosphorylation

RR Rafael Rivas-Santisteban

AL Alejandro Lillo

JL Jaume Lillo

JR Joan-Biel Rebassa

JC Joan S. Contestí

CS Carlos A. Saura

RF Rafael Franco

GN Gemma Navarro

This method is extracted from research article: Alzheimers Res Ther, Nov 2021

N-Methyl-D-aspartate (NMDA) and cannabinoid CB2 receptors form functional complexes in cells of the central nervous system: insights into the therapeutic potential of neuronal and microglial NMDA receptors

DOI: 10.1186/s13195-021-00920-6

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Hippocampal neurons, microglial cells, or HEK-293T cells cotransfected with the cDNA for the protomers of the NMDA receptor, GluN1 (1 μg) and GluN2B (0.75 μg), and/or with the cDNA for CB₂R (1 μg) were plated in transparent Deltalab 96-well microplates. Primary microglial cells were activated by incubating cells with 1 μM LPS and 200 U/mL IFN-γ during 48 h. Two hours before the experiment, the medium was substituted by serum-starved DMEM medium. Cells were treated or not for 10 min with the selective antagonists (MK-801 (1 μM) or SR-144528 (1 μM)) followed by 7 min treatment with the selective agonists (NMDA (15 μM) and/or JWH-133 (100 nM)). Cells were then washed twice with cold PBS before the addition of lysis buffer (15 min treatment). Ten microliters of each supernatant was placed in white ProxiPlate 384-well microplates and ERK1/2 phosphorylation was determined using an AlphaScreen®SureFire® kit (Perkin Elmer) following the instructions of the supplier and using an EnSpire® Multimode Plate Reader (PerkinElmer).

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