Abstract
The orphan receptor GPR80 (also called GPR99) was recently reported to be the P2Y15 receptor activated by AMP and adenosine and coupled to increases in cyclic AMP accumulation and intracellular Ca2+ mobilization (Inbe et al. J Biol Chem 2004; 279: 19790–9[12]). However, the cell line (HEK293) used to carry out those studies endogenously expresses A2A and A2B adenosine receptors as well as multiple P2Y receptors, which complicates the analysis of a potential P2Y receptor. To determine unambiguously whether GPR80 is a P2Y receptor subtype, HA-tagged GPR80 was either stably expressed in CHO cells or transiently expressed in COS-7 and HEK293 cells, and cell surface expression was verified by radioimmunoassay (RIA). COS-7 cells overexpressing GPR80 showed a consistent twofold increase in basal inositol phosphate accumulation. However, neither adenosine nor AMP was capable of promoting accumulation of either cyclic AMP or inositol phosphates in any of the three GPR80-expressing cells. A recent paper (He et al. Nature 2004; 429: 188–93 [15]) reported that GPR80 is a Gq-coupled receptor activated by the citric acid cycle intermediate, α-ketoglutarate. Consistent with this report, α-ketoglutarate promoted inositol phosphate accumulation in CHO and HEK293 cells expressing GPR80, and pretreatment of GPR80-expressing COS-7 cells with glutamate dehydrogenase, which converts α-ketoglutarate to glutamate, decreased basal levels of inositol phosphates. Taken together, these data demonstrate that GPR80 is not activated by adenosine, AMP or other nucleotides, but instead is activated by α-ketoglutarate. Therefore, GPR80 is not a new member of the P2Y receptor family.
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Introduction
Extracellular adenine and uridine nucleotides exert their physiological effects through two main receptor families: The ligand-gated ion channel P2X receptors and the G protein-coupled P2Y receptors [1]. Molecular cloning and functional studies by a number of laboratories have identified eight functional mammalian P2Y receptor subtypes (P2Y1, P2Y2, P2Y4, P2Y6, P2Y11, P2Y12, P2Y13, and P2Y14) [2]. These receptors can be subdivided pharmacologically into the adenosine nucleotide-preferring P2Y receptors activated primarily by ATP and/or ADP (P2Y1, P2Y11, P2Y12, and P2Y13), the uridine nucleotide-preferring receptors (P2Y4, P2Y6, and P2Y14) activated by UTP, UDP or UDP sugars, and a receptor (P2Y2) activated equipotently by both ATP and UTP. From a phylogenetic, structural, and signaling point of view, P2Y receptors fall into two subfamilies. The P2Y1 receptor subfamily, which encompasses P2Y1, P2Y2, P2Y4, P2Y6 and P2Y11 receptors, shares 35%–52% sequence identity (with exception of 28%–30% identity of the P2Y11 receptor to the other four members) and couples to Gq thereby activating phospholipase C. The P2Y12 receptor subfamily, which includes P2Y12, P2Y13, and P2Y14 receptors, is located in a gene cluster on chromosome 3, shares 45%–55% identity, and couples to Gi/o and thereby inhibits adenylyl cyclase.
The identification and naming of new P2Y receptors has been controversial and has led to considerable confusion in P2Y receptor nomenclature. For example, four receptors were originally identified as P2Y receptors (P2Y5, P2Y7, P2Y9, and P2Y10) [3, 4] but were shown later either to not respond to nucleotides (P2Y5, P2Y7) [5, 6] and/or to be activated by a non-nucleotide ligand (P2Y7, P2Y9) [7, 8]. Moreover, two additional receptors, chick P2Y3 [9] and Xenopus P2Y8 [10] receptors, are likely species homologues of human P2Y6 and P2Y4 receptor subtypes, respectively [11]. Problems in identifying new P2Y receptors arise in part because of (1) the low sequence identity between bona fide P2Y receptor subtypes, (2) the lack of a generally applicable radioligand for P2Y receptors, (3) endogenous expression of one or more subtypes of P2Y and adenosine receptors on model cell lines in which potentially new receptors are expressed and characterized, and (4) extracellular metabolism and inter-conversion of nucleotides, which can lead to unintended or misleading responses to added nucleotides. Thus, identification of a new receptor in the P2Y family requires rigorous demonstration of receptor activity.
