Abstract
The nociceptin/orphanin FQ (N/OFQ) peptide (NOP) receptor is the fourth and most recently discovered member of the opioid receptor superfamily that also includes μ, δ, and κ opioid receptor subtypes (MOR, DOR, and KOR, respectively). The widespread anatomic distribution of the NOP receptor enables the modulation of several physiologic processes by its endogenous agonist, N/OFQ. Accordingly, the NOP receptor has gained a lot of attention as a potential target for the development of ligands with therapeutic use in several pathophysiological states. NOP receptor activation frequently results in effects opposing classic opioid receptor action; therefore, regulation of the NOP receptor and conditions affecting its modulatory tone are important to understand. Mounting evidence reveals a heterologous interaction of the NOP receptor with other G protein–coupled receptors, including MOR, DOR, and KOR, which may subsequently influence their function. Our focus in this review is to summarize and discuss the findings that delineate the cellular mechanisms of NOP receptor signaling and regulation and the regulation of other receptors by N/OFQ and the NOP receptor.
Introduction
The multiplicity of opioid receptor subtypes enables opiates and endogenous opioid peptides to elicit diverse physiologic and pharmacological actions. Before the cloning of the NOP receptor [also known as opioid receptor–like 1, KOR3, OP4 (Bunzow et al., 1994; Chen et al., 1994; Fukuda et al., 1994; Mollereau et al., 1994; Wang et al., 1994; Wick et al., 1994; Pan et al., 1995)], the opioid receptor superfamily consisted of the classical MOR, DOR, and KOR. The NOP receptor sequence is approximately 50–60% identical to the classic opioid receptors; however, neither endogenous opioid peptides nor selective MOR, KOR, and DOR ligands [with the exception of KOR agonist, dynorphin A (Zhang et al., 1998)] bind to or activate the NOP receptor (Bunzow et al., 1994; Chen et al., 1994; Mollereau et al., 1994; Wang et al., 1994; Wick et al., 1994; Fukuda et al., 1997). Subsequently, two groups independently identified an endogenous neuropeptide similar to KOR agonist dynorphin A with little or no affinity for classic opioid receptor subtypes but high affinity for NOP receptor, emphasizing that this peptide and the NOP receptor are pharmacologically unique from the other opioid receptors (Meunier et al., 1995; Reinscheid et al., 1995). Reinscheid et al. named this heptadecapeptide orphanin FQ (OFQ), where “orphanin” refers to the peptide affinity for the recently cloned orphan opioid receptor; “F” (phenylalanine) and “Q” (glutamine) denote the first and last amino acids of the peptide, respectively (Reinscheid et al., 1995). Meunier et al. chose to name the peptide nociceptin (N) because of its pronociceptive activity (Meunier et al., 1995). For the purpose of this review, we have used both terms as denoted by N/OFQ for addressing this peptide.
Corresponding to the widespread distribution of the NOP receptor in the central and peripheral nervous systems [reviewed in Mollereau and Mouledous (2000) and Civelli (2008)], N/OFQ activation of the NOP receptor modulates many physiologic responses/systems, including anxiety (Jenck et al., 1997), food intake (Pomonis et al., 1996), learning (Sandin et al., 1997), locomotor (Reinscheid et al., 1995; Florin et al., 1996), respiratory (Fischer et al., 1998; Shah et al., 1998), immune (Peluso et al., 2001; Serhan et al., 2001), and cardiovascular and renal functions (Kapusta et al., 1997). To maintain this important modulatory role, the N/OFQ/-NOP receptor system therefore requires extensive and intricate regulation. Our focus in this review is to outline the findings that have advanced our understanding of NOP receptor signaling at the cellular level, how that signaling impacts NOP receptor function, and how N/OFQ and NOP receptors modulate other receptors.
NOP Receptor Signaling
The NOP receptor, like other opioid receptors, is a prototypical G protein–coupled receptor (GPCR) that couples to pertussis toxin–sensitive (Ma et al., 1997) and –insensitive (Chan et al., 1998) G proteins. After agonist activation, the NOP receptor triggers intracellular signaling events, including inhibition of adenylyl cyclase (Ma et al., 1997) and activation of protein kinase C (PKC) (Lou et al., 1997), phospholipase A (Fukuda et al., 1998) and C (Lou et al., 1997), extracellular signal-regulated kinases 1 and 2 (ERK1/2) (Fukuda et al., 1997; Lou et al., 1997), p38 mitogen-activated protein kinase (Zhang et al., 1999a), c-Jun N-terminal kinase (JNK) (Chan and Wong, 2000), nuclear factor κB (NFκB) (Donica et al., 2011), and modulation of calcium (Connor et al., 1996b) and potassium channel conductance (Connor et al., 1996a). N/OFQ-mediated inhibition of presynaptic, voltage-gated calcium channels has been demonstrated in vitro (Connor et al., 1996b) and in vivo (Knoflach et al., 1996). Furthermore, activation of the NOP receptor opens inwardly, rectifying potassium channels, and produces a postsynaptic hyperpolarization, preventing excitation or propagation of action potentials (Vaughan et al., 1997). The significance of kinase activation and channel modulation by N/OFQ directly relates to the ability of N/OFQ to modulate neurotransmitter release, immune function, and transcriptional activation.
N/OFQ modulation of ion channel activity appears to be responsible for its inhibition of acetylcholine, serotonin, dopamine, β-endorphin, norepinephrine, glutamate, and GABA neurotransmission in several brain regions, including, but not limited to, the locus coeruleus, periaqueductal gray (PAG), dorsal raphe nucleus, hippocampus, hypothalamus, ventral tegmental area, spinal cord, and rostral ventral medulla (Connor et al., 1996a; Vaughan and Christie, 1996; Vaughan et al., 1997; Yu et al., 1997; Connor and Christie, 1998; Wagner et al., 1998; Vaughan et al., 2001; Zheng et al., 2002; Lu et al., 2010).
