Institut de Recherches Servier, Centre de Recherches de Croissy,
Psychopharmacology Department, Paris, France
The benzofurane (+)-S 14297, the benzamide nafadotride, the aminoindane
U 99194 and the arylpiperazine GR 103,691 have been proposed as
"selective" antagonists at dopamine D3 vs.
D2 receptors. Herein, we compared their in vitro
affinities and in vivo actions to those of the aminotetralin
D3 antagonists (+)-AJ 76 and (+)-UH 232. Affinities at
recombinant, human (h)D3 and/or hD2 sites were determined by employing the mixed D2/D3
antagonist [125I]-iodosulpride and the preferential
D3 ligands [3H]-(+)-PD 128,907 and
[3H]-(+)-S 14297. [3H]-(+)-PD 128,907, [3H]-(+)-S 14297 and [125I]-iodosulpride
yielded an essentially identical pattern of displacement at
D3 sites, which suggests that they recognize the same
population of receptors. The rank order of potency
(Ki values in nM vs.
[3H]-(+)-PD 128,907) was GR 103,691 (0.4) 
nafadotride
(0.5) > haloperidol (2) (+)-UH 232 (3) (+)-S 14297 (5) > (+)-AJ 76 (26) > U 99194 (160). The rank order of preference
(Ki ratio, D2:D3) for
D3 receptors (labeled by [3H]-PD 128,907)
vs. D2 sites (labeled by
[125I]-iodosulpride) was (+)-S 14297 (61) GR 103,691 (60) > U 99194 (14) > nafadotride (9) (+)-UH 232 (8) (+)-AJ
76 (6) > haloperidol (0.2). (+)-S 14297 and GR 103,691 also showed
greater than 100-fold selectivity at dopamine hD3
vs. hD4 and hD1 sites. However, GR 103,691 showed marked affinity for serotonin1A receptors
(5.8 nM) and alpha-1 adrenoceptors (12.6 nM). In
vivo, all antagonists except GR 103,691 prevented the induction of
hypothermia by (+)-PD 128,907 (0.63 mg/kg s.c.) and a further
preferential D3 agonist, (+)-7-OH-DPAT (0.16 mg/kg s.c.).
On the other hand, haloperidol, (+)-AJ 76, (+)-UH 232 and nafadotride
all induced catalepsy in rats, whereas (+)-S 14297, U 99194 and GR
103,691 were inactive. Haloperidol, (+)-AJ 76, (+)-UH 232, nafadotride
and (weakly) U 99194 also enhanced prolactin secretion and striatal
dopamine synthesis, whereas (+)-S 14297 and GR 103,691 were inactive.
However, despite its high affinity at 5-HT1A receptors and
alpha-1 adrenoceptors, both of which are present on
raphe-localized serotonergic neurons, GR 103,691 (0.5 mg/kg i.v.)
failed to influence their basal firing rate or the inhibition of their
electrical activity by the 5-HT1A agonist (±)-8-OH-DPAT
(0.005 mg/kg i.v.), a result that casts doubt on its activity in
vivo. In conclusion, both (+)-S 14297 and GR 103,691 are markedly
selective ligands that permit the characterization of actions at
hD3 vs. hD2 receptors in
vitro, but (+)-S 14297 appears to be of greater utility for the
evaluation of their functional significance in vivo.
Nevertheless, to develop a better understanding of the respective roles
of dopamine D3 and D2 receptors, we need
additional, chemically diverse antagonists of improved potency and
selectivity.
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Introduction |
DA
is implicated in the modulation of several physiological functions,
including endocrine secretion, motor behavior, thermoregulation and
mood (Creese and Fraser, 1987
). Its actions are expressed via at least five different receptor types. On the basis of
their molecular structure and pharmacological properties, these
receptors have been divided into two families: D1-like,
including D1 and D5 receptors, and
D2-like, including D2, D3 and
D4 receptors (Sokoloff and Schwartz, 1995; Strange, 1993).
As concerns the D2 receptor family, the low level of
expression of mRNA encoding D4 receptors in rodent and
human tissue, and the hitherto lack of selective radioligands for
D4 sites, have complicated the elucidation of their
functional significance, although selective D4 antagonists are now becoming available (Boyfield et al., 1996; Bristow
et al., 1997; Kulagowski et al., 1996; Merchant
et al., 1996; Millan et al., 1996). In contrast,
both in situ hybridization and polymerase chain reaction
amplification studies have allowed for the localization of mRNA
encoding D3 receptors in rodent and human brain, and the use of antibodies directed against D3 receptors has
permitted localization of the corresponding protein (Bouthenet et
al., 1991; Landwehrmeyer et al., 1993; Lévesque
et al., 1992). These approaches, together with studies of
the preferential D3 agonists [3H]-(+)-PD
128,907 and [3H]-(+)-7-OH-DPAT (Hall et al.,
1996; Herroelen et al., 1994), suggest that D3
sites are predominantly localized in limbic regions such as the
olfactory tubercles, the nucleus accumbens and the islands of Calleja.
This restricted D3 receptor distribution contrasts with the
broad distribution of D2 receptors (Gehlert et
al., 1992; Larson and Ariano, 1995; Levant et al.,
1993; Murray et al., 1994; Richtand et al.,
1995). In addition, a minor population of D3 autoreceptors
may exist with D2 autoreceptors on dopaminergic cell bodies
of the ventral tegmental area and substantia nigra, pars compacta (Diaz
et al., 1995; Gobert et al., 1995; Koeltzow et al., 1998; Meador-Woodruff et al., 1996).
Despite the utility of gene knockout and antisense strategies (Accili
et al., 1996; Baik et al., 1995; Carta et
al., 1996, Tepper et al., 1997), ligands that interact
selectively with D3 vs. D2 receptors
are essential for an improved knowledge of their localization,
modulation and functional significance. In the absence of appropriate
tissue preparations, the characterization of novel ligands has
generally been performed by using mammalian cell lines transfected with
human or rodent D2 or D3 receptor subtypes and radioligands such as [125I]-iodosulpride or
[3H]-spiperone that do not differentiate these sites
(Chio et al., 1993; Millan et al., 1995; Sokoloff
et al., 1992; Tang et al., 1994). On the basis of
such studies, the aminotetralins (+)-AJ 76 and (+)-UH 232 were found to
display a modest (about 2-5-fold) preference for D3 over
D2 sites (Lévesque, 1996; Sokoloff et al.,
1992; Van Vliet et al., 1996). Subsequently, several
antagonists with improved selectivity at D3 vs.
