Abstract
To investigate the roles of individual transmembrane segments (TM) of the human D3 dopamine receptor in its ligand-receptor interactions, we generated chimeric receptors in which its TMs were replaced, one at a time, partially or entirely, by the corresponding TM of the homologous human D1 receptor. Ligand binding properties of the chimeras, as expressed heterologously in Sf9 cells using recombinant baculoviruses, indicate that the critical binding regions for D3-selective (over D1) ligands reside at narrow regions (6 to 8 residues) near the extracellular surface for TMI, II, IV and VI, while TMV seems to be minimally involved in the ligand selectivity. For TMIII and TMVII, the critical regions seem to be deeper, involving at least the 10 residues near the extracellular surface for TMIII, and the entire TM segment for TMVII. This is based on our current observations that the chimeras with the D3 sequence in the critical regions, although the rest of the TM is of D1 origin (except TMVII), showed the binding properties indistinguishable from those of the wild-type receptor. The chimeras with the D1 sequence in the regions, on the other hand, showed ligand binding characteristics wildly variable depending on substituted TMs: Most marked decreases in ligand affinities were observed with the chimeras of TMIII and VII, and intermediate changes with those of TMIV and VI. Replacements of TMV produced no appreciable effects on the affinities of 14 test ligands (except for one). The chimeras of TMI and II with the D1sequence in the critical regions showed no appreciable specific binding for several radioactive D3-selective ligands, possibly reflecting their critical roles in assembly and folding of the receptor. These critical regions of the D3 receptor were highly homologous to those of the D2 receptor, except for several nonconservatively substituted residues, which could be exploited to develop ligands selective for the D3 over D2 dopamine receptor or vice versa.
Dopamine receptors are G protein-coupled receptors with seven transmembrane domains, and consist of five distinct subtypes (D1-D5) and their splicing variants, which are classified into the families of D1-like and D2-like receptors (Kebabian and Calne, 1979; Civelli et al., 1993;Gingrich and Caron, 1993; Seeman and Van Tol, 1994). Recently, the D2-like receptors, which include D2, D3 and D4 subtypes, have been the focus of many investigations because of the potential usefulness of their ligands for psychotic disorders and Parkinson’s disease (O’Dell et al., 1990; Sokoloff et al., 1990, 1992; Sokoloff and Schwarz, 1995). The D3 dopamine receptor, in particular, has received much attention as a potential target of antipsychotic drugs without extrapyramidal side effects, because of its highly localized distribution in limbic brain regions, in contrast to the D2 dopamine receptors, which are widely distributed in all dopamine projection fields (Sokoloff and Schwarz, 1995). Development of subtype-specific ligands is essential to test this hypothesis, and is critically dependent on the knowledge on ligand binding pockets of individual subtypes.
Ligand binding pockets for the dopamine receptors seem to be primarily contributed by TMs as shown by earlier studies with catecholamine receptors, analogous members of the superfamily of G protein coupled receptors (Frielle et al., 1988; Ostrowski et al., 1992; Strader et al., 1994). Although the sequences of TM segments among the dopamine receptor subtypes are considerably homologous, the ligand binding pockets of D2-like receptors are distinct from those of D1-like receptors (Civelli et al., 1993; Gingrich and Caron, 1993), judging from the existence of numerous ligands with higher affinity for the D2- over D1-like receptors (several orders of magnitude). This provides a unique opportunity to characterize binding pockets for D2-like dopamine receptors (D3 in particular) via a homolog-scanning mutagenesis (Cunningham et al., 1989). It is likely that D3/D1 chimeras, for instance, would maintain the receptors without gross disruptions of the wild-type conformation and nonspecific perturbations of the tertiary structures of the receptor (Cunningham et al., 1989). Characterization of such chimeras would enable us to understand contributions of individual TM segments to dopamine ligand binding pockets and would be useful for development of subtype-selective ligands. In this study, we generated a number of human D3 receptor chimeras in which its TM segments, ranging from 22 to 26 amino acid residues, were replaced, one at a time, partially or entirely, with the corresponding segments of human D1 receptor; we report ligand binding properties of the D3/D1 chimeras, as expressed in Sf9 cells using recombinant baculoviruses carrying the chimeric cDNAs.
Materials and Methods
Construction of chimeric receptors.
