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ALTERATIONS OF “SLEEPING TIME” IN THE RAT INDUCED BY DRUGS WHICH MODULATE CENTRAL MONOAMINERGIC SYSTEMS
British Journal of Anaesthesia 1990; 64: 594-600
ALTERATIONS OF "SLEEPING TIME" IN THE RAT INDUCED BY DRUGS WHICH MODULATE CENTRAL MONOAMINERGIC SYSTEMS
for the LC system was proposed: the modulation of action of barbiturate-like drugs. Subsequent The effects of adrenoceptor agonists and antago- investigations [15] showed that i.p. injection of nists have been determined on "sleeping time " some adrenoceptor agonists and antagonists given in the rat—that is, with the animal immobile and before thiopentone could produce significant adopting a sleeping posture. Alterations in their changes in the duration of the resultant anaesgross behaviour patterns were assessed also. The thesia. It was suggested that these drugs might specific CL2-adrenoceptor agonists (yohimbine, influence the overall activity of the LC systems WY 26393, RX 781094 and RS 21361) de- which, in turn, could alter the coerulear moducreased sleeping time, as did the fi-adrenoceptor lation of cortical arousal, wakefulness or the agonist c/enbuterol. The specific ^-adreno- processing of sensory information and thus affect ceptor agonist clonidine gave a large increase in the duration of the anaesthetic effect. sleeping time at doses in excess of 25 ng kg-''. However, behavioural studies in other laboraThe same effect was seen with the ^-antagonist tories have shown wide ranging psychotropic propranolol and the specific fi2-antagonist ICI effects induced by adrenoceptor agonists and 118551. antagonists in man and animals. For example, drugs which caused a prolongation of thiopentone anaesthesia (clonidine and propranolol) have been KEY WORDS reported previously to possess sedative [16] and Brain: central monoamines. Sleep. tranquillizing actions [17], respectively. These effects would imply a general depressant action on It is widely accepted that the majority of central the central nervous system. Generally, if two noradrenergic (NA) neurones originate in the sedatives are administered concurrently, a simple locus coeruleus (LC) [1]. From this small pontine additive or potentiating effect of one upon the nucleus the dorsal noradrenergic bundle (DNB) other would be observed. Conversely, a central ascends to innervate the thalamus, hypothalamus, nervous stimulant would be expected to antagothe basal telencephalon and the entire neocortex nize the depressant action of an anaesthetic [18]. [2-6]. With its extensive distribution, it is not It is thus possible that drug-induced alterations of surprising to find that the LC is implicated in the duration of action of anaesthetic agents might neuronal modulation over a large part of the have been caused solely by non-specific drugbrain. It appears that the LC may play a role in drug interactions per se and not by any modulatory paradoxical sleep, attentional processes, modu- action of a noradrenergic system implicated in the lation of electrophysiological responses of cerebral action of the anaesthetic. Consequently, expericortical neurones, the regulation of autonomic ments have been performed to assess the action of output and the mechanisms underlying vigilance and behavioural arousal [7-13]. Angel and Mason [14] showed that, in the rat, A. ANGEL, B.SC., PH.D. ; A. B. A. MAJEED*, B.SC., PH.D. ; Departof Biomedical Science, The University, Sheffield destruction of the DNB with the selective neuro- ment S10 2TN. Accepted for Publication: December 14, 1989. toxin 6-hydroxydopamine potentiates barbiturate *Present address: Department of Physiology, School of anaesthesia. From this observation, another role Pharmacy, Universiti sains Malaysia, Pilau Penang, Malaya. SUMMARY
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A. ANGEL AND A. B. A. MAJEED
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SLEEP AND ADRENERGIC RECEPTORS
Determination of sleeping time
Sleeping time
The animals were placed singly in a rat cage suspended upon a movement transducer [21]. Briefly, this consisted of a length of silicon rubber tubing filled with mercury and connected as one arm of a Wheatstone bridge, the output of which was amplified, full-wave rectified and integrated over 1-s periods. The integrated signal was displayed on a pen recorder. After a 30-min period of acclimatization the animals were treated with either a drug (made up in normal saline) at concentrations to keep the volume of injectate to 2 ml kg"1, or saline alone. The total amount of "sleeping time", denned as the total amount of time during which the activity from the transducer did not exceed baseline, during the period 20-80 min after injection of drug was then determined. The baseline activity for the animal was represented by the level of activity recorded during the pre-injection period when the animal was immobile and had adopted a sleeping posture. All experiments were carried out at the same time of day for each animal in a quiet room. Each animal was investigated as its own control and for drug treatments. The animals were housed under normal conditions of 12-h light-dark cycle and the experiments were performed between 10:00 and 16:00—that is, during the normal sleeping period. Mean value of sleeping time from control and treated animals were compared for statistical difference using Student's two-tailed t test.
The results for all the drugs tested are summarized in table I. Saline controls. In the 1-h assessment period the animals were quiescent for 29.4 (SEM l)min. The variation in total sleeping time for the 10 animals tested was from 24 to 35 min.
a-Adrenoceptor drugs. Three of the four a^adrenoceptor antagonists produced a dose-dependent decrease in sleeping time with a potency order of: yohimbine > WY 26392 > RS 21361. For example, at a dose of 1 mg kg"1, yohimbine almost halved sleeping time (15.6 (1.1) min; P < 0.001) compared with a 30% reduction with WY 26392 (21.4 (0.5) min; P<0.01), whereas RS 21361 (29.6 (1.9) min) was ineffective. Of particular interest was RX 781094, which showed a biphasic dose-response relationship. At low doses (0.01 mg kg"1) it caused a slight, but statistically significant increase in sleeping time (38.2 (2.2) min; P<0.01), whereas at greater doses (:> 0.1 mg kg"1) sleeping time was decreased. This can possibly be attributed to a dual action on a-adrenoceptors, acting as an agonist at low doses and an antagonist at high doses [24]. The a,-adrenoceptor agonist clonidine also showed a biphasic dose-response curve. At a dose of 0.01 mg kg"1 it produced a small but statistically significant (21.4 (1.9) min; P < 0.01) decrease in sleeping time, whereas with doses > 0.1 mg kg"1, statistically significant increases in Drugs sleeping time were observed. The dose for agonist 1 The following drugs were used in this study: to antagonist transition was about 0.025 mg kg" clonidine hydrochloride and clenbuterol (Boeh- in the present series of experiments. The sleepringer & Ingelheim); propranolol, yohimbine HC1 promoting effect of clonidine developed extremely and pyrogallol (Sigma); 2[2-(l,4-benzo- rapidly. Values of sleeping time for clonidine and diaxonyl)]-2-imidazoline HC1 (RX 781094, saline during the first 20 min after injection are
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drugs which modulate the effectiveness of the Reckitt & Colman); 2(l-ethyl-2-imidazolyl central noradrenergic pathways to see if they had methyl)-1,4-benzodiaxan (RS 21361, Syntex); Nany effect upon natural sleep in the unanaesthe- [2p",l lbot)-1,3,4,6,7,1 lb-hexahydro-2H-benzotized rat. Brief reports of this work have appeared (a)-quinolizin-2-yl]-N-methylpropane sulphonamide HC1 (WY 26392, Wyeth); erythro-DLelsewhere [19, 20]. l-(7-methylindan-4-yloxy)-3-isopropylaminobutan-2-ol (ICI 118551); chlordiazepoxide (Librium, Roche) and amphetamine. ICI 118551 MATERIALS AND METHODS was heated gently until it dissolved; all other Male albino rats (Sheffield strain) in the weight drugs were dissolved in saline at 37 °C. range 200-300 g were housed in groups of three and allowed free access to food and water except for the short period of testing. RESULTS
