Functional Characterization of the Recombinant Human 5-Hydroxytryptamine7(a) Receptor Isoform Coupled to Adenylate Cyclase Stimulation

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Vol. 287, Issue 2, 508-514, November 1998

Functional Characterization of the Recombinant Human 5-Hydroxytryptamine_7(a) Receptor Isoform Coupled to Adenylate Cyclase Stimulation

Nika Adham, John M. Zgombick, Jonathan Bard and Theresa A. Branchek

Synaptic Pharmaceutical Corporation, Paramus, New Jersey

	Abstract

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Functional characterization of the recombinant human 5-hydroxytryptamine_7(a) (h5-HT_7(a)) receptor isoform was performed usingstably transfected LM(tk) cells. Expression levels of the h5-HT_7(a) receptor determinedfrom saturation studies using either a labeled agonist ([³H]5-HT) or antagonist ([³H]LSD) were very similar (B_max = 160-190 fmol/mg protein), suggestingthat all receptors may exist in the high affinity (G protein-coupled)state. In intact cells, 5-HT produced a concentration-dependentelevation of intracellular cAMP levels ([cAMP]_i) with an EC₅₀value of 80 nM and a maximal response of 5-fold increase abovebasal levels. The rank order of agonist potencies in the secondmessenger assay paralleled their rank order of binding affinities:5-carboxamidotryptamine > 5-hydroxytryptamine $>=$ 5-methoxytryptamine> 8-hydroxy N,N-dipropyl aminotetralin > sumatriptan. Agonistpotencies (EC₅₀ values) to stimulate [cAMP]_i were more than 25-foldlower relative to their respective binding affinities (K_ivalues) obtained in [³H]5-HT competition assays. In contrast, antagonist potencies (K_bvalues) to block 5-HT-stimulated [cAMP]_i were in close agreementwith their corresponding K_i values. These data may indicatelow efficiency of receptor-effector coupling to adenylate cyclasestimulation. Pretreatment of stably transfected cells with choleratoxin abolished the 5-HT-mediated elevation of [cAMP]_i, indicatingthat the 5-HT_7(a) subtype directly interacts with G_s protein(s)to activate adenylate cyclase(s). Clonal cell lines stably expressingh5-HT₇ receptor isoforms will serve as valuable cellular modelsto study their function and regulation, as well as assist in thedevelopment of selective 5-HT₇ receptor agents to uncover thebiological roles and potential therapeutic applications of thisnovel receptorsubtype.

	Introduction

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Serotonin receptors display the greatest molecular diversity of any family of G protein-coupled receptors. Fourteen receptorsubtypes have been cloned and subdivided into seven distinct subfamilies(5-HT_1-7) based on structural (deduced amino acid sequence,transmembrane homology), operational (binding properties, pharmacology)and transductional (effector coupling) criteria (Hoyer et al.,1994). With the exception of the 5-HT₃ receptor that is a ligand-gatedion channel, all other serotonin receptors are members of thesuperfamily of G protein-coupled receptors including three subtypesthat couple to the stimulation of adenylate cyclase (5-HT₄, 5-HT₆and 5-HT₇). Identifying the functional correlates of the clonedserotonin receptors and hence their therapeutic potential is challenging,particularly for the more novel subtypes such as 5-HT₆ and 5-HT₇receptors, because selective compounds have yet to bedeveloped.

One functional correlate of 5-HT₇ receptor activation includes smooth muscle relaxation observed in a variety of isolatedtissue preparations, in which elevations of [cAMP]_i concentrationswere also detected (Branchek and Zgombick, 1997; Eglen et al.,1997 for reviews). Further evidence for the mediation of the relaxantresponse via the 5-HT₇ receptor is provided by the localizationof mRNA transcripts encoding the 5-HT₇ receptor in many bloodvessels by RT-PCR (Ullmer et al., 1995). An additional physiologicalresponse that may be mediated by the 5-HT₇ receptor is the regulationof photic entrainment of circadian rhythms (Ying and Rusack, 1997),potentially via an inhibition of a GABA_A receptor-activated current(Kawahara et al., 1994). However, neither the 5-HT₇ receptor norits mRNA has been localized to the hypothalamic suprachiasmaticnuclei (Lovenberg et al., 1993; To et al., 1995; Gustafson etal., 1996). In other in vitro and in vivo preparations, 5-HT₇responses are intermixed with one or more additional serotonineffects. For example, the 5-HT₇ receptor mediates the high affinityportion of the biphasic stimulation of adenylate cyclase by 5-CTin guinea pig hippocampal membranes (Tsou et al., 1994). Similarly,the 5-HT₇ receptor may also be involved in the tertiary, prolongedhypotensive response to i.v. administration of 5-HT in the rat(De Vries et al., 1997).