The ability of N/OFQ and the NOP receptor to inhibit neurotransmitter release is the basis for its modulation of the many biologic functions that rely on synaptic transmission, including nociception, anxiety, and reward. For instance, the influx of calcium through the N-type calcium channel plays a critical role in regulating nociceptive signaling in the spinal cord. The NOP receptor associates with and inhibits N-type calcium channels, even in the absence of N/OFQ (Beedle et al., 2004). The constitutive regulation of N-type calcium channels in the dorsal root ganglion (DRG) cells by the NOP receptor is thought to be modulated by NOP receptor expression (Beedle et al., 2004). Although there is agreement over the ability of N/OFQ-NOP receptor system to inhibit N-type calcium channels, there is still some debate about whether this involves NOP receptor–mediated internalization of those channels. For instance, N/OFQ treatment induces N-type calcium channel internalization in a PKC-dependent manner, effectively inhibiting calcium influx into the cell (Altier et al., 2006). However, a recent study examining the effect of NOP receptor activation on N-type calcium channels in a highly N/OFQ-sensitive subpopulation of rat DRG and spinal cord neurons found that, although N/OFQ treatment inhibited primary afferent excitatory postsynaptic currents on dorsal horn neurons, it did not induce internalization of N-type calcium channels in the cell body or nerve terminals of DRG neurons (Murali et al., 2012). Thus, the precise means by which the NOP receptor regulates calcium channels in vivo is still under debate.
N/OFQ and NOP receptor are expressed on lymphocytes, monocytes, and peripheral blood mononuclear cells and in T cell and B cell lines, where they modulate synthesis and release of neuromodulators (Halford et al., 1995; Wick et al., 1995; Peluso et al., 1998; Arjomand et al., 2002). N/OFQ blocks synthesis of proinflammatory cytokines in the spinal cord, astrocytes, and splenocytes (Fu et al., 2007; Miller and Fulford, 2007) and inhibits Complete Freund’s adjuvant-induced increase in proinflammatory interleukin-6, interleukin-1β, and tumor necrosis factor–α mRNA in cultured astrocytes (Fu et al., 2007). N/OFQ-NOP receptor interactions also induce neutrophil chemotaxis (Fiset et al., 2003; Serhan et al., 2001), block antibody formation in vivo and in vitro in rodent spleen cells (Anton et al., 2010), and inhibit T cell function (Waits et al., 2004). Although the mechanisms underlying these actions have yet to be determined, they undoubtedly involve signaling through one or more of the aforementioned protein kinases. We recently reported that N/OFQ activates NFκB transcription factor, a critical player in immune system regulation (Donica et al., 2011). Activation of NFκB provides one mechanism by which the NOP receptor regulates immune system function. NOP receptor activation also leads to transcriptional changes, resulting in sustained regulation of biologic processes. NOP receptor activation of ERK1/2 stimulates the Elk-1 transcription factor, which has been implicated in disorders, such as drug addiction, depression, and long-term memory (Bevan et al., 1998), whereas activation of JNK stimulates c-Jun and activating transcription factor–2 (ATF-2) (Chan and Wong, 2000). ATF-2 stimulates transcription in response to stressors, such as hypoxia and infection, and is important in development, innate immunity, and oncogenesis (Seong et al., 2012). N/OFQ activation of G16-coupled NOP receptor phosphorylates STAT3, a regulator of myeloid cell differentiation that provides another means of regulating immune function (Wu et al., 2003). Prolonged N/OFQ exposure up-regulates the transcription factors NFκB (Donica et al., 2011), activating protein-2 (Thakker and Standifer, 2002a) and Oct-2 (Thakker and Standifer, 2002b), a protein associated with development (He et al., 1989), immune cell maturation and activation (Kang et al., 1992; Humbert and Corcoran, 1997), and inflammation (Ensor et al., 1996). The ability of NOP receptor to modulate gene transcription and acute functions underscores its significance and potential as a therapeutic target.
Homologous NOP Receptor Desensitization
Analogous to the cellular regulation of other GPCRs, the NOP receptor is regulated by the process of homologous desensitization. Homologous desensitization is a state of decreased responsiveness of the receptor resulting from persistent exposure to its agonist. Receptor desensitization strongly contributes to mechanisms of drug tolerance experienced after drug administration, such that more of the drug is required to produce the same response or effect. Desensitization of the NOP receptor occurs after both acute (Connor et al., 1996a; Mandyam et al., 2000; Mandyam et al., 2002; Thakker et al., 2007) and chronic (Hashimoto et al., 2002; Thakker and Standifer, 2002a) agonist exposures. Desensitization to all known NOP receptor cellular functions has been observed after agonist treatment, including inhibition of adenylyl cyclase (Cheng et al., 1997; Ma et al., 1997) and voltage-gated calcium channels (Morikawa et al., 1998) and activation of inwardly rectifying potassium channels (Connor et al., 1996a), ERK1/2 (Hawes et al., 1998), and p38 (Zhang et al., 1999b).
According to the accepted model of prototypical GPCR desensitization, GPCRs undergo three states/phases of desensitization: (1) phosphorylation, (2) internalization, and (3) down-regulation and degradation (Gainetdinov et al., 2004). NOP receptor desensitization is discussed in this context in the following paragraphs.
NOP Receptor Phosphorylation.
After activation by N/OFQ, the NOP receptor, like other GPCRs, couples to its corresponding heterotrimeric G-protein, where the Gα and βγ subunits initiate the aforementioned signaling cascades. After uncoupling from the Gα subunit, Gβγ subunits recruit intracellular G protein-coupled receptor kinases (GRKs) to the cell surface that phosphorylate the agonist-bound NOP receptor. The phosphorylated receptor is thought to undergo a rapid conformational change that prevents it from coupling to G-proteins or to bind agonists until the receptor is dephosphorylated. This is the earliest phase of desensitization.
Kinases regulate GPCRs by phosphorylating threonine and serine residues. The human NOP receptor contains several serine and threonine residues in its intracellular loops and carboxyl terminus that serve as potential phosphorylation sites for intracellular serine/threonine protein kinases (highlighted residues in Fig. 1). PKC also plays an important role in mediating NOP receptor desensitization. N/OFQ binding to the NOP receptor activates PKC, as demonstrated by translocation of cytosolic PKC to the plasma membrane and increased phosphorylation of proteins by PKC in cell lines that endogenously express or have been transfected to stably express the NOP receptor (see Table 1 for specific names of cell lines, phenotype, level of expression, and use) (Lou et al., 1997; Pei et al., 1997; Pu et al., 1999; Mandyam et al., 2002; Ozsoy et al., 2005). Pretreatment with the phorbol ester, phorbol 12-myristate 13-acetate, a PKC activator, facilitates the acute desensitization of the NOP receptor (Pu et al., 1999). Depletion of PKC with persistent phorbol 12-myristate 13-acetate treatment or inhibition by nonselective and conventional PKC isoform-selective inhibitors blocks the homologous desensitization of NOP receptor after acute (≤1 hour) treatment by N/OFQ (Pei et al., 1997; Mandyam et al., 2002). Indeed, N/OFQ-induced translocation of PKC involved only conventional PKC isoforms (Lou et al., 1997; Mandyam et al., 2002).