D2 sites have been identified: the aminoindane U 99194 (Waters et al., 1993), the benzofurane (±)-S 11566 and its
active (+)-isomer (+)-S 14297 (Gobert et al., 1995, 1996;
Millan et al., 1994; 1995; Morris et al., 1997),
the arylpiperazine GR 103,691 (Murray et al., 1995) and the
benzamide derivative nafadotride (Sautel et al., 1996). Of
these, (+)-S 14297 has been extensively employed in the functional
evaluation of the potential significance of D3 receptors
in vivo. It has been shown that (+)-S 14297 inhibits the
hypothermia induced by dopaminergic agonists such as (+)-7-OH-DPAT and
quinpirole in rodents, which suggests an involvement of D3
receptors in the control of CT (Millan et al., 1994; 1995;
Rivet et al., 1996). At comparable doses, (+)-S 14297 neither modifies PRL secretion nor induces catalepsy in rats, two
responses reflecting blockade of D2 receptors (Brocco
et al., 1995; Millan et al., 1995; 1997). Interestingly, (+)-S 14297 does not modify the synthesis or release of
DA in cerebral tissues, and it fails to modify the activity of ventral
tegmental area-localized dopaminergic neurons (Gobert et
al., 1995; Lejeune and Millan, 1995; Millan et al.,
1995; Rivet et al., 1994; 1996). These observations suggest
that D2 rather than D3 autoreceptors tonically
inhibit the activity of central dopaminergic neurons. Nevertheless,
(+)-S 14297 attenuates the inhibitory influence of (+)-7-OH-DPAT and
(+)-PD 128,907 upon DA release and synthesis, which suggests that
D3 (auto)receptors may contribute to the "phasic"
inhibition of dopaminergic pathways (Gobert et al., 1995;
Lejeune and Millan, 1995; Rivet et al., 1994).
Evidently, there now exist several antagonists and agonists of
potential utility for the in vitro and in vivo
functional characterization of actions mediated by D3
receptors. However, there has not yet been any comparative evaluation
of the properties of these ligands. Thus, using the radioligands
[3H]-(+)-S 14297 and [3H]-(+)-PD 128,907, both of which have recently been radiolabeled (Akunne et
al., 1995; Newman-Tancredi et al., 1995), as well as the mixed D2/D3 antagonist
[125I]-iodosulpride, the present study undertook a
comparative evaluation of the binding profiles of (+)-S 14297, nafadotride, U 99194, GR 103,691, (+)-AJ 76, (+)-UH 232 and haloperidol
at recombinant hD2 and hD3 receptors. In
addition, we examined their in vivo actions in models of
putative activity at D3 receptors (hypothermia) and
D2 receptors (catalepsy, PRL secretion and DA synthesis). These analyses allowed for the classification of drugs in terms of 1)
their rank order of potency at hD3 receptors and 2) their rank order of selectivity for hD3 vs.
hD2 receptors. In addition, a direct comparison of drug
doses in putative models of D3 as compared with
D2 receptor-mediated activity was possible.
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Material and Methods |
Binding at cloned, human D2 and D3
receptors.
Binding studies were carried out at recombinant
hD2 receptors (Receptor Biology, Beltsville, MA) and
hD3 receptors (J.-C. Schwartz, INSERM, Paris, France)
expressed in CHO cell lines as described previously (Millan et
al., 1995). Briefly, affinities at hD2 and
hD3 receptors were determined using
[125I]-iodosulpride (0.1 and 0.2 nM for D2
and D3, respectively), [3H]-(+)-S 14297 (7 nM
for D3) and [3H]-(+)-PD 128,907 (2 nM for
D3). Nonspecific binding was defined using 10 µM
raclopride. Binding conditions for [125I]-iodosulpride
and [3H]-(+)-S 14297 were as previously described
(Newman-Tancredi et al., 1995; Sokoloff et al.,
1992), and they were the same for [3H]-(+)-PD 128,907 except that incubations were carried out for 90 min.
Binding at other sites.
Binding conditions at other receptor
sites were as described in Millan et al. (1995). For each
receptor, the tissue, radioligand and ligands used to define
nonspecific binding were as follows: hD4 receptors
(4-repeat variant) expressed in CHO cells; [3H]-spiperone
(0.2 nM); haloperidol 10 µM; rat striatal D2 receptors; [3H]-spiperone (0.1 nM), raclopride 10 µM; rat
hippocampal 5-HT1A receptors and cloned, human serotonin
(h5-HT1A) receptors expressed in CHO cells;
[3H]-(±)-8-OH-DPAT (0.4 nM); 5-HT 10 µM; cloned, human
muscarinic (hM1) receptors expressed in CHO cells;
[3H]-N-methylscopolamine (0.5 nM); atropine 10 µM; rat
frontal cortex alpha-1 adrenoceptors;
[3H]-prazosin (0.2 nM); phentolamine 10 µM.
Influence on CT.
For evaluation of the influence of drugs
alone on CT, basal CT was determined, drug or vehicle was administered,
and CT was determined again 30 min later. This time corresponds to that
at which (+)-PD 128,9078 and (+)-7-OH-DPAT exert their maximal
influence on CT (Salmi et al., 1993; Dekeyne, A.,
unpublished observation). The difference between basal and postdrug
values was calculated. For antagonist studies, the procedure was as
follows. Basal CT was measured, drug or vehicle was administered and
(+)-7-OH-DPAT, (+)-PD 128,907 or vehicle was administered 30 min later.
A further 30 min later, CT was reevaluated and the difference from
basal values calculated. The percent of drug inhibition of the actions of (+)-7-OH-DPAT and (+)-PD 128,907 was computed as
1-[(antagonist + agonist) 
vehicle alone)/(vehicle + agonist) vehicle alone)] × 100. Drug potency was expressed as
ID50 95% CL.