Alternative splicing of the mRNA encoding intron-containing serotonin receptors contributes to further structural diversity,resulting in the generation of additional receptor variants. Thishas been demonstrated for genes encoding two G_s-coupled serotoninreceptors, the 5-HT₄ (Gerald et al., 1995; Blondel et al., 1998)and 5-HT₇ (Bard et al., 1993; Heidmann et al., 1997; Jasper etal., 1997; Stam et al., 1997) subtypes, in which splice variantsdiffer in length of their predicted carboxy termini. An intron-containingh5-HT₇ receptor gene (5-HT_7(a)) was first isolated by Bard andcolleagues (1993) from a genomic library and was found to encodea protein of 445 amino acids. Subsequently, several groups reportedthe cloning of a cDNA encoding a second h5-HT₇ receptor isoform(5-HT_7(b)) identical to that described by Bard et al. (1993),except that it contained a truncated carboxy terminus (Heidmannet al., 1997; Stam et al., 1997; Jasper et al., 1997). A thirdsplice variant of the h5-HT₇ receptor (5-HT_7(d)) was identifiedcontaining an additional exon and hence a longer carboxy tailthan the other two 5-HT₇ receptor isoforms (Heidmann et al., 1997).The 5-HT_(7d) splice variant represents a minor molecular species(<5%) compared to the relative abundance of the other two 5-HT₇receptor isoforms (Heidmann et al., 1997). Although the bindingproperties of the human 5-HT_7(a) and 5-HT_7(b) splice variantshave been well characterized (Bard et al., 1993; Jasper et al.,1997), detailed functional characterization has only been reportedfor the h5-HT_7(b) receptor (Jasper et al., 1997). In our study,a clonal cell line was generated expressing the h5-HT_7(a) receptorisoform to determine the potencies and intrinsic activities ofreference serotonergic agents using the elevation of [cAMP]_i asa functional measure of compoundactivity.

	Methods and Materials

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Generation of the stable cell line. The entire coding region of the h5HT_7(a) receptor gene was subcloned into the expression vector pcEXV-3 (Bard et al., 1993).Murine fibroblasts (LMtk) were used as the transfection host to establish a stable cellline expressing this subtype by the calcium phosphate method usingG-418 as a selection marker (Zgombick et al., 1991). Clonal cellswere grown as adherent monolayers under standard conditions (5%CO₂, 37°C) in serum-free media (AIM V, GIBCO BRL, Grand Island,NY). Transfected cells reached approximately 90% confluency priorto use in radioligand binding and second messengerassays.

[³H]5-HT and [³H]LSD binding assays. Membranes were prepared from clonal cells using standard techniques (Branchek et al., 1990). Radioligand binding studies wereperformed according to the methodology outlined by Zgombick andcolleagues (1991). Expression levels of the h5-HT_7(a) receptorwere determined from both [³H]5-HT (agonist) and [³H]LSD (antagonist) saturation studies using eight concentrationsof radioligand (0.2-20 and 0.5-60 nM, respectively). Competitionstudies were performed using 5 nM [³H]5-HT and 10 concentrations of competitor. Unlabeled 5-HT (10µM) defined nonspecific binding. Membranes were incubated for30 min at 37°C and the assay was terminated by vacuum filtration.Protein concentrations were determined by the method of Bradford(1976) using bovine serum albumin as thestandard.

