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Vol. 294, Issue 1, 187-194, July 2000
Department of Pharmacology and Human Physiology, University of Bari, Bari, Italy
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Abstract |
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 Top
 Abstract
 Introduction
Materials and Methods
Results
Discussion
References
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1,2,3,3a,8,8a-Hexahydro-1,3a,8-trimethylpyrrolo[2,3-b]indol-5-ol
2-ethylphenylcarbamate N-oxide hydrochloride
(3aS-cis) (CHF2819) is a novel
acetylcholinesterase inhibitor that produces central cholinergic
stimulation after oral administration in rats. In vivo studies show
that CHF2819 (0.5, 1.5, and 4.5 mg/kg p.o.) significantly increases
acetylcholine levels in young adult rat hippocampus in a dose-dependent
manner. Moreover, aged animals, which show a significant decrease in
basal acetylcholine levels with respect to young adult rats, also
exhibit a marked increase in the hippocampal concentrations of this
neurotransmitter after the administration of CHF2819. This compound
(1.5 mg/kg p.o.) significantly attenuates scopolamine-induced amnesia
in a passive avoidance task. Furthermore, CHF2819 induces a significant
decrease in dopamine levels and a significant elevation of
extracellular concentrations of 5-hydroxytryptamine, whereas it does
not modify norepinephrine and 
-aminobutyric acid levels in the
hippocampus of young adult rats. Functional observational battery
screening demonstrates that CHF2819 (1.5 and 4.5 mg/kg p.o.) does not
affect activity, excitability, autonomic, neuromuscular, and
sensorimotor domains, as well as physiological end points (body weight
and temperature). However, this compound induces involuntary motor movements (ranging from mild tremors to myoclonic jerks) in a dose-dependent manner. These findings suggest that the anti-amnestic properties of CHF2819, together with its stimulatory effect on cholinergic and serotonergic functions, might have a therapeutic potential mainly for the symptomatic treatment of Alzheimer's disease
patients in which the cognitive impairment is accompanied by a
depressive syndrome.
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Introduction |
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Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
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Alzheimer's
disease (AD) is a complex and multifaceted neurodegenerative disease
affecting aged populations. The pathogenesis and the etiology remain
unknown, although a "cholinergic deficit hypothesis" has been
suggested (Perry, 1986
). In fact, among the multiple transmitter
deficits that have been described in AD, one of the most specific and
consistent features is an early and severe degeneration of forebrain
cholinergic system, as revealed by the correlation observed between the
cholinergic pathology and dementia (Geula and Mesulam, 1994).
Therefore, the enhancement of brain cholinergic transmission in AD
remains a major goal for many putative therapeutic agents that are in
use or under development.
Acetylcholinesterase (AChE) has long been an attractive target for
the rational design of mechanism-based inhibitors because of the
pivotal role it plays in the central nervous system. Currently, only
the AChE inhibition approach, which enhances the function of central
cholinergic neurons by permitting acetylcholine (ACh) to remain in the
synaptic cleft longer through reducing ACh hydrolysis, seems to produce
encouraging symptomatic improvements in clinical trials. In fact, the
resulting increase in extracellular ACh concentrations might reverse
central cholinergic hypofunction and improve cognitive functions in AD
(Kelly, 1999).
To date, most of the drugs used therapeutically have proved to
ameliorate AD symptomatically, but it is controversial whether there is
an effect on the disease progression (Giacobini, 1998).
The clinical usefulness of AChE inhibitors (AChEIs) has been limited by
either an extremely short or an excessive long half-life, hepatotoxicity, and severe peripheral cholinergic side effects (Giacobini, 1998; Kelly, 1999). To obtain greater therapeutic benefit,
newer AChEIs that circumvent these problems are needed.
