Your search keyword '"Free RB"' showing total 2 results

1. Surface and intracellular nicotinic receptors expressed in intact adrenal chromaffin cells: direct measurements using [3H]epibatidine.

Author

Free RB and McKay DB

Subjects

Adrenal Medulla cytology, Adrenal Medulla drug effects, Adrenal Medulla metabolism, Alkylation, Animals, Antibiotics, Antineoplastic pharmacology, Catecholamines biosynthesis, Cattle, Cells, Cultured, Dactinomycin pharmacology, Down-Regulation physiology, Immunohistochemistry, Intracellular Membranes metabolism, Microscopy, Confocal, Bridged Bicyclo Compounds, Heterocyclic, Chromaffin Cells metabolism, Nicotinic Agonists, Pyridines, Receptors, Cell Surface biosynthesis, Receptors, Nicotinic biosynthesis

Abstract

The presence and importance of assembled, intracellular neuronal nicotinic acetylcholine receptors (nAChRs) has not been established in native systems. In these studies [3H]epibatidine binding techniques were used to characterize surface and intracellular sites expressed in intact bovine adrenal chromaffin cells in culture. Permeant (300 microM nicotine) and impermeant (5 mM carbachol) cholinergic agents were used to define specific [3H]epibatidine binding to total (surface and intracellular) sites and surface sites, respectively. Intracellular [3H]epibatidine binding sites were characterized after eliminating surface binding sites via alkylation. Equilibrium binding to all sites was reached within 30 min at room temperature. Homologous (epibatidine) competition experiments on total (surface and intracellular) binding sites demonstrated a significant fraction of the high affinity sites were localized to intracellular compartments. Saturation binding assays to surface and intracellular sites revealed K(d) values of 1.9+/-1.1 and 3.6+/-1.9 nM, respectively. These binding studies document the existence of a significant population of high affinity, intracellular binding sites in native neuronal cells and support their characterization as assembled, alpha3beta4* nAChRs. Although the intracellular nAChRs represent approximately 70% of the total, high-affinity nAChRs expressed in cultured chromaffin cells, they do not appear to be involved in functional recovery after nAChR down-regulation.

Published

2003

2. Receptor protection studies to characterize neuronal nicotinic receptors: tubocurarine prevents alkylation of adrenal nicotinic receptors.

Author

Free RB and McKay DB

Subjects

Acetylcholine pharmacology, Adrenal Medulla drug effects, Alkylation drug effects, Animals, Binding, Competitive drug effects, Binding, Competitive physiology, Catecholamines metabolism, Cattle, Cells, Cultured, Chromaffin Cells drug effects, Drug Interactions physiology, Neurons drug effects, Receptors, Nicotinic drug effects, Adrenal Medulla metabolism, Chromaffin Cells metabolism, Neurons metabolism, Nicotinic Antagonists pharmacology, Receptors, Nicotinic metabolism, Tubocurarine pharmacology

Abstract

Our laboratory has evidence that multiple nicotinic acetylcholine receptor subtypes regulate bovine adrenal catecholamine release. In the following studies, receptor protection assays were used to differentiate adrenal nicotinic receptor subpopulations. Under alkylating conditions, bromoacetylcholine (30 microM) reduced nicotinic receptor-stimulated adrenal catecholamine secretion by approximately 80%. When 100 microM tubocurarine was present during alkylation, nicotine-stimulated secretion was reduced by less than 30%. Hexamethonium (500 microM), decamethonium (500 microM), mecamylamine (50 microM), pentolinium (50 microM), adiphenine (50 microM), methyllycaconitine (1 microM) and alpha-bungarotoxin (1 microM) afforded no protection when present during alkylation. When the pharmacology of residual, tubocurarine-protected receptors was investigated, the EC50 value for nicotine's stimulatory effects on secretion significantly increased from 4.0 (2.5-6.5) microM in control cells to 9.1 (7.2-11.4) microM in tubocurarine-protected cells. In addition, the IC50 value for tubocurarine's inhibitory effects on release significantly decreased from 0.7 (0.5-0.9) microM in control cells to 0.3 (0.2-0.4) microM in tubocurarine-protected cells. These studies support the use of protection assays to characterize nicotinic receptor subpopulations.

Published

2001