P2Y Receptors Modulate Ion Channel Function through Interactions Involving The C-Terminal Domain

doi:10.1124/mol.63.4.878

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Vol. 63, Issue 4, 878-885, April 2003

P2Y Receptors Modulate Ion Channel Function through Interactions Involving The C-Terminal Domain

So Yeong Lee, Samuel C. Wolff, Robert A. Nicholas, and Scott M. O'Grady

Department of Physiology and Molecular Veterinary Biosciences Graduate Program (S.Y.L.) and Departments of Physiology and Animal Science (S.M.O.), University of Minnesota, St. Paul, Minnesota; and Department of Pharmacology, University of North Carolina School of Medicine, Chapel Hill, North Carolina (S.C.W., R.A.N.)

	Abstract

Top Abstract Introduction Materials and Methods Results and Discussion References

Nucleotide stimulation of G_q-coupled P2Y receptors expressed in Xenopus laevis oocytes produces the activation of an endogenousvoltage-gated ion channel, previously identified as the transientinward (T_in) channel. Expression of human P2Y₁, human P2Y₂, ratP2Y₆, human P2Y₁₁, or skate P2Y receptors in oocytes resultedin modulation of the voltage dependence and inactivation gatingof the channel. Expression of the human P2Y₄ receptor, rat M₁-muscarinicreceptor, and human B₁-bradykinin receptor did not alter the propertiesof the T_in channel. Replacement of the C-terminal domain of thehuman B₁-bradykinin receptor with the C-terminal domains of eitherthe human P2Y₁ or human P2Y₂ receptor resulted in voltage dependenceand inactivation-gating properties, respectively, of the T_in channelthat were similar to those elicited by the respective native P2Yreceptor. Systematic truncation of the C-terminal region of thehuman P2Y₁ receptor identified a short region responsible formodulation of the T_in channel. This region contains a conservedsequence motif found in all P2Y receptors that modulates the voltagedependence of the T_in channel. Synthetic 20-mer peptides fromthe C-terminal domains of human P2Y₁ and P2Y₂ receptors produceda shift in the voltage dependence and slowed inactivation gating,respectively, after injection into oocytes expressing human B₁-bradykininor truncated human P2Y₁ receptors. These results indicate thatcertain P2Y receptors are capable of modulating the voltage sensitivityand inactivation gating of an endogenous oocyte ion channel throughinteractions involving the C-terminal region of the receptor.Such modulation of ion channel function could also exist in nativemammalian cells that express P2Yreceptors.

	Introduction

Top Abstract Introduction Materials and Methods Results and Discussion References

Extracellular nucleotides (ADP, ATP, UDP, and UTP) function as signaling molecules that mediate a variety of biological effectsthrough a family of cell surface receptors known as P2 receptors.This family is divided into two groups: the ionotropic P2X receptorsand the metabotropic P2Y receptors (Dubyak and el-Moatassim, 1993;Boarder et al., 1995; Boarder and Hourani, 1998; Ralevic and Burnstock,1998). Currently, seven mammalian P2X receptors (P2X_1-7)and eight mammalian P2Y receptors (P2Y₁, P2Y₂, P2Y₄, P2Y₆, P2Y₁₁,P2Y₁₂, P2Y₁₃, and P2Y₁₄) have been cloned and functionally characterized(Ralevic and Burnstock, 1998; von Kugelgen and Wetter, 2000; Communiet al., 2001; Nicholas, 2001; Sak and Webb, 2002). P2X receptorsfunction as nonselective cation channels with inwardly rectifyingcurrent-voltage relationships (Dubyak and el-Moatassim, 1993;Ralevic and Burnstock, 1998). Activation of these receptors withATP or 2-methylthio-ATP (2MeS-ATP) produces membrane depolarization.P2Y₁, P2Y₂, P2Y₄, and P2Y₆ receptors couple to G_q/11 and activatephospholipase C, resulting in increased inositol phosphate-3 formationand mobilization of intracellular Ca²⁺ (Parr et al., 1994; Communi et al., 1995; Schachter et al., 1996;Lazarowski et al., 2001). The P2Y₁₁ receptor activates both phospholipaseC and adenylyl cyclase (Communi et al., 1997), whereas P2Y₁₂ andP2Y₁₃ receptors are coupled solely to G_i and inhibition of adenylylcyclase (Daniel et al., 1998; Hollopeter et al., 2001). P2Y₁₄receptors are orphan G protein-coupled receptors that are activatedby UDP-glucose and couple to the G_i/o class of G proteins (Chamberset al., 2000). The skate (s) P2Y receptor has 61 to 64% sequencesimilarity to the human (h) P2Y₁ receptor, is coupled to G_q/phospholipaseC, and has a rank order of potency similar to the P2Y₁ receptor(Dranoff et al., 2000).

