EFFECT OF SOLVENT ON THE HISTAMINE-RELEASING, ENZYME-RELEASING, AND MITOGENIC PROPERTIES OF THE CALCIUM IONOPHORE-A23187

The potency of the calcium ionophore A23187 in inducing three activities of human leukocytes (histamine secretion from basophils, enzyme secretion from PMNs, and proliferation of lymphocytes) was markedly dependent on the solvent (DMSO versus ethanol versus aqueous buffer) used for its initial sonication. While 0.1 μg/ml of DMSO- and ethanol-solubilized A23187 induced maximal histamine release from basophils and histaminase release from PMNs, concentrations of aqueous buffer-sonicated ionophore of ≥ 1 μg/ml were required for an equivalent response. Ionophore sonicated in organic solvents caused a maximum release of 40% of PMN ß-glucuronidase, at an optimal concentration tenfold higher than that required for maximal histamine release; ionophore sonicated in aqueous buffers, even at high concentrations, effected a release of less than 5% of cellular ß-glucuronidase. A23187 also induced lymphocyte proliferation over a narrow concentration range; 0.05 μg/ml of DMSO-sonicated ionophore induced optimal proliferation and concentrations ≥0.2 μg/ml were toxic. Twofold higher concentrations of ethanol-sonicated ionophore and fourfold higher concentrations of aqueous-sonicated ionophore were necessary for maximal proliferation, and the magnitude of the maximal response with aqueous-sonicated A23187 was only one-half that of DMSO-solubilized agent. Ionophore-induced release of histamine from basophils and enzymes from PMNs was not cytotoxic, since ionophore induced neither LDH nor histamine release from heat-treated (47°C) cells. These results explain several previous, discortant reports on the presence or absence of an effect of A23187 on cellular secretory events, on differing dose-response relationships, and on cytotoxic versus noncytotoxic mechanisms of action. © 1979.