This study describes the biochemical and neurobehavioral profile of
CHF2819 (Fig. 1), a novel geneserine
derivative with AChE inhibitory activity (Pietra et al., 1999). The
characterization of CHF2819 started with an in vivo (microdialysis
technique) investigation of the effects of this compound, administered
by the oral route or by local perfusion via the dialysis probe, on the
extracellular concentrations of ACh in young adult rat hippocampus, the
main target region, together with the cerebral cortex, for symptomatic treatment of AD. This was followed by an investigation of
behavioral correlates of central cholinergic function in young adult
rats (scopolamine-induced amnesia in a passive avoidance task).
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A functional observational battery (FOB) of tests was used to assess
functional domains (sensory, motor, and autonomic) in young adult rats
to investigate potential neurotoxic effects of CHF2819.
Moreover, because a recovery of extracellular ACh levels in aged
rats has been obtained after the administration of AChEIs as well as
drugs acting on brain cholinergic neurons with different mechanisms
(Quirion et al., 1995; Scali et al., 1997a; Vannucchi et al., 1997),
the effects of CHF2819 on extracellular ACh levels in the hippocampus
of aged rats were also measured in this study.
However, noncholinergic neurochemical abnormalities that may contribute
to the behavioral and cognitive disorders associated with AD have been
identified (Zubenko et al., 1990; Camacho et al., 1996). Furthermore,
experimental and clinical data have shown interactions between central
cholinergic and catecholaminergic, serotonergic, and -aminobutyric
acid (GABA)ergic systems (Bianchi et al., 1982; Memo et al., 1988;
Robinson et al., 1989; Decker and McGaugh, 1991). Therefore, it is
likely that the efficacy of AChEIs in the treatment of demented
patients could be due not only to cholinesterase inhibition but also to
other neurochemical effects. In this study, we therefore also
investigated, in addition to ACh, the effects of CHF2819 on
extracellular concentrations of dopamine (DA), 5-hydroxytryptamine
(5-HT), norepinephrine (NE), and GABA in the rat hippocampus.
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Materials and Methods |
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Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
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Animals. Young adult (2-3 months old) and aged (20-22 months old) male Wistar rats (Harlan, S. Pietro al Natisone, Udine, Italy) were used. They were housed at constant room temperature (22 ± 1°C) and relative humidity (55 ± 5%) under a 12-h light/dark cycle (lights on from 8:00 AM to 8:00 PM). Food and water were freely available.
Chemicals. CHF2819 (Fig. 1) was provided by Chiesi Farmaceutici S.p.A. (Parma, Italy). The drug was dissolved in saline and administered p.o. in a volume of 2 ml/kg. All doses refer to the salt form (HCl). All other chemicals were obtained from commercial sources.
Dialysis Procedure.
As previously described (Cagiano et al.,
1998), rats were anesthetized with 3 ml/kg i.p. of a solution
containing 1.2 g of pentobarbital, 5.3 g of chloral hydrate,
2.7 g of MgSO4, 49.5 ml of propylene glycol,
12.5 ml of ethanol, and 58 ml of distilled water.
2.4 mm
according to a stereotaxic atlas (Paxinos and Watson, 1982). A short
piece of dialysis fiber made of copolymer of acrylonitrile sodium
methallyl sulfonate (AN69 Hospal S.p.A; 20,000 Da cutoff) was
covered with epoxy glue to confine dialysis to the area of interest
(6-mm glue-free zone). The skull of the rat was exposed, and two holes
were made on the lateral surface at the level of the head of the dorsal
hippocampus. A dialysis fiber, held straight by a tungsten wire inside,
was inserted transversely into the brain so that the glue-free zone was
located exactly in the target area. The tungsten wire was withdrawn,
and stainless steel cannulas (22-gauge diameter, 15 mm long) were glued
to the ends of the fibers. These ends were bent up and fixed vertically
to the skull using dental cement and modified Eppendorf tips. Finally,
the skin was sutured, and the rats were allowed to recover from
anesthesia for at least 15 h before the neurotransmitter release
study. On the day of the experiment, the fibers were perfused with a
Krebs-Ringer solution containing 138 mM NaCl, 11 mM KCl, 1.5 mM
CaCl2, 1 mM MgCl2 and 11 mM
NaHCO3 in distilled water. The solution was
buffered at pH 7.4 with a 2 mM sodium-phosphate buffer, filtered (0.22 µm), and degassed. No AChEIs were administered through the dialysis probe to increase ACh detection capability. The fibers were perfused at
a constant flow rate of 2 µl/min with a CMA/100 microinjection pump
(CMA Microdialysis, Stockholm, Sweden). After a 60-min washout period,
consecutive 20-min samples of perfusate were collected, and
neurotransmitter concentrations were assayed by HPLC. Once a stable
basal neurotransmitter output was obtained (no more than 10%
difference between three consecutive samples), rats were administered the drug. The position of the microdialysis probe was verified by
histological procedures at the end of each experiment. Only rats in
which probe tracks were exactly located in the target area were
considered in Results.