Recently, the orphan receptor GPR80 (also called GPR99), which encodes a protein of 337 amino acids with 25%–36% sequence identity (43%–58% similarity) to members of the P2Y1 receptor subfamily, was reported to be the P2Y15 receptor and to mediate AMP- and adenosine-promoted increases in cyclic AMP accumulation and mobilization of intracellular Ca2+ [12]. However, the cell line (HEK293) used to examine the pharmacological selectivity of recombinant GPR80 endogenously expresses P2Y1, P2Y2, P2Y4, P2Y12 and P2Y13 receptors as well as A2A and A2B adenosine receptors [12–14], which markedly obfuscates the potential study of recombinant receptors activated by either nucleotides or nucleosides. Moreover, a recent study reported activation of GPR80 by the citric acid cycle intermediate α-ketoglutaric acid [15], which further calls into question the assertion that GPR80 is a receptor for adenosine and AMP.
To determine unambiguously whether GPR80 is a new P2Y receptor subtype, HA-tagged GPR80 was stably expressed in CHO cells or transiently expressed in COS-7 and HEK293 cells, and activation by AMP and adenosine was evaluated by measuring both inositol phosphate and cyclic AMP accumulation. Our data demonstrate that GPR80 is not activated by adenosine, AMP, or any other nucleotides, but instead is activated by the citric acid cycle intermediate, α-ketoglutarate, as reported by He et al. [15].
Materials and methods
Materials
All cell culture reagents were supplied by the tissue culture facility in the Lineberger Comprehensive Cancer Center (University of North Carolina at Chapel Hill). AMP, adenosine, ADP, UDP, α-ketoglutarate, adenosine deaminase (ADA), Ro20-1724, glutamate dehydrogenase, and carbachol were from Sigma (St Louis, Missouri, USA). ATP, UTP, and the transfection reagent FuGENE6 were from Roche Biochemicals (Indianapolis, Indiana, USA). Forskolin was purchased from Calbiochem (La Jolla, California, USA). Suramin and PPADS (pyridoxal-phosphate-6-azophenyl-2′, 4′-disulphonic acid) were from RBI (Natick, Massachusetts, USA).
Construction of HA-tagged GPR80 cDNA
The coding sequence of GPR80 was amplified by PCR with Pfu polymerase (Stratagene) from human genomic DNA. The 5′ primer (5′-GAGACGCGTCCAATGAGCCACTAGACTATTTA-3′) was complementary to codons 2–7 of GPR80 and contained an MluI site at the 5′ end, while the 3′ primer (5′-AGACTCGAGTCAAGGGTTGTTTGAGTAACTGATT-3′) was complementary to codons 337–331 and contained a XhoI site following the stop codon. The amplified cDNA was digested with MluI and XhoI and ligated in-frame into a similarly digested pLXSN retroviral expression vector containing an upstream EcoRI restriction site, Kozak initiation sequence, initiating methionine residue, and the hemagglutinin (HA) epitope tag (YPYDVPDY) to yield pLXSN-GPR80. To construct pcDNA3-GPR80, pLXSN-GPR80 was digested with EcoRI and XhoI and ligated into the similarly digested expression vector, pcDNA3.
Transient expression of GPR80 in COS-7 and HEK293 cells
All cells were maintained in DMEM-High Glucose (DMEM-H) with 10% serum. Transient transfection of COS-7 and HEK293 cells was performed according to protocols supplied with the FuGENE6 reagent. Briefly, 1.5×106 cells per 60-mm dish were incubated overnight in 4 ml medium. The next day, 8 µl FuGENE6 and 2.8 µg of either pcDNA3 or pcDNA3-GPR80 in 400 µl serum-free DMEM-H was added to the cells for 5–6 h. The transfected cells then were trypsinized and seeded in 24-well plates for assays.