Previously, we showed that agonist activation of the P2Y₁ receptor expressed in Xenopus laevis oocytes stimulated a slowlyactivating inward current that inactivated within seconds afterstimulation (O'Grady et al., 1996). The channel exhibits steady-stateinactivation at strong hyperpolarizing potentials. This inwardcurrent was identified previously as the transient inward (T_in)current and was first observed after injection of mRNA from ratbrain (Parker et al., 1985) and subsequently observed when cloned5-hydroxytryptamine-1a and 5-hydroxytryptamine-2c receptors wereexpressed in oocytes (Ni et al., 1997). The channel is expressedin stage V and VI oocytes but seems to be absent in earlier stagesof oocyte maturation. It is reversibly blocked by polyvalent cationsincluding Ba²⁺, Mn²⁺, and La³⁺. T_in current activation requires membrane hyperpolarization andan increase in intracellular Ca²⁺ (Parker et al., 1985; Ni et al., 1997). Expression of G $alpha$ _q inmature oocytes was found to be sufficient for activation of theT_in current (Guttridge et al., 1995). The channel responsiblefor the T_in current has not been cloned and seems to representa new family of ion channels that has not been previouslycharacterized.

Interactions between expressed membrane proteins and endogenous ion channels that produce altered properties of these channelshave been documented previously. For example, previous studiesof Ca²⁺-activated Cl channels (CaCC) in bovine artery endothelial cells showed thatbiophysical properties of the channel could be modulated by expressionof cystic fibrosis transmembrane conductance regulator (CFTR)(Wei et al., 2001). Stimulation of the cells with forskolin and3-isobutyl-1-methylxanthine produced activation of CFTR and simultaneouslyinhibited ATP-dependent activation of endogenous CaCC activity.This effect of CFTR on the regulation of CaCC function was independentof the PDZ domain located at the C terminus of CFTR, but was shownto involve sequences within the R domain. CFTR has also been shownto modulate the function of amiloride-sensitive Na⁺ channels expressed in X. laevis oocytes (Boucherot et al., 2001).In this study, the first functional nucleotide-binding domain(NBF1) was proposed to be an interaction site between the twochannels because mutations in the NBF1 region of CFTR resultedin a decrease in its ability to inhibit amiloride-sensitive Na⁺ channelactivity.

In this study, we examined the effects of native P2Y receptor subtypes on channel function and observed that several membersof the P2Y receptor family modified the functional propertiesof the channel. To address the hypothesis that these receptorsmodulate the gating and voltage dependence of the T_in channelthrough membrane-delimited interactions involving specific structuraldomains of the receptor, we constructed truncation mutants andchimeric receptors involving the C-terminal regions of hP2Y₁ andhP2Y₂ receptors and determined the effects of these mutationson the biophysical properties of the T_in channel. Our resultsindicate that the C-terminal domains of these P2Y receptors areinvolved in regulating voltage dependence or inactivation gatingof the T_in channel. An analysis of C-terminal sequences of P2Yreceptors suggests that there are protein-protein interactiondomains, distinct from their PDZ-binding motifs, which are involvedin the coupling and modulation of channelfunction.

	Materials and Methods

Top Abstract Introduction Materials and Methods Results and Discussion References

Materials. X. laevis frogs were purchased from Xenopus I (Ann Arbor, MI) and maintained in aquaria as suggested by the supplier. Collagenaseand gentamicin were obtained from Invitrogen (Carlsbad, CA). 2MeS-ADPand 2MeS-ATP were obtained from Sigma/RBI (Natick, MA). UDP, UTP,carbachol, bradykinin, and isoproterenol were obtained from Sigma(St. Louis, MO). [D-Pen²,D-Pen⁵]-enkephalin was obtained from Bachem Biosciences (King of Prussia,PA).