Despite having an important role in NOP receptor desensitization, direct phosphorylation of the NOP receptor by PKC has yet to be demonstrated. However, N/OFQ-induced activation of PKCα does promote the membrane translocation (Mandyam et al., 2000) and phosphorylation (Ozsoy et al., 2005) of GRK2/3, resulting in GRK2/3-mediated desensitization of the NOP receptor (Mandyam et al., 2002). GRKs phosphorylate serine residues 334 and 335 on the C-terminal tail of the rat NOP receptor (corresponding to Ser337 in the human NOP receptor) (Fig. 1), such that a single mutation at each site reduced receptor desensitization. A double S334A/S335A mutation almost abolished homologous desensitization and significantly impaired phosphorylation of the NOP receptor (Wang et al., 2006).
GRK2 and GRK3 also contribute to NOP receptor desensitization, which ensues after long-term (24 hour) stimulation by N/OFQ. Using two different human neuroblastoma cell lines that endogenously express the NOP receptor, we demonstrated that prolonged activation of the NOP receptor increases GRK2 and GRK3 levels by 2.2–2.5-fold (Thakker and Standifer, 2002a). PKC activation facilitates NOP receptor–mediated GRK3 up-regulation, and increases in GRK2 are ERK1/2 dependent (Thakker and Standifer, 2002a). Blockade of GRK2/3 up-regulation by PKC inhibition, ERK inhibition, or GRK antisense DNA treatment prevented NOP receptor desensitization. Of interest, homologous NOP receptor desensitization in BE(2)-C cells was mediated by GRK3; knockdown of GRK2 had no effect (Thakker and Standifer, 2002a).
NOP Receptor Internalization.
Receptor internalization can occur through clathrin-dependent and/or -independent (e.g., caveolae/lipid rafts) processes. To date, there are no reports that NOP receptor internalization occurs by clathrin-independent endocytosis; thus, discussion here is limited only to the role of clathrin-dependent processes in NOP receptor internalization. Phosphorylated GPCRs serve as targets for adaptor proteins, such as β-arrestins, which further disrupt the G protein–mediated actions of the receptor (Krupnick and Benovic, 1998) and trigger the formation of clathrin-coated pits to transport surface receptors to intracellular compartments through clathrin-mediated endocytosis. Clathrin-coated vesicles are trafficked to early endosomal compartments, where the receptor is completely internalized. Agonist-induced receptor internalization is the intermediate phase of GPCR desensitization, where the receptor is now inaccessible for activation by the extracellular agonist, thereby inhibiting further agonist-mediated cellular responses. However, it is also an essential process for resensitization of receptors (Gainetdinov et al., 2004), as explained below.
It was initially reported that, although the stably transfected human NOP receptor did not internalize after N/OFQ treatment, it internalized in response to treatment with the nonpeptide agonist, Ro 64-6198 ([(1S,3aS)-8-(2,3,3a,4,5,6-hexahydro-1H-phenalen-1-yl)-1-phenyl-1,3,8-triaza-spiro[4.5]decan-4-one]), as determined by radioligand binding (Dautzenberg et al., 2001; Corbani et al., 2004). In contrast, immunofluorescent and confocal microscopic approaches and radioligand binding studies in intact cells demonstrated internalization of the NOP receptor after N/OFQ treatment in endogenously expressing or stably transfected cells (Spampinato et al., 2001, 2002; Corbani et al., 2004). These studies also confirmed the temperature and ATP dependence of NOP receptor internalization via clathrin-mediated endocytosis (Dautzenberg et al., 2001; Spampinato et al., 2001, 2002; Corbani et al., 2004). Variability between studies may be attributable to possible differences in the cellular components of the cell lines [human embryonic kidney (HEK)293, Chinese hamster ovary (CHO), SK-N-BE] that are crucial for NOP receptor internalization, levels of NOP receptor expression, and/or to the efficacy of peptide versus nonpeptide agonists. NOP receptor expression in HEK293 cells (1.3 pmol/mg protein; Table 1) (Dautzenberg et al., 2001) was 10–20-fold higher than that in CHO (110 fmol/mg protein) or SK-N-BE (38 fmol/mg protein) cells used by Spampinato et al. (2001, 2002). It is possible that little internalization was noted because of the presence of numerous spare receptors in the Dautzenberg study (Dautzenberg et al., 2001). Of interest, partial agonists did not induce NOP receptor endocytosis and recruited less GRK2 to the membrane, but did produce robust NOP receptor desensitization after 1 hour of pretreatment (Spampinato et al., 2001; Corbani et al., 2004; Spampinato and Baiula, 2006). This indicates that endocytosis is important for NOP receptor resensitization.
GPCR internalization is a net result of receptor endocytosis and recycling back to the surface. This process involves acidification of endocytic vesicles and activation of GPCR phosphatases for dephosphorylating the internalized NOP receptor (Spampinato et al., 2001, 2002). Dephosphorylated receptors then transit in a recycling compartment or recycle directly back to the cell surface, ready for reactivation by their agonist. The percentage of internalized receptors at any given time, therefore, depends on the net result of endocytosis and recycling to the surface. Interfering with vesicular acidification not only reduces NOP receptor recycling to the cell surface, but also prolongs NOP receptor desensitization (Spampinato et al., 2001, 2002). NOP receptor recycling to the cell surface is a default trafficking pathway that occurs regardless of whether the agonist remains bound (Spampinato et al., 2001).
Although receptor recycling contributes to the rapid recovery of many cell surface NOP receptors, some receptors remain internalized for as long as 2 hours after washout of N/OFQ (Spampinato et al., 2001, 2002). Agonist-induced phosphorylation is required for efficient NOP receptor internalization. Agonists that induce robust NOP receptor internalization enable the NOP receptor to resume signaling more rapidly than do agonists that induce slower NOP receptor internalization (Spampinato et al., 2001; Corbani et al., 2004; Spampinato and Baiula, 2006).