Stable expression of GPR80 in CHO cells
The procedure for stable receptor expression was described in detail previously [16]. Briefly, recombinant retrovirus particles were produced by calcium phosphate-mediated transfection of PA317 cells with pLXSN or pLXSNGPR80 and used to infect CHO cells. Geneticin-resistant cells were selected with DMEM-H containing 1 mg/ml G418.
Assays for inositol phosphate and cyclic AMP accumulation
CHO cells were seeded in 24-well plates at 5×104 cells/well and assayed 3 days later. For transiently transfected COS-7 and HEK293 cells, 2×105 cells/well were seeded in 24-well plates and assayed 2 days later. Inositol lipids were radiolabelled by overnight incubation of the cells with 200 µl serum-free, inositol-free DMEM containing 0.4 µCi myo-[3H]inositol per well. Agonists or antagonists were added at 5× concentration in 50 µl of 50 mM LiCl, 250 mM HEPES, pH 7.25. Following a 10-min incubation (30 min incubation in Figures 1C and 5) at 37 °C, the reaction was terminated by aspirating the medium and adding 0.75 ml boiling EDTA, pH 8.0. [3H]Inositol phosphates were resolved with Dowex AG1-X8 columns.
To monitor cyclic AMP accumulation, cells were labeled with 200 µl serum-free DMEM containing 0.8 µCi of [3H]adenine for 2 h. Twenty minutes prior to the assay, cells were supplemented with 50 mM HEPES, pH 7.4. Ro20-1724 (100 µM), which in contrast to IBMX used by Inbe and coworkers [12] does not inhibit adenosine receptors, was added 10 min prior to the initiation of the assay to inhibit cyclic nucleotide phosphodiesterases. Drugs were added at 6× concentration in 50 µl of Hank’s balanced salt solution (HBSS) for 10 min at 37 °C. Reactions were terminated by aspiration of the drugcontaining medium and addition of 1 ml of ice-cold 5% trichloroacetic acid. [3H]Cyclic AMP was purified using Dowex and alumina columns and quantified by scintillation counting.
Radioimmunoassay (RIA) to quantify cell surface expression
Cells were seeded in 24-well plates at the densities described above and assayed 2–3 days later as described previously [17]. Cells were fixed in 4% paraformaldehyde, washed, blocked, and then incubated with a 1:1,000 dilution of mouse anti-HA monoclonal antibody (clone HA.11) for 1 h. Cells were washed twice with HBSS containing 1 mM Ca2+ and Mg2+, followed by incubation with [125I]-labeled rabbit anti-mouse antibody. After incubating for 2 h, the cells were washed twice with HBSS containing Ca2+ and Mg2+, solubilized with 1 M NaOH, and transferred to glass tubes for quantitation of radioactivity by γ-counting.
Results
Transient expression of GPR80 in COS-7 cells
To identify the ligand(s) that activate GPR80, we first expressed the HA-tagged receptor transiently in COS-7 cells. GPR80 was well expressed in COS-7 cells as determined by a cell-surface RIA (Figure 1A). To assess the capacity of adenosine or AMP to activate GPR80, COS-7 cells were transfected with pcDNA3 or pcDNA3-GPR80 either with or without a plasmid encoding chimeric Gqiα [18], and then challenged with high concentrations (up to 100 µM) of adenosine or AMP. Gqiα is a chimeric Gα subunit in which the last five amino acids of Gqα have been replaced with the corresponding residues from Gia, allowing Gi-coupled receptors to activate phospholipase C and increase inositol phosphate accumulation.
Neither adenosine nor AMP promoted inositol phosphate accumulation in either vector- or GPR80-transfected cells (Figure 1B). Similarly, ATP, ADP, UTP, UDP and UDP-glucose (all at 100 µM) failed to promote inositol phosphate accumulation (data not shown).1 However, we consistently observed an approximately twofold increase in basal inositol phosphate accumulation in GPR80-transfected cells compared to vector-transfected cells, and this increase in basal levels was not affected by co-expression of Gqiα. The increase in basal inositol phosphate levels in GPR80-transfected cells and the absence of a further increase when GPR80 was co-expressed with Gqiα suggests that GPR80 is coupled to Gq/phospholipase C.