Construction of Truncated and Chimeric Receptors. Truncated P2Y receptors were constructed by polymerase chain reaction using a 3' primer with a stop codon at the desired locationand an XhoI restriction site to aid in subcloning. Chimeric receptorswere generated by overlap-extension polymerase chain reaction(Ho et al., 1989). All receptor constructs were verified by sequencingand were subcloned intopcDNA3.

Preparation of RNA for Injection. cRNA was synthesized from linear cDNA encoding either wild-type P2Y receptor or mutants using Megascript (Ambion, Austin,TX).

Oocyte Isolation and Injection. Ovarian lobes from adult X. laevis frogs were removed from anesthetized animals under sterile condition. The tissue mass wasdissociated with collagenase solution (90 mM NaCl, 1 mM KCl, 0.82mM MgSO₄, 10 mM HEPES, pH 7.4, and 250 units/ml collagenase).Stage V and VI oocytes were sorted, defolliculated, and maintainedin modified Barth's saline solution (MBS solution: 90 mM NaCl,2 mM KCl, 0.82 mM MgSO₄, 0.74 mM CaCl₂, and 10 mM HEPES, pH 7.4,supplemented with 0.05 µg/µl gentamicin) at 19 to 20°C. Oocyteswere injected with cRNA transcripts (46 ng/oocyte) using a Nanojectoocyte injection system (Drummond Scientific (Broomall, PA). Controloocytes were injected with 46 nl of sterile water. Oocytes werestored for 2 to 7 days in MBS solution beforeanalysis.

Peptide Synthesis and Purification. Peptides of 20 amino acids corresponding to the C-terminal sequence of the hP2Y₁ receptor (RKASRRSEANLQSKSEDMTL) or the hP2Y₂receptor (RRSDRTDMQRIGDVLGSSED) were synthesized by the MicroChemicalFacility at the University of Minnesota (St. Paul, MN). Peptideswere purified by high-pressure liquid chromatography before injection,and the appropriate amino acid composition was confirmed by aminoacidanalysis.

Electrophysiological Measurements. Electrophysiological measurements were made using the two-electrode voltage-clamp technique at 20°C. Recordings were conductedin Cl-free MBS solution (90 mM NaMeSO₄, 2 mM KMeSO₄, 0.82 mM MgSO₄,0.74 mM calcium gluconate, and 10 mM HEPES, pH 7.4). Electrodeswere placed in a separate Cl-containing MBS solution and connected to the oocyte bathing solutionwith an agar bridge. Current- and voltage-measuring electrodeswere pulled from borosilicate filament glass to resistances between2 and 5 M $Omega$ when filled with 0.5 M KCl. Data acquisition and analysiswas performed with a Pentium PC using pCLAMP 8 software (AxonInstruments, Inc., Union City,CA).

Analysis and Statistics. Statistical significance was determined using Student's t test. Statistical significance was accepted at p < 0.05. Conductance-voltagerelationships were analyzed using a Boltzmann function (Y = 1/1+ exp(V₅₀ $-$ X/slope factor), where V₅₀ represents the voltageat which the conductance is half-maximal, slope factor representsthe relative degree of voltage dependence (steepness of the curve),Y represents the normalized conductance, G/G_{140 mV}, andX represents a specificvoltage.

	Results and Discussion

Top Abstract Introduction Materials and Methods Results and Discussion References

We previously reported that 2MeS-ADP stimulation of X. laevis oocytes expressing the hP2Y₁ receptor activated a voltage-dependentcurrent with gating characteristics that were identical with theendogenous T_in channel in oocytes (O'Grady et al., 1996). Theability to measure these currents was dependent on receptor expressionand on the presence of agonist. We followed up on these initialstudies and report here that although all G_q-coupled P2Y receptorsare capable of activating T_in channel currents in the presenceof their cognate agonists, the electrophysiological propertiesof the channel vary markedly depending on the subtype of thereceptor.