Initially, we constructed seven D3 chimeras, in which each transmembrane segment of the human D3 dopamine receptor from TMI to TMVII was replaced with the corresponding region of the D1 receptor by using the procedure of gene splicing by overlap extension (Horton et al., 1989). Briefly, a pair of linker primers were synthesized for each chimera. A sense primer contained its 3′ end sequence (about 20 nucleotides) complementary to the proximal part of a target TM of D1 receptor, and its other half (about 20 nucleotides long) complementary to the D3sequence adjoining its corresponding TM. A similar antisense primer was prepared covering the distal side of the target TM. We used another pair of outside primers that were selected to contain a unique restriction site at the 3′ and 5′ ends of the D3receptor cDNA, outside of the target TM. After the polymerase chain reaction procedures (Horton et al., 1989), we obtained a D3 cDNA fragment with a D1TM sequence in the middle and unique restriction sites at the 5′ and 3′ ends. The final polymerase chain reaction fragments were digested with proper restriction enzymes to yield sticky ends and then were cloned into the PCRscript vector containing the D3dopamine receptor cDNA with the complementary ends. All chimeras were confirmed initially with restriction digestion maps and subsequently with dideoxy sequencing. They are designated as D3/D1-TMI (31–52), D3/D1-TMII (66–94), D3/D1-TMIII (104–126), D3/D1-TMIV (151–172), D3/D1-TMV (188–209), D3/D1-TMVI (327–353) and D3/D1-TMVII (364–384), with the numbers in the parentheses denoting the range of replaced residues (D1) at the beginning and the end of the D3 TM regions, as noted earlier (Civelli et al., 1993). The numbering refers to the D3 dopamine receptor throughout this report. Two or three additional mutants from each chimera were generated in which a cluster of seven or 14 residues of the amino-terminal (TMX-1 or -2) or seven residues at carboxyl-terminal side (TMX-3) of a given TM was mutated back to the D3 sequence. These chimeras were generated in the same manner as described above, and their correct constructs were confirmed with dideoxy sequencing. Each D3 chimeric insert was transferred to PVL1394 (a shuttle vector for baculovirus), which was used to prepare the recombinant baculovirus, using a Baculo Gold kit (PharMingen, San Diego, CA) following the vender’s protocol. The recombinant baculovirus was plaque-purified, and the titer of final purified viral stocks ranged near 1 × 108 plaque-forming particles/ml. The culture of Sf9 cells (1 × 106 cells/ml) was infected with 5 × 106 viral particles/ml, and harvested 60 to 72 hr after infection. The membranes were prepared as described elsewhere (Pregenzer et al., 1993).
Binding measurements.
Binding of radioactive ligands was measured in membranes obtained from Sf9 cells expressing recombinant receptors, using filtration techniques as described elsewhere (Pregenzer et al., 1993). Briefly, [3H]spiperone binding was measured in the medium containing 150 mm NaCl, 2 mmMgCl2, 1 mm EDTA, 20 mmHEPES/Tris, pH 7.4, the radioactive ligand at varying concentrations (0.1 to 30 nm for typical binding profiles), and 5 to 100 μg of membrane protein depending on the receptor density of a given membranes, in a total volume of 500 μl at 4° for 60 min. In some experiments, the reaction volume was raised to 2500 μl to lower the ratio of bound/free ligand. The mixture was filtered over a Whatman GF/B filter (Whatman, Clifton, NJ) under vacuum. The filters were washed three times with 4 ml of an ice-cold 50 mmTris·HCl buffer, pH 7.4. Nonspecific binding was estimated in the presence of excess unlabeled spiperone (10 μm). All the stock solutions for ligands were prepared in 0.1% ascorbic acid. Displacement experiments of [3H]spiperone binding by test compounds (competition assay) were carried out in the same assay buffer with the radioactive ligand at 0.5 to 10 nm depending on the dissociation constant of chimeras. The binding data were analyzed using a nonlinear regression method (Sigma Plot), and presented with the mean and standard errors from three or more experiments.
Results
We examined each chimeric receptor in Sf9 cells with [3H]spiperone binding, a selective antagonist for D2-like receptors (D2, D3 and D4). The ratio of its specific to nonspecific binding at 2 nm was at least 4 or greater with the following chimeras: D3/D1-TMI-1(39–51), D3/D1-TMII-3(66–88), D3/D1-TMIII-2(123–126) and D3/D1-TMIII-3(104–114), D3/D1-TMIV-2(166–172), D3/D1-TMIV-3(151–164), D3/D1-TMV (188–209), D3/D1-TMVI (327–353), D3/D1-TMVI-2(347–353), D3/D1-TMVI-3(327–346), D3/D1-TMVII (364–384), D3/D1-TMVII-1(371–384) and D3/D1-TMVII-2(381–384). Again, the two numbers in the parenthesis denote the range of residues at the beginning and the end of a D3 TM region that was replaced with the D1counterparts. Scatchard analysis using the binding equation for a single class of binding sites fit well (linearity) with the binding data from the D3 dopamine receptor as well as those from the above chimeras (data not shown). The dissociation constant for [3H]spiperone ranged from 0.38 to 29 nm, and the maximal binding sites from 3 to 37 pmol/mg protein (Table 1).