Intracellular cAMP assays. The h5-HT_7(a) receptor-mediated elevations of [cAMP]_i were determined using a protocol described previously (Zgombick et al.,1993), with the exception that forskolin was omitted from theassay. Transfected cells were plated in 96-well microtiter plates(5 × 10³ cells/well) and allowed to grow for 96 hr. Cells were preincubatedfor 20 min in N-2-hydroxyethylpiperazine-N'-2-ethanesulfonic acid(HEPES)-buffered saline (150 mM NaCl, 10 mM HEPES, 5 mM theophylline,10 µM pargyline, pH 7.4 at 37°C). Antagonists were also incubatedduring this preincubation period in a subset of experiments. Inseparate experiments, cholera toxin (20 µg/ml) was added 18 hrbefore the assay. Cells were incubated with 10 concentrationsof agonist for an additional 10 min (5% CO₂, 37°C) to generateCRCs. The assay was terminated by the removal of medium and theaddition of 160 µl of 0.1 M HCl. Intracellular cAMP was determinedby radioimmunoassay (PerSeptive Diagnostics, Cambridge,MA).

Data analysis. Binding (K_d, B_max and IC₅₀ values) and response (EC₅₀ and E_max) parameters were determined by nonlinear regressionanalysis (GraphPAD Prism, San Diego, CA). IC₅₀ values were convertedto K_i values using the Cheng-Prusoff equation (1973).Apparent dissociation constants of antagonists (K_b values)were determined from the shift of the EC₅₀ value of 5-HT in theabsence and presence of one concentration of antagonist (~10 ×K_i values) by the method of Arunlakshana and Schild (1959).

Drugs. [³H]LSD (specific activity 76.7 Ci/mmol) and [³H]5-HT (25.2 Ci/mmol) were obtained from New England Nuclear (Boston, MA). 5-Carboxamidotryptamine,5-hydroxytryptamine, 5-methoxytryptamine, N,N-dipropyl-5-carboxamidotryptamine,N,N-dimethyl-5-methoxytryptamine, 2-methyl-5-hydroxytryptamine, $alpha$ -methyl-5-hydroxytryptamine, tryptamine, 8-hydroxy N,N-dipropylaminotetralin, 1-naphthylpiperazine, methiothepin, dihydroergotamine,mesulergine, metergoline, clozapine, ritanserin, spiperone, cyproheptadine,ketanserin and rauwolscine were purchased from Research BiochemicalsInc. (Natick, MA). d-LSD was supplied from the National Instituteof Drug Abuse (Bethesda,MD).

	Results

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Expression levels (B_max values) of the recombinant h5-HT_7(a) receptor in membranes derived from stably transfected murinefibroblasts were determined from parallel saturation experimentsutilizing both [³H]5-HT (agonist) and [³H]LSD (antagonist). Both [³H]LSD and [³H]5-HT bound with high affinity and in a saturable manner to membranesderived from this clonal cell line (fig. 1, A and B). Bindingparameters for the [³H]radioligands (K_d and B_max values) are summarized intable 1. The site densities of the 5-HT_7(a) receptor in clonalcell membranes determined from [³H]antagonist and [³H]agonist saturation studies were very similar.

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Fig. 1. [³H]LSD (A) and [³H]5-HT (B) binding isotherms using membranes harvested from stable transfectants expressing the recombinant human 5-HT_7(a) receptor. Transformed data are represented in the form of Scatchard plots (inset). Binding parameters (K_d and B_max values) are summarized in table 1.

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TABLE 1
Equilibrium dissociation constants (K_d values) and maximal binding site density (B_max values) determined from [³H]5-HT and [³H]LSD saturations using membranes harvested from cells stably expressing the recombinant human 5-HT_7(a) receptor