Bradykinin Activation of the hB₁-Bradykinin Receptor Elicits T_in Currents in X. laevis Oocytes. Figure 1A shows representative T_in current traces recorded from oocytes expressing the G_q-coupled hB₁-bradykinin receptor.Oocytes were held at 0 mV and then stepped to $-$ 140 mV and +80mV in the presence of a 2 µM bradykinin. In the absence of eitherreceptor mRNA or bradykinin, no time-dependent currents were observedupon hyperpolarization. In contrast, bradykinin elicited a characteristicT_in channel current in oocytes injected with hB₁-bradykinin receptormRNA but not in noninjected oocytes (data not shown). Resultsfor several G_q-coupled P2Y receptors were very similar, with theexception that a varying amount of T_in channel activation wasobserved under basal conditions in oocytes expressing P2Y receptorsbefore agonist stimulation (O'Grady et al., 1996). This basalactivation was probably caused by the accumulation in the bathingsolution of nucleotides released from oocytes, a result similarto that observed in mammalian cells (Parr et al., 1994; Schachteret al., 1996).

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Fig. 1. Voltage dependence of the T_in current elicited by agonist-activated G_q-coupled receptors expressed in X. laevis oocytes. A, representative current traces recorded from oocytes expressing the hB₁-bradykinin receptor. Oocytes were held at 0 mV and then stepped from $-$ 140 mV to +80 mV in 20-mV increments. The data represent peak inward current at each voltage step. The I-V relationship was fit with a Boltzmann function. The reversal potential of hB₁-bradykinin receptor was determined from the fit and had a value of +13 mV. B, normalized conductance as a function of voltage for the T_in channel activated by hP2Y₁ (n = 13), hP2Y₄ (n = 9), rM₁-muscarinic (n = 16), and hB₁-bradykinin (n = 13) receptors. C, normalized conductance as a function of voltage for hB₁-bradykinin (n = 13), hP2Y₁ (n = 13), hP2Y₁₁ (n = 15), and the sP2Y (n = 12) receptors. The V₅₀ values and slope factors for each conductance are listed in Table 1. D, the effects of hP2Y₁ receptor expression levels on the conductance-voltage relationship of the T_in channel; inset: conductance values obtained from oocytes injected with increasing amounts of hP2Y₁ receptor mRNA (nanograms).

Voltage Dependence of the T_in Current Elicited by Agonist-Activated G_q-Coupled Receptors Expressed in X. laevis Oocytes. Figure 1B shows the normalized conductance-voltage relationships for G_q-coupled receptors expressed in X. laevis oocytes.Only G_q-coupled receptors elicited T_in channel currents, becauseagonist-activated $beta$ ₂-adrenergic (50 µM isoproterenol; G_s-coupled), $delta$ -opioid (5 µM [D-Pen²,D-Pen⁵]-enkephalin; G_i-coupled), M₂-muscarinic (10 µM carbachol; G_i-coupled),and P2Y₁₂ (20 µM 2MeS-ADP; G_i-coupled) receptors were unable toactivate T_in currents after hyperpolarization (data not shown).The conductance-voltage curves were analyzed using a Boltzmannfunction, where V₅₀ represents the voltage at which the conductancewas half-maximal (described under Materials and Methods). TheV₅₀ value for the conductance activated by the hP2Y₁ receptor,but not the rat (r) M₁-muscarinic or hP2Y₄ receptor, was shiftedmarkedly to a more negative voltage compared with the conductanceactivated by the hB₁-bradykinin receptor and was significantlydifferent from the V₅₀ value elicited by the hB₁-bradykinin receptor(Table 1). Two other P2Y receptors, the hP2Y₁₁ and the sP2Y receptors,also activated currents with significantly more negative V₅₀ valuesthan the currents activated by the hB₁-bradykinin or the rM₁-muscarinicreceptor (Fig. 1C) (Table 1).

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TABLE 1
V₅₀and slope factor values of T_in currents elicited by agonist-activated receptors

To investigate the effect of receptor expression levels on the voltage sensitivity of the T_in channel, we injected increasingamounts of hP2Y₁ receptor mRNA into oocytes and monitored theconductance-voltage relationships after receptor activation witha maximum activating concentration (20 µM) of 2MeS-ADP (O'Gradyet al., 1996

) (Fig. 1D). Whereas increasing hP2Y₁ receptor mRNAelicited higher peak conductance levels, it had no effect on thevoltage sensitivity of the T_in channel. These data strongly suggestthat the modulation of T_in channel voltage sensitivity by thehP2Y₁ receptor is independent of the level of receptorexpression.