Increasing expression of β-arrestin 2 increases the rate of NOP receptor internalization (Spampinato et al., 2001). Conversely, reducing the expression of β-arrestin 2 and GRK3 via siRNA significantly inhibits N/OFQ-induced NOP receptor internalization (Zhang et al., 2012a). When Ser363, a putative GRK phosphorylation site on the NOP receptor, was mutated to an alanine, cytosolic β-arrestin 2 was not recruited to the cell surface after N/OFQ treatment and the mutant S363A demonstrated significantly reduced NOP receptor internalization (Zhang et al., 2012a). Of interest, Ser363 of the NOP receptor aligns with the putative GRK2 phosphorylation sites of MOR and DOR (Fig. 1). Development of phospho-specific antibodies will be very useful to confirm the role of NOP receptor phosphorylation in internalization, recycling, and postendocytic receptor trafficking.
NOP Receptor Down-Regulation.
Receptors that remain internalized are often degraded, resulting in NOP receptor down-regulation. Long-term treatment with agonist often causes internalized receptors to be transported from endosomes to either proteosomes or lysosomes for degradation. The consequent decrease in total receptor number is referred to as receptor down-regulation, which generally ensues after chronic (hours or days) activation by an agonist. Down-regulation is the last phase of desensitization, where the total number of receptors in the cell is reduced, and therefore, responsiveness to the agonist is reduced until new receptors are synthesized and targeted to the cell surface.
NOP receptor down-regulation was observed after acute (≤1 hour) exposure to the nonpeptide agonist, Ro 64-6198 (Dautzenberg et al., 2001), but not the peptide agonist, N/OFQ, in HEK293 (stably transfected) or BE(2)-C cells (endogenously) expressing the human NOP receptor (Dautzenberg et al., 2001; Mandyam et al., 2002). Prolonged (24–48 hours) incubation with N/OFQ resulted in marked NOP receptor down-regulation in CHO cells expressing recombinant NOP receptor (Hashimoto et al., 2002). Significant NOP receptor down-regulation was also observed in membranes from rat brain homogenates 3 hours after a single intraperitoneal injection of Ro 64-6198 (Dautzenberg et al., 2001). NOP receptor levels recovered 24 hours after Ro 64-6198 injection, with a half-life of approximately 5.5 hours. Of interest, when Ro 64-6198 was administered intraperitoneally once daily for 15 days, tolerance to the drug (as indicated by loss of anti–anxiety-like behavior) was not noted, correlating well with no net loss of NOP receptor (Dautzenberg et al., 2001). This suggests that repeated long-term exposure to a NOP receptor nonpeptide agonist activates compensatory mechanisms to ensure that NOP receptor expression is maintained in vivo or that intermittent dosing regimens that allow receptor expression to recover after down-regulation is different from sustained dosing regimens that ultimately lead to degradation and down-regulation. It is possible that peptide NOP receptor agonists, such as N/OFQ, differentially induce down-regulation in a time-dependent manner, compared with nonpeptide (Ro 64-6198) agonists, because acute but not chronic Ro 64-6198 treatment produced NOP receptor down-regulation, whereas the reverse is true with N/OFQ. Furthermore, Ro 64-6198 also modulates NOP receptor function differently than N/OFQ in the vas deferens, ileum, and ventrolateral PAG (Calo et al., 1996; Rizzi et al., 2001; Chiou et al., 2004). For instance, Ro 64-6198 regulates only 60% of N/OFQ-sensitive NOP receptors in rat PAG slices, suggesting that Ro 64-6198 only regulates a specific subset of NOP receptors (Chiou et al., 2004). Whether this can be attributed to expression of NOP receptor splice variants (Pan et al., 1995, 1998; Xie et al., 1999), spare receptors, or receptor dimerization (Pan et al., 2002) is not clear. Differences in neuronal (rat brain) versus nonneuronal cell phenotype (CHO and HEK cells) expression in different backgrounds (native versus recombinant) and in levels of NOP receptor expression also may account for some of these differences.
These differences underscore the need to investigate the role of NOP receptor expression levels and neuronal cellular environment on NOP receptor regulation. To address the role of NOP receptor density, an ecdysone-inducible expression system was used to express human NOP receptors at different levels in CHO cells to determine the functional activity of several partial agonists (McDonald et al., 2003). These studies found that receptor density dictated the level of agonist or antagonist effect on receptor binding and cAMP inhibition (McDonald et al., 2003). For instance, with use of 35S-GTPγS binding as a functional readout, N/OFQ(1–13)–NH2 was a full NOP receptor agonist when the NOP receptor was expressed at approximately 25 fmol/mg, whereas [F/G]N/OFQ(1–13)–NH2 failed to stimulate any 35S-GTPγS binding at this expression level. In fact, [F/G]N/OFQ(1–13)–NH2 was a full NOP receptor agonist only after NOP receptor levels reached ∼70 fmol/mg (McDonald et al., 2003). When measuring inhibition of cAMP accumulation, N/OFQ(1–13)–NH2 remained a full agonist at all receptor densities (25–1100 fmol/mg), whereas [F/G]N/OFQ(1–13)–NH2 was a full agonist only at high receptor density (McDonald et al., 2003). Increasing receptor expression from physiologic (194 fmol/mg) to supra-physiologic (473 fmol/mg) levels increased N/OFQ-induced 35S-GTPγS binding and, thus, increased N/OFQ efficacy via G-protein coupling to the NOP receptor (McDonald et al., 2003; Barnes et al., 2007). However, N/OFQ potency was unaffected by NOP receptor density (Barnes et al., 2007). Furthermore, pretreatment with N/OFQ produced similar desensitization of the NOP receptor response, regardless of receptor density. Of note, low-density receptor expression (25 fmol/mg) in CHO cells using the ecdysone-inducible system was similar to NOP receptor levels in SK-N-BE and SH-SY5Y human neuroblastoma cells, whereas mid-range (200 fmol/mg) and high expression (1100 fmol/mg) were similar to levels seen in rat cortex and stably transfected CHO cells, respectively (Okawa et al., 1999; Peluso et al., 2001). Altogether, this suggests that, in non-neuronal cell background, NOP receptor desensitization induced by N/OFQ is not dependent on the amount of NOP receptor (Barnes et al., 2007). The role of receptor density on NOP receptor regulation in a neuronal cell background remains to be addressed.