Evaluation of catalepsy.
Catalepsy was determined in rats
using a previously described procedure (Waldmeier and Delini-Stula,
1979). The animals were placed in a position whereby the left and right
hind paws were crossed over the ipsilateral front paws; the time during
which this position was maintained was determined up to a maximum of 30 sec. The mean value of three consecutive tests, separated by intervals
of 1 min, was determined. Cataleptogenic potency was expressed in terms
of AD50 (95% CL)
that is, the dose required for the
induction of a half-maximal response (equivalent to 15 sec).
Evaluation of PRL secretion.
As described previously (Gobert
et al., 1995), we measured PRL 30 min after drug
administration in plasma by radioimmunoassay, using a highly specific
(<0.5% cross-reactivity to all other hormones examined) antibody
against rat PRL (Amersham, Buckingham, England). The detection limit
was 70 pg/tube, and the intravariation and interassay variation were
5% and 15%, respectively. Because there is no theoretical limit to
PRL levels in plasma, the MED was defined as the lowest dose
significantly different (P < .05) from vehicle control values in
Dunnett's test after ANOVA.
Evaluation of DA turnover.
The method we used was described
previously (Gobert et al., 1995). The effect of drugs alone
was determined 30 min after their s.c. injection. The striatum, nucleus
accumbens, olfactory tubercle and frontal cortex were examined (the
inclusion of a portion of cingulate cortex in "frontal" cortex
should be noted).
Tissues were homogenized in 500 µl of 0.1 M HClO4
containing 0.5% Na2S2O5 and 0.5%
EDTA Na2 and centrifuged at 15,000 × g for
15 min at 4°C. Supernatants were diluted in the mobile phase and
injected into a HPLC column (Hypersil ODS 5 µm, C18, 150 × 4.6 mm (Thermo Quest, Les Ulis, France) maintained at 25°C). The mobile
phase of the HPLC was KH2PO4, 100 mM; EDTA
Na2, 0.1 mM; sodium octylsulphonate, 0.5 mM; methanol 5%
adjusted to pH 3.15 with PO4H3. The flow rate
was 1 ml/min. Electrochemical detection was performed using a Waters
M460 detector with a working potential of 850 mV against an Ag/AgCl
reference. Quantitative determinations were made by comparison with
appropriate external standards. Levels of DA and DOPAC were expressed
as a function of the tissue content of protein, with bovine serum
albumin (Sigma Chemical Co., St. Louis, MO) as the standard. As an
index of turnover, the ratio of DOPAC:DA was calculated. For each
experiment, the mean levels of DA and DOPAC and the DOPAC:DA ratios
were determined. They were expressed relative to values in animals
treated with vehicle (defined as 100%). The influence of drugs was
expressed as a percentage thereof. Drug potency was expressed as
AD50 (95% CL)that is, an increase in DOPAC:DA ratios to
150% relative to vehicle values.
Electrical activity of serotonergic neurons in the DRN.
As
described in detail previously (Lejeune et al., 1994), rats
were anesthetized with chloral hydrate (500 mg/kg s.c.). The femoral
vein was cannulated and the rat placed in a stereotaxic apparatus. A
tungsten electrode was lowered into the DRN, and the firing activity
was measured by means of a Spike 2 analysis system obtained from
Cambridge Electronic Design (Cambridge, U.K.). Drug effects were
quantified over 60-sec bins at their time of maximal effect (1-2 min)
after their injection i.v. Administered alone, GR 103,691 was injected
in cumulative doses every 2 min. It was also injected at a single dose
2 min after administration of the 5-HT1A receptor agonist
(±)-8-OH-DPAT (0.005 mg/kg i.v.). Firing rates were expressed as a
percentage of basal, preinjection values (defined as 100%). The mean,
basal firing rate was 1.1 Hz.
Data analysis and statistics.
All binding data were analysed
with nonlinear regression ("Prism," GraphPad, San Diego, CA).
Ki values were calculated according to the
Cheng-Prussof equation, Ki = IC50/(1 + L/Kd), where
IC50 is the concentration of compound that gives 50%
inhibition of radioligand binding, L is the concentration of
radioligand and Kd is the dissociation constant
of the radioligand. In vivo dose-response curves were
initially analyzed by ANOVA followed by Dunnett's test, for which the
level of significance was set at P < .05. As indicated above,
MEDs, ID50 values, AD50 values or
AD150 values were determined to estimate drug potencies.
MOEs of drugs were also calculated.
Drugs and chemicals.
[125I]-Iodosulpride (2000 Ci/mmol) and [3H]-(+)-PD 128,907 (90-130 Ci/mmol) were
purchased from Amersham, and [3H]-(+)-S 14297 (145 Ci/mmol) was radiolabeled by C.E.A (Gif-sur-Yvette, France). For
in vitro binding studies, drugs were dissolved in water or
in dimethylsulfoxide. For in vivo studies, drugs were dissolved in sterile water, plus a few drops of lactic acid if necessary, and pH was adjusted to as close to neutrality (>5.0) as
possible. Drugs were injected s.c., and doses are expressed in terms of
the base. Drug sources, salts and structures were as follows: (+)-AJ 76 and (+)-UH 232 (Tocris Cookson, Southampton, England); (+)-7-OH-DPAT
HCl (J. Besselièvre, CNRS, Paris, France); (+)-PD 128,907 HCl and
(±)-8-OH-DPAT HBr (Research Biochemicals, Inc., Natick, MA) and
haloperidol base (Sigma, Chesnes, France). (±)-S 11566 HCl, (+)-S
14297 dibenzoyltartrate, ()-S 17777 dibenzoyltartrate, U 99194 HCl,
GR 103,691 and nafadotride were synthesized by Servier chemists (J.-L.
Peglion and G. Lavielle).
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Results |
In vitro ligand binding at hD3 and
hD2 receptors.
In an initial series of experiments, we
investigated the binding characteristics of [3H]-(+)-PD
128,907 to hD3 receptors. [3H]-(+)-PD 128,907 associated rapidly and monophasically with a t1/2 of
21 ± 3 min. Dissociation of [3H]-(+)-PD 128,907 from hD3 receptors was biphasic with a t1/2 value for the first component of the isotherm of 58 ± 8 min
(k
1 = 0.013 ± 0.002 min1).