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TABLE I. Effects of adrenoceptor agonists-antagonists, pyrogallol, amphetamine and saline on sleeping time in rats. Values are mean (SEM) and were evaluated for significance of difference vs saline controls using an unpaired two-tailed Student's t test: *P<0.05; **P<0.01; ***P < 0.001. Values in [brackets] showed a significant increase in sleeping time. n = 6 in all cases except for saline (n = 10). ns = Not significant. COMT-I = catechol-o-methyl transferase inhibitor. (For drug doses see references cited)
Drug
Action
Dose (mg kg"1)
0,-Agonist
0.010 0.025 0.125 0.25
RX 781094 [36]
a,-Agonist a,-Antagonist
0.01
0.5 0.1 1.0
10.0 Yohimbine [15]
0,-Antagonist
WY 26392 [36]
o^-Antagonist
RS 21361 [36]
a,-Antagonist
0.1 0.5 1.0 0.2 0.5 1.0 2.0 1.0 2.0
10.0 20.0 Clenbuterol [32]
(5-Agonist
2.0
20.0 Propranolol [32]
f$- Antagonist
ICI 118551 [32]
p,-Antagonist
Pyrogallol [22] Librium [23] Amphetamine [23] Saline
COMT-I Anxiolytic Stimulant Control
shown in table II. At all doses tested, clonidine was found to produce a statistically significant decrease in activity during this time period. /?- Adrenoceptor drugs. The P-adrenoceptor agonist clenbuterol produced a significant decrease in sleeping time at a dose of 20 mg kg"1 (18.5 (3.1) min; P < 0.01). In contrast, both propranolol (a P-adrenoceptor antagonist) and ICI 118551 (a selective P,-adrenoceptor antagonist) caused a marked increase in sleeping time at the same dose (35.9 (1.4) and 37.3 (2.0) min,
1.0 2.0
10.0 20.0 10.0 20.0 30.0 125.0 20.0 2.0
21.4(1.9) ** 30.6 (5.3) ns [41.5(2.6)]*** [45.8(1.6)]*** [47.7 (2.2)]*** [38.2 (2.2)]** 24.7(1.3) * 21.4(2.1) ** 19.0 (0.9) *** 20.0(1.5) *** 18.9(1.8) *** 15.6(1.2) *** 33.4 (1.7) ns 24.8(1.3) * 21.4(0.5) ** 20.9(1.7) ** 29.6(1.9) ns 28.8 (1.9) ns 23.5 (3.3) ns 13.0 (2.4) *** 24.4 (3.7) ns 18.5(3.1) ** 26.4 (2.2) ns 29.3 (1.3) ns 32.4 (3.0) ns [35.9(1.4)]** 28.2 2.4 ns [37.3 (2.0)]** [42.8 (2.9)]*** 34.1 (2.0) ns [43.0 (2.7)]*** 0
29.4 1.0
respectively). As was seen with clonidine, the sleep-promoting effect of these two drugs was apparent also in the 20-min period immediately after administration. Paradoxically, during this period, a low dose of propranolol was found to cause a small but statistically significant decrease in sleeping time (table I). Anxiolytic agent. Chlordiazepoxide 20 mg kg"1 produced a significant increase in sleeping time (43 (2.7) min)—an effect which also showed a rapid development (table II).
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Clonidine [15]
Sleeping time (min)
SLEEP AND ADRENERGIC RECEPTORS
597
TABLE II. Total sleeping time during the first 20 min immediately after the injection. Significance compared with saline controls: * P < 0 . 0 5 ; **P<0.01; * * * P < 0.001. Values in [brackets] show a decrease in sleeping time
Drug
Action a,-Agonist
Propranolol
p-Antagonist
ICI 118551
P,-Antagonist
Librium Saline
Anxiolytic Control
Sleeping tune (min)
0.010 0.025 0.125 0.25 0.5 1.0 2.0 10.0 20.0 10.0 20.0 30.0 20.0
4.8 (0.8) * 5.6(1.4)* 6.2 (0.9) *** 7.6(1.2) *** 8.5(1.4) *** [1.1(0.4)]** 4.5 (1.3) ns 7.0 (1.7) ns 10.0(1.4) ** 4.8 (1.7) ns 4.5 (0.9) ns 7.2(1.5) *** 9.4(1.1) *** 2.9 (0.3)
COMT inhibitor. The catechol-o-methyl transCatecholamine and catecholaminergic neurones ferase inhibitor, pyrogallol [25], gave only a slight have been implicated in the mechanism of action increase in sleeping time which was not stat- of anaesthetic agents. Muller and Frouts [28] istically significant (table I). reported that adrenergic blocking drugs caused a prolongation of hexobarbitone sleeping time in Psychostimulant drug. None of the animals mice. Such action was attributed to both a drugtreated with amphetamine 2 mg kg"1 showed any induced inhibition of liver microsomal enzymes signs of sleep during the entire period of ob- and decrease in body temperature. On the other hand, Miller, Way and Eger [29], suggested that servation. the anaesthetic requirement for volatile anaesthetics (the minimal alveolar concentration, DISCUSSION MAC) might be related to the NA content of the In the present series of experiments, we have brain. Their hypothesis was based on the findings attempted to use the same variable as that in the that patients receiving drugs which effectively previously reported experiments on potentiation reduced brain NA (guanethidine or methyldopa) of barbiturate anaesthesia, that is, the duration of required lesser concentrations of halothane than time during which the total locomotor activity of normal patients. Similar observations were made the animal did not exceed the level of a pre- by Johnston, Way and Miller [30], who showed determined baseline (see below). The descriptive that acute treatment with D-amphetamine resulted term "sleeping time" was adopted rather than in an increase in halothane MAC in animals. "time of zero locomotor activity", "immobility Conversely, chronic treatment with drugs which time", "period of inactivity " etc., for a variety of deplete brain catecholamines caused a decrease in reasons. The baseline was taken as that at which halothane MAC. Later Roizen and colleagues [31] the animal was completely immobile and assumed showed that halothane and cyclopropane could a sleeping posture. None of the drugs used alter NA concentrations in discrete brain nuclei produced motor freezing (no locomotor activity such as the LC and nucleus accumbens. without the adoption of a sleeping posture). In More recently, Mason and Angel [15,32] addition, it has been shown that clonidine pro- demonstrated that the duration of barbiturate duces changes in EEG pattern which resemble anaesthesia was dependent upon the overall those seen in sleep in the rat [26] and clinically it activity of the central NA system. Drugs which produces prolonged sleep in man [27]. reduced the activity of the system, for example a2-
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Clonidine
Dose (mg kg"1)
598
demonstrated a strong inhibitory action of clonidine on discharge of central NA neurones [37-39]. However, propranolol has been shown to be without action on the firing rate of LC cells [40] even at very high i.v. doses. Thus it is possible that drug-induced alterations of sleeping time may not be dependent upon the availability of NA at the LC neuronal terminations per se. In the present studies pyrogallol, a COMT inhibitor, which would tend to increase the accumulation of NA in the vicinity of the postsynaptic adrenoceptors, failed to cause a shortening of sleeping time. This chemical did, however, produce a small increase in sleeping time at a dose of 125 mg kg"1. At this dose, in the chick, it produces complete somnolence [Angel and Dewhurst, unpublished observations]. There have been some contradictory suggestions on the mechanism of the central action of propranolol. Mason and Angel [32] proposed that its P-blocking action might be responsible for potentiation of thiopentone anaesthesia in the rat. Murman, Almirante and Saccani-Guelfi [41] and Hermansen [42] suggested that the prolongation of hexobarbitone action in mice could be caused by a pure depressant action of propranolol on the CNS. Similarly, the tranquillizing [17] and anticonvulsant [41] effects of propranolol have been attributed to an intrinsic CNS depressant action [43]. There have been reports also of the sleepinducing effect of propranolol in mice [44] and rats [45]. Many, but not all, of the pharmacological effects of P-blockers may be attributed to their Padrenoceptor antagonist activity per se. They do, however, possess other properties, such as acting as local anaesthetics or having intrinsic sympathomimetic activity. There have been suggestions that aberrant activity of drugs may be related to their chemical structure. Lesvkovsky and Tardos [43] proposed that the CNS-depressant action of propranolol might be a result of the presence of a methyl group, and a similar explanation has been essayed for the naphthyl group of pronethalol [41]. In the present study both propranolol and ICI 118551 (which has an indalyl group) induced an increase in sleeping time. The latter and another P-blocker, pindalol, have been shown to potentiate the effect of thiopentone in the rat [32] and pindalol has been shown to increase the effectiveness of chloral hydrate in mice [44]. From these observations it is interesting to note