For the cells infected with the wild-type baculovirus, the ratio of specific to nonspecific binding of [3H]spiperone was < 1. Similar low ratios were observed with the chimeras of D3/D1-TMI(31–51), D3/D1-TMI-3(31–41), D3/D1-TMII(66–94), D3/D1-TMII-1(75–94), D3/D1-TMII-2 (89–94), D3/D1-TMIII(104–126), and D3/D1-TMIV(151–172). Their ratios did not improve with other commercially available radioactive ligands such as [3H]dopamine, [3H]YM-09151–2 and [3H]raclopride. These chimeras were not examined further in this study.
With the chimeras showing high levels of specific [3H]spiperone binding, competition binding experiments were carried out with various ligands selective for the D3 receptor (representing the D2-like receptors) over the D1 receptor. The ligands represent several well known templates such as butyrophenones (spiperone and haloperidol), ergots (lisuride and cabergoline), aminotetralins (UH-232 and AJ-76), pyrrolidinyl-methyl benzamides (raclopride), and phenothiazines (chlorpromazine). Also included are several agonists such as quinpirole, pramipexole and apomorphine. It should be noted, however, that agonist affinities here represent their low affinity states (uncoupled receptors) because of extremely high density of the cloned receptors (0.3 to 37 pmol/mg protein). Table2 lists theKi values for the test ligands in the wild-type receptor (D3) and the chimeras, as obtained using Cheng-Prusoff equation (Cheng and Prusoff, 1973). We also found that all the chimeras we examined here interacted poorly with SCH23390, a D1-specific ligand (Kd of 0.37 nmfor D1), with theKi values of above 1000 nm as measured by its ability to inhibit [3H]spiperone binding.
TMI mutant.
The TMI sequence (Y31-C51) of the D3 receptor shows that twelve residues are divergent from the D1 receptor. The chimera TMI-1 (39–50) contains the five divergent D1 residues near the carboxyl-terminal side, but retains the D3 sequence at the amino-terminal side (near the extracellular surface). In the chimera, the dissociation constant (Kd ) for [3H]spiperone was 0.38 ± 0.03 nm, similar to that for the wild-type receptor (0.42 ± 0.1 nm), and theKi values for the other ligands were indistinguishable from those for the wild-type receptor (Fig.1). This indicates a minimal contribution of the five divergent residues near the carboxyl-terminal side of TMI (near the intracellular surface) to ligand selectivity. The chimeras with the D1 sequence at the amino-terminal side [TMI(31–52) or TMI-3 (31–41)], on the other hand, displayed no noticeable level of specific binding of [3H]spiperone, [3H]dopamine, [3H]raclopride, and [3H]YM-09151–2. This could imply that the amino-terminal side of TMI (near the extracellular surface) is important not only in ligand binding but also in assembly and folding of the receptor.
TMII mutant.
Twelve divergent residues are found in the TMII sequence (Y66-G94) of the D3 and D1 receptors. The only TMII chimera we were able to examine here was the TMII-3(66–88) with the D1 sequence at the amino-terminal side (including eight divergent residues) and the D3 sequence at the carboxyl-terminal side (89–94) near the extracellular surface. With this chimera, we obtained the aKd value for [3H]spiperone of 0.54 ± 0.04 nm, which is similar to that for the wild-type receptor (0.42 ± 0.1 nm) (Table 1). Also, all the test ligands displayedKi values nearly identical to those obtained with the wild-type receptor (Table 2; Fig. 1). This indicates that the eight divergent residues at the amino-terminal side of TMII, near the intracellular surface, may not be critical for ligand binding. The chimeras with the D1 sequence at the carboxyl-terminal side (near extracellular surface), on the other hand, showed no appreciable level of specific binding, as is the case for TMI. Point mutations in the region would be useful for further characterization of its functional roles.
TMIII mutants.