Role of the hP2Y₁ Receptor C Terminus in Modulating T_in Channel Voltage Sensitivity. The data presented above suggest that the hP2Y₁ and hP2Y₁₁ receptors not only activate T_in channels, but also modulate channelproperties, possibly through direct protein-protein interactions.To test this hypothesis, we examined the conductance-voltage relationshipof the T_in current elicited by a chimeric hB₁-bradykinin receptorin which the C-terminal domain was replaced by the C-terminalregion from the hP2Y₁ receptor (hB₁/Y₁). Figure 2A shows thatthe conductance-voltage relationship of the T_in channel elicitedby the hB₁/Y₁ chimeric receptor was essentially identical withthat elicited by the activated hP2Y₁ receptor. These data demonstratea "gain in function" of the hB₁-bradykinin receptor containingthe hP2Y₁ receptor C-terminal domain and strongly suggest thatthe C-terminal region of the hP2Y₁ receptor is involved in regulatingthe properties of the T_in channel.

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Fig. 2. Effect of C-terminal truncation on the conductance-voltage relationship. A, normalized conductance as a function of voltage for T_in currents elicited by activated hB₁-bradykinin (n = 13), hP2Y₁ (n = 13), and hB₁/Y₁ chimeric (n = 6) receptors. B, location of truncation mutations introduced into the hP2Y₁ receptor. The last four amino acids, DTSL, represent a consensus class 1 PDZ-binding motif. C, normalized conductance as a function of voltage for T_in currents elicited by activated hB₁-bradykinin (n = 13), hP2Y₁ (n = 13), hP2Y₁360tr (n = 17), and hP2Y₁369tr (n = 10) receptors. D, normalized conductance as a function of voltage for T_in currents elicited by activated hP2Y₁ (n = 13), hP2Y₁334tr (n = 9), hP2Y₁342tr (n = 18), and hP2Y₁349tr (n = 9) receptors. The V₅₀ values and slope factors for each conductance are listed in Table 1.

To further characterize the region of the hP2Y₁ receptor C-terminal domain involved in modulating the biophysical propertiesof the T_in channel, we analyzed the conductance-voltage relationshipsof the T_in current elicited by a series of carboxyl terminal truncations(Fig. 2B). Removal of either the PDZ-binding motif (hP2Y₁369tr)or the last 13 amino acids (hP2Y₁360tr) from the C terminus ofthe hP2Y₁ receptor had no effect on the V₅₀ values for the T_inchannel compared with the full-length wild-type receptor (Fig.2C) (Table 1). In contrast, deletion of either 31 (hP2Y₁342tr)or 39 (hP2Y₁334tr) amino acids from the C terminus resulted inV₅₀ values that were very similar to those elicited by hB₁-bradykinin,rM₁-muscarinic, and hP2Y₄ receptors (Fig. 2D) (Table 1). Deletionof 24 amino acids (hP2Y₁349tr) resulted in an intermediate phenotype,with a V₅₀ value in between the full-length hP2Y₁ receptor andthe truncation mutant missing the entire C-terminaldomain.

Role of the C-Terminal Domain of the hP2Y₂ and rP2Y₆ Receptors in T_in Channel Inactivation Gating. We also observed a marked difference in the inactivation gating of the T_in channel depending on which P2Y receptor was responsiblefor activating the current. Thus, whereas the current elicitedby the hP2Y₁ receptor was almost completely inactivated within3 s of the hyperpolarizing pulse, the current elicited by eitherthe hP2Y₂ (stimulated with 40 µM UTP) or the rP2Y₆ receptor (stimulatedwith 40 µM UDP) showed significantly slower inactivation. (Fig.3A). As observed with the voltage gating of the channel, the timecourse of inactivation was dependent on the identity of the C-terminaldomain of the receptor. Thus, the inactivation time courses ofthe hP2Y₁ receptor containing the hP2Y₂ C-terminal domain (hY₁/Y₂chimera) (Fig. 3A) or the hB₁-bradykinin receptor containing thehP2Y₂ C-terminal domain (hB₁/Y₂) (Fig. 3B) were identical withthat of the wild-type hP2Y₂ receptor (Fig. 3A).