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agonists and P-antagonists, potentiated thiopentone sleeping time, whilst drugs which enhance LC-NA activity, for example, a2-antagonists and P-agonists, gave a decrease in the effectiveness of thiopentone. However, not all anaesthetic agents have their activity modulated by interference with the central NA system. Adrenergic drugs were shown to have no effect on ketamine, urethane or Althesin (alphadolone/alphaxalone) anaesthesia [15,32]. In the present series of experiments it has been found that drugs which shortened thiopentone sleeping time could induce "stimulant" effects in unanaesthetized rats. Assessment of behavioural signs such as awareness, consciousness, spontaneous activity, stereotyped movements and motor co-ordination generally showed an increase. The degree of CNS excitation obtained was, however, not as great as that produced by the more conventional CNS stimulants. For example, the increased motor activity seen after yohimbine was intermittent compared with the continuous activity seen after amphetamine. Nonetheless, by measuring total locomotor activity it has been shown that yohimbine, WY 26392 and RS 21361, all selective a2-adrenoceptor antagonists, caused an increase in central excitation, reflected as a decrease in the total time spent immobile after adopting a sleeping posture. The P-adrenoceptor agonist, clenbuterol, also reduced sleeping time. For this drug, a direct stimulation of the postsynaptic P-adrenoceptors would lead to excitation of central NA neurones. It has been shown that electrical stimulation of the LC leads to the release of NA in the cerebral cortex [33], which could then lead to electrocortical and behavioural arousal [34, 35]. The possible correlation between the activity of LC cells and the duration of sleeping time receives support from the action of RX 781094. At low doses it produced an increase in sleeping time, possibly via a presynaptic a2-agonist action. Conversely, higher doses caused a reduction in sleeping time, presumably by autoreceptor block. Both behavioural studies using the thiopentoneinduced sleeping time model [36] and electrophysiological recordings of rate of discharge of LC cells [24] have shown a similar biphasic response with RX 781094. However, the enhancement of sleeping time produced by propranolol, clonidine and ICI 118551 cannot be attributed solely to modulation of coerulear discharge. Many workers have
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SLEEP AND ADRENERGIC RECEPTORS
ACKNOWLEDGEMENT We thank Reckitt & Colman, Syntex, Wyeth and ICI for the generous gifts of the drugs used in this study.
REFERENCES 1. Dahlstrom A, Fuxe K. Evidence for the existence of monoamine containing neurones in the CNS. I. Demonstration of monoamines in the cell bodies of brain stem neurones. Acta Physiologica Scandinavica 1965; (Suppl. 62) 232: 1-55. 2. Ungerstedt U. Stereotaxic mapping of the monoamine pathways in the rat brain. Acta Physiologica Scandinavica 1971; (Suppl.) 367: 1-19. 3. Lindvall O, Bjorklund A, Nobin A, Stenevi U. The adrenergic innervation of the rat thalamus as revealed by the glyoxylic acid fluorescence method. Journal of Comparative Neurology 1974; 154: 317-348. 4. Pickel VM, Segal M, Bloom FE. A radioautographic study of the efferent pathways of the nucleus locus coeruleus. Journal of Comparative Neurology 1974; 155: 15-^2. 5. Shimuzu N, Ohnishi S, Tohyama M, Maeda T. Demonstration by degeneration silver method of the ascending projection from the locus coeruleus. Experimental Brain Research 1974; 20: 375-384. 6. Jones BE, Moore RY. Ascending projections of the locus coeruleus in the rat. Autoradiographic study. Brain Research 1977; 127: 23-53. 7. Amaral DG, Sinnamon HM. The locus coeruleus: neurobiology of a central noradrenergic nucleus. Progress in Neurobiology 1977; 9: 147-196. 8. McNaughton N, Mason ST. The neurophysiology and the neuropharmacology of the ascending dorsal noradrenergic bundle. Progress in Neurobiology 1980; 14: 157-219. 9. Mason ST. Noradrenaline in the brain: progress in theories of behavioural function. Progress in Neurobiology 1981; 16: 263-303. 10. Robinson TE, Vanderwolf CH, Pappas BA. Are the dorsal noradrenergic bundle projections from the locus coeruleus important for neocortical and hippocampal activation? Brain Research 1977; 138: 75-98. 11. Olpe HR, Glare A, Laszlo J, Schellenberg A. Some electrophysiological and pharmacological properties of the cortical noradrenergic projection of the locus coeruleus in the rat. Brain Research 1980; 186: 9-19. 12. Beiner PB. Clonidine inhibits central noradrenergic neurons in unanaesthetized cats. European Journal of Pharmacology 1985; 115: 249-257. 13. De Sarro GB, Ascioti C, Froio F, Libri V, Nistico G. Evidence that locus coeruleus is the site where clonidine and drugs acting at otl- and a,-adrenoceptors affect sleep and arousal mechanisms. British Journal of Pharmacology 1987; 90: 675-685. 14. Angel A, Mason ST. 6-Hydroxydopamine-induced depletion of noradrenaline potentiates barbiturate anaesthesia. Journal of Physiology (London) 1982; 324: 75P. 15. Mason ST, Angel A. Anaesthesia: the role of adrenergic mechanisms. European Journal of Pharmacology 1983; 91: 29-39. 16. Delbarre B, Schmitt H. Sedative effects of a-sympathomimetic drugs and their antagonism by adrenergic and cholinergic blocking drugs. European Journal of Pharmacology 1971; 13: 356-363. 17. Bainbridge JG, Greenwood D T . Tranquilizing effects of propranolol demonstrated in rats. Neuropharmacology 1971; 10: 453-458. 18. Bloom FE. Neurohumoral transmission and the CNS. In: Goodman LS, Gilman A, eds. The Pharmacological Basis
Downloaded from http://bja.oxfordjournals.org/ at The University of British Colombia Library on July 9, 2015
that P-blockers with a double ring structure on the aromatic moiety of the molecule produce a sedative or depressant action, whereas compounds with a phenyl group such as nifenalol and dichloroisoproterenol cause central excitation. Similarly sotalol, dichloroisoproterenol and Ko 1336 shortened, whereas practolol did not alter, chloral hydrate sleeping time [44]. The significance of structure—activity relationships of a2-adrenoceptor antagonists has been demonstrated [46]. Thus the possibility of a similar structure-dependent action of P-adrenoceptor antagonists cannot be ruled out. The sedative action of clonidine has been attributed to its activation of presynaptic a2adrenoceptors on LC cells causing a decrease in the activity of this ascending NA pathway projecting diffusely to subcortical and cortical areas. However, such a simplistic mechanism of action can, at best, provide only a partial explanation for its wide-ranging central effects. In the present study its action resembled that of an anaesthetic rather than a sleep-inducing agent. Electrophysiological studies [47] have shown that clonidine in high dose (^ 100 (ig kg"1) potentiates the effect of urethane and has an action identical to that of several general anaesthetic agents as measured by electrocortical activity, cerebral evoked responses and its ability to suppress thalamic and cortical, but not cuneate, cellular responsiveness to electrical stimulation of the periphery. The same authors reported a reverse action of clonidine at small doses. Such a biphasic dose-dependent action was seen also in the present study (table I). In support of this suggestion for a separate, non-adrenergic, mechanism of action of clonidine-induced CNS depression, Nassif and colleagues [48] have shown that a neurochemical lesion of the LC system does not suppress its sedative action. Moreover, yohimbine, a specific a2-adrenoceptor antagonist, has no effect on spontaneous electrocortical activity, cerebral evoked responses or cellular responses to peripheral stimulation at cuneate, thalamic or cortical sites [49]. Thus not all of the central actions of clonidine can be ascribed to an otj-agonist action. It may in addition exert a mild anaesthetic-like action. The exact site, or sites, of such action should be determined.