Additional evidence for N/OFQ regulation of NOP receptor expression comes from pre-pro-N/OFQ knockout (KO) mice. Clarke et al. (2003) observed significant NOP receptor up-regulation in several brain regions of the pre-pro-N/OFQ KO mice. This up-regulation may represent a type of denervation supersensitivity of postsynaptic cells, resulting in increased NOP receptor expression in response to the loss of tonic neurotransmitter (N/OFQ) release from the presynaptic nerve terminals (Clarke et al., 2003) in the N/OFQ KO mice. Alternatively, other compensatory changes during the development of pre-pro-N/OFQ KO mice may also account for such regulation of the NOP receptor (Clarke et al., 2003). Further characterization of these events is required to confer a definitive role for N/OFQ in regulating NOP receptor expression in vivo.
Heterologous Regulation of the NOP Receptor
In addition to the homologous regulation by its own agonists, heterologous regulation of the NOP receptor occurs in a cell-specific manner and may increase or decrease NOP receptor activity or expression. Heterologous receptor desensitization is a state of reduced responsiveness of a receptor to its agonist because of activation of a second receptor system. This can occur by a simple heterologous effect or by heterologous modulation of homologous desensitization.
Regulation by MOR Agonists.
MOR agonists induced heterologous desensitization of the NOP receptor in a cell-specific manner. Short-term pretreatment (1 hour) of MOR and NOP receptor with the MOR agonist [D-Ala2, N-MePhe4, Gly-ol]-enkephalin (DAMGO) robustly desensitized N/OFQ/NOP receptor–induced inhibition of cAMP accumulation in BE(2)-C human neuroblastoma cells (Mandyam et al., 2000, 2003). However, the same treatment had no effect on the N/OFQ response in SH-SY5Y cells, despite the fact that both cell lines expressed both MOR and NOP receptor (Mandyam et al., 2003). This may result from differences in signal transduction components in the two cell lines, as described above. In SH-SY5Y cells, MOR agonists increased PKCε translocation, not translocation of a conventional isoform (such as PKCα) that produced homologous NOP receptor desensitization in BE(2)-C cells (Mandyam et al., 2002). Similar results were noted in HEK 293 or CHO cells expressing recombinant NOP receptor and MOR. In those studies, pretreatment with a MOR agonist had no effect on NOP receptor–mediated inhibition of cAMP (Wang et al., 2005) or stimulation of ERK1/2 (Hawes et al., 1998). In contrast, MOR agonist treatment internalized recombinant NOP receptor expressed with MOR in tsA-201 cells (Evans et al., 2010). Therefore, because the specific components of signaling cascades, especially kinase isoforms, activated by MOR agonists vary between cell types, the ability of MOR agonists to regulate NOP receptor activity also varies among cell types.
MOR agonist treatment also heterologously regulates homologous NOP receptor desensitization (e.g., 10 minutes incubation with N/OFQ to measure NOP receptor inhibition of cAMP accumulation; NOP receptor desensitization of this response normally does not occur within 10 minutes). However, if GRK2 or 3 levels at the plasma membrane (Mandyam et al., 2003) or in the cell (Thakker and Standifer, 2002a) were up-regulated by 1 hour or 24 hours of DAMGO pretreatment, respectively, the rate of NOP receptor desensitization increased; the subsequent 10 minutes exposure to N/OFQ resulted in a rightward shift or flattening of the concentration-response curve. Down-regulation of GRK2 and 3 or blockade of their up-regulation prevented NOP receptor desensitization (Thakker and Standifer, 2002a; Mandyam et al., 2003). MOR-mediated NOP receptor desensitization in SH-SY5Y cells involved GRK2, whereas NOP receptor desensitization in BE(2)-C cells was PKC and GRK3 dependent. Therefore, the ability of a MOR agonist to up-regulate or translocate GRK2 or 3 serves as a critical factor for producing heterologous modulation of homologous NOP receptor desensitization.
The role of the MOR in regulating NOP receptor expression also was examined in vivo using MOR knockout mouse strains and chronic MOR agonist treatment. NOP receptor expression in the brains of MOR knockout mice did not differ from levels in wild-type mice (Slowe et al., 2001), suggesting that activation of MOR by endogenous agonists does not regulate the expression of NOP receptor supraspinally. In contrast, chronic activation of MOR with morphine increased NOP receptor expression in the dorsal spinal cord in mice and rats (Gouarderes et al., 1999; Ueda et al., 2000; Zhang et al., 2012b). Whether chronic morphine treatment also increases NOP receptor expression supraspinally is not yet known.
Regulation by DOR or KOR Agonists.
Heterologous regulation of the NOP receptor by DOR or KOR agonists is far less characterized than that by MOR agonists. DOR agonists were unable to desensitize NOP receptor–mediated inhibition of cAMP accumulation (Cheng et al., 1997; Ma et al., 1997) or activation of p38 (Zhang et al., 1999b) in SK-N-SH human neuroblastoma and NG108-15 rat neuroblastoma-glioma hybrid cells that natively express NOP receptor and DOR. Of interest, significant NOP receptor up-regulation was observed in the brains of DOR KO mice, suggesting that basal activation of DOR by endogenous peptides exerted inhibitory control over NOP receptor expression (Slowe et al., 2001).
In contrast to DOR KO mice, NOP receptors were down-regulated in the brains of KOR KO mice (Slowe et al., 2001), indicating that endogenous KOR signaling increased NOP receptor expression or prevented its degradation. NOP receptor coupling to G16 (a pertussis toxin–insensitive G protein commonly expressed in hematopoietic cells) also increased after KOR and NOP receptor coexpression of the NOP receptor with the KOR in COS-7 African green monkey kidney cells (Ho et al., 2002). The mechanism of this enhanced coupling of NOP receptor to the G16 by increased KOR expression is unknown.
Regulation by GABAB Receptor Agonists.
