Unifying Perspectives of the Mechanisms Underlying the Development of Tolerance and Physical Dependence to Opioids

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Vol. 297, Issue 1, 11-18, April 2001

Unifying Perspectives of the Mechanisms Underlying the Development of Tolerance and Physical Dependence to Opioids

David A. Taylor and William W. Fleming

Department of Pharmacology and Toxicology, Robert C. Byrd Health Sciences Center, West Virginia University School of Medicine, Morgantown, West Virginia

	Abstract

Top Abstract Introduction Cellular Mechanisms of Acute... Effects of Chronic Exposure... Conclusions and Future... References

The cellular basis of tolerance to, and dependence upon, many types of drugs, including opioids, has long defied identification.Tolerance to opioids cannot be explained solely on the basis ofmodification of opioid receptors or altered metabolism or dispositionof the opioid. The development of tolerance following chronicexposure to opioids presents at least three different types ofchange in cellular responsiveness, each of which has been suggestedto represent some type of adaptive modification in cellular responsiveness.These different forms of tolerance are distinguishable on thebasis of their time course and whether or not the tolerance isspecific for opioid receptor agonists (homologous) or extendsto agonists of other systems (heterologous). The adaptive modulationof responsiveness via regulation of cellular proteins has beenproposed to be the basis for both longer-term forms of tolerance.The divergent signaling pathways activated by G-protein-coupledreceptors like the µ-opioid receptor provide multiple downstreamtargets for both short- and long-term regulation of cell functionthat is associated with the development of tolerance and/or dependence.Since the magnitude of receptor activation is an important determinantof the degree to which various signaling pathways are activated,the expressed characteristics of tolerance and/or dependence maybe functionally related to which of these diverse pathways arestimulated to the greatest degree. Thus, the possibility thatdifferent signaling events are activated either sequentially orconcurrently offers the possibility to explain the interactionbetween these different forms of tolerance and/ordependence.

	Introduction

Top Abstract Introduction Cellular Mechanisms of Acute... Effects of Chronic Exposure... Conclusions and Future... References

The chronic use of opioids is often accompanied by the development of tolerance and/or dependence upon these agents due toadaptive changes in the response of the subject to the agent.Tolerance may be defined as a reduction in sensitivity to an agentfollowing repeated exposure, while dependence is generally thoughtof as the absolute requirement for the agent to maintain normalphysiological function. A complication in identifying cellularmechanisms of the adaptation is the presence of multiple formsof tolerance and dependence that include both homologous and heterologouschanges in responsiveness. Dependence also presents in differentforms that are defined by the presence of a withdrawal reaction(physical dependence) and/or the presence of a "drug-craving"component (psychic dependence). The existence of multiple formsof these phenomena raises the possibility that each componentmay possess different cellular mechanisms and, furthermore, thatmultiple mechanisms could be concurrently operating to producethe complex behavior normally associated with drug dependenceand tolerance in humans. Indeed, a number of potential mechanismsfor these states of altered responsiveness have been suggestedfrom animal and isolated tissue studies. Providing a perspectivefrom which multiple mechanisms, each based upon sound scientificmodeling, could interact to produce these effects on cell responsivenessis a challenging goal. To achieve such a goal within this limitedformat requires the liberal use of review citations from whichthe reader can retrieve the original references discussed anda limited number of individual citations for eachobservation.

To avoid the complications of the phenomena that are created through the impact on neuronal networks, attention will be devotedto the mechanisms that have been described at the level of theindividual neuron or can reasonably be inferred to that level.It is obvious that adaptation to opioid responses in one neuronwithin the framework of a network can induce adaptations in secondaryneurons that may not possess opioid receptors, for example, thosethat follow chronic opioid action involving a compensatory elevationin the activity of glutamatergic neurons whose actions are mediatedthrough N-methyl-D-aspartate (NMDA) receptors (Mao, 1999). Such"network" adaptations are clearly beyond the limits of this analysis.Clearly, psychic dependence is a phenomenon of complexity wellbeyond the adaptation of individual neurons and has been reviewedby Koob et al. (1998).