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Fig. 3. Inactivation gating of receptor-activated T_in currents. A, representative traces of the T_in conductance elicited by activated hP2Y₁, rP2Y₆, hP2Y₂, and hY₁/Y₂ chimeric receptors. T_in channels were monitored for 5 s in the presence of the appropriate receptor agonist. UTP (40 µM) and UDP (40 µM) were used to stimulate the hP2Y₂ and rP2Y₆ receptors, respectively (Parr et al., 1994

; Communi and Boeynaems, 1997

). 2MeS-ADP (20 µM) was used to activate the hP2Y₁ receptor and hY₁/Y₂ chimeric receptors. B, representative traces of currents elicited by agonist-activated hB₁-bradykinin and hB₁/Y₁, and hB₁/Y₂ chimeric receptors after step hyperpolarization to $-$ 140 mV. C, I_final/I_max is the current amplitude at the end of the voltage pulse (as indicated by the open arrows in parts A and B) divided by the maximum inward current and represents the degree of T_in channel inactivation gating. This ratio was significantly increased in hP2Y₂ (n = 10), rP2Y₆ (n = 11), hY₁/Y₂ (n = 7), hY₂/Y₁ (n = 7)_, and hB₁/Y₂ (n = 7) chimeric receptors (p < 0.05).

Figure 3C shows the ratio of the current amplitude at the end of the voltage pulse ( $-$ 140 mV, 3.8 s) to the maximum inwardcurrent elicited by a series of activated receptors. As suggestedby the current traces in Fig. 3, A and B, the ratio derived fromthe hP2Y₁ receptor-activated currents was near zero. In contrast,the ratio was nearly 0.8 for the current elicited by the hP2Y₂receptor, rP2Y₆ receptor, and the hY₁/Y₂ chimera, indicating slowinactivation. Although the ratio of the current elicited by thehY₂/Y₁ chimera was significantly decreased compared with wild-typehP2Y₂ receptor, it was still significantly greater than that observedafter hP2Y₁ and hP2Y₄ receptoractivation.

C-Terminal Sequence Comparisons of P2Y Receptors. Figure 4 compares the C-terminal sequences of all five of the G_q-coupled P2Y receptors (P2Y₁, P2Y₂, P2Y₄, P2Y₆, and P2Y₁₁).Within the C-terminal domains of the hP2Y₁, hP2Y₁₁, and sP2Y receptor,all of which modulate the voltage activation of the T_in channel,a common sequence motif was observed (RRSE $---$ QXK/RSE)(bold letters identify conserved amino acids between P₂Y receptorsubtypes). Importantly, this sequence motif falls within the narrowregion of the hP2Y₁ receptor C-terminal domain shown to be involvedin modulating voltage sensitivity (Fig. 2). Likewise, a differentconserved sequence motif (QRXG/R) was observed in the C-terminaldomains of the hP2Y₂ and rP2Y₆ receptor, both of which modulateT_in channel inactivation. This motif is not present in the otherP2Y receptors.

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Fig. 4. C-terminal sequence comparisons between P2Y receptors. The underlined and bolded amino acids represent potential sequences involved in protein-protein interactions with the T_in channel. hP2Y₁, hP2Y₁₁, and sP2Y receptors modulate voltage dependence, whereas hP2Y₂ and rP2Y₆ receptors modulate inactivation gating. A similar sequence motif affecting inactivation gating of the channel is present in the mouse (m) P2Y₆ receptor. The boxed amino acids in the hP2Y₁ and hP2Y₂ receptor sequences indicate the peptide sequences used for experiments shown in Fig. 5.

Effects of Y1 and Y2 C-Terminal Peptides on the Conductance-Voltage Relationships and Inactivation Gating of the T_in Channel. To examine whether the unique sequence motif present in the C-terminal region of the hP2Y₁ receptor was able to modulate theconductance-voltage relationship of the T_in current, a syntheticpeptide (Y1 peptide) (boxed region in Fig. 4) was injected intohP2Y₁342tr-expressing oocytes (final concentration $approx$ 500 nM),and the conductance-voltage relationship of the T_in channel wasdetermined (Fig. 5A). The V₅₀ value of the conductance elicitedby the hP2Y₁342tr receptor with 500 nM Y1 peptide ( $-$ 72.3 mV) wassignificantly different from the value elicited by the hP2Y₁342trreceptor alone (V₅₀ = $-$ 49.0 mV) and similar to that elicited bythe wild-type hP2Y₁ receptor (V₅₀ = $-$ 72.5 mV) (Table 1). TheY1 peptide produced a similar negative shift in the V₅₀ value( $-$ 68.0 mV) in oocytes expressing the hB₁-bradykinin receptor comparedwith the hB₁-bradykinin receptor alone ( $-$ 43.0 mV) (Fig. 5B).