The second component of the isotherm dissociated slowly, with 27% ± 1% of binding still remaining after 6 hr of incubation. An estimate of
the Kd derived from the association and
dissociation (rapid component) constants yielded a value of 0.6 nM. In
saturation binding experiments, [3H]-(+)-PD 128,907 yielded a Kd value at hD3 receptors
of 1.61 ± 0.31 nM. The Bmax value
(6.06 ± 0.59 pmol/mg) was similar to that determined with
[125I]-iodosulpride in the same membrane preparation (not
shown). Antagonist competition binding isotherms at hD3
receptors were derived for the preferential D3 receptor
agonist [3H]-(+)-PD 128,907, the D3
antagonist [3H]-(+)-S 14297 and the
D2/D3 antagonist
[125I]-iodosulpride (fig.
1). Ki values at
hD3 receptors were similar regardless of the radioligand
used (table 1). The rank order of
antagonist potency against [3H]-(+)-PD 128,907 binding at
hD3 sites was GR 103,691 > nafadotride > haloperidol > (+)-UH 232 > (+)-S 14297 > (±)-S
11566 > (+)-AJ 76 > U 99194 > ()-S 17777. The
agonists (+)-7-OH-DPAT and (+)-PD 128,907 yielded biphasic isotherms at
hD2 receptors (table 1, legend). The selectivity ratios
(Ki, hD2/Ki,
hD3) for the three radioligands are shown in table 1.
(±)-S 11566, its isomer (+)-S 14297 and GR 103,691 exhibited the
highest selectivity for hD3 receptors. Affinities at
hD3 receptors correlated positively between radioligands
with coefficients (r values) of +0.98 to +0.99. The affinity
of the antagonists at other key receptor subtypes was determined.
Ki values are shown for hD4,
h5-HT1A and hM1 receptors and for rat
alpha-1 adrenoceptors (table
2). (+)-AJ 76 was only 8-fold more
selective for hD3 than for hD4 receptors, and
GR 103,691 was only 11-fold more selective for hD3 than for
h5-HT1A receptors. (+)-S 14297 exhibited modest affinity at
hM1 receptors, for which its affinity was 30-fold less than
at hD3 receptors labeled by [3H]-PD 128,907 (Millan et al., 1995).
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Fig. 1.
Competition binding of dopaminergic antagonists at
cloned, hD3 and hD2 receptors expressed in CHO
cells. [3H]-(+)-PD 128,907, hD3 (panel A),
[3H]-(+)-S 14297, hD3 (panel B) and
[125I]-iodosulpride, hD3 (panel C).
Competition binding experiments at hD2 receptors were
carried out against [125I]-iodosulpride (panel D). Points
shown are means of triplicate determinations from a single,
representative experiment performed at least three times.
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TABLE 1
Affinities of dopaminergic antagonists at hD3, hD2 and
rat D2 receptors determined by competition with different
radioligands
Ki values (nM) are expressed as mean ± S.E.M.
of at least three determinations in triplicate. D2:D3
Ki ratios are shown for the different radioligands
(PD = [3H]-(+)-PD 128,907; S 14297 = [3H]-(+)-S 14297 and Iodosulp = [125I]-iodosulpride). Irrespective of radioligand used,
binding isotherms at hD3 receptors were all best fitted by
one-site analysis (Hill numbers not significantly different from
unity). At hD2 receptors, the agonists (+)-7-OH-DPAT and (+)-PD
128,907 yielded biphasic competition isotherms. nH values,
KH (% sites), KL as follows:
(+)-7-OH-DPAT: 0.73 ± 0.07, 19.7 ± 7 nM (47.7 ± 7%),
159 ± 37 nM. (+)-PD 128,907: 0.58 ± 0.01, 20 ± 5 nM
(28 ± 3%), 895 ± 108 nM.
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TABLE 2
Binding affinities (Ki values) of dopaminergic
ligands at key receptors
Ki values at D3 receptors are those obtained
with [3H]-(+)-PD 128,907. Values are the means of 2 to 3 determinations, each performed in triplicate.
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Electrical activity of DRN-localized serotonergic neurons.
Administered at a dose of 5 µg/kg i.v., (±)-8-OH-DPAT completely
abolished the firing rate of DRN serotonergic neurons (100.0 ± 0.0% relative to vehicle values, defined as 0%). Further, the alpha-1 adrenoceptor antagonist prazosin (150 µg/kg i.v.)
reduced firing levels to 77.9 ± 6.4% of vehicle values. Both
effects were significant in Student's two-tailed t test
(P < .05). By contrast, administered in incremental doses up to
500 µg/kg i.v., GR 103,691 failed (±0.0 ± 5.5%) to modify the
firing rate of these neurons. Similarly, at a dose of 250 µg/kg i.v.,
GR 103,691 did not modify the influence of 8-OH-DPAT on DRN firing
(100.0 ± 0.0%).
Blockade of (+)-PD 128,907- and (+)-7-OH-DPAT-induced
hypothermia.
Both (+)-PD 128,907 and (+)-7-OH-DPAT
dose-dependently elicited hypothermia (fig.
2). Their actions were prevented by
(±)-S 11566, as well as by its active eutomer (+)-S 14297, whereas the inactive distomer ()-S 17777 was ineffective (table
3; fig. 3).
(+)-AJ 76, (+)-UH 232, nafadotride and U 99194 also antagonized (+)-PD
128,907- and (+)-7-OH-DPAT-induced hypothermia, whereas GR 103,691 was
inactive (table 3; fig. 3). Haloperidol was active at low doses.
Antagonist potencies in blocking PD 128,907- and (+)-7-OH-DPAT-induced
hypothermia were highly correlated (r = 0.97, P < .01).
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Fig. 2.
Dose-dependent induction of hypothermia by the
preferential agonists at hD3 receptors, (+)-PD 128,907 and
(+)-7-OH-DPAT. The data represent the difference between basal and
post-treatment values and are means ± S.E.M. (n  5 per value). ANOVA results: (+)-PD 128,907, F(6,31) = 55.8, P < .01 and (+)-7-OH-DPAT, F(4,38) = 51.1, P < .01. * Significantly different from vehicle values in
Dunnett's test after ANOVA; P < .05.