There is clear evidence that the expression of tolerance in individual neurons occurs with different characteristics thatcan be distinguished by the specificity of change in responsivenessand the temporal development. One form (i.e., "desensitization")is highly specific for opioids (homologous), develops rapidlyfollowing receptor occupation (seconds to minutes), is due touncoupling of the receptor from its cognate G-protein (with orwithout internalization), and is often produced by exposure tohigh concentrations of agonist (Johnson and Fleming, 1989; Lawand Loh, 1999). Another form is also homologous but develops ona somewhat slower time course (hours) and has been proposed tobe due to changes in the adenylyl cyclase (AC) cascade (Nestleret al., 1994; Nestler and Aghajanian, 1997). A third form developsand decays even more slowly (days), exhibits nonspecific changesin responsiveness (heterologous), and has been suggested to bedue to a partial depolarization resulting from down-regulationof the sodium pump and a reduction in its electrogenic contributionto membrane potential (Fleming and Taylor, 1995; Fleming, 1999).Interestingly, the expression of these different types of "tolerance"can be observed in a variety of individual neurons and may developseparately or concurrently, depending upon the method used toinduce tolerance (Johnson and Fleming, 1989).

The concept that tolerance and physical dependence upon opioids are expressions of individual neuronal adaptation has beenthe subject of several reviews (Johnson and Fleming, 1989; Nestleret al., 1994; Fleming and Taylor, 1995; Christie et al., 1997;Nestler and Aghajanian, 1997), although no single mechanism hasbeen clearly identified to underlie the development of the phenomena.Increasing emphasis has been placed on the regulation of cellprotein levels as a general mechanism by which long-term adaptationsin cellular responsiveness occur (Nestler et al., 1994; Flemingand Taylor, 1995; Nestler and Aghajanian, 1997). Certain criteriamust be met for any proposed cellular mechanism of adaptationto be confidently established as being responsible for the changein responsiveness. The proposed cellular change must: 1) be inducedby experimental procedures identical to those that induce toleranceand/or dependence; 2) follow a similar time course as the toleranceand/or dependence in that tissue; 3) quantitatively account forthe tolerance and/or dependence; 4) account for the qualitativecharacteristics of the tolerance and/or dependence; and 5) occurin the very cells upon which the opioid is acting. It is alsoassumed that the cellular changes develop as a consequence ofactivation of the acute signaling pathway by theopioid.

These criteria were first explicitly expressed in the review by Fleming and Taylor (1995). However, they have been implicitlyapplied for decades in studies of adaptation in non-neuronal cells.For example, all of the criteria have been met in identifyingthe spread of cholinoceptors outward from the end-plate as thecause of the highly specific supersensitivity of denervated skeletalmuscle (Thesleff, 1960; Fleming and Westfall, 1988). Similarly,all of the criteria have been met for the role of partial depolarizationand reduced Na⁺, K⁺ pump function underlying the nonspecific supersensitivity toexcitatory agonists in the rabbit aorta (Abel et al., 1981) andthe guinea pig vas deferens (see Discussion in Hershman et al.,1995), which follow chronic interruption of adrenoceptor activation.These criteria have not been established fully for any proposedmechanism of opioid tolerance to date, although the collectivedata supporting a role for membrane depolarization and reducedfunction of the Na⁺, K⁺ pump in myenteric neurons come close to meeting all of the criteria(see Effects of Chronic Exposure to Opioids below). The criteriagenerally lacking for other mechanisms are numbers 3 and 4 andsometimes2.

It is particularly intriguing to consider the possibility that multiple mechanisms could be concurrently activated to affectthe adaptation associated with chronic exposure to opioids, asdiscussed later. Since activation of the receptor-mediated signaltransduction pathway is an obligatory component in the developmentof all types of tolerance, examination of the acute effects ofopioids should identify potential molecular targets that couldunderlie the long-term modification inresponsiveness.

	Cellular Mechanisms of Acute Opioid Action

Top Abstract Introduction Cellular Mechanisms of Acute... Effects of Chronic Exposure... Conclusions and Future... References

The actions of opioids in any biological system are a combination of multiple independent components acting in concert. Thefirst source of diversity is the receptor where at least threemajor types of opioid receptors (i.e., µ, $kappa$ , and $delta$ ) mediate theresponse to exogenous or endogenous opioid ligands (di Chiaraand North, 1992). Each of these receptors is a member of the superfamilyof G-protein-coupled receptors (GPCR) characterized by seven transmembrane-spanningtertiary structures with a large intracellular loop between TM5and TM6 where the presumed contact with the cognate G-protein $alpha$ -subunit resides. Since the µ-opioid receptor subtype (hereaftertermed the µ-receptor) is predominately responsible for the productionof both analgesia and euphoria by the more common opioids, considerationof the mechanisms of development of tolerance/dependence willfocus primarily on this receptorsubtype.