Competition experiments were performed using [³H]5-HT to determine the affinity constants (K_i values) of serotonergiccompounds for the h5-HT_7(a) receptor in a stably expressing cellline since we previously reported K_i values using membranesfrom transiently-transfected Cos-7 cells. These binding studiespermitted a direct comparison between compound affinities andtheir potencies (agonist and/or antagonist) determined in thecAMP second messenger assay. Binding affinities (K_i values)for agonists and antagonists are listed in tables 2 and 3, respectively.The rank order of binding affinities was consistent with 5-HT₇receptor pharmacology: 5-CT > 5-HT $>=$ 5-MeOT $>=$ methiothepin > mesulergine> 8-OH-DPAT > spiperone > sumatriptan > ketanserin > rauwolscine.Higher binding affinities (2- to 4-fold) were noted for compoundsthat were identified as agonists in our cAMP assay relative totheir previously reported K_i values. This discrepancyis due to the lower affinity (K_d = 8 nM) of [³H]5-HT for the h5-HT_7(a) receptor in Cos-7 membranes (Bard etal., 1993) than that obtained with the stable cell line used inthis study (table 1). Much higher expression levels of the h5-HT_(7a)receptor were obtained in Cos-7 cells (7 pmol/mg protein; Bardet al., 1993) and may have contributed to the lower affinity for[³H]5-HT if endogenous G_s were rate-limiting. In contrast,no significant differences in binding affinities were noted foragents identified as antagonists in the cAMP second messengerassay since these compounds are less sensitive to the affinitystate of the receptor as compared to agonists.

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TABLE 2
Agonist potencies to stimulate [cAMP]_i by the recombinant human 5-HT_7(a) receptor isoform stably expressed in murine fibroblasts

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TABLE 3
Antagonist potencies to block 5-HT-stimulated [cAMP]_i mediated by the recombinant human 5-HT_7(a) receptor isoform stably expressed in murine fibroblasts

In stably transfected LM(tk) cells, 5-HT produced a concentration-dependent elevation of [cAMP]_i, with an EC₅₀ value of 80nM and a maximal stimulation of 5.4 ± 0.4-fold above basal values(n = 50; fig. 2; table 2). The rank order of agonist potenciesin the 5-HT_7(a) receptor second messenger assay paralleled theirrank order of binding affinities: 5-CT > 5-HT $>=$ 5-MeOT > 8-OH-DPAT> sumatriptan (fig. 2; table 2). Agonist potencies to stimulatecAMP production was more than 25-fold lower relative to theirrespective binding affinities (table 2). For tryptamine derivatives,the magnitude of the potency/affinity ratios (EC₅₀/K_i)was inversely related to their binding affinity constants (i.e.,the higher the binding affinity the smaller the discrepancy inpotency). A high correlation index (r² = 0.81) was obtained between the K_i values and EC₅₀/K_iratios for a series of tryptamine congeners (fig. 3).

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Fig. 2. CRCs for the stimulation of [cAMP]_i by serotonergic agonists in intact cells stably expressing the recombinant human 5-HT_7(a) receptor. Data was normalized to 100% relative to the maximal response elicited by 5-HT. Each data point represents a single determination. Experiments (n = 5-10) were performed as described in "Materials and Methods." $bullet$ , 5-CT; $open circle$ , 5-HT;

, 5-MeOT;

, DP-5-CT; $black-triangle$ , 5-MeO-DMT; $triangle$ , 1-NP; $black-lozenge$ , 8-OH-DPAT; $diamond$ , Sumatriptan.

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Fig. 3. Correlation between potency/binding affinity ratios (EC₅₀/K_i) and binding affinities (K_i) of tryptamine derivatives obtained with the recombinant human 5-HT_7(a) receptor. The correlation index (r²) is listed in the graph. Numbers correspond to the following compounds: 1, 5-CT; 2, 5-HT; 3, 5-MeOT; 4, DP-5-CT; 5, 5-MeO-DMT; 6, tryptamine; 7, $alpha$ -Me-5-HT.

Methiothepin and several ergot alkaloids (i.e., d-LSD) antagonized the 5-HT-mediated elevation in [cAMP]_i (fig. 4). In contrastto agonists in which large variations were obtained between K_iand EC₅₀ values, the apparent K_b values of antagonistsdetermined for the h5-HT_7(a) receptor in the second messengerassay were in close agreement with their respective K_ivalues in binding assays (table 3). Compounds identified as antagonistsdid not display inverse agonism in our heterologous expressionsystem.