HPLC Analysis. ACh concentrations were determined by HPLC using a microbore column and enzyme reactor coupled with electrochemical detection in reduction mode and a glassy carbon electrode (6 mm) coated with peroxidase with +0.0 V applied (wired electrode system; Bioanalytical Systems, West Lafayette, IN; Sepstik 530- mm × 1-mm analytical column and ACh/Ch IMER). The mobile phase used was 80 mM sodium phosphate with 5 ml/l Kathon (Bioanalytical Systems) at pH 8.5. The flow rate used was 125 µl/min, and detection sensitivity for ACh was 0.1 nM (10 µl injected).
DA, 3,4-dihydroxyphenilacetic acid (DOPAC), homovanillic acid (HVA), 5-HT, 5-hydroxyindolacetic acid (5-HIAA), and NE levels were determined by microbore HPLC using a Spherisorb 15-cm × 2- mm column (3-µm packing). The detection was accomplished with a Unijet cell (BAS) with a 6-mm-diameter glassy carbon electrode at +0.65 V, connected to a Waters 460 electrochemical detector, as previously described (Kendrick et al., 1996). Detection limits for a 10-µl injection volume were 100 to 200 pM. GABA concentrations were measured by HPLC with fluorescence
detection (Gilson, 157) after derivatization with
o-phthaldialdehyde as previously described (Kendrick et al.,
1996) and with a detection limit of 5 nM for a 10-µl sample volume.
Passive Avoidance Behavior. A stepdown-type apparatus was used. It consisted of a compartment (25 × 24 × 24 cm) constructed of black Plexiglas and equipped with a grid floor to which an elevated compartment (13 × 24 × 16 cm) with solid Plexiglas floor was attached. The opening between the elevated compartment and the large compartment was separated by a guillotine door (9 × 10 cm). A 25-W lamp illuminated the elevated compartment, whereas the large compartment remained dark. Scrambled foot shocks were delivered from a Letica shock generator (LI 2750 U; Barcelona, Spain). The experiments were performed in a sound-attenuating chamber (Amplifon G-type cabin) that was dark except for the illumination of the elevated compartment of the apparatus. Each animal was removed from the home cage and placed in a holding cage adjacent to the apparatus. Two minutes later, the rat was placed in the illuminated compartment, and after a 10-s delay, the guillotine door was raised; thereafter, its latency (approach latency) to enter the dark compartment was recorded and a single 2-s unavoidable scrambled foot shock (0.8 mA) was immediately delivered after entering the dark compartment. The retention of the passive avoidance response was tested 24 h after the learning trial. The animal was placed on the elevated compartment, and the latency to reenter (avoidance latency) the dark compartment was recorded. Both acquisition and retention trials lasted for a maximal observation time of 180 s. CHF2819 (0.5, 1.5, and 4.5 mg/kg) was administered orally 90 min before the acquisition trial. Scopolamine hydrobromide (0.75 mg/kg) was dissolved in saline and injected s.c. 30 min before the acquisition trial.
FOB.