599
600
BRITISH JOURNAL OF ANAESTHESIA
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of Therapeutics, 6th Edn. London: Collier-MacMillan, effects of stimulation of the nucleus locus coeruleus in the 1980; 235-257. stumptailed monkey, Macaca arctoides. Brain Research 1976; 116: 502-510. 19. Angel A, Majeed ABA. The effects of some centrally active adrenergic drugs on sleeping time in the rat. Journal 35. Koella WP. The organization and regulation of sleep. A of Physiology {London) 1986; 378: 45P. review of the experimental evidence and a novel integrated model of the organizing and regulating apparatus. Experi20. Angel A, Majeed ABA. Effects of centrally active entia 1984; 40: 309-338. adrenoceptor agonists and antagonists on sleeping time in the rat. In: Proceedings of the First Congress of the Asian 36. Mason ST. Alpha-2 receptor antagonists and thiopentone and Oceanian Physiological Societies, Bangkok, Thailand, anaesthesia in the rat. Journal of Physiology (London) November 26-29, 1986. 1985; 360: 37P. 21. Angel A. Two simple, relatively inexpensive, devices to 37. Svensson TH, Bunney BS, Aghajanian GK. Inhibition of measure the locomotor activity of anaesthetized or unboth noradrenergic and serotonergic neurons in brain by anaesthetized animals. British Journal of Pharmacology •^-agonist clonidine. Brain Research 1975; 92: 291-306. 1970; 39: 243P. 38. Cedarbaum JM, Aghajanian GK. Catecholamine re22. Angel A, Rogers KJ. An analysis of the convulsant activity ceptors on locus coeruleus neurons: Pharmacological of substituted benzenes in the mouse. Toxicology and characteristics. European Journal of Pharmacology 1977; Applied Pharmacology 1972; 21: 214-229. 44: 375-385. 23. Barnes CD, Etherington LG. Drug Dosage in Laboratory 39. Marwaha J, Kehne JH, Comnissaris RL, Lakoski J, Shaw Animals—A Handbook, revised Edn. California: UniW, Davis M. Spinal clonidine inhibits neural firing in versity of California Press, 1973. locus coeruleus. Brain Research 1983; 276: 379-382. 24. Goldstein JM, Knobloch LC, Malick JB. Electro- 40. Dahlof C, Engberg G, Svensson TH. Effects of 0adrenoceptor antagonists on the firing rate of norphysiological demonstration of both a,-agonist and anadrenergic neurones in the locus coeruleus of the rat. tagonist properties of RX781094. European Journal of Naunyn Schmiederbergs Archive of Pharmacologie 1981; Pharmacology 1983; 91: 101-105. 317: 26-30. 25. Ross SB, Haljasma O. Catechol-O-methyl transferase inhibitors: in vivo inhibition in mice. Ada Pharmacologica 41. Murman W, Almirantc L, Saccani-Guelfi M. Central nervous system effects of four P-adrenergic receptor et Toxicologica 1964; 21: 215-225. blocking agents. Journal of Pharmacy and Pharmacology 26. Kleinlogel H, Scholtysik G, Sayers AC. Effects of 1966; 18: 317-318. clonidine and BS100-141 on the EEG sleep pattern in rats. European Journal of Pharmacology 1975; 33: 159-163.42. Hermansen K. Effects of different P-adrenergic receptor blocking agents on hexobarbital induced narcosis in mice. 27. Davies DS, Wing LMH, Reid JL, Neill E, Tippett P, Acta Pharmacologica et Toxicologica 1969; 27: 453-^60. Dollery CI. Pharmacokinetics and concentration-effects of intravenous and oral clonidine. Clinical Pharmacology 43. Leszkovsky G, Tardos L. Some effects of propranolol on the central nervous system. Journal of Pharmacy and and Therapeutics 1977; 21: 593-601. Pharmacology 1965; 17: 518-519. 28. Muller JO, Frouts JR. Prolongation of hcxobarbital sleeping time and inhibition of hepatic drug metabolism by 44. Delbarre B, Schmitt H. A further attempt to characterize sedative receptors activated by clonidine in chickens and adrenergic blocking agents in mice. Biochemical Pharmice. European Journal of Pharmacology 1973; 22: macology 1965; 14: 305-311. 355-359. 29. Miller RD, Way WL, Eger El. The effects of otmethyldopa, reserpine, guanethidine and iproniazid on 45. Torbati D. Effect of propranolol on cortical electrical activity in conscious and anaesthetized rats. Neurominimum alveolar anesthetic requirement (MAC). Anespharmacology 1986; 25: 1251. thesiology 1968; 29: 1153-1158. 30. Johnston RR, Way WL, Miller RD. Alteration of 46. Pettibone DJ, Pfleuger AB, Totaro JA. Comparison of the effects of recently developed ot,-adrenergic antagonists anesthetic requirement by amphetamine. Aneslhesiology with yohimbine and rauwolscine on monoamine systems 1972; 36: 357-363. in rat brain. Biochemical Pharmacology 1985; 34: 109331. Roizen MF, Kopin IJ, Thoa NB, Zivin J, Muth EA, 1097. Jacoboitz D. The effect of two anaesthetic agents on norepinephrine and dopamine in discrete brain nuclei, 47. Angel A, Goldman P, Halsey MJ, Majeed ABA, Kendig J. A possible anaesthetic action of clonidine. Journal of fibre tracts and terminal regions of the rat. Brain Research Physiology {London) 1986; 378: 10P. 1976; 110: 515-522. 32. Mason ST, Angel A. Brain noradrenaline and anaesthesia: 48. Nassif S, Kempf E, Cardo B, Velley L. Neurochemical lesion of the locus coeruleus of the rat does not suppress Further characterization of the beta receptor. Neurothe sedative effect of clonidine. European Journal of pharmacology 1983; 22: 1065-1069. Pharmacology 1983; 91: 69-76. 33. Tanaka C, Inagaki C, Fujiwara H. Labelled noradrenaline release from rat cerebral cortex following electrical 49. Angel A, Majeed ABA. An electrophysiological study on the central action of yohimbine in the rat. Journal of stimulation of locus coeruleus. Brain Research 1976; 106: 384-389. Physiology {London) 1987; 392: 58P. 34. Redmond DE, Huang YH, Snyder DR. Behavioural
ALTERATIONS OF "SLEEPING TIME" IN THE RAT INDUCED BY DRUGS WHICH MODULATE CENTRAL MONOAMINERGIC SYSTEMS
for the LC system was proposed: the modulation of action of barbiturate-like drugs. Subsequent The effects of adrenoceptor agonists and antago- investigations [15] showed that i.p. injection of nists have been determined on "sleeping time " some adrenoceptor agonists and antagonists given in the rat—that is, with the animal immobile and before thiopentone could produce significant adopting a sleeping posture. Alterations in their changes in the duration of the resultant anaesgross behaviour patterns were assessed also. The thesia. It was suggested that these drugs might specific CL2-adrenoceptor agonists (yohimbine, influence the overall activity of the LC systems WY 26393, RX 781094 and RS 21361) de- which, in turn, could alter the coerulear moducreased sleeping time, as did the fi-adrenoceptor lation of cortical arousal, wakefulness or the agonist c/enbuterol. The specific ^-adreno- processing of sensory information and thus affect ceptor agonist clonidine gave a large increase in the duration of the anaesthetic effect. sleeping time at doses in excess of 25 ng kg-''. However, behavioural studies in other laboraThe same effect was seen with the ^-antagonist tories have shown wide ranging psychotropic propranolol and the specific fi2-antagonist ICI effects induced by adrenoceptor agonists and 118551. antagonists in man and animals. For example, drugs which caused a prolongation of thiopentone anaesthesia (clonidine and propranolol) have been KEY WORDS reported previously to possess sedative [16] and Brain: central monoamines. Sleep. tranquillizing actions [17], respectively. These effects would imply a general depressant action on It is widely accepted that the majority of central the central nervous system. Generally, if two noradrenergic (NA) neurones originate in the sedatives are administered concurrently, a