The TMIII sequence (D104-I126) of the D3 receptor shows nine residues divergent from the D1 receptor. The chimera TMIII-3(104–114) includes the D1 segment, with eight divergent residues that span the amino-terminal side of the TMIII near the extracellular surface. This mutation differentially affected the affinity of the test ligands (Table 2; Fig.2), ranging from 15-fold to more than 5000-fold affinity changes. Those with moderate affinity changes (a ≤ 40-fold increase in theirKi values) are spiperone, butaclamol, haloperidol, the ergots (lisuride and cabergoline). Those with noticeable affinity changes (100–500-fold increases inKi value, as noted in parentheses) are YM-09151–2 (97), chlorpromazine (155), AJ-76 (321), apomorphine (454), and UH-232 (575). Those with marked affinity changes include quinpirole (775), pramipexole (1366), and raclopride (5500).
The TMIII-2 chimera contains the D1 TM III sequence at the carboxyl-terminal side, including the two remaining divergent residues, and the D3 sequence at the amino-terminal side near the extracellular surface. This alteration had no appreciable effect on the affinity of all the tested compounds; their Ki values were nearly identical to those observed with the wild-type receptor (Table 2; Fig. 2).
TM IV mutants.
Comparison of the TMIV sequence of the D3 (A151-F172) and D1receptor reveals 18 divergent residues. The chimera TMIV-3 (151–165), containing the D1 sequence at the amino-terminal side (near the intracellular surface) with 11 divergent residues, showed ligand Ki values ≅ or < 6-fold changes compared with those for the wild-type receptor (Table2; Fig. 2). This indicates marginal contributions to ligand binding by the amino-terminal region (A151 to S165), which includes the 11 divergent residues.
The chimera TMIV-2 (166–172) contains the D1sequence at the carboxyl-terminal side (near the extracellular surface) with seven divergent residues. This mutation differentially affected the affinity of the test ligands (Fig. 2). The compounds with minimal affinity changes (≤ 4-fold) were the aminotetralins (UH-232 and AJ-76), YM-09151–2, apomorphine, (−)3-PPP, and the ergots (lisuride and cabergoline). Those with noticeable increases in theirKi (15- to 100-fold) are spiperone (15), butaclamol (17), chlorpromazine (30), and raclopride (38), haloperidol (58), pramipexole (74) and quinpirole (85). Apparently, the seven divergent residues at the carboxyl-terminal side (near the extracellular surface) of TM IV seem to play considerable roles in ligand binding for the D3 receptor.
TM V mutant.
Despite 13 divergent residues between the TMV of D1 and D3 receptors (F188-A209), the chimera TMV(188–209), containing the D1 TM V segment in its entirety, had no appreciable effect on the affinity of most test ligands, except for raclopride, which showed a 240-fold increase in itsKi (Fig.3). Because of this lack of general effects on ligand affinity by TMV, here we did not study TMV further.
TM VI mutant.
The TM VI sequence (A327-T353) of the D3 receptor shows 19 residues divergent from the D1 receptor. The chimera TMVI(327–353), containing the D1 TM VI segment in its entirety, altered affinities of only few ligands. Quinpirole and pramipexole showed a 235- and 45-fold decrease in their affinity to the chimera, respectively, whereas the other ligands showed no noticeable affinity changes compared with those observed with the wild-type receptor (Table2; Fig. 3). The chimera TMVI-2 (347–353) contains the seven divergent D1 residues at the carboxyl-terminal side (near the extracellular surface) and displayed ligand affinity changes nearly identical to those observed with the chimera TMVI, with theKi values of quinpirole and pramipexole 323 and 93 times greater, respectively, than the wild-type receptor, but no appreciable affinity changes with the rest of test ligands (Table 2; Fig. 3). On the other hand, the chimera TMVI-3 (327–346), which contains the D3 sequence at the carboxyl-terminal side and the D1 sequence at the amino-terminal side (near the intracellular surface) including 12 divergent residues, displayed ligand-binding characteristics nearly identical to those of the wild-type receptor, including its affinities for quinpirole and pramipexole (Table 2). Thus, the key molecular determinant for quinpirole and pramipexole seems to reside at the carboxyl-terminal side (near the extracellular surface) of TMVI.
TM VII mutants.