The FOB consisted of measures of sensory, motor, and
autonomic function. The evaluation of the end points considered and the scoring criteria used have been extensively described elsewhere (Moser,
1997). Briefly, the rat was placed on a flat surface (open field with a
perimeter barrier, 60 × 60 cm) covered with a clean absorbent
pad. The rat was observed for 3 min, and during that time, the
frequency of rearing responses was recorded. At the same time, gait
characteristics were noted and ranked; the ease with which the rat
moved about was also ranked, and arousal, tremor, convulsions, and
abnormal postures were evaluated. At the end of the 3 min, the number
of the fecal boluses and urine pools on the absorbent pad were
recorded. Reflex testing then consisted of recording the responses of
each rat to the approach of a blunt object such as a pencil, a touch of
an object to the posterior flank, and an auditory click stimulus.
Responsiveness to a pinch on the tail and the ability of the pupil to
constrict to light were then assessed. These measures were followed by
a test for the righting reaction and then followed by measures of
forelimb and hindlimb grip strength, body weight and rectal
temperature, and, finally, hindlimb landing foot splay. The entire
battery of tests required approximately 6 to 8 min per rat. Animals
were subjected to FOB screening 90 min and 24 h after dosing.
Data Analysis. Neurochemical data were expressed as percentages of baseline, which was defined as the average of at least three consecutive samples with stable level of neurotransmitters. Actual data were analyzed by two-way ANOVA for repeated measures with treatment (tr) as the between-subject factor and time (t) as the within-subject factor. Conservative F tests using the Greenhouse-Geisser correction were performed to account for possible violations of the sphericity assumption. Post hoc comparisons were made by Dunnett's and Tukey's tests where appropriate. The adoption of nonparametric tests (Wilcoxon's paired signed rank test) was due to the nonhomogeneity of variances, as shown by Bartlett's test.
Statistical analysis of behavioral data (passive avoidance task) was based on Kruskal-Wallis ANOVA. The Mann-Whitney U test was used for individual comparisons between groups. The data collected with FOB assessment fall into these different classes: categorical (i.e., presence or absence of a sign), ordinal (i.e., ranking of the severity of a sign), or continuous (i.e., a range of motor activity counts) values. Analyses of the individual FOB measures, as well as the physiological measures (body weight and body temperature), were conducted as previously described (Moser, 1997).
Animal Care. The experiments were conducted in accordance with guidelines released by Italian Ministry of Health (D.L. 116/92), the Declaration of Helsinki, and the Guide for the Care and Use of Laboratory Animals as adopted and promulgated by the National Institutes of Health.
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Results |
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Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
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Effects of CHF2819 Administration on Extracellular ACh
Concentrations in Young Adult and Aged Rats.
Constant
extracellular concentrations of ACh were detectable in the 20-min
baseline samples collected for 6 h from the hippocampus of
conscious, freely moving young adult rats (mean ± S.E. = 1.2 ± 0.2 nM; n = 36) (Fig.
2). The effects of the oral
administration of CHF2819 on the basal extracellular concentrations of
ACh were determined for 4 h after administration of the drug (Fig.
2). Two-way ANOVA for repeated measures showed the following
differences: [F(tr)3,240 = 13.11, P < .0001;
F(t)12,240 = 3.94, P < .01; F(tr × t)36,240 = 3.93, P < .01]. The post hoc test showed that CHF2819 (0.5, 1.5, and 4.5 mg/kg
p.o.) dose dependently increased ACh levels. The maximal stimulatory
effect of CHF2819 was found at 4.5 mg/kg 120 min after its
administration (732% increase above the baseline). The increase in ACh
concentrations was still significant 4 h after treatment (Fig. 2).
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73%) (Fig. 4,
inset). The post hoc test showed that CHF2819, administered p.o. at the
dose of 4.5 mg/kg, induced a significant increase in extracellular ACh concentrations that peaked 20 min after treatment and disappeared within 60 min [F(tr)1,8 = 14.93, P < .005;
F(t)9,72 = 3.37, P < .005; F(tr × t)9,72 = 3.29, P < .005] (Fig. 4).