simple locus coeruleus (LC) [1]. From this small pontine additive or potentiating effect of one upon the nucleus the dorsal noradrenergic bundle (DNB) other would be observed. Conversely, a central ascends to innervate the thalamus, hypothalamus, nervous stimulant would be expected to antagothe basal telencephalon and the entire neocortex nize the depressant action of an anaesthetic [18]. [2-6]. With its extensive distribution, it is not It is thus possible that drug-induced alterations of surprising to find that the LC is implicated in the duration of action of anaesthetic agents might neuronal modulation over a large part of the have been caused solely by non-specific drugbrain. It appears that the LC may play a role in drug interactions per se and not by any modulatory paradoxical sleep, attentional processes, modu- action of a noradrenergic system implicated in the lation of electrophysiological responses of cerebral action of the anaesthetic. Consequently, expericortical neurones, the regulation of autonomic ments have been performed to assess the action of output and the mechanisms underlying vigilance and behavioural arousal [7-13]. Angel and Mason [14] showed that, in the rat, A. ANGEL, B.SC., PH.D. ; A. B. A. MAJEED*, B.SC., PH.D. ; Departof Biomedical Science, The University, Sheffield destruction of the DNB with the selective neuro- ment S10 2TN. Accepted for Publication: December 14, 1989. toxin 6-hydroxydopamine potentiates barbiturate *Present address: Department of Physiology, School of anaesthesia. From this observation, another role Pharmacy, Universiti sains Malaysia, Pilau Penang, Malaya. SUMMARY
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A. ANGEL AND A. B. A. MAJEED
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SLEEP AND ADRENERGIC RECEPTORS
Determination of sleeping time
Sleeping time
The animals were placed singly in a rat cage suspended upon a movement transducer [21]. Briefly, this consisted of a length of silicon rubber tubing filled with mercury and connected as one arm of a Wheatstone bridge, the output of which was amplified, full-wave rectified and integrated over 1-s periods. The integrated signal was displayed on a pen recorder. After a 30-min period of acclimatization the animals were treated with either a drug (made up in normal saline) at concentrations to keep the volume of injectate to 2 ml kg"1, or saline alone. The total amount of "sleeping time", denned as the total amount of time during which the activity from the transducer did not exceed baseline, during the period 20-80 min after injection of drug was then determined. The baseline activity for the animal was represented by the level of activity recorded during the pre-injection period when the animal was immobile and had adopted a sleeping posture. All experiments were carried out at the same time of day for each animal in a quiet room. Each animal was investigated as its own control and for drug treatments. The animals were housed under normal conditions of 12-h light-dark cycle and the experiments were performed between 10:00 and 16:00—that is, during the normal sleeping period. Mean value of sleeping time from control and treated animals were compared for statistical difference using Student's two-tailed t test.
The results for all the drugs tested are summarized in table I. Saline controls. In the 1-h assessment period the animals were quiescent for 29.4 (SEM l)min. The variation in total sleeping time for the 10 animals tested was from 24 to 35 min.
a-Adrenoceptor drugs. Three of the four a^adrenoceptor antagonists produced a dose-dependent decrease in sleeping time with a potency order of: yohimbine > WY 26392 > RS 21361. For example, at a dose of 1 mg kg"1, yohimbine almost halved sleeping time (15.6 (1.1) min; P < 0.001) compared with a 30% reduction with WY 26392 (21.4 (0.5) min; P<0.01), whereas RS 21361 (29.6 (1.9) min) was ineffective. Of particular interest was RX 781094, which showed a biphasic dose-response relationship. At low doses (0.01 mg kg"1) it caused a slight, but statistically significant increase in sleeping time (38.2 (2.2) min; P<0.01), whereas at greater doses (:> 0.1 mg kg"1) sleeping time was decreased. This can possibly be attributed to a dual action on a-adrenoceptors, acting as an agonist at low doses and an antagonist at high doses [24]. The a,-adrenoceptor agonist clonidine also showed a biphasic dose-response curve. At a dose of 0.01 mg kg"1 it produced a small but statistically significant (21.4 (1.9) min; P < 0.01) decrease in sleeping time, whereas with doses > 0.1 mg kg"1, statistically significant increases in Drugs sleeping time were observed. The dose for agonist 1 The following drugs were used in this study: to antagonist transition was about 0.025 mg kg" clonidine hydrochloride and clenbuterol (Boeh- in the present series of experiments. The sleepringer & Ingelheim); propranolol, yohimbine HC1 promoting effect of clonidine developed extremely and pyrogallol (Sigma); 2[2-(l,4-benzo- rapidly. Values of sleeping time for clonidine and diaxonyl)]-2-imidazoline HC1 (RX 781094, saline during the first 20 min after injection are
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drugs which modulate the effectiveness of the Reckitt & Colman); 2(l-ethyl-2-imidazolyl central noradrenergic pathways to see if they had methyl)-1,4-benzodiaxan (RS 21361, Syntex); Nany effect upon natural sleep in the unanaesthe- [2p",l lbot)-1,3,4,6,7,1 lb-hexahydro-2H-benzotized rat. Brief reports of this work have appeared (a)-quinolizin-2-yl]-N-methylpropane sulphonamide HC1 (WY 26392, Wyeth); erythro-DLelsewhere [19, 20]. l-(7-methylindan-4-yloxy)-3-isopropylaminobutan-2-ol (ICI 118551); chlordiazepoxide (Librium, Roche) and amphetamine. ICI 118551 MATERIALS AND METHODS was heated gently until it dissolved; all other Male albino rats (Sheffield strain) in the weight drugs were dissolved in saline at 37 °C. range 200-300 g were housed in groups of three and allowed free access to food and water except for the short period of testing. RESULTS
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TABLE I. Effects of adrenoceptor agonists-antagonists, pyrogallol, amphetamine and saline on sleeping time in rats. Values are mean (SEM) and were evaluated for significance of difference vs saline controls using an unpaired two-tailed Student's t test: *P<0.05; **P<0.01; ***P < 0.001. Values in [brackets] showed a significant increase in sleeping time. n = 6 in all cases except for saline (n = 10). ns = Not significant. COMT-I = catechol-o-methyl transferase inhibitor. (For drug doses see references cited)
Drug
Action
Dose (mg kg"1)
0,-Agonist
0.010 0.025 0.125 0.25
RX 781094 [36]
a,-Agonist a,-Antagonist
0.01
0.5 0.1 1.0
10.0 Yohimbine [15]
0,-Antagonist
WY 26392 [36]
o^-Antagonist
RS 21361 [36]
a,-Antagonist
0.1 0.5 1.0 0.2 0.5 1.0 2.0 1.0 2.0
10.0 20.0 Clenbuterol [32]
(5-Agonist
2.0
20.0 Propranolol [32]
f$- Antagonist
ICI 118551 [32]
p,-Antagonist
Pyrogallol [22] Librium [23] Amphetamine [23] Saline
COMT-I Anxiolytic Stimulant Control
shown in table II. At all doses tested, clonidine was found to produce a statistically significant decrease in activity during this time period. /?- Adrenoceptor drugs. The P-adrenoceptor agonist clenbuterol produced a significant decrease in sleeping time at a dose of 20 mg kg"1 (18.5 (3.1) min; P < 0.01). In contrast, both propranolol (a P-adrenoceptor antagonist) and ICI 118551 (a selective P,-adrenoceptor antagonist) caused a marked increase in sleeping time at the same dose (35.9 (1.4) and 37.3 (2.0) min,
