MEASUREMENT OF CHANGES IN FUNCTIONAL MUSCARINIC ACETYLCHOLINE-RECEPTOR DENSITY IN SINGLE NEUROBLASTOMA-CELLS USING CALCIUM-RELEASE KINETICS

Calcium release in response to the activation of muscarinic M1 and histamine H-1 receptors was studied in single N1E-115 cells using Fura-2 imaging. The objective was to relate changes in the kinetics of Ca release with reductions in functional receptor density resulting from receptor desensitization. Calcium release increased and ifs time course accelerated with increasing carbachol concentration with an EC(50) = 98 +/- 8 mu M This value is similar to the binding K-D (100 mu M) and the similarity shows that the activation of calcium release is limited by the number of muscarinic receptors. In contrast, the EC(50) for Ca release in response to histamine is 4.0 +/- 0.7 mu M while the binding K-D is 8.3 mu M and, therefore, H-1 receptors appear to be in approximately 2-fold excess over the minimum number necessary to fully engage the Ca release mechanism. Functional surface receptor number was assayed in the population of cells by counting the total number of cells responding to agonist. A 5 min exposure to 1 mW carbachol caused 12% of cells to lose their ability to respond to carbachol, with no change in their response to histamine. Interpolating from the dose-response curve taken before desensitization, this is equivalent to an average 23% reduction in the number of muscarinic receptors. In individual cells the latency to Ca release is dose-dependent in the absence of excess receptors. The loss of functional receptors was therefore estimated from the increase in latency after desensitization, and varied from 5-48% of receptors (22 +/- 18%). Muscarinic desensitization did not depend on IP3-evoked Ca release, Ca entry, protein kinase C, NO, or cGMP. We conclude that in a population, the number of cells responding and in single cells, the latency to Ca release can serve as measures of functional receptor density.