The G-proteins that couple these receptors to the intracellular effectors exist as heterotrimers derived from three differentprimary classes of subunits: G [18 subunit isoforms fromfour families (G_s, G_i/o, G_q, and G₁₂)];G (5 subunit isoforms), and G (11 subunit isoforms)(Hildebrandt, 1997). Each heterotrimer, consisting of a single $alpha$ -subunit isoform combined with a dimer of $beta$ $gamma$ -subunits, can linka different GPCR with a specific downstream effector system. Substantialmechanistic diversity can be achieved through this type of combinatorialcell signaling involving only two partners, a GPCR and a G-proteinheterotrimer, as depicted in Fig. 1. As illustrated, the µ-receptoris activated by agonist forcing the replacement of GDP bound tothe $alpha$ -subunit by GTP, which then forces the dissociation of $alpha$ -and $beta$ $gamma$ -subunits. The activated $alpha$ -subunit (i.e., G * GTP)and $beta$ $gamma$ -subunits can each mediate downstream effects providinga locus for the two entities to couple to multiple cellular effectorslike enzymes and ion channels (Fig. 1). According to this scheme,opioid receptor activation could not only change ion conductancebut also act upon other cellular effectors simultaneously throughthe combined actions of the $alpha$ - and $beta$ $gamma$ -subunits (see activitiesin Table 1). Through this type of coupling between a single ligand-receptor-transducercomplex and multiple effectors, the potential for activating pathwayswhose primary targets are separated between short- and long-termregulation of cellular function is markedly enhanced. Given thatadaptive processes underlying tolerance and/or dependence utilizemultiple signaling systems, the possibility that one pathway maybe predominately activated over another by varying the conditionsof agonist exposure must be considered. Thus, when high concentrationsof agonist are used, the specific pathway that exerts the primaryeffect could change from that used in the normal acute situationor under conditions of chronic low-concentration agonist exposure.

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Fig. 1. Schematic representation of the signaling pathways activated acutely by µ-opioid receptor activation. The G-protein-coupled receptor can modify the activity of a variety of cellular effectors through the combined action of the dissociated $alpha$ - (i.e., GTP-bound) and $beta$ $gamma$ -subunits. The action of the cellular effectors are amplified further by the capacity to simultaneously produce multiple cell signals that can then interact with multiple downstream effectors within the cell. The cellular effectors that have been identified to be modified acutely by µ-opioid receptor agonists are presented in Table 1. The phosphoproteins component actually represents another potential site of regulation through modification of the phosphorylation/dephosphorylation state. The cellular loci highlighted in red represent those entities that have been proposed or demonstrated to be modified during the production of acute changes in responsiveness (i.e., desensitization through receptor uncoupling or receptor sequestration and internalization).

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TABLE 1
Impact of µ-opioid receptor activation on various cellular elements that may be involved in production of tolerance and/or dependence upon opioids

The inactivation of G-protein-linked signaling through GTP hydrolysis offers another unique site for regulation that may bedependent upon the level of receptor activation. Since the $alpha$ -subunitspossess intrinsic GTPase activity (see Dohlman and Thorner, 1997),the potential for signal regulation to occur through inactivationprompted efforts to identify other GTPase or GTPase-activatingproteins. A family of 20 known protein isoforms called Regulatorsof G-protein Signaling (RGS proteins) have beenidentified that exhibit high specificity as GTPase-activatingproteins that function to accelerate the exchange of GTP for GDPon the $alpha$ -subunits of G_i, G_o, and G_q (see Dohlman and Thorner,1997). The mRNAs encoding these different proteins are differentiallydistributed throughout the rat brain (Gold et al., 1997). ThemRNA for three of these proteins (i.e., RGS4, -7, and -8) hasbeen found in high abundance in the rat locus ceruleus (LC), whiletwo other areas heavily studied with respect to acute and chronicopioid effects, the nucleus accumbens and ventral tegmental area,express RGS8 mRNA in high abundance with moderate amounts of RGS4mRNA also present in the nucleus accumbens. As illustrated inFig. 1, these RGS proteins would increase the rate of GTP hydrolysisforcing the reassociation of the $beta$ $gamma$ -subunits with an $alpha$ -subunitand thereby turning off the signal mediated by both G-proteincomponents. This process has been suggested to participate inacute desensitization of µ-receptor-mediated activation of inwardlyrectifying K⁺ channels (GIRK) (Doupnik et al., 1997; Chuang et al., 1998).