1.0 2.0
10.0 20.0 10.0 20.0 30.0 125.0 20.0 2.0
21.4(1.9) ** 30.6 (5.3) ns [41.5(2.6)]*** [45.8(1.6)]*** [47.7 (2.2)]*** [38.2 (2.2)]** 24.7(1.3) * 21.4(2.1) ** 19.0 (0.9) *** 20.0(1.5) *** 18.9(1.8) *** 15.6(1.2) *** 33.4 (1.7) ns 24.8(1.3) * 21.4(0.5) ** 20.9(1.7) ** 29.6(1.9) ns 28.8 (1.9) ns 23.5 (3.3) ns 13.0 (2.4) *** 24.4 (3.7) ns 18.5(3.1) ** 26.4 (2.2) ns 29.3 (1.3) ns 32.4 (3.0) ns [35.9(1.4)]** 28.2 2.4 ns [37.3 (2.0)]** [42.8 (2.9)]*** 34.1 (2.0) ns [43.0 (2.7)]*** 0
29.4 1.0
respectively). As was seen with clonidine, the sleep-promoting effect of these two drugs was apparent also in the 20-min period immediately after administration. Paradoxically, during this period, a low dose of propranolol was found to cause a small but statistically significant decrease in sleeping time (table I). Anxiolytic agent. Chlordiazepoxide 20 mg kg"1 produced a significant increase in sleeping time (43 (2.7) min)—an effect which also showed a rapid development (table II).
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Clonidine [15]
Sleeping time (min)
SLEEP AND ADRENERGIC RECEPTORS
597
TABLE II. Total sleeping time during the first 20 min immediately after the injection. Significance compared with saline controls: * P < 0 . 0 5 ; **P<0.01; * * * P < 0.001. Values in [brackets] show a decrease in sleeping time
Drug
Action a,-Agonist
Propranolol
p-Antagonist
ICI 118551
P,-Antagonist
Librium Saline
Anxiolytic Control
Sleeping tune (min)
0.010 0.025 0.125 0.25 0.5 1.0 2.0 10.0 20.0 10.0 20.0 30.0 20.0
4.8 (0.8) * 5.6(1.4)* 6.2 (0.9) *** 7.6(1.2) *** 8.5(1.4) *** [1.1(0.4)]** 4.5 (1.3) ns 7.0 (1.7) ns 10.0(1.4) ** 4.8 (1.7) ns 4.5 (0.9) ns 7.2(1.5) *** 9.4(1.1) *** 2.9 (0.3)
COMT inhibitor. The catechol-o-methyl transCatecholamine and catecholaminergic neurones ferase inhibitor, pyrogallol [25], gave only a slight have been implicated in the mechanism of action increase in sleeping time which was not stat- of anaesthetic agents. Muller and Frouts [28] istically significant (table I). reported that adrenergic blocking drugs caused a prolongation of hexobarbitone sleeping time in Psychostimulant drug. None of the animals mice. Such action was attributed to both a drugtreated with amphetamine 2 mg kg"1 showed any induced inhibition of liver microsomal enzymes signs of sleep during the entire period of ob- and decrease in body temperature. On the other hand, Miller, Way and Eger [29], suggested that servation. the anaesthetic requirement for volatile anaesthetics (the minimal alveolar concentration, DISCUSSION MAC) might be related to the NA content of the In the present series of experiments, we have brain. Their hypothesis was based on the findings attempted to use the same variable as that in the that patients receiving drugs which effectively previously reported experiments on potentiation reduced brain NA (guanethidine or methyldopa) of barbiturate anaesthesia, that is, the duration of required lesser concentrations of halothane than time during which the total locomotor activity of normal patients. Similar observations were made the animal did not exceed the level of a pre- by Johnston, Way and Miller [30], who showed determined baseline (see below). The descriptive that acute treatment with D-amphetamine resulted term "sleeping time" was adopted rather than in an increase in halothane MAC in animals. "time of zero locomotor activity", "immobility Conversely, chronic treatment with drugs which time", "period of inactivity " etc., for a variety of deplete brain catecholamines caused a decrease in reasons. The baseline was taken as that at which halothane MAC. Later Roizen and colleagues [31] the animal was completely immobile and assumed showed that halothane and cyclopropane could a sleeping posture. None of the drugs used alter NA concentrations in discrete brain nuclei produced motor freezing (no locomotor activity such as the LC and nucleus accumbens. without the adoption of a sleeping posture). In More recently, Mason and Angel [15,32] addition, it has been shown that clonidine pro- demonstrated that the duration of barbiturate duces changes in EEG pattern which resemble anaesthesia was dependent upon the overall those seen in sleep in the rat [26] and clinically it activity of the central NA system. Drugs which produces prolonged sleep in man [27]. reduced the activity of the system, for example a2-
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Clonidine
Dose (mg kg"1)
598
demonstrated a strong inhibitory action of clonidine on discharge of central NA neurones [37-39]. However, propranolol has been shown to be without action on the firing rate of LC cells [40] even at very high i.v. doses. Thus it is possible that drug-induced alterations of sleeping time may not be dependent upon the availability of NA at the LC neuronal terminations per se. In the present studies pyrogallol, a COMT inhibitor, which would tend to increase the accumulation of NA in the vicinity of the postsynaptic adrenoceptors, failed to cause a shortening of sleeping time. This chemical did, however, produce a small increase in sleeping time at a dose of 125 mg kg"1. At this dose, in the chick, it produces complete somnolence [Angel and Dewhurst, unpublished observations]. There have been some contradictory suggestions on the mechanism of the central action of propranolol. Mason and Angel [32] proposed that its P-blocking action might be responsible for potentiation of thiopentone anaesthesia in the rat. Murman, Almirante and Saccani-Guelfi [41] and Hermansen [42] suggested that the prolongation of hexobarbitone action in mice could be caused by a pure depressant action of propranolol on the CNS. Similarly, the tranquillizing [17] and anticonvulsant [41] effects of propranolol have been attributed to an intrinsic CNS depressant action [43]. There have been reports also of the sleepinducing effect of propranolol in mice [44] and rats [45]. Many, but not all, of the pharmacological effects of P-blockers may be attributed to their Padrenoceptor antagonist activity per se. They do, however, possess other properties, such as acting as local anaesthetics or having intrinsic sympathomimetic activity. There have been suggestions that aberrant activity of drugs may be related to their chemical structure. Lesvkovsky and Tardos [43] proposed that the CNS-depressant action of propranolol might be a result of the presence of a methyl group, and a similar explanation has been essayed for the naphthyl group of pronethalol [41]. In the present study both propranolol and ICI 118551 (which has an indalyl group) induced an increase in sleeping time. The latter and another P-blocker, pindalol, have been shown to potentiate the effect of thiopentone in the rat [32] and pindalol has been shown to increase the effectiveness of chloral hydrate in mice [44]. From these observations it is interesting to note