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Effects of CHF2819 Administration on Extracellular DA, DOPAC, HVA,
5-HT, 5-HIAA, NE, and GABA Concentrations.
Data are reported in
Fig. 5. For DA, the two-way ANOVA for
repeated measures showed that significant differences between
treatments were time-independent
[F(tr)3,240 = 12.27, P < .001;
F(t)12,240 = 1.02, N.S.;
F(tr × t)36,240 = 1.26, N.S.], and therefore individual comparisons between marginal
means (pooled data of 13 samples for each treatment) were made. Results
showed that at the highest dose, CHF2819 significantly decreased DA
levels (baseline, 0.67 ± 0.39 nM) (Fig. 5, inset). Concentrations
of DA metabolites DOPAC and HVA were not affected by any of the doses
tested: DOPAC: [F(tr)3,240 = 0.71, N.S.; F(t)12,240 = 1.29, N.S.; F(tr × t)36,240 = 0.69, N.S.]; HVA: [F(tr)3,240 = 0.23, N.S.; F(t)12,240 = 1.56, N.S.; F(tr × t)36,240 = 1.86, N.S.].
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Effects of CHF2819 Administration on Passive Avoidance
Behavior.
Kruskal-Wallis ANOVA for approach latencies showed no
significant differences (H = 0.87; df = 4, N.S.) among groups (data not shown). Conversely, Kruskal-Wallis
ANOVA for avoidance latencies showed the following significant
differences: H = 11.78; df = 4;
P < .05. Individual comparisons between groups
indicated that CHF2819, at a dose of 1.5 mg/kg, significantly
attenuated scopolamine-induced decrease of avoidance latencies, whereas
both the lowest (0.5 mg/kg) and the highest (4.5 mg/kg) doses did not
affect this behavioral end point (Fig.
6).
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FOB Assessment.
Results of neurobehavioral screening battery
showed that oral administration of CHF2819 (1.5 and 4.5 mg/kg) did not
significantly affect activity, excitability, autonomic, neuromuscular,
and sensorimotor domains (data not shown). In particular, the following
end points were not influenced by this AChEI: handling (ease of
removal, handling, lacrimation, palpebral closure, piloerection,
salivation), open field (rears, urination, defecation, gait, gait
score, mobility score, arousal, vocalizations, stereotypy), reflexes
(approach response, touch response, click response, tail pinch
response, pupil response, righting reflex, landing foot splay), grip
strength (forelimb, hindlimb), and physiological (body weight, body
temperature). However, at 90 min after dosing, this compound induced
involuntary motor movements (ranging from mild tremors to myoclonic
jerks) in a dose-dependent manner (Fig.
7). These alterations were not observed
24 h after treatment.
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Discussion |
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Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
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The severity of cognitive decline in AD has been shown to be
mainly correlated with alterations of the cholinergic function (Mountjoy et al., 1984), and this has led to the hypothesis that impaired learning and memory would be ameliorated by the restoration of
cholinergic neurotransmission. In this regard, an overwhelming amount
of evidence suggests the importance of hippocampal cholinergic transmission in cognitive processes. It has been demonstrated that a
number of cholinomimetic agents enhance memory (Bartus, 1987);
furthermore, it has been shown that several AChEIs stabilize most AD
patients at their present cognitive and behavioral state for a period
of at least 1 year (Giacobini, 1998).
At present, a novel AChEI that is orally administrable, efficacious, tolerable, and relatively safe remains a major therapeutic goal for further validation of the cholinergic deficit hypothesis of AD and successfully treatment of AD patients. This study suggests that the novel geneserine derivative CHF2819 may be an important candidate in this respect.