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Fig. 4. Determination of the apparent dissociation constant (K_b value) of d-LSD for the recombinant human 5-HT_7(a) receptor. CRCs for the stimulation of [cAMP]_i by 5-HT were generated in the absence ( $open circle$ ) and presence ( $bullet$ ) of 50 nM d-LSD. Data were normalized to 100% relative to the maximal response elicited by 5-HT. Each data point represents a single determination. Experiments (n = 5) were performed as described in "Materials and Methods." Apparent K_b values were determined from the Schild equation and are summarized in table 3.

Pretreatment of clonal cells with cholera toxin (20 µg/ml for 18 hr) abolished the 5-HT-mediated elevation of [cAMP]_i (fig.5). No changes in inositol phosphate production or intracellularcalcium concentrations were observed after exposure of stabletransfectants to 1 µM 5-HT (data not shown). These data indicatethat the h5-HT_7(a) receptor directly interacts with G_s protein(s)and does not couple to G_q/G₁₁ or G_i pathways. Similar observationswere reported previously in which the h5-HT_7(b) receptor isoformcoupled only to adenylate cyclase stimulation in transfected HEK293 cells (Jasper et al., 1997).

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Fig. 5. Effect of cholera toxin pretreatment on the 5-HT-induced elevation of [cAMP]_i in intact cells stably expressing the recombinant human 5-HT_7(a) receptor. CRCs for the stimulation of [cAMP]_i by 5-HT was generated in control ( $open circle$ ) and cholera toxin-pretreated ( $bullet$ ) cells. Data were normalized to 100% relative to the maximal response elicited by 5-HT. Each data point represents a single determination. Experiments (n = 3) were performed as described in "Materials and Methods."

	Discussion

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RT-PCR studies have assisted in the identification of four mammalian 5-HT₇ receptor isoforms that are structurally divergentin their predicted intracellular carboxy termini. The 5-HT_7(a)receptor was the first isoform cloned from human with a predictedlength of 445 amino acids (Bard et al., 1993). Alternative splicingof a second intron in the coding region located near the carboxyterminus of the human gene generates a 13 amino acid truncatedreceptor isoform (5-HT_7(b)) due to a five nucleotide base insertionwhich introduces an in-frame stop codon (Jasper et al., 1997;Heidmann et al., 1997; Stam et al., 1997). Two additional splicevariants, designated 5-HT_7(c) (rat) and 5-HT_7(d) (human), areproduced by a retained exon cassette, which is distinct betweenthe two species. These other isoforms encode gene products withunique carboxy-terminal amino acid sequences different from boththe 5-HT_7(a) and 5-HT_7(b) receptors as well as from each other(Heidmann et al., 1997). The 5-HT_7(a) and 5-HT_7(b) receptor isoformsrepresent the predominant splice variants in both rat and human(Heidmann et al., 1997).

The binding properties of the recombinant human 5-HT_7(a) (Bard et al., 1993) and 5-HT_(7b) (Jasper et al., 1997) receptor isoformshave been reported previously. The discriminating properties ofh5-HT₇ receptor pharmacology include a rank order of binding affinities:5-CT > 5-HT $>=$ 5-MeOT $>=$ methiothepin > 8-OH-DPAT > spiperone >sumatriptan > ketanserin > rauwolscine. In addition, a seriesof antipsychotic and tricyclic antidepressant compounds displayhigh affinity for the 5-HT₇ receptor (Roth et al., 1994). Becausedetailed functional information (intrinsic activities and potencies)of reference serotonergic compounds has been determined only forthe h5-HT_(7b) splice variant (Jasper et al., 1997), the h5-HT_(7a)receptor isoform was stably expressed in murine fibroblasts (LMtk) and second messenger responses were investigated to gain furtherinsight into the pharmacological properties of the different splicevariants of the h5-HT₇receptor.

Low site densities of the h5-HT_7(a) receptor in LM(tk) membranes were obtained from saturation studies using both [³H]5-HT and [³H]LSD (163 and 189 fmol/mg protein, respectively) (table 1).The similar (and low) receptor expression levels obtained withboth [³H]agonist and [³H]antagonist radioligands are suggestive that endogenous G_sprotein(s) is not rate limiting in this cell line and that h5-HT_7(a)receptors exist in the high affinity (G protein-coupled) state.However, the relationship between the high affinity state of thereceptor (detected from [³H]5-HT competition studies) and the affinity state of the h5-HT_7(a)receptor that mediates the stimulation of adenylate cyclase(s)is not known atpresent.