Another mechanism by which GPCR signaling is acutely down-regulated involves receptor phosphorylation and subsequent internalizationor sequestration of the receptor into caveolae or clathrin-coatedpits. Phosphorylation of the receptor occurs through the actionof a family of six different protein isoforms known as G-protein-coupledReceptor Kinases (GRK, also known as $beta$ ARK). TheseGRK proteins are serine/threonine-phosphorylating proteins thatare differentially distributed and regulated in a wide varietyof tissues (see Krupnick and Benovic, 1998). Simplistically, theGRK-phosphorylated receptor is bound to one of a family of cytosolicproteins, $beta$ -arrestins, that uncouples the receptor from its cognateG-protein and targets the complex for sequestration in clathrin-coatedpits (see Krupnick and Benovic, 1998). Thus, the cellular machineryexists to regulate the responsiveness of the system in the shortterm via receptor availability rather than receptor abundance,and recent studies have demonstrated that the activation of G-proteinsby opioids and subsequent activation of GRK proteins plays animportant role in this process (Zaki et al., 2000). Receptor uncouplingand sequestration is an example of a mechanism that clearly associateswith tolerance. However, it is more difficult to explain physicaldependence by such amechanism.

An additional component of the GPCR signaling pathways impacting upon the levels of available receptors is the family of receptortyrosine kinases. This signaling pathway is activated by cellularprocesses that produce free G and/orG subunits or elevate intracellular Ca²⁺ (Luttrell et al., 1997) and eventually lead to the phosphorylationof mitogen-activated protein kinases (MAP kinases) (van Biesenet al., 1995). This protein family includes the Extracellularsignal-Regulated protein Kinases (ERKs) and theJun protein Kinases (JNKs), which phosphorylatedifferent transcription factors and serve as central intermediatesin signal transduction from the plasma membrane to the nucleus(see Segal and Greenberg, 1996). The participation of this seriesof proteins in a signaling cascade can also be directly influencedthrough the intracellular regulation of Ca²⁺ concentration and/or activation of protein kinase C (PKC). Bothchronic and acute exposure to morphine elevates the levels ofspecific ERKs in the rat brain (Berhow et al., 1996) and transfectedcell lines (Gutstein et al., 1997; Belcheva et al., 1998). Confocalimaging studies have also suggested a role for receptor internalizationfollowing µ-receptor stimulation in the activation of the MAPkinase pathway (Ignatova et al., 1999) that involves free Gsubunits and Ras (Belcheva et al., 1998).

Understanding the acute effects that follow occupation of µ-receptors provides signaling cascades that could participate ineither the short- or long-term regulation of responsiveness toopioids. One prominent acute action mediated by the µ-receptorthat is responsible for reduced neuronal excitability is the hyperpolarizationof the cell membrane due to activation of GIRK. The activationof GIRK by µ-receptors has been demonstrated in guinea pig myentericneurons (Cherubini et al., 1984), guinea pig and rat LC neurons(see Christie, 1991), rat nodose ganglion neurons (Ingram andWilliams, 1994), rat and guinea pig spinal trigeminal substantiagelatinosa neurons (Grudt and Williams, 1994), rat parabrachialneurons (Christie and North, 1988), rat anterior cingulate corticalneurons (Tanaka and North, 1994), rat periaqueductal gray neurons(Chieng and Christie, 1994), neurons in the hippocampal formation(Wimpey and Chavkin, 1991), as well as in expression systems transfectedwith µ-receptor and GIRK1 (Chuang et al., 1998). In particular,in both guinea pig myenteric neurons and rat LC neurons, the activationof GIRK has been demonstrated to occur without the requirementfor production of any diffusable substance like cyclic AMP (Miyakeet al., 1989; Johnson and Pillai, 1990).