Our results have shown clearly that in the hippocampus of both young
and aged rats, CHF2819 given either systemically or directly potently
increases extracellular ACh concentrations. The highly sensitive
detection methods used for determining ACh concentrations in the
microdialysis samples made it possible to determine these effects
without having to add other AChEIs. The use of such inhibitors has
often restricted interpretation of previous studies on ACh release
where neostigmine or physostigmine was required to be added to
dialysates for efficient detection of basal ACh levels. The addition of
these inhibitors has been reported previously to alter ACh release
profiles (de Boer et al., 1990) and complicate the interpretation of
systemically administered AChEI effects (Messamore et al., 1993).
Incorporation of neostigmine in the dialysis medium also modifies the
calcium dependence and tetrodotoxin sensitivity of extracellular ACh
levels (Damsma et al., 1988). Furthermore, in several studies, it has
been demonstrated that the increase in ACh levels induced by
retrodialysis application of neostigmine or physostigmine induces a
muscarinic autoregulatory mechanism that appears to be quiescent under
basal conditions (de Boer et al., 1990; Kawashima et al., 1991).
The increase in endogenous hippocampal ACh levels after the oral administration of CHF2819 in young adult rats was dose-dependent. At the maximum dose used (4.5 mg/kg), this compound induced a 732% increase in ACh concentrations above baseline between 80 and 120 min after its administration orally. Furthermore, the ACh increase was long lasting, with levels of this neurotransmitter still being significantly elevated above baseline 240 min after treatment.
This long-lasting effect was not found after the oral administration of
other AChEIs, such as metrifonate or tacrine. In fact, metrifonate (80 mg/kg) and tacrine (3 mg/kg) induced a significant elevation of
hippocampal ACh, which lasted 140 and 100 min, respectively (Scali et
al., 1997a,b).
Infusions of CHF2819 through the dialysis probe allowed us to confirm its direct action on in vivo hippocampal neurotransmitter concentrations. Under these circumstances, elevated ACh levels occurred immediately in the sample where the drug was first infused and were initially higher in the hippocampus than after systemic administration (1970% increase above baseline at 20 min). However, ACh levels remained significantly elevated for only 20 min after the end of the infusion, although preinfusion levels were not completely restored for 80 to 100 min. These neurochemical changes were paralleled by behavioral effects showing that CHF2819 significantly attenuated scopolamine-induced amnesia in a passive avoidance task.
The attenuation of scopolamine-induced amnesia elicited by CHF2819
occurred at a lower dose level (1.5 mg/kg) than that (4.5 mg/kg)
producing the peak effect on extracellular concentrations of ACh, thus
suggesting that the lower increase in ACh levels elicited by 1.5 mg/kg
CHF2819 is sufficient to antagonize scopolamine-induced memory
impairment. Literature data have clearly shown that the administration
of AChEIs is followed by AChE inhibition and an increase in
extracellular ACh levels in various brain areas. In turn, this is
accompanied by an improvement in learning and memory deficits
associated with cholinergic hypofunction (Pepeu, 2000). However, no
straightforward correlation can be established between the intensity of
AChE inhibition, the increase in ACh, and the beneficial effect on
cognitive function. In some cases, improvements have been observed with
doses of AChEIs with effects on AChE and ACh levels that were
undetectable. For example, previous findings have shown that
scopolamine-induced impairment of the passive avoidance response was
prevented by metrifonate also at doses (10-15 mg/kg p.o.) that did not
significantly increase cortical ACh levels in rats (Itoh et al., 1997).
Therefore, it has been assumed that small undetectable increases in ACh
levels at critical synapses are sufficient to ameliorate the cognitive
impairment induced by scopolamine (Pepeu, 2000).