In agreement with previous studies, 5-HT evoked a concentration-dependent elevation of [cAMP]_i in intact cells expressingthe h5-HT_7(a) receptor (fig. 2). The rank order of agonist potenciesto stimulate cAMP formation paralleled their rank order of bindingaffinities: 5-CT > 5-HT $>=$ 5-MeOT > 8-OH-DPAT > sumatriptan. However,agonist potencies ranged from 25-950-fold lower than their respectivebinding affinities (table 2). Jasper and colleagues (1997) alsonoted significantly lower agonist potencies relative to theirbinding affinities for the h5-HT_7(b) receptor stably expressedin HEK 293 cells, although smaller differences were observed (8-to 75-fold) relative to that obtained in our study. Agonist potenciesfor the h5-HT_7(a) receptor (table 2) were 3- to 17-fold lowerthan for the same subset of compounds for the h5-HT_7(b) receptor(Jasper et al., 1997). The 3-fold higher binding affinities ofagonists for the h5-HT_7(b) receptor (Jasper et al., 1997) relativeto the h5-HT_7(a) splice variant (table 2) may underlie a portionof the observed agonist potency differences between the receptorisoforms. Indeed, Jasper and colleagues (1997) determined thebinding properties of the two splice variants of the h5-HT₇ receptorin parallel using [³H]5-CT and observed small variations in receptor pharmacology,with a conservation of the rank order of binding affinities. Thesedata would suggest that differences in experimental methodologiesemployed in the two investigations (i.e., radioligands, buffer,transfection host) contribute to the lower binding affinitiesreported in this study relative to those of Jasper et al. (1997).The much higher expression of the h5-HT_7(b) receptor in HEK 293cells (>7 pmol/mg protein; Jasper et al., 1997) relative to thelower density of the h5-HT_7(a) receptor in LM(tk) cells (~200 fmol/mg protein; fig. 1) may contribute to the observedvariations in agonist potencies between the two studies. Differentialexpression of native G_s and adenylate cyclase isoforms inthe two transfection hosts could also lead to differences in theefficiency of receptor coupling to adenylate cyclase stimulation(and hence agonist potencies) by the two splice variants. Thelow potency of agonists to elicit functional responses has alsobeen noted in native 5-HT₇ receptor systems from various species,suggestive that low efficiency in receptor-effector coupling maybe an inherent property of this subtype (Tsou et al., 1994; Leunget al., 1996; Schoeffter et al., 1996; Terrón, 1996; Eglen etal., 1997 forreview).

The high EC₅₀/K_i ratios reported here and by others (see above) for the 5-HT₇ receptor, is not necessarily unexpected.In the context of current receptor theory, one would expect anEC₅₀ value for an agonist in a functional assay to be less thanor equal to its affinity for the uncoupled state of the receptor(K_low) calculated from antagonist competition binding studiesperformed in the presence of guanine nucleotides. Indeed, thisaffinity state (K_low) corresponds to that derived from receptorinactivation studies (K_A) using the method of Furchgott(Furchgott and Bursztyn, 1967). In contrast, the K_i valuesmeasured in our binding studies are presumably the affinity ofagonists for the G protein-coupled state of the receptor (K_(high))because [³H]5-HT was used as the radioligand in the absence of guanine nucleotides.The nature of the relationship between K_(high) and the EC₅₀ foran agonist is unclear currently. As the designation implies, thebinding affinity (K_i) of a compound is a "constant" dependentprimarily upon its molecular structure, whereas agonist potency(EC₅₀) varies as a function of its intrinsic efficacy and thedegree of receptor reserve present in the assay system. Therefore,the EC₅₀/K_i ratios might be expected to vary similarlysuch that one would expect highly efficacious compounds to showa higher ratio as compared to partial agonists. The calculatedEC₅₀/K_i ratios obtained in our study may be an indirectmeasure of the intrinsic efficacy of the agonist tested and wouldbe expected to vary analogous to the K_low/K_high ratios. It hasbeen demonstrated for several G protein-coupled receptors thatthe magnitude of agonist K_low/K_high ratio (guanine nucleotideshift) calculated from binding studies is an estimate of the intrinsicefficacy of that compound, with the most efficacious agonistsdisplaying the largest ratios (Kenakin, 1993).