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Fig. 3.
Dose-dependent blockade of (+)-PD 128,907-induced
hypothermia by dopaminergic antagonists. Antagonists were given 30 min
before (+)-PD 128,907 (0.63 mg/kg s.c.) (closed symbols) or vehicle
(open symbols). Data are means ± S.E.M. (n 4 per value). ANOVA results follow. Panel A: (±)-S 11566/vehicle,
F(3,25) = 4.4, P < .05; (±)-S 11506/(+)-PD 128,907, F(3,15) = 24.5, P < .001; (+)-S 14297/vehicle,
F(3,33) = 8.5, P < .001; (+)-S 14297/(+)-PD 128,907, F(3,15) = 12.4, P < .001; ()-S 17777/vehicle,
F(2,12) = 3.1, P > .05; ()-S 17777/(+)-PD 128,907, F(3,16) = 3.7, P < .05. Panel B: (+)-UH 232/vehicle,
F(3,10) = 0.3, P > .05; (+)-UH 232/(+)-PD 128,907, F(3,17) = 15.7, P < .01; (+)-AJ 76/vehicle,
F(3,30) = 4.0, P < .05; (+)-AJ 76/(+)-PD 128,907, F(3,14) = 12.5, P < .01; nafadotride/vehicle,
F(3,13) = 1.6, P > .05. Panel C: nafadotride/(+)-PD
128,907, F(4,18) = 19.4, P < .01; U 99,194/vehicle,
F(3,11) = 0.2, P > .05; U 99,194/(+)-PD 128,907, F(4,26) = 11.1, P < .01 and GR 103,691/(+)-PD 128,907, F(3,13) = 0.8, P > .05. * Significantly different
from vehicle/(+)-PD 128,907 values in Dunnett's test after ANOVA:
P < .05.
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Induction of catalepsy, PRL secretion and DA synthesis by
dopaminergic antagonists.
Haloperidol potently elicited catalepsy,
increased plasma PRL levels and elevated DA synthesis (tables
4 and 5;
fig. 4). (+)-AJ 76, (+)-UH 232 and
nafadotride likewise induced both PRL secretion and DA synthesis
(tables 4 and 5; fig. 4). U 99194 failed to elicit catalepsy and
increased PRL release and DA turnover only at very high doses (40.0 mg/kg). (+)-S 14297 and GR 103,691 were devoid of activity in each of
these models (tables 4 and 5; fig. 4).
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TABLE 4
Induction of catalepsy and PRL secretion by dopaminergic antagonists
Doses are in mg/kg s.c. The MOE is in seconds for catalepsy and in
nanograms per milliliter for PRL levels. N.C. = not computable.
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Fig. 4.
Dose-dependent induction by dopaminergic antagonists
of catalepsy (panel A), PRL secretion (panel B) and striatal DA
synthesis (panel C). Data are means ± S.E.M. (n 4 per value). ANOVA results follow. Catalepsy: (+)-AJ 76, F(4,26) = 4.8, P < .05; GR 103,691, F(3,18) = 0.6, P > .05; haloperidol, F(4,43) = 58.3, P < .05; nafadotride, F(3,26) = 11.8, P < .05; (+)-UH 232, F(3,19) = 11.7, P < .05; U 99194, F(2,8) = 0.8, P > .05 and (+)-S 14297, F(2,12) = 1.5, P > .05. Prolactin secretion: (+)-AJ 76, F(4,32) = 9.7, P < .05; GR 103,691, F(3,30) = 0.8, P > .05;
haloperidol, F(5,47) = 18.7, P < .05; nafadotride,
F(5,36) = 24.3, P < .05; (+)-UH 232, F(3,13) = 5.8, P < .05; U 99194, F(4,15) = 17.7, P < .05 and (+)-S 14297, F(4,28) = 0.5, P > .05. Striatal DA synthesis: GR 103,691, F(1,6) = 3.5, P > .05; nafadotride, F(4,19) = 90.5, P < .01;
(+)-UH 232, F(3,12) = 34.5, P < .01; U 99194, F(3,17) = 108.2, P < .01 and S 14297, F(3,31) = 0.7, P > .05. (+)-AJ 76 and haloperidol data
are from Gobert et al., (1995). * Significantly different
from vehicle values in Dunnett's test after ANOVA; * P < .05.
|
|
| |
Discussion |
Competition binding studies.
All antagonists displayed similar
affinities at hD3 receptors irrespective of the radioligand
used, though slightly higher affinities were generally observed with
[3H]-(+)-PD 128,907. This observation may reflect the
capacity of agonist radioligands to stabilize
hD3 receptors in a high-affinity conformation, an
interpretation consistent with its slow dissociation ("Results")
and implied by a ternary complex model of receptor coupling (Kenakin,
1996). In any case, a similar order of hD2/hD3 selectivity was observed regardless of the D3 radioligand.
With subnanomolar affinities, GR 103,691 and nafadotride were potent ligands at hD3 receptors (Murray et al., 1995;
Sautel et al., 1996). The hD2/hD3
selectivity ratio of nafadotride was, however, only modest, whereas GR
103,691 showed 60-fold selectivity. Because of a higher affinity at
D2 sites in our hands, this value is about 2-fold less than
that previously reported (table 1; Murray et al., 1995) but
is still pronounced. (±)-S 11566 and its active eutomer (+)-S 14297 also exhibited marked selectivity ratios at D3
vs. D2 sites, whereas a modest
hD2/hD3 selectivity ratio was obtained for the
less active distomer ()-S 17777, as well as for U 99194 (Millan
et al., 1994; 1995; Waters et al., 1993). Overall, the lowest D2/D3 ratios were observed
for (+)-AJ 76 and (+)-UH 232 and the highest for (+)-S 14297 and GR
103,691 (table 1). However, GR 103,691 displayed high affinity at
5-HT1A receptors and alpha-1 adrenoceptors
(table 2), in accordance with the findings of Murray et al.