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agonists and P-antagonists, potentiated thiopentone sleeping time, whilst drugs which enhance LC-NA activity, for example, a2-antagonists and P-agonists, gave a decrease in the effectiveness of thiopentone. However, not all anaesthetic agents have their activity modulated by interference with the central NA system. Adrenergic drugs were shown to have no effect on ketamine, urethane or Althesin (alphadolone/alphaxalone) anaesthesia [15,32]. In the present series of experiments it has been found that drugs which shortened thiopentone sleeping time could induce "stimulant" effects in unanaesthetized rats. Assessment of behavioural signs such as awareness, consciousness, spontaneous activity, stereotyped movements and motor co-ordination generally showed an increase. The degree of CNS excitation obtained was, however, not as great as that produced by the more conventional CNS stimulants. For example, the increased motor activity seen after yohimbine was intermittent compared with the continuous activity seen after amphetamine. Nonetheless, by measuring total locomotor activity it has been shown that yohimbine, WY 26392 and RS 21361, all selective a2-adrenoceptor antagonists, caused an increase in central excitation, reflected as a decrease in the total time spent immobile after adopting a sleeping posture. The P-adrenoceptor agonist, clenbuterol, also reduced sleeping time. For this drug, a direct stimulation of the postsynaptic P-adrenoceptors would lead to excitation of central NA neurones. It has been shown that electrical stimulation of the LC leads to the release of NA in the cerebral cortex [33], which could then lead to electrocortical and behavioural arousal [34, 35]. The possible correlation between the activity of LC cells and the duration of sleeping time receives support from the action of RX 781094. At low doses it produced an increase in sleeping time, possibly via a presynaptic a2-agonist action. Conversely, higher doses caused a reduction in sleeping time, presumably by autoreceptor block. Both behavioural studies using the thiopentoneinduced sleeping time model [36] and electrophysiological recordings of rate of discharge of LC cells [24] have shown a similar biphasic response with RX 781094. However, the enhancement of sleeping time produced by propranolol, clonidine and ICI 118551 cannot be attributed solely to modulation of coerulear discharge. Many workers have
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ACKNOWLEDGEMENT We thank Reckitt & Colman, Syntex, Wyeth and ICI for the generous gifts of the drugs used in this study.
REFERENCES 1. Dahlstrom A, Fuxe K. Evidence for the existence of monoamine containing neurones in the CNS. I. Demonstration of monoamines in the cell bodies of brain stem neurones. Acta Physiologica Scandinavica 1965; (Suppl. 62) 232: 1-55. 2. Ungerstedt U. Stereotaxic mapping of the monoamine pathways in the rat brain. Acta Physiologica Scandinavica 1971; (Suppl.) 367: 1-19. 3. Lindvall O, Bjorklund A, Nobin A, Stenevi U. The adrenergic innervation of the rat thalamus as revealed by the glyoxylic acid fluorescence method. Journal of Comparative Neurology 1974; 154: 317-348. 4. Pickel VM, Segal M, Bloom FE. A radioautographic study of the efferent pathways of the nucleus locus coeruleus. Journal of Comparative Neurology 1974; 155: 15-^2. 5. Shimuzu N, Ohnishi S, Tohyama M, Maeda T. Demonstration by degeneration silver method of the ascending projection from the locus coeruleus. Experimental Brain Research 1974; 20: 375-384. 6. Jones BE, Moore RY. Ascending projections of the locus coeruleus in the rat. Autoradiographic study. Brain Research 1977; 127: 23-53. 7. Amaral DG, Sinnamon HM. The locus coeruleus: neurobiology of a central noradrenergic nucleus. Progress in Neurobiology 1977; 9: 147-196. 8. McNaughton N, Mason ST. The neurophysiology and the neuropharmacology of the ascending dorsal noradrenergic bundle. Progress in Neurobiology 1980; 14: 157-219. 9. Mason ST. Noradrenaline in the brain: progress in theories of behavioural function. Progress in Neurobiology 1981; 16: 263-303. 10. Robinson TE, Vanderwolf CH, Pappas BA. Are the dorsal noradrenergic bundle projections from the locus coeruleus important for neocortical and hippocampal activation? Brain Research 1977; 138: 75-98. 11. Olpe HR, Glare A, Laszlo J, Schellenberg A. Some electrophysiological and pharmacological properties of the cortical noradrenergic projection of the locus coeruleus in the rat. Brain Research 1980; 186: 9-19. 12. Beiner PB. Clonidine inhibits central noradrenergic neurons in unanaesthetized cats. European Journal of Pharmacology 1985; 115: 249-257. 13. De Sarro GB, Ascioti C, Froio F, Libri V, Nistico G. Evidence that locus coeruleus is the site where clonidine and drugs acting at otl- and a,-adrenoceptors affect sleep and arousal mechanisms. British Journal of Pharmacology 1987; 90: 675-685. 14. Angel A, Mason ST. 6-Hydroxydopamine-induced depletion of noradrenaline potentiates barbiturate anaesthesia. Journal of Physiology (London) 1982; 324: 75P. 15. Mason ST, Angel A. Anaesthesia: the role of adrenergic mechanisms. European Journal of Pharmacology 1983; 91: 29-39. 16. Delbarre B, Schmitt H. Sedative effects of a-sympathomimetic drugs and their antagonism by adrenergic and cholinergic blocking drugs. European Journal of Pharmacology 1971; 13: 356-363. 17. Bainbridge JG, Greenwood D T . Tranquilizing effects of propranolol demonstrated in rats. Neuropharmacology 1971; 10: 453-458. 18. Bloom FE. Neurohumoral transmission and the CNS. In: Goodman LS, Gilman A, eds. The Pharmacological Basis
Downloaded from http://bja.oxfordjournals.org/ at The University of British Colombia Library on July 9, 2015
that P-blockers with a double ring structure on the aromatic moiety of the molecule produce a sedative or depressant action, whereas compounds with a phenyl group such as nifenalol and dichloroisoproterenol cause central excitation. Similarly sotalol, dichloroisoproterenol and Ko 1336 shortened, whereas practolol did not alter, chloral hydrate sleeping time [44]. The significance of structure—activity relationships of a2-adrenoceptor antagonists has been demonstrated [46]. Thus the possibility of a similar structure-dependent action of P-adrenoceptor antagonists cannot be ruled out. The sedative action of clonidine has been attributed to its activation of presynaptic a2adrenoceptors on LC cells causing a decrease in the activity of this ascending NA pathway projecting diffusely to subcortical and cortical areas. However, such a simplistic mechanism of action can, at best, provide only a partial explanation for its wide-ranging central effects. In the present study its action resembled that of an anaesthetic rather than a sleep-inducing agent. Electrophysiological studies [47] have shown that clonidine in high dose (^ 100 (ig kg"1) potentiates the effect of urethane and has an action identical to that of several general anaesthetic agents as measured by electrocortical activity, cerebral evoked responses and its ability to suppress thalamic and cortical, but not cuneate, cellular responsiveness to electrical stimulation of the periphery. The same authors reported a reverse action of clonidine at small doses. Such a biphasic dose-dependent action was seen also in the present study (table I). In support of this suggestion for a separate, non-adrenergic, mechanism of action of clonidine-induced CNS depression, Nassif and colleagues [48] have shown that a neurochemical lesion of the LC system does not suppress its sedative action. Moreover, yohimbine, a specific a2-adrenoceptor antagonist, has no effect on spontaneous electrocortical activity, cerebral evoked responses or cellular responses to peripheral stimulation at cuneate, thalamic or cortical sites [49]. Thus not all of the central actions of clonidine can be ascribed to an otj-agonist action. It may in addition exert a mild anaesthetic-like action. The exact site, or sites, of such action should be determined.