Unexpectedly, we observed a reverse correlation between EC₅₀/K_i ratios and K_i values of agonists (table2; fig. 3). For example, we expected this ratio to be lower for5-MeOT, $alpha$ -Me-5-HT and 8-OH-DPAT as compared to 5-HT and 5-CT,because the former compounds have been shown to be either inactiveor partial agonists (and therefore possess lower intrinsic efficacythan the latter compounds) in several 5-HT₇ receptor-expressingsystems (Lovenberg et al., 1993; Leung et al., 1996; Schoeffteret al., 1996; Terrón, 1996). The higher intrinsic efficaciesof $alpha$ -Me-5-HT and 8-OH-DPAT in transfected cell lines (table 2)(Jasper et al., 1997) relative to native systems implies thata degree of receptor reserve may be present in the clonal cells,even though receptor expression may be low (<200 fmol/mg protein;table 1). The significance of the relationship between EC₅₀/K_iratios and intrinsic efficacies obtained in this study and itsrelevance to signal transduction is not clear at present, butour results indicate that these ratios may not be predictive ofthe intrinsic efficacy of compounds in mediating physiologicalresponses at native 5-HT₇ receptors. Differences in receptor-effectorcoupling, species variations in pharmacology or the experimentalmethodologies employed may contribute to variations in the intrinsicefficacy of the above agonists in different systems. Studies usingtransfected cells expressing lower number of receptors may providea more accurate estimate of intrinsic efficacy and may permitthe identification of partial agonism for compounds such as $alpha$ -Me-5-HT,since the degree of receptor reserve could be adequately low for1-NP (arylpiperazine; table 2) but not for a structurally divergentseries as the tryptamines. Determination of K_low values of agonistsin [³H]LSD (antagonist) competition binding assays using nonhydrolyzableGTP analogues and generation of K_A values by partialreceptor alkylation may also assist in elucidating further theunderlying molecular mechanisms involved between receptor activationand the generation of the second messenger response for thissubtype.

In accordance with 5-HT₇ receptor pharmacology, methiothepin and several ergot alkaloids such as d-LSD competitively antagonizedthe h5-HT_7(a) receptor-mediated elevation of [cAMP]_i (fig. 4;table 3). These compounds did not display inverse agonism inour heterologous expression system. With the exception of ketanserin,antagonist potencies (K_b values) to block 5-HT-mediatedcAMP production were in close agreement with affinity constants(K_i values) derived from [³H]5-HT competition binding (<3-fold; table 3), which contrastthe results obtained with agonists (see above). These data differmarkedly from those reported by Jasper et al. (1997) using theh5-HT_(7b) receptor, in which antagonist K_b values determinedin second messenger studies were 5- to 40-fold lower than theirrespective affinity constants obtained from binding studies. Theseauthors postulated that the receptor may attain different conformationalstates during functional interactions with G_s in second messengerand radioligand binding assays. Alternatively, the disparitiesmay reflect differences in experimental methodology between thetwo investigations (radioligands, transfection hosts). To betterevaluate the apparent variations in agonist and antagonist potenciesobserved between the two h5-HT₇ splice variants, it is criticalto perform parallel studies by expressing both receptor isoformsin the same cell line at similar and physiologically relevantlevels.