The GPR80-dependent increase of basal inositol phosphate accumulation could be due either to constitutive activity of the receptor or to the activation of GPR80 by endogenously released compounds. To assess whether adenosine is released and activates the receptor, cells were preincubated with 1 or 4 U/ml of adenosine deaminase for 1 h prior to the addition of Li and incubation for an additional 30 min. No decrease in inositol phosphate accumulation was observed in the presence of the adenosine-metabolizing enzyme (Figure 1C). We also tested the capacity of non-selective P2 receptor antagonists, PPADS and suramin, to inhibit basal accumulation of inositol phosphates, but both of these compounds had no effect.
Stable expression of GPR80 in CHO cells
CHO cells were utilized as an additional cell line to investigate the signaling properties of GPR80. HA-tagged GPR80 was stably expressed in CHO cells following retroviral infection, and immunoassays indicated that the receptor was well expressed in CHO cells (Figure 2A). Neither AMP nor adenosine (at 100 µM) promoted inositol phosphate or cyclic AMP accumulation (Figures 2B and D). In contrast, carbachol, which activates an endogenous muscarinic receptor, promoted a robust increase in inositol phosphates in both wild-type and GPR80-expressing cells (Figure 2B), and ATP (100 µM) promoted large increases in inositol phosphate accumulation in CHO cells exogenously expressing the P2Y11 receptor (Figure 2C). These data provide additional data in a different cell line demonstrating that neither AMP nor adenosine is an agonist for GPR80.
Transient expression of GPR80 in HEK293 cells
The studies of Inbe et al. [12] reporting AMP- and adenosine-promoted increases in intracellular calcium mobilization and cyclic AMP accumulation were carried out in HEK293 cells transiently transfected with GPR80. Although we did not observe the agonist activity of AMP or adenosine at GPR80 in either COS-7 or CHO cells, the possibility remained that an endogenous factor exists in HEK293 that combines with GPR80 to convey nucleotide/ nucleoside sensitivity to the receptor. To test this possibility, we transiently expressed GPR80 in HEK293 cells and tested the capacity of ATP, AMP and adenosine to promote inositol phosphate or cyclic AMP accumulation. Although HA-tagged GPR80 was well expressed in HEK293 cells (Figure 3A), neither AMP nor adenosine (up to 100 µM) promoted increases in inositol phosphate accumulation (Figure 3B) in cells transfected with GPR80 compared to the cells transfected with empty vector. A slight increase in inositol phosphate accumulation was observed with ATP, which presumably occurred due to activation of endogenous P2Y1 and P2Y2 receptors in HEK293 cells [13]. Both AMP and adenosine promoted cyclic AMP accumulation in HEK293 cells, but no difference was observed in cells transfected with empty vector versus cells expressing GPR80 (Figure 3C). Taken together, our data in three different cell lines demonstrate that GPR80 is not a receptor for either adenosine or AMP.
A citric acid cycle intermediate, α-ketoglutarate, is an agonist for GPR80
During the course of this work, α-ketoglutarate, a citric acid cycle intermediate, was reported to activate GPR80, promoting intracellular calcium mobilization and inositol phosphate accumulation through a Gq-mediated pathway [15]. To confirm these results, we assessed the capacity of α-ketoglutarate to promote inositol phosphate accumulation in CHO-GPR80 and in GPR80-transfected HEK293 cells. As shown in Figure 4, α-ketoglutarate increased inositol phosphate accumulation in a concentration-dependent manner in both cell lines, with an EC50 of 140 ± 10 µM in CHOGPR80 cells and 160 ± 20 µM in HEK293-GPR80 cells.