(1994). (+)-S 14297 also showed modest (about 30 fold-lower) activity
at muscarinic hM1 receptors (Millan et al.,
1995). Nevertheless, among the ligands tested, (+)-S 14297 presents a
reasonable combination of marked hD3 affinity, pronounced hD3/hD2 selectivity and modest interactions at
other receptor sites. Indeed, (+)-S 14297 shows 100-fold lower
affinity at hD1 and hD5 receptors, multiple
serotonergic and adrenergic receptors and all other sites (>50) as yet
examined, with the exception of 
1 sites, for which it
shows modest affinity (196 nM) (Millan et al., 1995).
Induction and blockade of hypothermia.
In a recent study, the
comparative importance of D2 and D3 sites in
mediating hypothermia was addressed in detail (Millan et
al., 1994; 1995; Rivet et al., 1996). In a result
consistent with a putative role of D3 receptors, (+)-PD
128,907 elicited hypothermia herein (fig. 2). Notwithstanding its
superior affinity at D3 (and D2) receptors as
compared with (+)-7-OH-DPAT (table 1; Akunne et al., 1995;
Bristow et al., 1996), (+)-PD 128,907 was less
potent in decreasing CT. We have also noted an inferior potency of
(+)-PD 128,907 relative to (+)-7-OH-DPAT in a diversity of in
vivo models in which pre- and/or postsynaptic D3
and/or D2 receptors are implicated, including a reduction
of locomotion, inhibition of the firing rate of ventral tegmental
area-localized dopaminergic neurons and suppression of PRL secretion
(Brocco et al., 1995; Gobert et al., 1995;
Lejeune, F., unpublished observation). Collectively, these observations
suggest that (+)-PD 128,907 is a less potent ligand than
(+)-7-OH-DPAT in vivo, which probably reflects differential
absorption, metabolism or access to the CNS.
(±)-S11566 and (+)-S 14297, but not ()-S 17777, stereospecifically
block the induction of hypothermia by (+)-7-OH-DPAT (table 3; fig. 3)
(Millan et al., 1994; 1995). These data are extended herein
to antagonism of the hypothermic actions of (+)-PD 128,907. The
inability of GR 103,691 to block hypothermia, even at high doses, may
reflect its poor in vivo bioavailability (see below). By
contrast, the preferential D3 antagonists U 99194 and
nafadotride both antagonized hypothermia elicited by (+)-7-OH-DPAT and
(+)-PD 128,907 (table 3; fig. 3). The modestly preferential
D3 antagonists (+)-UH 232 and (+)-AJ 76 likewise blocked
the actions of (+)-7-OH-DPAT and (+)-PD 128,907, and, like all other
antagonists, they did not modify basal CT. The lack of influence of
(+)-UH 232 on basal CT is of note inasmuch as a recent study of
transfected NG 10815 cells, employing stimulation of mitogenesis as a
measure of coupling efficacy, suggested that (+)-UH 232 behaves as a
weak partial agonist at D3 receptors (Griffon et
al., 1995). However, it is difficult to compare efficacies at
heterologously expressed receptors in cell lines to those at native
receptors in situ. Further, the NG 10815/hD3
receptor expression system possesses a high receptor density and is
probably of greater sensitivity than the population of postsynaptic
D3 receptors thought to mediate hypothermia (Lajiness et al., 1993; Millan et al., 1995; Sautel
et al., 1995). Although the present data are consistent with
a role of D3 receptors in the induction of hypothermia, a
role of D2 sites should not be excluded, and the
availability of more selective D2 and D3
receptor antagonists, as well as studies in transgenic mice, will be
necessary for a further evaluation of the respective roles of
D3 and D2 receptors in controlling CT.
PRL secretion, DA synthesis and catalepsy: blockade of tonically
active D2 receptors.
Tuberoinfundibular dopaminergic
pathways exert a tonic, inhibitory control on the secretion of PRL
(Ben-Jonathan et al., 1989; McDonald et al.,
1984). Although multiple dopaminergic receptor types may indirectly
modulate PRL secretion via these tuberoinfundibular neurons
(Berry and Gudelsky, 1990), dopaminergic ligands modulate PRL secretion
primarily via actions at dopaminergic receptors on
lactotrophs in the adenohypophysis (McChesney et al., 1991). Neuroanatomical studies have indicated that these are of the
D2 type (Levant et al., 1993; Lévesque,
1996). Pharmacological support for a predominant role of D2
receptors has also been obtained. Thus the relative potencies of
dopaminergic agonists and antagonists in decreasing and increasing PRL
secretion, respectively, correlate with their affinity at
D2 (but not D3) sites (Millan et
al., 1995; Rivet et al., 1996). Indeed, compared with
haloperidol, (+)-S 14297 modified PRL secretion very little (fig. 4).
Further, U 99194, in line with its low D2 affinity, exerted
only a weak influence on PRL levels. A previous study has also reported
that (+)-AJ 76 weakly modifies PRL secretion in vivo
(Eriksson et al., 1986). Although GR 103,691 was also
inactive, this observation must be interpreted in the light of the
following comments about its poor activity in vivo. Indeed,
the affinity of GR 103,691 at hD2 receptors is virtually
identical to that of (+)-UH 232, which potently elicited PRL secretion.
There is anatomical (Bouthenet et al., 1991; Diaz
et al., 1995; Gehlert et al., 1992; Herroelen
et al., 1994; Larson et al., 1995; Lévesque
et al., 1992; Richtand et al., 1995;
Meador-Woodruff et al., 1996),
electrophysiological (Devoto et al., 1995; Lejeune and
Millan, 1995), behavioral (Sanger et al., 1996) and
biochemical (Gainetdinov et al., 1995; 1996; Gobert et
al., 1995; 1996; O'Hara et al., 1996; Rivet et
al., 1994; 1996; Tang et al., 1994) evidence that
D3 receptors contribute to the phasic,
inhibitory control of ascending dopaminergic pathways. However,
D3 (auto)receptors do not appear to inhibit
tonically the activity of dopaminergic neurons
(Koeltzow et al., 1998; Millan et al., 1995).