In many brain regions, however, opioid receptor activation uses other mechanisms to regulate neuronal responsiveness includingthe regulation of transmitter release and/or postsynaptic membraneresponsiveness. One process activated by opioid receptor subtypes,especially $kappa$ , that could account for the presynaptic actions isthe interaction with calcium channels seen in several neuronalpopulations (see di Chiara and North, 1992; Moises et al., 1994).The µ-receptor-mediated activation of GIRK likely involves theG subunits released from G_i (Doupniket al., 1997; Chuang et al., 1998). One additional electrophysiologicaleffect that has been described for µ-receptor activation is inhibitionof a cAMP-dependent resting cation conductance in LC neurons (seeNestler and Aghajanian, 1997). However, the physiological relevanceand functional significance of these changes in LC neurons inthe production and propagation of the withdrawal response hasbeen questioned (Christie et al., 1997). Furthermore, the concentrationsof agonist required to activate this conductance are 100 to 200times greater than the concentration required to increase K⁺ conductance (see Fleming and Taylor, 1995). The latter effectclearly is important in the modulation of membrane potential byµ-receptor agonists (see di Chiara and North, 1992; Christie etal., 1997).

Other acute effects of µ-receptor activation have been identified that could be important in the signaling pathways that ultimatelylead to the adaptation. Particularly significant among these effectsis the inhibition of AC that has been described in a number ofneuronal populations (see Nestler et al., 1994; Fleming and Taylor,1995; Wang and Gintzler, 1997). The interaction of µ-receptorswith the AC cascade introduces an opportunity for the agoniststo impact on downstream effectors of the action of cAMP includingprotein kinase A (PKA) and the cyclic AMP response element-bindingprotein (CREB). This latter protein provides access of the cascadeto the nucleus for activation of transcription factors as suggestedin Fig. 1. However, µ-receptor activation has also been demonstratedto activate and/or translocate PKC in guinea pig longitudinalmuscle/myenteric plexus (LM/MP) (Wang et al., 1996), rat centralneurons (Mayer et al., 1995; Ventayol et al., 1997), and in vitroexpression systems (Kramer and Simon, 1999a,b). In periaqueductalgray neurons, acute µ-receptor-mediated responses involve activationof a voltage-dependent K⁺ conductance through an action on phospholipase A₂ (Ingram etal., 1998) thereby offering another cell signaling pathway thatalso is a site for the synergy that exists between the opioidsand nonsteroidal anti-inflammatory agents. Finally, µ-receptorshave also been shown to acutely activate the MAP kinase cascadethrough a Ras-dependent mechanism in expression systems (Gutsteinet al., 1997; Belcheva et al., 1998; Ignatova et al., 1999) aswell as the immediate early genes (e.g., fos) in brain tissue,permitting communication between the extracellular signal andthe nucleus (see Nestler et al., 1994; Nestler and Aghajanian,1997). Thus, the divergent acute effects of µ-receptor activationcan account for both the acute electrical events that regulateneuronal responsiveness in the short term as well as permit sufficientcross-talk among different signaling cascades between the cellsurface and the nucleus to provide a scaffold for regulation ofcellular protein abundance and, ultimately, neuronal sensitivityin the longterm.

	Effects of Chronic Exposure to Opioids

Top Abstract Introduction Cellular Mechanisms of Acute... Effects of Chronic Exposure... Conclusions and Future... References

Following chronic exposure to opioids, Cox (1978) identified two components of subsensitivity to opioids that differed incharacteristics and temporal relationships (see Johnson and Fleming,1989). One component decayed rapidly after drug removal and wasapparently dependent on the presence of the tolerance-inducingdrug, while the second component outlasted the presence of thedrug and was associated with long-lasting changes in the propertiesof opioid-sensitive neurons. A similar two-phase response hasbeen described during morphine withdrawal in rat behavior andin LC neurons (Rasmussen et al., 1990). Marked changes in behaviorand increases in LC firing rate occurred with a rapid declineover 4 h, followed by a lesser, prolonged effect that was undiminishedfor 24 h with complete recovery requiring 72 h. In the guineapig ileum, three components of subsensitivity have been identified.The first is the rapidly decaying homologous tolerance, probablyresulting from receptor uncoupling and internalization (Johnsonand Fleming, 1989). Second, chronic treatment with opioid leadsto sustained changes in G-proteins (Ammer et al., 1991) and theAC system (Wang et al., 1996; Wang and Gintzler, 1997) as indicatedin Table 1. Third, there is a slowly disappearing, heterologoustolerance that results from changes in resting membrane potentialdue to an alteration in electrogenic sodium pumping (see Table1 and Fleming, 1999).