As shown above (Figures 1B and 1C), expression of GPR80 in COS-7 cells resulted in increased basal accumulation of inositol phosphates. To determine if GPR80-dependent increases in inositol phosphate accumulation was due to the presence of α-ketoglutarate in the medium, we utilized the enzyme glutamate dehydrogenase (GluDH), which catalyzes the conversion of α-ketoglutarate to glutamate in the presence of NADH, NH4 +, and ADP. COS-7 cells expressing GPR80 or empty vector were preincubated for 60 min with PBS, reaction buffer (135 µM NADH, 200 µM NH4Cl, 85 mM EDTA, and 100 µM ADP, final concentrations), or reaction buffer plus GluDH, and basal accumulation of inositol phosphate accumulation was assessed. As seen in Figure 5, pre-incubation with GluDH significantly lowered basal inositol phosphate accumulation in GPR80-expressing cells, although the levels were still higher than those in empty vector-transfected COS-7 cells.
Discussion
The nomenclature for P2Y receptors is confusing at best. Six receptors have erroneously been designated as P2Y receptors, which has led to considerable confusion and controversy in the P2 receptor field. Thus, all reports of potential new P2Y receptors should be viewed with caution until the results are independently verified by other labs. We show here that GPR80, which was reported to be the P2Y15 receptor activated by adenosine and AMP [12], is not a receptor for these compounds, and, consequentially, should not be included in the P2Y receptor family. By either stably or transiently expressing GPR80 in three different cell lines (COS-7, CHO, and HEK293), we have provided compelling evidence that although GPR80 is a functional Gq-coupled receptor, it is not activated by adenosine, AMP and other common nucleotides and nucleotide sugars, but instead is activated by the citric acid cycle intermediate, α-ketoglutarate, as first reported by He and coworkers [15].
In the study by Inbe et al. [12], AMP and adenosine promoted both intracellular Ca2+ mobilization and cyclic AMP accumulation in HEK293 cells expressing GPR80 but not in wild-type cells. However, our data from three different cell lines expressing GPR80, including HEK293 cells, demonstrate that AMP and adenosine have no such activity. What might be the source(s) of this discrepancy? Our data with HEK293 cells demonstrate that adenosine and to a lesser extent AMP promote robust cyclic AMP accumulation, whether or not GPR80 was expressed in these cells. Perhaps the stimulation of cyclic AMP accumulation in HEK293 cells stably expressing GPR80 versus wild-type HEK293 cells reflects a difference in the level of endogenous receptors expressed in the two cell lines, leading to the erroneous conclusion that stimulation was due to activation of GPR80. The Ca2+ mobilization response to adenosine and AMP observed in GPR80 cells also may have been due to differential expression of endogenous P2Y receptors and their activation by small amounts of contaminating nucleotides or by bioconversion of added nucleotides by ecto-enzymes. This is particularly relevant given the fact that the signal amplification inherent in Ca2+ measurements can result in large signals from activation of a receptor even at low receptor occupancy.
Although we were unable to observe a response to adenosine or AMP in GPR80-expressing COS-7 and CHO cells, one possibility to explain the discrepancy between our results and those of Inbe et al. [12] is that the HEK293 cells used to express GPR80 in the previous study might express an endogenous factor that was required for receptor activity. For example, P2Y1, P2Y2 , P2Y4 , P2Y12 and P2Y13 receptors or A2a and A2b receptors, all of which are expressed in HEK293 cells [12–14], might potentially form a heterodimer with overexpressed GPR80 and result in a receptor with novel pharmacological selectivity. For example, this phenomenon has been observed with mu and delta opioid receptors [19, 20] and with GABAB receptors [21] as well as with other receptors [22]. However, as in COS-7 and CHO cells, expression of GPR80 in HEK293 cells did not confer capacity of either adenosine or AMP to increase inositol phosphate or cyclic AMP accumulation over levels observed in vector-transfected cells. Thus, heterodimerization or expression of an endogenous factor in HEK293 cells apparently does not explain the results of Inbe et al. [12].