In addition to opioid receptors, the metabotropic GABAB receptor is another GPCR that modulates NOP receptor function. Only a brief (1 minute) activation of the GABAB receptor is sufficient to desensitize the NOP receptor in hippocampal neurons (Pu et al., 1999). Both GABAB receptor and NOP receptor homologous desensitization are PKC dependent (Pei et al., 1997; Pu et al., 1999; Mandyam et al., 2002); however, whether heterologous desensitization of NOP receptor by GABAB occurs via PKC activation remains to be determined. GABAB and NOP receptors are important for the modulation of pain (Malcangio and Bowery, 1995; Mogil and Pasternak, 2001) and are colocalized in several neurons implicated in the actions of opioids (Vaughan and Christie, 1996; Connor and Christie, 1998; Pu et al., 1999). Therefore, a detailed investigation of their interaction will possibly shed more light on the diverse actions of N/OFQ on pain perception and its regulation of opioid actions via GABAB receptors.
Regulation by CB1 Receptor Agonists.
Cannabinoids have pharmacological characteristics and physiologic effects similar to those of the NOP receptor system (Pertwee, 2008). Long-term (24 hours) treatment with the CB1 agonist, delta9-tetrahydrocannabinol, dose-dependently decreased NOP receptor mRNA and protein expression in SH-SY5Y human neuroblastoma cells (Cannarsa et al., 2012). However, the molecular mechanism responsible for NOP receptor down-regulation by delta9-tetrahydrocannabinol is not known.
Regulation by N-Methyl-D-Aspartate Receptor Ligands.
N-methyl-D-aspartate (NMDA) receptors also regulate NOP receptor function. Stimulation of the NMDA receptor promotes calcium influx and augmentation of intracellular calcium, which in turn, leads to the activation of PKC (Etoh et al., 1991). Because enhanced calcium levels are required for NOP receptor desensitization (Pu et al., 1999), short-term exposure (5 minutes) to NMDA promotes the desensitization of NOP receptor in neuronal cells. NMDA receptor antagonists in the same cells also inhibit homologous NOP receptor desensitization by blocking calcium influx (Zhao et al., 1998). As mentioned above, presynaptic NOP receptor activation decreases calcium influx and inhibits neurotransmitter release. Desensitization of NOP receptor by acute NMDA receptor activation would permit calcium influx and, thus, facilitate neurotransmission.
Heterologous Regulation by N/OFQ
Activation of the NOP receptor by N/OFQ or other NOP receptor agonists can also heterologously regulate the activity of other receptors.
Classic Opioid Receptors.
Because of its ability to modulate morphine analgesia and morphine tolerance, it is important to understand how N/OFQ can regulate the MOR. Indeed, N/OFQ pretreatment produced MOR desensitization (Hawes et al., 1998; Mandyam et al., 2000, 2002; Thakker and Standifer, 2002a; Ozsoy et al., 2005), phosphorylation (Ozsoy et al., 2005), internalization (Evans et al., 2010), and down-regulation (Mandyam et al., 2002) in cells endogenously expressing and stably transfected with NOP receptor. However, mechanisms of N/OFQ-mediated MOR desensitization also are cell, time, and signal pathway specific. Short-term N/OFQ pretreatment reduced the ability of the MOR agonists DAMGO (Mandyam et al., 2002; Wang et al., 2005) and morphine (Mandyam et al., 2000) to inhibit cAMP and to stimulate mitogen-activated protein kinase (Hawes et al., 1998). Acute desensitization of MOR responses by N/OFQ in BE(2)-C cells involves translocation of PKCα, GRK2, and GRK3 to the plasma membrane. By increasing GRK2 levels at the plasma membrane during N/OFQ pretreatment, MOR phosphorylation was enhanced significantly during subsequent challenge with DAMGO, compared with MOR phosphorylation in the absence of N/OFQ pretreatment (Mandyam et al., 2002; Ozsoy et al., 2005). N/OFQ-mediated MOR desensitization and phosphorylation was blocked by inhibition of PKC and down-regulation of GRK2, but not by down-regulation of GRK3. Furthermore, MORs lacking the GRK2 phosphorylation site, Ser375, were not phosphorylated or desensitized by acute N/OFQ pretreatment (Ozsoy et al., 2005). Therefore, acute exposure to N/OFQ enhanced MOR-mediated homologous desensitization in BE(2)-C human neuroblastoma cells. The mechanism(s) by which acute N/OFQ-desensitized MOR responses in CHO and HEK cells were not investigated (Hawes et al., 1998; Wang et al., 2005).
Although prolonged N/OFQ treatment reduced the ability of MOR agonists to inhibit cAMP accumulation in BE(2)-C and SH-SY5Y cells (Thakker and Standifer, 2002a), it did not alter the ability of MOR to activate ERK1/2 (Thakker and Standifer, 2002b). The desensitization of the cyclase response by N/OFQ involved up-regulation of GRK2 (SH-SY5Y) and GRK3 (BE(2)-C and SH-SY5Y) (Thakker and Standifer, 2002a); MOR desensitization was blocked in both cell lines by blocking up-regulation of the respective GRK. This is consistent with the mechanism of acute N/OFQ-mediated MOR desensitization. It would appear that MOR-mediated ERK1/2 activation is not sensitive to GRK up-regulation, but the role of GRK in DAMGO-stimulated ERK1/2 activation and desensitization has not been examined directly.
Acute N/OFQ prechallenge failed to desensitize DOR-mediated inhibition of cAMP accumulation in NG108-15 neuroblastoma cells (Ma et al., 1997). However, N/OFQ treatment also reduced MOR (Zhang et al., 2005) and KOR (Zhang et al., 1998) agonist-induced inhibition of calcium currents in freshly isolated rat DRG neurons. It is not clear whether the mechanism for this effect involves desensitization or competition for intracellular signaling components/G protein subunits or results from receptor internalization, as reported more recently (Evans et al., 2010). Indeed, N/OFQ induced internalization of MOR, KOR, and DOR when each was coexpressed with the NOP receptor (Evans et al., 2010). This issue is discussed further in the heterodimerization section below.
Of interest, MOR, KOR, or DOR receptor expression was unaltered in NOP receptor KO rats, compared with wild-type animals (Homberg et al., 2009), suggesting that endogenous N/OFQ tone was not important for basal expression of those receptors.
Cytokine Receptors.
The chemotactic effect mediated through CXCR4, an important HIV-1 coreceptor, was desensitized in primary leukocytes, U937 monocytes, and Jurkat T cells after N/OFQ treatment (Kaminsky and Rogers, 2011). This further supports a role for N/OFQ in immunomodulation.