The physiological significance of multiple splice variants of the h5-HT₇ receptor has yet to be fully appreciated. However,recent evidence suggests that these alternatively spliced 5-HT₇receptor isoforms may be differentially expressed in human brainand smooth muscle. RT-PCR studies have identified the 5-HT_7(a)receptor as the predominant molecular species in the human brainalthough the 5-HT_(7b) receptor as the primary transcript in humansmooth muscle (Hamblin and Heidmann, 1997). Structural differencesin the carboxy termini of the h5-HT₇ receptor splice variantsindicate potential differential interactions with PDZ-domain-containingproteins, determinants of protein organization with the plasmamembrane (Martin et al., 1998). Additionally, these two splicevariants may display differential coupling to G_s isoforms.Splice variants of the h5-HT₇ receptor differ in their lengthof their C-termini, and this region of G_s-coupled receptors isa structural domain implicated in molecular interactions withG_s (Strader et al., 1994). However, it is highly unlikelythat the human 5-HT_(7a) and 5-HT_(7b) receptor isoforms are differentiallydown-regulated by phosphorylation because neither splice variantcontains known consensus sequences for potential phosphorylationin their predicted intracellular carboxy termini. In contrast,the h5-HT_(7d) possesses two phosphorylation consensus sites (Heidmannet al., 1997) and may be regulated in a phosphorylated-dependentmanner.

The detailed pharmacological characterization of the cloned h5-HT_7(a) receptor and other related splice variants in heterologousexpression systems will continue to facilitate the interpretationof in vivo and in vitro responses to 5-HT in native tissues andaid in the identification of additional 5-HT₇ receptor-mediatedresponses. The physiological roles and potential therapeutic significanceof splice variants of this receptor are only now becoming appreciated.The development of selective 5-HT₇ receptor agents will acceleratethe investigation of receptor function and regulation as wellas assist in the delineation of the role of 5-HT₇ receptor isoformsin a humanpathophysiology.

	Acknowledgments

The authors acknowledge the expert technical assistance of Ms. Anastasia Kokkinakis, Ms. Deborah Tambe and Mr. George Stepan.We also thank Mr. George Moralishivilli for preparing thefigures.

	Footnotes

Accepted for publication June 23, 1998.

Received for publication March 6, 1998.

¹ Current address: Wyeth Ayerst Research, CNS Department, Monmouth Junction, NJ08852.

Send reprint requests to: Dr. Nika Adham, Synaptic Pharmaceutical Corporation, 215 College Road, Paramus, NJ 07652.

	Abbreviations

[cAMP]_i, intracellular cAMP concentrations; CRC, concentration-response curve; EC₅₀, concentration of agonist required to produce 50% maximal response; E_max, maximal response; h5-HT_7(a), human 5-hydroxytryptamine_7(a); K_b, apparent antagonist dissociation constant; K_i, affinity constant; RT-PCR, reverse transcriptase polymerase chain reaction; 5-CT, 5-carboxamidotryptamine; 5-HT, 5-hydroxytryptamine; 5-MeOT, 5-methoxytryptamine; DP-5-CT, N,N-dipropyl-5-carboxamidotryptamine; 5-MeO-DMT, N,N-dimethyl-5-methoxytryptamine; 2-Me-5-HT, 2-methyl-5-hydroxytryptamine; $alpha$ -Me-5-HT, $alpha$ -methyl-5-hydroxytryptamine; 8-OH-DPAT, 8-hydroxy N,N-dipropyl aminotetralin; 1-NP, 1-naphthylpiperazine.

	References

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				C. P. Bengtson, D. J. Lee, and P. B. Osborne Opposing Electrophysiological Actions of 5-HT on Noncholinergic and Cholinergic Neurons in the Rat Ventral Pallidum In Vitro J Neurophysiol, July 1, 2004; 92(1): 433 - 443. [Abstract] [Full Text] [PDF]

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				E. M. Chapin and R. Andrade A 5-HT7 Receptor-Mediated Depolarization in the Anterodorsal Thalamus. I. Pharmacological Characterization J. Pharmacol. Exp. Ther., April 1, 2001; 297(1): 395 - 402. [Abstract] [Full Text]

				T. Ishine, I. Bouchelet, E. Hamel, and T. J. F. Lee Serotonin 5-HT7 receptors mediate relaxation of porcine pial veins Am J Physiol Heart Circ Physiol, March 1, 2000; 278(3): H907 - H912. [Abstract] [Full Text] [PDF]

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