Twelve divergent residues are found in the TM VII sequence (L364-T384) when comparing the D3and D1 receptors. Three TM VII chimeras were examined in this study: TMVII(364–384), TMVII-1(371–384), and TMVII-2(381–384). The chimera TMVII(364–384), containing the D1 sequence in its entirety, bound most test ligands with noticeably low affinity, although this affinity varied from ligand to ligand (Fig. 2). Only the ergots (lisuride and cabergoline) showed no appreciable change in their affinities, displaying only 2- to 3-fold increases in theirKi values compared with those obtained with the wild-type receptor. The ligands with moderate affinity decreases (40- to 150-fold) include butaclamol (45), chlorpromazine (40), UH-232 (56), spiperone (60), YM-09151–2 (97), and haloperidol (144). The ligands of markedly low affinity (over 200-fold) included apomorphine (239), AJ-76 (318), quinpirole (3071), raclopride (4291), and pramipexole (5375). Moreover, (−)3-PPP even at 50 μm showed no detectable inhibition of [3H]spiperone binding (in Fig. 2, we indicated a 600-fold change in affinity for comparison’s sake).
In the chimera TMVII-1(371–384), where the six divergent residues at the amino-terminal side (near the extracellular surface) were reverted to the D3 residues, the binding affinities of several ligands improved compared with those observed with the chimera TMVII (Table 2). The most pronounced improvement was noted with AJ-76, a 200-fold decrease in its Ki , nearly approaching its wild-type value, followed by haloperidol and pramipexole with about 20 to 30-fold affinity increases. Only marginal improvements (ranging from 2- to 5-fold changes) were seen with the rest of the test compounds. In the chimera TMVII-2(381–384), where the D3 sequence extended almost all the way to the carboxyl-terminal side except for two divergent residues (381 and 384), most ligands displayed binding affinity comparable with those observed with the wild-type receptor, including spiperone, butaclamol, chlorpromazine, YM 09151–2, UH-232, raclopride and (−)3-PPP (Fig. 2). Interestingly, however, the affinities of quinpirole, apomorphine, and pramipexole were still 45-, 28-, and 21-fold lower, respectively, compared with their wild-type values. This suggests that the remaining two divergent residues, V381 and T384, at the extreme carboxyl-terminal side of TMVII, may contribute to interactions of these ligands with the receptor.
Discussion
We found no systematic studies on D3/D1 chimeras in the literature, but few analogous ones such as the D1chimera with the D2 carboxyl-terminal region, TMVII and TMVI (MacKenzie et al., 1993; Kozell et al., 1994). This chimera retained binding affinity to [3H]SCH23390, a selective ligand for the D1 receptor, and at the same time improved affinity toward quinpirole, a selective agonist for D2-like receptors. This suggests the importance of the region of TM VI and TM VII for quinpirole binding but provided little information about contributions by individual TM segments to ligand binding pockets. In this study, with a number of ligands selective for the D3 over the D1 dopamine receptor, we characterized the binding properties of various D3 chimeric receptors in which its individual TM segments were replaced one at a time, partially or entirely, with the corresponding D1 TM sequence. Our results showed that relative changes in ligand affinity were widely variable from chimera to chimera, depending on substituted TM segments. The chimeras with the D1 TMIII (TM III-3 in particular) or TMVII segment showed marked affinity changes for a broad spectrum of ligands, with a maximal affinity decrease of nearly 5000-fold (e.g., raclopride and pramipexole). The replacement of TMIV with the corresponding D1 sequence near the extracellular surface (TM IV-2) produced rather moderate affinity alterations for most ligands, with a maximal affinity decrease up to 80-fold for pramipexole and quinpirole. Similar replacements of TMV or -VI sequence, despite 13 and 19 divergent residues, respectively, selectively affected the affinities of few ligands, raclopride for the TMV chimera (a 244-fold increase in its Ki value), and quinpirole and pramipexole for the TMVI chimera (236- and 40-fold increases in their Ki values, respectively), with no noticeable effects on the affinity of the other test ligands.