Heterodimerization
Heterodimerization of the NOP receptor with other GPCRs was examined using coimmunoprecipitation (Pan et al., 2002; Wang et al., 2005; Evans et al., 2010) and immunofluorescence microscopy approaches (Evans et al., 2010). Heterodimerization also appears to play a role in opioid receptor regulation and function by altering receptor binding, functional activity, and trafficking. MOR/NOP receptor dimerization increased the affinity for MOR agonist binding (Pan et al., 2002), but had no effect on N/OFQ/NOP receptor–mediated inhibition of cAMP or activation of ERK1/2 in the absence of MOR agonist stimulation. In contrast, MOR/NOP receptor dimerization decreased MOR agonist potency in both signaling pathways in the absence of N/OFQ (Wang et al., 2005). Pretreatment with N/OFQ desensitized the MOR/NOP receptor heterodimers, similar to results described above with endogenously coexpressed MOR and NOP receptor. MOR/NOP receptor heterodimerization also required the C-terminal portions of both receptors (Pan et al., 2002; Wang et al., 2005), sites of GRK-mediated phosphorylation required for receptor desensitization and agonist-mediated internalization. The NOP receptor interacts with and regulates N-type calcium channels (Beedle et al., 2004); thus, regulation of the NOP receptor by MOR agonists may also modulate calcium channel activity. Of interest, MOR does not physically associate with N-type calcium channels, nor does the MOR agonist DAMGO induce calcium channel internalization unless coexpressed with NOP receptor. When all three molecules are coexpressed, DAMGO stimulates MOR/NOP receptor/calcium channel internalization. The ability of NOP receptor and MOR/NOP receptor heterodimers to regulate calcium currents and to internalize N-type calcium channels allows these opioid systems to regulate calcium influx (Evans et al., 2010) and, thus, to potentially regulate neurotransmission and nociceptive signaling. Although MOR/NOP receptor heterodimerization has yet to be demonstrated in the brain, MOR and NOP receptors are functionally coexpressed in neurons of the PAG, RVM, hypothalamus, dorsal root ganglion, trigeminal ganglion, locus coeruleus, and nucleus tractus solitarius (Connor et al., 1996a; Wagner et al., 1998; Borgland et al., 2001; Vaughan et al., 2001, 2003; Endoh, 2006; Murali et al., 2012). The potential for MOR/NOP receptor heterodimerization in these regions may provide an additional level of MOR and NOP receptor modulation of nociceptive processing and reproductive behavior. However, development of additional tools will be necessary to move this discussion past the speculative stage.
The NOP receptor also heterodimerizes with KOR and DOR (Evans et al., 2010). In both cases, it resulted in N/OFQ- and U50,488- (KOR agonist), or deltorphin- (DOR agonist) mediated heterodimer internalization. Of interest, heterodimerization of NOP receptor with KOR or DOR reduced N/OFQ reduction of peak calcium current inhibition, especially with NOP receptor/DOR dimerization (Evans et al., 2010). This suggests that up-regulation of DOR or KOR in cells expressing the NOP receptor would be one means of reducing N/OFQ-mediated calcium channel modulation. Although autoradiographic and/or in situ hybridization studies suggest that KOR and NOP receptors are regionally colocalized in the descending analgesic reward pathways (Mansour et al., 1995; Berthele et al., 2003) and that DOR and NOP receptors are regionally colocalized in the cortex, nucleus accumbens, amygdala, and dorsal horn (Neal et al., 1999; Berthele et al., 2003), these methods do not confirm colocalization at a cellular level. However, functional evidence also supports cellular colocalization of KOR/NOP receptor in PAG and RVM, suggesting that KOR/NOP receptor heterodimerization may mediate nociceptive processing (Vaughan et al., 2001, 2003). DOR and NOP receptors colocalize at the cellular level in neurons in the PAG and the medial vestibular nucleus (Sulaiman et al., 1999; Vaughan et al., 2003), suggesting that heterodimers may modulate nociceptive processing and vestibular reflex.
NOP Receptor Function, Pain, and Inflammatory Response: The Role of NOP Receptor Regulation
One of the hallmarks of the opioid receptor family is regulation of pain. As indicated by its name, N/OFQ and the NOP receptor play a unique role in nociception and nociceptive processing. Depending on a number of factors, including species and strain, dose, time of testing after drug administration, or the testing paradigm itself, N/OFQ may produce a hyperalgesic or an analgesic response (Mogil and Pasternak, 2001). Although both hyperalgesic and analgesic actions of supraspinally administered N/OFQ are noted, spinally administered N/OFQ predominantly produces analgesia (Mogil and Pasternak, 2001). The biphasic effect (hyperalgesic versus analgesic) after supraspinal administration may be explained by NOP receptor desensitization, trafficking, and/or dimerization, but that is not yet clear.
The N/OFQ-NOP receptor system also modulates the actions of other opioids. Several reports document the anti-opioid activity of N/OFQ by demonstrating its ability to block supraspinal analgesia produced by selective MOR, DOR, and KOR agonists (Mogil et al., 1996a,b; Zhu et al., 1996). This effect is largely attributed to the expression of NOP receptors on cells regulating descending analgesia (Heinricher, 2005). However, it is possible that heterologous regulation of the other opioid receptors by the NOP receptor also contributes to the regulation of nociceptive transmission. N/OFQ treatment desensitizes the MOR in vitro (Hawes et al., 1998; Mandyam et al., 2000, 2002; Thakker and Standifer, 2002a; Ozsoy et al., 2005; Evans et al., 2010), raising the possibility that supraspinal NOP receptor agonist treatment attenuates MOR responsiveness in vivo, thus reducing the analgesic actions of MOR agonists.