On the other hand, at the highest dose (4.5 mg/kg) used in this study,
CHF2819 did not significantly affect scopolamine-induced amnesia. These
results are in agreement with those reported in recent studies (Wang
and Tang, 1998) showing the effectiveness of other AChEI agents
[()-huperazine, donepezil, and tacrine] in antagonizing the
disruptive effect of scopolamine on memory in rats (bell-shaped
dose-effect curve). Interestingly, more than 20 years ago, when
discussing the possible role of the cholinergic system in memory,
Deutsch (1973) proposed that "as physostigmine prolongs the effects
of ACh by inhibiting AChE, then this drug should strengthen weak
memories but weaken strong memories because there will be excessive ACh
which will result in a depolarization block". Moreover, because
CHF2819 induced involuntary motor movements (ranging from mild tremors
to myoclonic jerks) in a dose-dependent manner, the lack of
antiamnestic effect at the highest dose (4.5 mg/kg) could be in part
due to the marked neurotoxic alteration caused by this AChEI.
Cognitive impairment in aged rats seems to be in part due to
cholinergic hypofunction, and activation of the brain cholinergic system under these circumstances is often accompanied by an improvement in cognitive dysfunction (Riekkinen et al., 1991; Ikari et al., 1995).
Our data have demonstrated that in aged rats, there is a significant
(73%) reduction in basal ACh concentrations in the hippocampus and
that CHF2819 is also capable of producing marked elevations in levels
in these animals that were of a similar magnitude to those found in
young animals.
Findings from previous electrophysiological, biochemical, and
pharmacological experiments are consistent with the hypothesis that
there is a close functional interaction between central cholinergic and
monoaminergic and GABAergic neurotransmitter systems (Bianchi et al.,
1982; Robinson et al., 1989; Decker and McGaugh, 1991).
Our current results show that CHF2819 can increase 5-HT concentrations
and decrease those of DA in the hippocampus of freely moving rats.
These data are in agreement with previous in vitro studies showing that
tacrine, an AChEI agent, evokes the release of radiolabeled 5-HT in
rodent brain (Robinson et al., 1989).
To our knowledge, this is the first in vivo report showing a
concomitant increase of ACh and 5-HT levels in rat hippocampus after
AChEI administration. Indeed, previous studies have reported no
consistent changes in rat brain of 5-HT or 5-HIAA efflux after the
systemic or local administration of various AChEIs (Cuadra et al.,
1994; Mori et al., 1995; Giacobini et al., 1996; Warpman et al., 1996).
Increased 5-HT levels produced by CHF2819 could be of particular
interest in AD treatment. Indeed, depressive disorders have been
reported in some AD patients (Gottfries, 1996). Furthermore,
significant decreases in 5-HT and 5-HIAA levels have been shown in
discrete areas of the brain of the AD patient as well as a reduced
number of 5-HT nerve terminals (Gottfries et al., 1983; Gottfries,
1990).
As far as the dopaminergic and noradrenergic system is concerned, our
present data show that CHF2819 does not affect NE concentrations, whereas it significantly decreases DA levels, without affecting DA
metabolism. Previous findings have demonstrated that AChEI-induced stimulation of cholinergic activity induces an increase in DA levels
(Grenhoff and Svensson, 1992; Warpman et al., 1996), whereas other
studies have shown no significant effect (Westerink et al., 1990;
Dajas-Bailador et al., 1996). However, interactions between cholinergic
and dopaminergic systems seem to play a role in the modulation of
memory processes. In fact, a specific cholinergic control of the DA
system located in brain areas involved in cognitive functions
(hippocampus and cerebral cortex) has been shown (Memo et al., 1988).
Cholinergic agonists increase DA turnover and release in vivo (Xu et
al., 1989), and the systemic administration of muscarinic antagonists
impairs performance on cognitive tests and reduces DA turnover in
frontal cortex (Memo et al., 1988). Moreover, previous studies have
shown a reciprocal interaction of DA and ACh, as well as an elevation
of cortical DA levels, after physostigmine administration (Day and
Fibiger, 1992; Cuadra et al., 1994).
