During recent years several examples have been reported of neurons in which a neuropeptide coexists with a 'traditional' neurotransmitter of lower molecular weight, and evidence has been obtained that nerve stimulation may cause co-secretion of both (see Lundberg & Hokfelt 1983). In the postganglionic sympathetic nerves of rat vas deferens, the 36 amino acid peptide, neuropeptide Y (NPY, Tatemoto 1982) co-exists with noradrenaline (NA). Exogenous NPY has been reported to depress the twitch phase of the contractile response of rat vas deferens evoked by single shock electrical field stimulation, but not the contraction evoked by exogenous NA (Allen et al. 1982; Lundberg et al. 1982). This finding suggests that liberated endogenous NPY may interact with NA prejunctionally, by depressing the secretion of NA. In the present work we have examined this hypothesis more directly, by studying the effect of this peptide both on the secretion of 'H-NA and on the contraction evoked by electrical nerve stimulation, in rat isolated vas deferens.Briefly (for details concerning the experimental methods see Alberts et al. 19811, male Sprague Dawley rats were stunned and bled to death, and the vasa deferentia dissected out and preincubated at 37°C for 30 min with 2 pM 'H-NA (New England Nuclear Co.), in Tyrode's solution of the following composition (mM): NaCl 136.9, KCI 2.7, CaClz 1.8, MgCIz 0.5, NaHCO, 11.9, NaHzPOs 0.4, glucose 5.6, ascorbate 0.114. The preparation was then washed, mounted in a perspex chamber and perifused at 1 ml/min with Tyrode's solution. Desipramine (0.6 pM) and normetanephrine (10 pM) were added to block reuptake of liberated NA, and atropine (2.6 pM) to block possible interaction with cholinergic functions. The effluent was divided into 4 ml fractions and used for analysis of 'H-NA secretion. The nerves were excited by field stimulation with trains of 300 shocks at 1 Hz, via platinum ring electrodes at the top and bottom of the preparation, using a Grass S44 stimulator (90 V, 0.3 msec). The rise in longitudinal tension (resting tension adjusted to 10 mN) was recorded isometrically, using a force displacement transducer and amplifier (Hottinger Baldwin Messtechnik GmbH, Q 11/5 and KWS 3072, respectively) and an Omniscribe recorder (Houston Instrument). After addition of 2.5 ml Instagel (Packard Instruments) the ' H activity in 1 ml aliquots of the effluents and of extracts of the tissue, at the end of the experiment, was counted in a Packard liquid scintillation spectrometer. In order to separate 'H-NA from metabo-Fig. 1. Effect of NPY on the secretion of tracer NA evoked by electrical field stimulation (90 V, 0.3 msec) with trains of 300 shocks at 1 Hz. Open bars show fractional stimulus-evoked rise in 'H, hatched bars fractional rise in 'H-NA. Mean values, and range from two parallel experiments. NPY (0.2 pM) was present I5 min before and during the second stimulation period; after this NPYfree medium was admitted. Stimulation periods 3 and 4 started at 20 and 52 min, respectively, after discontinuing ...