In fact, all the chimeras examined here produced, more or less, differential effects on affinities of test ligands of various chemical templates, as if only a particular microbinding region or regions were perturbed in a given chimera. For instance, in the TM VII chimera, we observed a 5000-fold increase in theKi value for raclopride (benzamide), but no appreciable change in those for lisuride and cabergoline (ergots). These disparities among test ligands support the view that the observed affinity changes arise from alterations in critical binding domains for particular ligands, rather than from such nonspecific changes as global perturbations of receptor conformations. This apparent lack of nonspecific receptor alterations among the D3/D1 chimeras could be attributed not only to the high sequence homology between the D1 and D3 TM segments but also to substitutions of only small and discrete TM regions, one at a time, in these chimeras. Despite these efforts, however, several chimeras, particularly those involving regions toward the extracellular side of TM I and II, could not be examined here because of their low levels of specific binding for available D3-selective radioactive ligands. This perhaps could be interpreted to mean that TMI and II may play critical roles in assembly and/or folding of the receptors, and will necessitate even smaller substitutions, including point mutations, to assess their roles in receptor-ligand interactions. Besides TMI and II, the chimeras with the whole segment of D1 TMIII or IV also failed to show binding activity for D3 ligands (despite high homologies to the D3 counterparts), but these TMs differ from the TMI and II in that substitutions with smaller D1 TM fragments, including the critical regions retained ligand binding activity, albeit of lower affinity compared with the wild-type receptor. It seems that overall free energy changes from the two smaller substitutions in TMIII (TMII-2 and TMIII-3), for instance, could not predict the energy change encountered with the substitution of the whole TM segment. This unpredictable (probably much greater) free energy change could arise from structural interdependency of the residues within a helical structure as well as their cooperative interface interactions with the adjacent transmembrane helices. Otherwise, free energy changes from the smaller substitutions would be additive, as known for mutations of structurally independent regions. Also there are many conceivable scenarios leading to the chimeras’ failure to show ligand binding activity, such as their failed expression, their rapid degradation, a failure of their translocation to surface membranes, or their severely disturbed binding pockets. Discrimination of these various conformational possibilities for the chimeras with D1 TMI, II, III, and IV could be attempted in the future with various techniques in cell biology, including the uses of site-specific antibodies to the D3 receptor.
Here we evaluated how an overall similarity (or dissimilarity) of the substituted TM sequence for a given chimera is related to its relative changes in ligand affinity. As computed the similarity in the primary sequences of substituted TMs, using the Dayhoff Table (Schwarz and Dayhoff, 1978), we found that the overall similarity of the substituted region to the original D3 TM sequences shows no relationship with the degree of ligand affinity changes. For instance, the order of similarity (%) among the key chimeras follows TM III-3 (91.3%) > TMV (72.9%) > TM IV-2(72.7%) > TMVII (61.9%) > TM VI (59.3%), and the order hardly reflects their relative impact on ligand affinity (see the text, Table 2, and Figs. 1, 2, and 3). This again points out that alterations of critical binding regions in the chimeras, rather than overall dissimilarities in their sequences, are responsible for observed ligand affinity changes. Again, this negligible general structural factor is largely attributable to substitution of a small, discrete region for a given chimera with a homologous segment and could be recognized by the use of diverse ligands selective for the D3 over D1 receptor. From these considerations, we propose that individual TM segments disproportionately contribute to receptor ligand interactions of the D3 dopamine receptor, with the order of decreasing impact, TM VII, TMIII > TM IV >TM VI > TMV.
Furthermore, the current study enabled us to focus on the molecular determinants of individual TM segments for the D3receptor ligand interactions. Our observations indicate that the key molecular determinants of most TM segments confined to narrow regions near the extracellular surface. For instance, the TMIV-3 chimera that contains the seven residues of the D3 origin at the carboxyl-terminal side (near the extracellular surface), bound all the ligands with affinity comparable with that of the wild-type receptor, despite its D1 sequence at the amino-terminal side (A151-F164), which includes 11 divergent residues. On the other hand, the TMIV-2 chimera with the D1sequence at the carboxyl-terminal side and the D3sequence at the amino-terminal side, (its orientation of D1 sequence opposite to the TMIV-3 chimera), showed considerable changes in ligand affinity (Fig. 2). This difference in the behaviors of the TMIV-2 and TMIV-3 chimera could not be predicted from their overall sequence similarity to the wild-type receptor (63.7% for TMIV-3 and 72.7% for TMIV-2), and underscores the view that the key molecular determinants of the TMIV for ligand binding are confined to the residues near the extracellular surface. Similarly, the TMVI-3 with the D3 sequence near the extracellular surface bound all the ligands with affinities comparable with that of the wild-type receptor despite its 12 divergent D1 residues near the intracellular surface. On the other hand, the TMVI-2 with the seven divergent D1 residues near the extracellular surface showed selective affinity changes for quinpirole and pramipexole that were very similar to those of the TMVI, which contains the entire D1 TMVI sequence. The same view can be applied to the TMI, TMII, and TMVI. That is, no appreciable affinity changes for the test ligands were observed with the TMI-1, II-3, and VI-3, with the D3-sequence (6 to 8 residues deep) near the extracellular surface despite their D1 sequences in the rest of the TM segments. With the TMV, we did not pursue further because there were no noticeable affinity changes for test ligands other than raclopride. For the TMIII segment, the chimera with the D1 sequence near the extracellular surface (TMIII-3, 104–114) produced marked changes in ligand affinities compared with the wild-type receptor.1 This is also consistent with the view that the key molecular determinants for ligand binding confined to the regions near the extracellular surface, but the question of how far this critical region extends could not be answered with our current study because of the high sequence homology of the rest of the TMIII sequence (115TASILNLC122) between the D1 and D3 receptor. For example, the TMIII-2 chimera contains only two divergent D1 residues, A123V and I126V, at the distal carboxyl-terminal side (near the intracellular surface), and showed no changes in ligand binding properties.