The long-term nonspecific tolerance, membrane depolarization, and pump protein changes 1) are produced by the same procedure(i.e., morphine pellet implantation); 2) occur at the same time(i.e., 6-7 days after morphine pellet implantation, although acomplete time course has yet to be completed); 3) account forthe qualitative (nonspecific) characteristics of tolerance, includingthe subsensitivity to inhibitory agents and supersensitivity toexcitatory agents; 4) account for the magnitude of the subsensitivity(tolerance); and 5) occur in the same cells (the S-type myentericneurons). Compare to the five criteria presented earlier. Number4 above requires some elaboration. The half-maximum concentrationsof morphine and 2-chloroadenosine for twitch inhibition were determinedby Taylor et al. (1988). In that same study, maximum effect (i.e.,a doubling of the half-maximum effect) was achieved by concentrationsof each agonist approximately 10-fold greater. The depolarizationassociated with tolerance is 7 to 9 mV (Leedham et al., 1992).The approximate half-maximum concentrations of morphine and 2-chloroadenosine(from Taylor et al., 1988) hyperpolarized the control and tolerantS neurons by 6 to 8 mV (Meng et al., 1997). Because of the offsettingdepolarized state, to achieve the same twitch inhibition, twiceas much hyperpolarizing effect is required (see analysis by Fleming,1999). Doubling the half-maximum effect is achieved by a 10-foldincrease in concentration of each agonist (Taylor et al., 1988).Thus, a depolarized state should lead to a 10-fold subsensitivity,which is what is observed for twitch inhibition by either drugin tolerant preparations (Taylor et al., 1988). Since the low-efficacyagonist clonidine can only achieve 50% inhibition (Taylor et al.,1988), it cannot double its hyperpolarizing effect of 6 to 8 mV(Meng et al., 1997) to overcome the equal depolarized state intolerant neurons. Thus, it is predicted that clonidine's twitchinhibition should virtually disappear with tolerance; this iswhat is observed (Taylor et al., 1988). For the higher efficacyagonists, the maximum hyperpolarizing effect is limited by thepotassium equilibrium potential (E_k). Thus, depolarization, whichincreases the difference from E_k, allows for increases in themaximum opioid-mediated hyperpolarizations. In contrast, withclonidine, the low maximum effect is limited by its receptorsand associated signal transduction to ion channels, which do notchange (Meng et al., 1997).

The mechanism involves a global change in excitability with no evidence of altered receptor or signal transduction processesof only those neurons upon which the opioid acts (see Fleming,1999). Since this altered state of excitability is responsibleboth for subsensitivity to inhibitory substances and supersensitivityto excitatory substances, this mechanism is a clear example ofone that can explain both tolerance and physicaldependence.

Studies from this laboratory in the LM/MP (Leedham et al., 1989) have provided circumstantial evidence that homologous andheterologous tolerance may occur concomitantly. Analyzing thetime course over which tolerance develops and decays in the LM/MP,the concentration-response curve for morphine is shifted to theright nearly 2 times greater 4 days after pellet implantationas the shift observed for 2-chloroadenosine. However, by 7 daysafter implantation, the concentration-response curves are shiftedto the right by similar magnitudes, suggesting that both typesof tolerance may develop concomitantly in the same animal butwith different onset and/or decayrates.