Rather, this role is fulfilled by colocalized D2
autoreceptors (Bowery et al., 1994; 1996; Meador-Woodruff
et al., 1996; Mercuri et al., 1997; Millan
et al., 1995; Momiyama et al., 1993; Piercey
et al., 1996; Seabrook et al., 1995).
Correspondingly, the facilitation of DA synthesis and release in
mesolimbic, mesocortical and nigrostriatal pathways reflects
inactivation of D2 receptors, and this parameter was not
significantly affected by (+)-S 14297. Thus the increase in DOPAC:DA
levels provoked by (+)-UH 232 and (+)-AJ 76 supports previous studies
performed with other procedures in suggesting that they accelerate DA
turnover by blockade of D2 autoreceptors (Waters et
al., 1994a). Furthermore, the induction of DA synthesis by
nafadotride extends a previous study of Sautel et al. (1995) in which, over a similar dose range, nafadotride increased levels of DA
metabolites in the striatum. The modest influence of U 99194 on DA
turnover is also consistent with its weak affinity at these sites
(Waters et al., 1993).
An enhancement in striatal DA turnover is generally correlated with the
induction of catalepsy, a behavior attributed to blockade of
postsynaptic dopaminergic receptors in the striatum and predictive of
an extrapyramidal syndrome in the human (Casey, 1993). Support for an
opposite control of motor behavior by D3 vs.
D2 receptors, and for a role of D2 receptors in
mediating catalepsy, may be derived from several lines of study. First,
knockout mice that lack D2 receptors display a
catalepsy-like state, whereas mice with a null mutation for
D3 receptors are hyperactive (Accili et al.,
1996; Baik et al., 1995). Second, the preferential
activation of postsynaptic D2 and of D3
receptors enhances and depresses locomotor behavior, respectively
(Bristow et al., 1996; Depoortere et al., 1996;
Khroyan et al., 1995; Kling-Petersen et al.,
1995; Sanger et al., 1996). Third, blockade of postsynaptic
D2 and D3 receptors respectively suppresses and
enhances (though more variably) locomotor activity (Millan et
al., 1997; Sautel et al., 1996; Svensson et
al., 1994; Waters et al., 1993; 1994b). Fourth,
D2 and D3 receptors exert an opposite control
of gene expression of neurotensin in the nucleus accumbens, a
neuropeptide that modulates locomotor behavior (Diaz et al.,
1994). Fifth, the potency of dopaminergic antagonists in eliciting
catalepsy correlates closely with affinity at D2 receptors
(Millan et al., 1997). Sixth, (+)-S 14297 inhibits the
induction of catalepsy by haloperidol (Brocco et al., 1995;
Millan et al., 1997). In analogy to the lack of cataleptogenic potential of (+)-S 14297, U 99194 failed to elicit catalepsy herein (fig. 4) and increases locomotor activity by an action
at postsynaptic D3 receptors (Waters et al.,
1994b). Similarly, low doses of nafadotride increase motor behavior
(Sautel et al., 1995), whereas higher doses elicit catalepsy
(Sautel et al., 1995) (fig. 4). The cataleptic actions of
nafadotride, (+)-UH 232 and (+)-AJ 76 at high doses evidently reflect
blockade of D2 receptors. In analogy to the other models of
activity at D2 receptors, GR 103,691 was inactive.
Mechanisms underlying induction of catalepsy, PRL secretion and DA
turnover.
The patterns of data obtained in the models of PRL
secretion, induction of cerebral DA turnover and catalepsy were broadly similar. In contrast to the potent actions of haloperidol, (+)-S 14297 was inactive and U 99194 displayed modest activity. Nafadotride, (+)-UH
232 and (+)-AJ 76, which manifest only a mild preference for
D3 receptors, displayed an intermediate pattern of
behavior. Thus these in vivo findings correspond to the
relative preference of these antagonists for D3
vs. D2 sites in vitro. Interestingly, differences among the antagonists were apparent not only as concerns their relative potencies but also as regards their maximal effects. Thus haloperidol consistently produced the most marked actions, (+)-S
14297 was inactive, U 99194 was weakly active and the other antagonists
provoked intermediate responses (tables 4 and 5; fig. 4). The question
arises why maximal effects should differ. If antagonist actions simply
reflected interruption of the activity of spontaneously released DA at
D2 receptors, they should, in theory, all elicit the same
maximal effect. There are several possible explanations. First, the
non-D2 (or D3) receptor interactions of drugs
may modify their respective maximal effects. Second, the dose ranges of
drugs employed may have been insufficient to occupy D2
receptors substantially. This may be the case for (+)-S 14297, but
dose-response curves for other drugs were pursued up to doses at which
D2 antagonist properties are clearly expressed (Brocco
et al., 1995; Brocco, M., unpublished observation). Third, a
functional interplay between postsynaptic D2 and
D1 sites is well established (Creese and Fraser, 1987), and
D2 and D3 receptors colocalized on individual
neurons may mutually oppose each other's activities (Surmeier et
al., 1992; Le Moine and Bloch, 1996). Indeed, as mentioned above,
the enhancement of motor behavior by D3 receptor blockade
counters the motor-suppressive effects of D2 receptor
antagonism (Millan et al., 1995; 1997). Thus, for the
ligands tested herein, a progressive reduction in cataleptogenic potential paralleled a progressive reinforcement of D3
vs. D2 antagonist preference. A fourth
possibility is that haloperidol behaves as an inverse agonist at
D2 receptors (Hall and Strange, 1997; Nilsson et
al., 1996). A differential degree of inverse agonist activity at
D2 sites could explain the contrasting maximal effects of
antagonists on PRL secretion, etc. (fig. 4). However, the concept of
inverse agonist actions cannot easily explain the occurrence of
catalepsy in D2 knockout mice (Baik et al.,
1995). Further, like haloperidol, clozapine is an inverse agonist at D2 receptors, but it does not evoke catalepsy (Hall and
Strange, 1997). Irrespective of the reasons underlying the difference
in maximal effects, the present data suggest that antagonists
possessing a marked preference for D3 versus D2
receptors may have a low extrapyramidal syndrome potential.
The inactivity of GR 103,691.