As discussed above, the N/OFQ-NOP receptor system has an important immunomodulatory effect, although the mechanism(s) underlying this immunomodulation is somewhat unclear. N/OFQ and the NOP receptor are expressed on many different types of immune cells (Halford et al., 1995; Wick et al., 1995; Peluso et al., 1998; Arjomand et al., 2002) and modulate numerous processes within the immune and neuroimmune systems, including cytokine expression, antibody formation, neutrophil chemotaxis, and T cell function (Serhan et al., 2001; Fiset et al., 2003; Waits et al., 2004; Fu et al., 2007; Miller and Fulford, 2007; Anton et al., 2010). NOP receptor activation and up-regulation of transcription factors, including ATF-2, NFκB (Donica et al., 2011), activating protein-2 (Thakker and Standifer, 2002a), and Oct-2 (Thakker and Standifer, 2002b), provide potential molecular mechanisms for prolonged regulation of an inflammatory response. In addition to NOP receptor–mediated transcriptional regulation, the recent report of heterologous regulation of HIV-1 coreceptor CXCR4 by the NOP receptor (Kaminsky and Rogers, 2011) provides another mechanism for NOP receptor immunomodulation. Together, these studies demonstrate the breadth of NOP receptor signaling on immune system regulation and warrant a more thorough investigation to elucidate the potential mechanisms of this effect.
Numerous recent reviews have emphasized the importance of inflammatory factors, such as cytokines, chemokines, and infiltrating immune cells, and signaling molecules, such as substance P, calcitonin-related gene peptide, bradykinin, and prostaglandins, in developing, enhancing, and maintaining nociception (Fukuoka et al., 1994; Basbaum et al., 2009; Ren and Dubner, 2010; Kiguchi et al., 2012). NOP receptor activation has been suggested to play a role in the association between pain and inflammation (Mika et al., 2011). N/OFQ and NOP receptor expression are elevated in the dorsal root ganglion projections to the spinal dorsal horn, ventrolateral PAG, dorsal raphe nucleus, and the nucleus of raphe magnus in neuropathic or inflammatory pain models, consistent with N/OFQ-NOP receptor system involvement in neuropathic and inflammatory pain processing (Ma et al., 2005; Chen and Sommer, 2006). Intrathecal N/OFQ administration delays chronic constrictive nerve injury-induced hyperalgesia and abolishes sciatic nerve injury-induced pain (Yamamoto et al., 1997, 2000; Courteix et al., 2004). However, it also appears that N/OFQ exacerbates neuropathic pain states by inducing an influx of inflammatory mediators (Fu et al., 2007; Mika et al., 2011). It is possible that acute activation of the NOP receptor contributes partially to spinal analgesia by inhibiting proinflammatory cytokines, whereas persistent NOP receptor activation leads to NOP receptor desensitization and reduced ability of N/OFQ to inhibit proinflammatory cytokines. Therefore, NOP receptor desensitization would exacerbate neuropathic pain when NOP-mediated inhibition of inflammatory mediators is reduced. An inevitable limitation to the rising prospect of using NOP receptor agonists in the long-term management of several disorders, such as anxiety, drug abuse, asthma, and chronic neuropathic pain, is the development of tolerance to NOP receptor agonists. As discussed above, chronic N/OFQ exposure induces homologous desensitization, resulting in diminished cellular and behavioral function. Indeed, tolerance to the hyperalgesic (Kavaliers and Perrot-Sinal, 1996) and spinal analgesic actions of N/OFQ (Hao et al., 1997; Jhamandas et al., 1998) and its blockade of locomotor activity (Devine et al., 1996) and morphine-induced antinociception in vivo (Lutfy et al., 1999) have been reported. Although likely, it has yet to be reported whether the development of tolerance to chronic N/OFQ administration in vivo is the result of NOPr desensitization and down-regulation. N/OFQ tolerance, similar to that of other opioids (Nestler and Aghajanian, 1997), may possibly involve complex compensatory changes in the neuronal circuitry along with adaptations in intracellular signaling cascades and subsequent regulation of the NOP receptor that requires further investigation. As noted with NOP receptor internalization studies, the structure and efficacy of a ligand can alter its ability to regulate the receptor; examination of NOP receptor regulation by structurally distinct partial agonists also is warranted.
Conclusion
Almost two decades since the NOP receptor was cloned and its endogenous agonist, N/OFQ, identified, our understanding of NOP receptor cellular function and consequent regulation still has far to go. Activation of the NOP receptor initiates intracellular events similar to those initiated by the other opioid receptors, but NOP receptor–mediated actions oppose many antinociceptive actions of classic opioid agonists. Regulation of NOP receptor function also appears to follow a similar pattern of GPCR regulation, as observed for the other opioid receptors. Of note, however, a large percentage of NOP receptor signaling and regulation studies were performed using recombinant receptors overexpressed in cells with nonneuronal phenotypes. The significance of studying the receptor-effector coupling in a native environment has become increasingly evident with our understanding of how different cell types and levels of receptor expression impact receptor function (Kenakin, 1997, 2002). Therefore, a detailed examination of NOP receptor regulation in neuronal cells that endogenously express this receptor is an essential next step. Additional in vivo studies of NOP receptor regulation also is warranted to understand how the cellular actions of NOP receptor activation integrate with NOP receptor–mediated behavioral and physiologic outcomes.
Authorship Contributions
Wrote or contributed to the writing of the manuscript: Donica, Awwad, Thakker, Standifer.
Footnotes
- Received December 20, 2012.
- Accepted February 8, 2013.
This work was supported by the Oklahoma Center for the Advancement of Science and Technology’s OHRS Award [Project HR08-152]; the National Institutes of Health National Institute on Drug Abuse [Grant R01-DA017380]; and the Department of the Army [DMRDP W81XWH-11-2-0077].
The information and interpretations included in this article do not necessarily reflect the position or the policy of the Government, and no official endorsement should be inferred.
↵1Current affiliation: Medtronic Neuromodulation, Minneapolis, Minnesota.
Abbreviations
- ATF-2
- activating transcription factor–2
- CHO
- Chinese hamster ovary
- DOR
- δ opioid receptor
- ERK
- extracellular signal-regulated kinases
- GPCR
- G protein–coupled receptor
- GRK
- GPCR kinase
- HEK
- human embryonic kidney
- KOR
- κ opioid receptor
- KO
- knockout
- MOR
- µ opioid receptor
- NMDA
- N-methyl-D-aspartate
- N/OFQ
- nociceptin/orphanin FQ
- NOP receptor
- nociceptin/orphanin FQ peptide receptor
- NFκB
- nuclear factor kappa B
- PAG
- periaqueductal gray
- PKC
- protein kinase C
- Ro 64-6198
- [(1S,3aS)-8-(2,3,3a,4,5,6-hexahydro-1H-phenalen-1-yl)-1-phenyl-1,3,8-triaza-spiro[4.5]decan-4-one]
- U.S. Government work not protected by U.S. copyright.