A schematic summary of the major changes that have been documented in cell signaling proteins after chronic exposure to opioidsis presented in Fig. 2 and detailed in Table 1. In particular,Fig. 2 illustrates the fact that changes in a variety of signalingproteins and electrical excitability have been identified afterchronic treatment with opioid. In the rat LC and nucleus accumbens,chronic administration of opioids increases the abundance of ACand cyclic AMP-dependent protein kinase and decreases the abundanceof CREB immunoreactivity, all of which are consistent with subsensitivityto opioid-mediated inhibition of cAMP systems (Nestler et al.,1994; Nestler and Aghajanian, 1997). In addition, increases inthe levels of several cyclic AMP-dependent phosphoproteins, G-protein-coupledreceptor kinases ( $beta$ ARK1), and gene expression have been observedin the rat LC (see Nestler et al., 1994; Nestler and Aghajanian,1997). In the rat LC, chronic morphine increases the abundanceof the $alpha$ -subunits of G_i and G_o, while similar treatment decreasesthe levels of G_i in the rat nucleus accumbens. It is particularlyintriguing, however, that the elevated levels of G_i and G_o associatedwith tolerance and dependence in the rat LC disappear over a shorttime course similar to the rapid phase associated with behavioralchanges and changes in LC firing observed in homologous tolerance(Rasmussen et al., 1990). In the rat periaqueductal gray, chronictreatment with morphine induced a shift in coupling of µ-receptorsfrom a transduction process involving phospholipase A₂ to onethat was dependent upon AC and protein kinase A (Ingram et al.,1998). In addition, involvement of cAMP-dependent mechanisms hasbeen identified as a potential common locus to account for long-termchanges in GABAergic synaptic transmission in the ventral tegmentalarea following chronic cocaine or morphine treatment (Bonci andWilliams, 1996).

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Fig. 2. Schematic illustration of the identified modifications in cell signaling pathways and proteins that have been proposed to occur following chronic exposure to µ-opioid receptor agonist. The cellular substances that have been identified to change following chronic treatment with opioid are highlighted in red. The impact of changes in these cellular proteins on the characteristics of the tolerance that develops accounts for homologous tolerance if related to a specific signaling pathway or heterologous tolerance if the modification leads to generalized changes in cell excitability. The possibility that a change in one cellular locus (e.g., adenylyl cyclase) could actually evoke changes in other cellular effectors (e.g., sodium pump) through modification of gene expression is clearly an area of potentially fruitful research.

Changes in the AC system similar to those in the LC have been observed in the guinea pig LM/MP following chronic treatmentwith morphine. Interestingly, modulation of the AC cascade inthe LM/MP has been observed as a switch from a G_i-dependent inhibitionto a G_s-mediated stimulation of AC, phosphorylation of AC typeII (Chakrabarti et al., 1998), and an increase in AC type IV mRNA(Rivera and Gintzler, 1998). Furthermore, while there is a significantincrease in G_s (Wang and Gintzler, 1997) as seen in the rat LC,there was no significant change in G_i in these preparations. Themeaning of these observations, however, is still unclear sinceelectrophysiological data clearly indicate that modulation ofintracellular cAMP levels does not directly impact upon the electricalproperties of LM/MP neurons (Johnson and Pillai, 1990) and thealtered electrical properties adequately explain the tolerance,as discussed earlier in this review. These observations reinforcethe concept that multiple signaling pathways may be differentiallyinvolved in the short- and long-term effects of opioids in myentericneurons. It is important to emphasize that little attempt hasbeen made, thus far, to determine whether multiple pathways arealtered in other neuronalpopulations.

Studies from this laboratory evaluated the sensitivity of guinea pig nucleus tractus solitarius (nTS) and LC neurons 1 weekafter implantation of morphine or placebo pellets. Neurons ofthe nTS displayed a significant disinhibitory response to morphinethat was mediated by GABA (Malanga et al., 1997) similar to thatreported for neurons of the nucleus accumbens (Chieng and Williams,1998). When the disinhibitory effect of morphine was eliminatedby GABA_A receptor antagonism with bicuculline, neurons of theguinea pig nTS from animals treated chronically with morphinedisplay nonspecific (i.e., heterologous) subsensitivity to muscimol,2-chloroadenosine, clonidine, and morphine as well as supersensitivityto the excitatory effects of elevations of K⁺ in the bathing solution. This suggests that the cellular basisfor tolerance involves a general increase in excitability in neuronsof the nTS as in those of the myenteric plexus. Similarly, neuronsof the guinea pig LC display a reduced responsiveness to muscimoland µ-receptor activation following chronic treatment that isaccompanied by a reduced capacity of the sodium pump similar tothat of myenteric neurons (see Fleming, 1999).