Pharmacokinetic factors also
contribute to differential drug effects, and GR 103,691 was inactive,
even at high doses relative to its in vitro affinities, in
each of the in vivo paradigms employed herein. It was
recently shown that, in contrast to haloperidol, GR 103,691 does not
influence cerebral c-fos expression (Hurley et al., 1996).
Indeed, the only in vivo effect documented to date for GR
103,691 is its ability to block the locomotion elicited by infusion of
muscimol into the ventral tegmental area (Murray et al.,
1995). In this model, GR 103,691 (0.3 mg/kg s.c.) was 6-fold less
potent than haloperidol (0.05 mg/kg s.c.) despite its 5-fold higher
affinity at D3 receptors, an observation in line with the
present data indicating a lower bioavailability than anticipated.
However, its low affinity at D3 receptors
(Ki = 200 nM) notwithstanding, clozapine (0.005 mg/kg s.c.) was more potent than GR 103,691 in blocking the actions of
muscimol. This observation suggests that activity in this model may
reflect the involvement of receptors other than, or in addition to,
D3 sites. Thus, to date, there are no unambiguous data for
functional actions of GR 103,691 at D3 (or D2)
sites in vivo. We have, moreover, found that high doses of
GR 103,691 (10 mg/kg s.c.) are inactive in several other behavioral
models of D2 receptor-mediated activity in rats, including
inhibition of amphetamine-induced locomotion and reduction of
conditioned avoidance responses (Brocco, M., unpublished observation)
models, whereas haloperidol is active, with ID50 values of
0.04 and 0.05 mg/kg s.c., respectively. In addition, haloperidol
abolishes inhibition of the firing of dopaminergic neurons in the
ventrotegmental area by (+)-PD 128,905 with an ID50 of
0.003 mg/kg i.v. In contrast, even at an 80-fold higher dose of 0.25 mg/kg i.v., GR 103,691 only partially (about 40%) inhibits the action
of (+)-PD 128,907 (Lejeune, F., unpublished observation). Herein, we
also examined this issue by exploiting the marked affinity of GR
103,691 for 5-HT1A receptors and alpha-1 adrenoceptors. Agonists at 5-HT1A sites and antagonists at
alpha-1 adrenoceptors both inhibit serotonergic neurons in
the DRN (Hjorth and Sharp, 1990; Lejeune et al., 1994).
However, GR 103,691, at doses up to 0.5 mg/kg i.v., neither modified
basal firing rates of serotonergic neurons nor attenuated the
inhibitory influence on these of the 5-HT1A agonist
(±)-8-OH-DPAT (see "Results"). These observations suggest that a
lack of in vivo activity is a general property of GR 103,691 irrespective of the receptor type concerned. This electrophysiological
study was performed by the i.v. route in order to minimize problems of
metabolism. Further, GR 103,691 does not modify PRL secretion even
though the relevant D2 receptors are localized outside the
blood-brain barrier. Thus it is not clear whether rapid metabolism,
poor CNS penetration and/or other factors underlie the low activity of GR 103,691 in vivo.
General discussion.
Of the ligands examined, (+)-S 14297 and
GR 103,691 appear the most appropriate ligands for the characterization
and differentiation of activity at D3 as compared with
D2 receptors in vitro. In this regard, GR
103,691 possesses an advantage in terms of its higher affinity and
overall selectivity for D3 vs. D2
sites. However, GR 103,691 displays the disadvantage of marked affinity
at both 5-HT1A receptors and alpha-1
adrenoceptors. Although these properties may not interfere with its use
in transfected cell lines, they compromise its utility in functional
studies of more complex systems. Furthermore, GR 103,691 appears to
possess little bioavailability in vivo. In this respect,
although its modest affinity at hM1 and 1
receptors must be mentioned (Millan et al., 1995), (+)-S 14297 appears to be a more suitable ligand for in vivo
studies. In fact, few ligands have been reported that possess a marked D3 vs. D2 preference comparable to
that of (+)-S 14297 and GR 103,691 in vitro. Moreover,
in vivo data are generally not available. Nevertheless, the
recently described, 2-substituted 2-aminotetralin GR 218,231 [2-(R,S)-(dipropylamino)-6-(4-methoxyphenylsulfonylmethyl)-1,2,3,4-tetrahydronaphtalene] possesses >100-fold selectivity for D3 vs.
D2 sites, and its functional actions in vivo
will be of interest to explore (Murray et al., 1996).
Moreover, a modestly preferential (10-20-fold) antagonist, L 741,626, at D2 receptors has been documented (Bowery et
al., 1996). As concerns the D2 receptor "family"
in general, several potent and selective D4 receptor
antagonists have now become available, including S 18126 ({2-[4-(2,3-dihydro benzo [1,4]dioxin-6-yl) piperazin-1-yl
methyl] indan-2-yl}) and L 745,870 (3-(4-[4-chlorophenyl]piperazin-1-yl)methyl-1H-pyrrolo[2,3b]pyridine). Notably, both S 18126 and L 745,870 were inactive in the functional models employed herein, which indicates a lack of involvement of
D4 receptors (Boyfield et al., 1996; Bristow
et al., 1997; Kulagowski et al., 1996; Millan
et al., 1996 and in press).
Conclusion.
In conclusion, the present data underpin the
hypothesis that the selective blockade of D3 receptors does
not provoke extrapyramidal side effects and fails to perturb
dopaminergic transmission. On the other hand, whether an antagonist
action at D3 receptors contributes to the therapeutic
efficacy of antipsychotic drugs remains to be determined (Levant, 1997;
Sokoloff and Schwartz, 1995). More generally, the potential
significance of D3 receptors in depression, drug abuse and
other psychiatric disorders requires further evaluation (Acri et
al., 1995; Caine and Koob, 1993; Roberts and Ranaldi, 1995;
Sokoloff and Schwartz, 1995; Spealman, 1996; Strange, 1993; Wallace
et al., 1996; Willner, 1983). To develop an improved
understanding of the physiological and therapeutic significance of
D3 (and D2) receptors, we need additional,
chemically diverse, potent and selective D3 and
D2 receptor antagonists.
We thank V. Pasteau, S. Aubry, C. Chaput, L. Verrièle, H. Gressier and S. Girardon for their excellent technical assistance.
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Abstract
Introduction