Furthermore, tacrine administered to rats at doses that did not elevate
ACh levels caused a modest increase in DOPAC levels in the whole brain
(Nielsen et al., 1989). Conversely, a clear-cut increase in
extracellular NE concentrations and a smaller increase in DA were shown
after the systemic administration of heptylphysostigmine (Cuadra et
al., 1994). The systemic administration of a large dose of metrifonate
induced an increase in NE levels, whereas the systemic administration
of small doses of metrifonate induced an elevation of DA concentrations
in rat cortex (Mori et al., 1995). The systemic administration of
donepezil at the dose of 2 mg/kg i.p., which in rat cortex caused a
35% AChE inhibition associated with a 2100% increase in ACh
extracellular concentrations, was accompanied by increases of 100 and
80% in extracellular levels in the cortex of NE and DA, respectively
(Giacobini et al., 1996). It has been shown that NE inhibits ACh
release in the cerebral cortex by acting on presynaptic
2-heteroreceptors (Beani et al., 1986). The
possibility of enhancing the effects of AChE inhibition either by
blocking the 2-receptors or by inhibiting NE
release has been previously investigated. It has been shown that only the combination of AChEIs with a selective 2
antagonist, such as idazoxan, is able to potentiate the effect of AChE
inhibition on extracellular concentrations of ACh (Cuadra et al., 1994;
Cuadra and Giacobini, 1995).
Finally, this study shows that CHF2819 does not affect extracellular
GABA concentrations in rat hippocampus. To our knowledge, there is no
information available on the effects of AChEIs on GABAergic function,
even though this neurotransmitter system is affected by AD (Chu et al.,
1987).
In conclusion, the neurochemical and behavioral profile of CHF2819 (i.e., marked increase in ACh levels in the hippocampus of both young adult and aged rats, attenuation of scopolamine-induced amnesia, increase in hippocampal 5-HT concentrations) suggests that this orally active novel AChEI agent could be of clinical interest mainly for the symptomatic treatment of AD patients in which the cognitive impairment is accompanied by a depressive syndrome.
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Acknowledgments |
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We thank Prof. E. Giacobini for valuable suggestions and Carlos de la Riva and Michele Persichella for technical assistance.
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Footnotes |
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Accepted for publication March 21, 2000.
Received for publication February 3, 2000.
1 This work was supported by Chiesi Farmaceutici S.p.A. and Biotechnology and Biological Sciences Research Council.
2 Current address: Pharmacology Department, Chiesi Farmaceutici S.p.A., Via Palermo 26/A, 43100 Parma, Italy.
3 Current address: Department of Neurobiology, The Babraham Institute, Babraham, Cambridge, CB2 4AT UK.
Send reprint requests to: Luigia Trabace, Ph.D., Department of Pharmacology and Human Physiology, Medical School, University of Bari, Policlinico Piazza Giulio Cesare 11, 701 24 Bari, Italy. E-mail: trabace{at}farmacol.uniba.it
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Abbreviations |
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AD, Alzheimer's disease;
AChE, acetylcholinesterase;
AChEI, AChE inhibitor;
ACh, acetylcholine;
NE, norepinephrine;
DA, dopamine;
DOPAC, 3,4-dihydroxyphenilacetic acid;
HVA, homovanillic acid;
5-HT, 5-hydroxytryptamine;
5-HIAA, 5-hydroxyindolacetic acid;
GABA, -aminobutyric acid;
FOB, functional
observational battery.
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Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
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-aminobutyric acid-mediated.
J Pharmacol Exp Ther
236:
230-2362-Adrenoceptor antagonists potentiate acetylcholinesterase inhibitor effects on passive avoidance learning in the rat.
Psychopharmacology
124:
347-354[Medline].This article has been cited by other articles:
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), 1.5 (
), and 4.5 (
)
mg/kg CHF2819 and saline (
) administration on extracellular levels
of ACh in microdialysis samples from hippocampus of conscious, freely
moving young adult rats. CHF2819 was administered at time 0 ( 
).
Data are mean ± S.E. (n = 6 rats).
*P < .05 and #P < .01 versus saline (Tukey's test).