	Conclusions and Future Directions

Top Abstract Introduction Cellular Mechanisms of Acute... Effects of Chronic Exposure... Conclusions and Future... References

The lack of a unifying hypothesis defining the cellular basis of tolerance to and/or dependence upon opioids can be largelyattributed to the complexity of opioid action involving severaldifferent signaling pathways. The basis for this diversity canbe found in the number of opioid receptors mediating the effectsof the narcotics and the very nature of those receptors (i.e.,GPCR superfamily). Multiple forms of tolerance to and dependenceon opioids have been characterized in terms of both time to development(acute versus chronic) and specificity characteristics (homologousversus heterologous). These two characteristics and the differencesthat exist in cells and tissues exhibiting the phenomena suggestthat multiple mechanisms must be considered at the very leastand, furthermore, that the development of the various forms oftolerance may occur concurrently. The fact that multiple signalingpathways can be activated via a single agonist using a singlereceptor subtype through the G-protein transducers provides amechanism to simultaneously involve many components in the processof cellular adaptation. 1) There is a rapid, short-lived homologoustolerance associated with very high agonist levels and clearlydue to receptor desensitization/uncoupling. 2) There is a tolerance(possibly homologous) with a moderate half-life associated withalterations in second messenger and transduction proteins. 3)There is a long-lasting heterologous tolerance resulting froma generalized increase in cellular excitability, partial membranedepolarization, and reduction in Na⁺, K⁺ pump protein. The fact that these three mechanisms can overlapin a given neuronal population is especially clear in myentericneurons. Whether these adaptations are independent of each otheris uncertain. The first mechanism, uncoupling of the receptorfrom its transduction process, could either trigger or impedeadaptations via the other two mechanisms. Mechanism 2 clearlycan lead to transcriptional changes that could participate inthe long-term regulation of other proteins involved in cell function.It is possible, therefore, that the alteration in AC-regulatedproteins (i.e., mechanism 2) may induce the reduction in pumpprotein in mechanism 3 in some neurons, as schematically illustratedin Fig. 2. It is also possible that different mechanisms playa primary role in different neuronalpopulations.

The capacity of cells to preferentially activate different signaling pathways depending on the magnitude of receptor occupationprovides an avenue to involve multiple pathways in adaptive processes.In addition to coinciding in time, however, the proposed cellularmechanisms that underlie the development of tolerance to opioidsand other drugs must also account for both the acute effects ofthe agonist and the long-term changes in cellular responsivenessthat are consistent with the observed specificity of the alteredresponsiveness. It is highly probable that multiple mechanismsare responsible for the development of tolerance and dependenceto opioids and that these divergent signaling pathways are likelyto be activated concurrently but to different degrees dependingupon the level of receptor activation. Therefore, future effortsmust begin to explore the impact of the level of receptor occupationon the signaling pathways that are activated and to develop someorder in the processes that areidentified.

	Acknowledgments

We thank Drs. Jian-Qiang Kong, Peggy S. Biser, and Stephen G. Graber for helpful discussions and suggestions during the preparationof this manuscript. We also acknowledge the technical and graphicsart assistance of Kathleen A.Thayne.

	Footnotes

Accepted for publication November 15, 2000.

Received for publication September 13, 2000.

Funding for work from the authors' laboratory upon which this perspective is based has been provided by the National Instituteon Drug Abuse through National Institutes of Health Grants RO1DA03773 and DA03773S1 and through funds from the Mylan Chair ofPharmacology, West VirginiaUniversity.

Send reprint requests to: Dr. David A. Taylor, Department of Pharmacology and Toxicology, Robert C. Byrd Health Sciences Center, P.O. Box 9223, West Virginia University School of Medicine, Morgantown, WV 26506-9223. E-mail: dtaylor{at}hsc.wvu.edu

	Abbreviations

AC, adenylyl cyclase [ATP pyrophosphate-lyase(cyclizing); EC 4.6.1.1], CREB, cyclic AMP response element-binding protein; GPCR, G-protein coupled receptor; GRK, G-protein coupled receptor kinase; GIRK, inwardly rectifying K⁺channel(s); LM/MP, longitudinal muscle/myenteric plexus; LC, locus ceruleus; nTS, nucleus tractus solitarius; RGS, regulators of G-protein signaling; PKA, protein kinase A; PKC, protein kinase C; E_k, potassium equilibrium potential; MAP kinase, mitogen-activated protein kinase; GABA, $gamma$ -aminobutyric acid.

	References

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