For the TMVII segment, the critical binding region was probed with the three TMVII chimeras that have the D3 sequence extending progressively from the extracellular to intracellular surface (e.g., no D3 sequence for the TMVII chimera); the seven D3 residues near extracellular surface for TMVII-1; and the entire D3 sequence except for V381I and T384A at the extreme carboxyl-terminal side for the TMVII-2. Test ligand affinities steadily improved as the D3 sequence extended from the amino-terminal (extracellular surface) to the carboxyl-terminal side (intracellular surface), although the improvements were not uniform among the ligands (Table 2). Interestingly, the TMVII-2 chimera with only two divergent residues (V381I and T384A) showed 20 to 45-fold lower affinities to quinpirole, apomorphine, and pramipexole. Structurally, the two residues seem to reside at the nearly same face of the TMVII helix (3.6 amino acid residues per helical turn), and are adjacent to Pro380, a strictly conserved residue among dopamine receptors. It has been shown previously that the corresponding proline in D2is exposed to extracellular water-accessible binding-site crevice, as probed with the cysteine scanning mutagenesis, using a charged, hydrophilic sulfhydryl-specific agent (Fu et al., 1996). Pro380 probably contributes to ligand binding pockets, and its immediate surroundings could be altered by the mutations of the two adjacent residues, leading to the selective alterations of several agonist affinities. The fact that only the agonist affinities were altered by the mutations could be interpreted to mean that the region including Pro380 is somehow linked to receptor-G protein coupling. It seems that the contributions of the TMVII to ligand binding arise not only from the residues near the extracellular surface but also from those near the intracellular surface on the carboxyl-terminal side, even if not directly.
We list below the Ki values of test ligands as measured by competition assay with [3H]SCH23390 in human D1receptors expressed in Sf9 cells, under experimental conditions identical to the current study; for spiperone, 634 ± 98 nm; butaclamol, 19.8 ± 1.3 nm; chlorpromazine, 79 ± 4 nm; YM 09151–2, 3,072 ± 692 nm; UH-232, 312 ± 42 nm; AJ-76, 63,272 ± 3,841 nm; haloperidol, 55 ± 3 nm; raclopride, ≫64,000 nm; (−)3-PPP, 8,088 ± 498 nm; quinpirole, >64,000; pramipexole, >64,000; lisuride, 148 ± 24 nm, and cabergoline, 2,315 ± 110 nm. The affinity to D1 is quite variable among the test ligands; from the compounds of no appreciable affinity represented by raclopride (≫64,000 nm) to those of relatively high affinity represented by butaclamol (19.8 nm). It is of some interest to evaluate how the D1affinity of individual test ligands is reflected in their affinity to the D3/D1 chimeras where one D1 TM is placed in the D3 receptor environments. One would expect a tendency that the ligands with lower affinities to D1 would display more markedly altered affinities to the chimeras, and this seems to be true for most compounds (e.g., raclopride and pramipexole). Also, one tends to expect that ligand affinity changes in D3/D1chimeras would be limited within the range between its D3 and D1 values. This expectation, however, is based on the assumptions that (a) a given ligand shares the same set of binding regions between the D3 and D1 receptors, which could be distributed in several TMs, and (b) that the substituted D1 region contributes to the ligand binding in the same way as its D3 counterpart, except for the impact from divergent residues. This seems to be untrue for some compounds. For instance, the Ki values of butaclamol for certain D3/D1 chimeras far exceed its D1 Ki value. This could be interpreted to mean that butaclamol employs a set of binding regions in D3 different from those in D1, although the two receptors are homologous. Future study on the roles of individual D1 TMs in ligand binding is needed, and one may construct D1 chimeric receptors where one D3 TM is placed in the D1receptor environments. Studies with such chimeras would reveal whether ligand binding regions for a given ligand reside at the same set of TMs in D1 as observed with the D3. With such information on hand, one could dissect molecular basis of ligand selectivity for D3/D1 receptor.