Interestingly, we consistently observed a twofold increase in basal inositol phosphate accumulation when GPR80 was expressed in COS-7 cells. This increase in basal inositol phosphate accumulation was reminiscent of increases observed upon expression of P2Y receptors in 1321N1 astrocytoma and other cell lines [23], which is due to the cellular release of nucleotides and autocrine/paracrine receptor activation [24]. We reasoned that the increased basal accumulation of inositol phosphates might also be due to release of an endogenous compound(s) that activated GPR80. The increased basal accumulation was not affected by increasing adenosine deaminase levels in the medium (Figure 1C), suggesting that adenosine was not the activating endogenous compound. Upon confirmation that GPR80 was activated by α-ketoglutarate, we investigated whether the increased basal inositol phosphates was due to release of α-ketoglutarate and subsequent autocrine/paracrine activation of the receptor. Indeed, addition of GluDH, which converts α-ketoglutarate to glutamate, significantly decreased the basal levels of inositol phosphate accumulation when added 60 min prior to addition of LiCl (to block inositol monophosphatase), although this decrease represented only a fraction of the total increase. Several possibilities might explain the relative impotence of GluDH in reducing basal accumulation of inositol phosphate accumulation in GPR80-expressing cells. These include: (1) addition of a suboptimal amount of enzyme (the maximum amount added was 10 U/ml), (2) inability of the enzyme to reduce α-ketoglutarate levels in the ‘unstirred layer’ at the extracellular surface of the cells [25], and (3) relatively low levels of inositol monophosphatase in COS-7 cells, which would result in substantial amount of GluDH-insensitive inositol phosphate accumulation prior to the addition of LiCl. Whatever the reason, our results do suggest that α-ketoglutarate release is involved in increased basal activity of GPR80.
Surprisingly, the increase in basal accumulation of inositol phosphates was observed only in COS-7 cells and not in CHO or HEK293 cells. Although this observation suggests that only COS-7 cells release α-ketoglutarate into the medium, an alternative explanation follows from the fact that COS-7 cells contain the SV40 large T antigen, which supports runaway plasmid replication following transfection with plasmids (such as pcDNA3) containing the SV40 origin of replication and eventually results in lytic death [26]. Thus, cell death may occur following transfection of COS-7 cells resulting in release of intracellular compounds, including α-ketoglutarate.
One interesting aspect of this work and that of He et al. [15] is the relatively low potency of α-ketoglutarate for activation of GPR80. The potency of α-ketoglutarate ranged from 32 and 69 µM in the aequorin and FLIPR assays, respectively, described by He and coworkers [15] to ∼150 µM in inositol phosphate accumulation assays reported here (Figure 4). These values are considerably higher than the potency of most natural nucleotides for activation of P2Y receptors. However, the citric acid cycle ensures a large reservoir of α-ketoglutarate and the mean level of α-ketoglutarate in rat plasma is about 25 µM [27, 28]. Given that α-ketoglutarate has the potential to be released from cells in a regulated fashion following receptor activation or mechanical stimulation, the levels of extracellular α-ketoglutarate could easily reach levels sufficient for activation of GPR80. Moreover, the recent work by Joseph and coworkers [25] has highlighted the lack of correlation between the concentrations of nucleotides in the bulk medium versus at the extracellular surface. Thus, the relatively high EC50 may allow relevant extracellular regulation of GPR80 under physiological conditions.
Note
Notes
Small increases of similar magnitude were observed in both vectorand GPR80-transfected cells upon addition of ATP, ADP, and UTP, presumably from activation of endogenous P2Y1 and P2Y2 receptors.
Abbreviations
- ADA:
-
adenosine deaminase
- Ado:
-
adenosine
- GluDH:
-
glutamate dehydrogenase
- HA:
-
hemagglutinin
- HBSS:
-
Hank’s balanced salt solution
- PBS:
-
phosphate-buffered saline
- PPADS:
-
pyridoxal-phosphate-6-azophenyl-2′,4′-disulphonic acid
- RIA:
-
radioimmunoassay
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Acknowledgement
This work was supported in part by National Institutes of Health Grants HL71131 (to R.A.N.) and GM38213 (to T.K.H.).
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Qi, AD., Harden, T.K. & Nicholas, R.A. GPR80/99, proposed to be the P2Y15 receptor activated by adenosine and AMP, is not a P2Y receptor. Purinergic Signalling 1, 67–74 (2004). https://doi.org/10.1007/s11302-004-5069-0
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DOI: https://doi.org/10.1007/s11302-004-5069-0