599
600
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of Therapeutics, 6th Edn. London: Collier-MacMillan, effects of stimulation of the nucleus locus coeruleus in the 1980; 235-257. stumptailed monkey, Macaca arctoides. Brain Research 1976; 116: 502-510. 19. Angel A, Majeed ABA. The effects of some centrally active adrenergic drugs on sleeping time in the rat. Journal 35. Koella WP. The organization and regulation of sleep. A of Physiology {London) 1986; 378: 45P. review of the experimental evidence and a novel integrated model of the organizing and regulating apparatus. Experi20. Angel A, Majeed ABA. Effects of centrally active entia 1984; 40: 309-338. adrenoceptor agonists and antagonists on sleeping time in the rat. In: Proceedings of the First Congress of the Asian 36. Mason ST. Alpha-2 receptor antagonists and thiopentone and Oceanian Physiological Societies, Bangkok, Thailand, anaesthesia in the rat. Journal of Physiology (London) November 26-29, 1986. 1985; 360: 37P. 21. Angel A. Two simple, relatively inexpensive, devices to 37. Svensson TH, Bunney BS, Aghajanian GK. Inhibition of measure the locomotor activity of anaesthetized or unboth noradrenergic and serotonergic neurons in brain by anaesthetized animals. British Journal of Pharmacology •^-agonist clonidine. Brain Research 1975; 92: 291-306. 1970; 39: 243P. 38. Cedarbaum JM, Aghajanian GK. Catecholamine re22. Angel A, Rogers KJ. An analysis of the convulsant activity ceptors on locus coeruleus neurons: Pharmacological of substituted benzenes in the mouse. Toxicology and characteristics. European Journal of Pharmacology 1977; Applied Pharmacology 1972; 21: 214-229. 44: 375-385. 23. Barnes CD, Etherington LG. Drug Dosage in Laboratory 39. Marwaha J, Kehne JH, Comnissaris RL, Lakoski J, Shaw Animals—A Handbook, revised Edn. California: UniW, Davis M. Spinal clonidine inhibits neural firing in versity of California Press, 1973. locus coeruleus. Brain Research 1983; 276: 379-382. 24. Goldstein JM, Knobloch LC, Malick JB. Electro- 40. Dahlof C, Engberg G, Svensson TH. Effects of 0adrenoceptor antagonists on the firing rate of norphysiological demonstration of both a,-agonist and anadrenergic neurones in the locus coeruleus of the rat. tagonist properties of RX781094. European Journal of Naunyn Schmiederbergs Archive of Pharmacologie 1981; Pharmacology 1983; 91: 101-105. 317: 26-30. 25. Ross SB, Haljasma O. Catechol-O-methyl transferase inhibitors: in vivo inhibition in mice. Ada Pharmacologica 41. Murman W, Almirantc L, Saccani-Guelfi M. Central nervous system effects of four P-adrenergic receptor et Toxicologica 1964; 21: 215-225. blocking agents. Journal of Pharmacy and Pharmacology 26. Kleinlogel H, Scholtysik G, Sayers AC. Effects of 1966; 18: 317-318. clonidine and BS100-141 on the EEG sleep pattern in rats. European Journal of Pharmacology 1975; 33: 159-163.42. Hermansen K. Effects of different P-adrenergic receptor blocking agents on hexobarbital induced narcosis in mice. 27. Davies DS, Wing LMH, Reid JL, Neill E, Tippett P, Acta Pharmacologica et Toxicologica 1969; 27: 453-^60. Dollery CI. Pharmacokinetics and concentration-effects of intravenous and oral clonidine. Clinical Pharmacology 43. Leszkovsky G, Tardos L. Some effects of propranolol on the central nervous system. Journal of Pharmacy and and Therapeutics 1977; 21: 593-601. Pharmacology 1965; 17: 518-519. 28. Muller JO, Frouts JR. Prolongation of hcxobarbital sleeping time and inhibition of hepatic drug metabolism by 44. Delbarre B, Schmitt H. A further attempt to characterize sedative receptors activated by clonidine in chickens and adrenergic blocking agents in mice. Biochemical Pharmice. European Journal of Pharmacology 1973; 22: macology 1965; 14: 305-311. 355-359. 29. Miller RD, Way WL, Eger El. The effects of otmethyldopa, reserpine, guanethidine and iproniazid on 45. Torbati D. Effect of propranolol on cortical electrical activity in conscious and anaesthetized rats. Neurominimum alveolar anesthetic requirement (MAC). Anespharmacology 1986; 25: 1251. thesiology 1968; 29: 1153-1158. 30. Johnston RR, Way WL, Miller RD. Alteration of 46. Pettibone DJ, Pfleuger AB, Totaro JA. Comparison of the effects of recently developed ot,-adrenergic antagonists anesthetic requirement by amphetamine. Aneslhesiology with yohimbine and rauwolscine on monoamine systems 1972; 36: 357-363. in rat brain. Biochemical Pharmacology 1985; 34: 109331. Roizen MF, Kopin IJ, Thoa NB, Zivin J, Muth EA, 1097. Jacoboitz D. The effect of two anaesthetic agents on norepinephrine and dopamine in discrete brain nuclei, 47. Angel A, Goldman P, Halsey MJ, Majeed ABA, Kendig J. A possible anaesthetic action of clonidine. Journal of fibre tracts and terminal regions of the rat. Brain Research Physiology {London) 1986; 378: 10P. 1976; 110: 515-522. 32. Mason ST, Angel A. Brain noradrenaline and anaesthesia: 48. Nassif S, Kempf E, Cardo B, Velley L. Neurochemical lesion of the locus coeruleus of the rat does not suppress Further characterization of the beta receptor. Neurothe sedative effect of clonidine. European Journal of pharmacology 1983; 22: 1065-1069. Pharmacology 1983; 91: 69-76. 33. Tanaka C, Inagaki C, Fujiwara H. Labelled noradrenaline release from rat cerebral cortex following electrical 49. Angel A, Majeed ABA. An electrophysiological study on the central action of yohimbine in the rat. Journal of stimulation of locus coeruleus. Brain Research 1976; 106: 384-389. Physiology {London) 1987; 392: 58P. 34. Redmond DE, Huang YH, Snyder DR. Behavioural