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Fig. 5. Effect of Y1 and Y2 C-terminal peptides on the conductance-voltage relationship and inactivation gating of T_in currents. A, normalized conductance as a function of voltage of T_in currents elicited by the agonist-activated hP2Y₁342tr receptor (Y₁tr; n = 18), hP2Y₁342tr receptor with 500 nM Y1 peptide (n = 8), and hP2Y₁ receptor (n = 13). B, normalized conductance as a function of voltage of T_in currents elicited by the hB₁-bradykinin receptor (n = 13), the hB₁-bradykinin receptor with 500 nM Y1 peptide (n = 7), and the hP2Y₁ receptor (n = 13). C, I_final/I_max ratios of the T_in current elicited by the indicated receptors were calculated as described in the legend to Fig. 3. The ratios were significantly increased for the hP2Y₁342tr receptor with 500 nM Y2 peptide (n = 6), the hB₁-bradykinin receptor with 500 nM Y2 peptide (n = 6), and the hP2Y₂ receptor (n = 10) (p < 0.05).

To examine whether the proposed sequence motif present in the C-terminal region of the hP2Y₂ receptor was able to modulatethe inactivation gating of the T_in current, a 20 amino acid peptide(Y2 peptide) (boxed region in Fig. 4) from the C terminus of thehP2Y₂ receptor encompassing this sequence was injected into hP2Y₁342tr-or hB₁-bradykinin receptor-injected oocytes (final concentration $approx$ 500 nM), and the inactivation gating of the T_in channel wasdetermined. Figure 5C shows the ratio of the current amplitudeat the end of the voltage pulse ( $-$ 140 mV) to the maximum inwardcurrent observed after activation. The ratio obtained from thehP2Y₁342tr and hB₁-bradykinin receptor-activated currents wasnearly zero, whereas the ratio for the current elicited by hP2Y₁342tror hB₁-bradykinin receptor with Y2 peptide was significantly increased(although not to the same level) compared with hP2Y₁342tr andhB₁- bradykinin receptor-activated currents alone or hP2Y₁342trand hB₁-bradykin receptor-activated currents with Y1peptide.

Taken together, these data strongly suggest that the C termini of the hP2Y₁ and hP2Y₂ receptors interact in some manner withthe T_in channel to modulate its biophysical properties. We hypothesizethat two sequence motifs, RRSE $---$ QXK/RSE and QRXG/R,located in the C-termini of P2Y receptors, are important protein-proteininteraction sites between P2Y receptors and the T_in channel, oralternatively an intermediate adapter protein. The presence ofmultiple protein-protein interaction domains within the C-terminalregion of P2Y receptors suggests that these receptors can coupleto a variety of membrane-associated proteins and potentially influencetheir function, independent of G-protein activation. Future studiesdirected toward identifying additional interacting protein partnersshould provide better insight into the role of protein-proteininteractions in P2Y receptorsignaling.

	Acknowledgments

We thank Drs. Linda Boland and Ken Harden for helpful comments andsuggestions.

	Footnotes

Received October 17, 2002; Accepted January 3, 2003

This work was supported in part by a grant from the Minnesota Applied Ecological Services (project 82) to S.M.O.

Address correspondence to: Dr. Scott M. O'Grady, Departments of Physiology and Animal Science, University of Minnesota, 495 Animal Science/Veterinary Medicine Building, 1988 Fitch Avenue, St. Paul, MN, 55108. E-mail: ograd001{at}umn.edu

	Abbreviations

2MeS, 2-methylthio-; T_in, transient inward; CaCC, Ca²⁺-activated Cl channels; CFTR, cystic fibrosis transmembrane conductance regulator; PDZ, PSD-95, Disc-large, and ZO-1; MBS, modified Barth's saline; prefixes, s, skate; h, human; r, rat.

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