Structural studies with bacteriorhodopsin (Henderson et al., 1990) and β-adrenergic receptors (Frielle et al., 1988;Strader et al., 1994) indicate that TMIII and VII are most centrally located in the ligand binding pocket, which is flanked by the TM I, II, IV, V and VI. This model is compatible with our results with the D3 receptor in that replacements of TMIII and TMVII with the corresponding D1 sequence markedly affected the affinity for a broad spectrum of ligands while replacements of the flanking TMs had moderate (for TMIV) or no effects on ligand affinity except for few ligands (TMV or VI). Furthermore, asymmetrical involvements of TMs in the binding pocket are implied from our results; that is, the critical binding regions on the D3 receptor are confined to the six to eight residues near the extracellular surface for TMI, II, IV and VI, but extend considerably deeper to the intracellular surface for the TMVII, more or less a funnel-shaped binding pocket with its narrow apex provided by the TMVII and probably TMIII segments.
As discussed above, individual ligands showed widely variable binding affinities toward a given chimera. This probably reflects the supposition that the binding pockets for individual ligands consist of multiple regions, some of which are common and overlapping among the ligands but others of which are highly individualized. Here, we attempted to sort out the test ligands for their sensitivity to the various D3/D1 chimeras. Fig. 4 shows the competition binding profiles (with [3H]spiperone) for the five representative ligands showing differential sensitivities to the various chimeras we examined here. Raclopride is the most sensitive ligand, displaying markedly low affinity to the chimeras containing the D1 TMIII, IV, V, VI, or VII. Quinpirole (also pramipexole) was sensitive to the above chimeras except for the TMV chimera. Chlorpromazine, representing the group of butaclamol and haloperidol, was sensitive to only the TMIII, IV, and VII chimera. YM-09151–2, representing the group of spiperone, UH-232, AJ-76, (−)3-PPP, and apomorphine, was sensitive to only the TM III and VII chimeras. Finally, the ergots (lisuride and cabergoline) showed no sensitivity to the chimeras except for the TMIII chimera, in which they showed about 30-fold lower affinity. This insensitivity of ergots is remarkable considering their high selectivity for the D3 over D1 receptors [e.g., the Ki value of cabergoline was 1800-fold less for the D3 than for the D1 receptor, as measured with competition experiments using [3H]SCH23390 and [3H]spiperone under identical conditions (data not shown)]. This implies that the subtype selectivity of the ergots may arise from their selective interactions with the TMIII and the residues in the extracellular loops.
This grouping tends to assign compounds with the same chemical template into the same class, such as the ergots (lisuride and cabergoline) and aminotetralins (UH-232 and AJ-76, as one might expect, but also collects chemically divergent ligands into a group, such as quinpirole and pramipexole. The latter situation may arise from similarity in their steric configurations and would be useful for further classifications of ligands. It will be also of future interest to see how single point mutations would affect ligand affinity within such groups.
Because most of the test ligands we examined here bound the D3 and D2 receptors with similar high affinity, one would predict a high sequence identity of the critical binding regions between the D3 and D2 receptors. Indeed, as shown in Table3, the sequence of the D2long receptor is nearly identical in the hot binding regions except for eight residues, L34, S35, Y36, C37, A38 (TMI), T92 (TMII), F172 (TMIV), and T353 (TMVII), which are nonconservatively substituted on the D2receptor. These structural differences could be exploited to develop ligands selective for the D3 over D2 dopamine receptor or vice versa.
Footnotes
- Received August 28, 1997.
- Accepted April 22, 1998.
-
Send reprint requests to: Dr. Wha Bin Im, CNS Diseases Research, 725–209-512, Pharmacia & Upjohn, Inc., Kalamazoo, MI 49001. E-mail: wbim{at}am.pnu.com
-
↵1 Our recent mutation of cysteine 114 to serine (i.e., the tenth residue of the TMIII of the human D3receptor to the corresponding residue of the D1 receptor) led to marked changes in ligand affinities similar to those observed with the chimera TMIII-3. For instance, AJ-76 and UH-232 displayedK i values 100-fold greater than those obtained with the wild-type receptor. This further supports our proposal of the critical region for TMIII being deeper, involving at least the 10 residues near the extracellular surface.
Abbreviations
- TM
- transmembrane segment
- HEPES
- 4-(2-hydroxyethyl)-1-piperazineethanesulfonic acid
- 3-PPP
- 3-(3-hydroxyphenyl)-N-(1-propyl)piperidine
- The American Society for Pharmacology and Experimental Therapeutics