1. Changes in cytosolic free calcium concentration ([Ca2+]i) in response to cholinergic and adrenergic agents alone and in combination were investigated using fura-2 fluorescence imaging in intact non-pigmented epithelial cells of rabbit ciliary body.2. Resting ('baseline') [Ca2+]i was 147 + 6 nm (mean + S.E.M.). Acetylcholine (ACh, 10/uM) Ciliary body epithelium is considered responsible for the secretion of aqueous humour in the eye, but the regulatory mechanisms of aqueous humour formation are not yet fully understood (Brubaker, 1991). Though there is no evidence for direct neural innervation of ciliary body epithelial cells, both sympathetic and parasympathetic nerves have been observed within the ciliary processes in the vicinity of the epithelial cells (Stone, Kuwayama & Laties, 1987). Furthermore, agents synthesized in the eye and circulating hormones such as adrenaline may reach these cells by diffusion (Elayan, Kennedy & Ziegler, 1990).Since the ciliary body epithelium appears not to receive direct synaptic input, and since there is such a multitude of receptors present on these cells (see Wax, 1992), it seemed to us possible that the epithelial cells may be regulated by the combined effect of multiple receptor activation, as has been suggested for platelet aggregation (Ruffolo, Nichols, Stadel & Hieble, 1993). In this report, we show such an effect for combined application of muscarinic and adrenergic agonists. Whereas ACh and adrenaline applied by themselves each produce small increases in [Ca2+]i, simultaneous application produces an over 7-fold increase, in part as a result of Ca2+ influx across the plasma membrane. This influx appears to occur through a La3+-sensitive entry pathway.
METHODS Tissue isolationIntact ciliary body epithelial processes were isolated from pigmented rabbits by the following procedure. Rabbits weighing 2-3 kg were killed with a lethal dose of sodium pentobarbitone (200 mg). The eyes were then rapidly enucleated, collected and rinsed in Hepes-buffered Ringer solution (for formulation, see below). The anterior segments were isolated, pinned (cornea down) in a dissecting dish filled with Ringer solution, and the lens and lens capsule carefully removed. Single processes were sectioned from the ciliary body by cutting along the base of the process from the iridial margin to pars plana. Individual processes were laid on their sides in Ringer solution in 35 mm Petri dishes that had been modified by cementing a glass coverslip over a 13 mm hole drilled into the bottom of the dish. The processes were barely covered and held down with a 2-3 mm square piece of glass coverslip, to improve mechanical stability.A plexiglass insert was placed in the chamber to reduce the chamber volume. The process was continuously superfused 215 MS 3083, pp. 215-221
