Regulation of G Protein-Coupled Receptor Kinases and Arrestins During Receptor Desensitization

doi:10.1124/mol.63.1.9

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Vol. 63, Issue 1, 9-18, January 2003

MINIREVIEW

Regulation of G Protein-Coupled Receptor Kinases and Arrestins During Receptor Desensitization

Trudy A. Kohout and Robert J. Lefkowitz

The Howard Hughes Medical Institute and the Departments of Medicine and Biochemistry, Duke University Medical Center, Durham, North Carolina

	Introduction

Top Introduction Receptor Phosphorylation... Regulation of GRKs through... Regulation of GRKs by... GRK Specificity for GPCRs:... Regulation of Arrestins during... Of Mice and MEFs:... Summary and Perspectives References

With at least 1000 family members encoded by mammalian genomes, the G protein-coupled receptors (GPCRs) represent the mostdiverse group of signaling proteins known (Bockaert and Pin, 1999).GPCRs are involved in the regulation of a wide variety of physiologicalprocesses including, but not limited to, the sensory perceptionsof pain, light, odors and tastes, cognition, muscle contraction,endocrine and exocrine secretion, metabolism, inflammation, andimmunity.

The classic paradigm of the GPCR signal transduction process is that upon ligand binding, conformational changes in the receptorarise that allow it to couple to the heterotrimeric G proteins.This coupling stimulates the G protein to alter the activity ofa variety of downstream effector molecules (Neer, 1995). In additionto G protein coupling, activation of a GPCR by its ligand alsoinitiates the process of receptor desensitization, an adaptiveresponse used by cells to arrest G protein signaling, thereforepreventing the potentially harmful effects that can result frompersistent receptorstimulation.

Almost every GPCR that has been studied undergoes desensitization and, despite their diversity, all cells use a universalmechanism for desensitizing GPCRs. This involves the coordinatedactions of two families of proteins, the G protein-coupled receptorserine/threonine kinases (GRKs) and the arrestins (Freedman andLefkowitz, 1996; Krupnick and Benovic, 1998; Pitcher et al., 1998;Ferguson, 2001). After binding to its agonist, a GPCR assumesa conformation that allows it to bind one or more of the GRKs(of which there are seven) and, in doing so, becomes phosphorylatedat residues on its intracellular loops and carboxyl terminus.Phosphorylation of the receptor promotes the high-affinity bindingof the arrestin family of proteins (of which there are four) tothe receptor, which physically interdicts further coupling toG proteins. This hindrance of coupling can result in as much asan 80% diminution of receptor signaling (Attramadal et al., 1992;Lohse et al., 1992).

It is also known that phosphorylation of GPCRs by several other kinases, such as protein kinases A and C (PKA and PKC) (Benovicet al., 1985; Roth et al., 1991; Pitcher et al., 1992a) and c-Src(Fan et al., 2001), can result in receptor desensitization. Thisprocess of desensitization involves a feedback mechanism in whichthe second messenger generated by the agonist-stimulated GPCRactivates a kinase that decreases the activity of the receptorand ultimately attenuates production of the second messenger.Despite contributions of a feedback mechanism to the desensitizationof GPCRs, desensitization can be fully reconstituted in vitrousing highly purified receptors, GRKs, and arrestins (Benovicet al., 1987; Attramadal et al., 1992; Lohse et al., 1992). Receptordesensitization is, in fact, highly regulated both through differencesin activity exhibited by each of the individual GRK and arrestinsubtypes and through their modulation by the activities of manyaccessory proteins. Herein, we review our current understandingof how GPCR desensitization is regulated by GRKs andarrestins.

	Receptor Phosphorylation Requires Recruitment of GRKs to the Plasma Membrane

Top Introduction Receptor Phosphorylation... Regulation of GRKs through... Regulation of GRKs by... GRK Specificity for GPCRs:... Regulation of Arrestins during... Of Mice and MEFs:... Summary and Perspectives References

For an agonist-occupied receptor to become phosphorylated by a GRK, the kinase first must be recruited to the plasma membraneand into a complex with the receptor. Of the seven GRK types identified,three are known to be constitutively associated with the plasmamembrane through covalent attachment of either fatty acids orisoprenes to their carboxyl termini: GRK4 (Premont et al., 1996)and GRK6 (Stoffel et al., 1994) are palmitoylated, whereas GRK1(Inglese et al., 1992) is farnesylated. Furthermore, GRK7 (Hisatomiet al., 1998; Weiss et al., 1998) has a CAAX sequence at its carboxylterminus that predicts geranylgeranyl modification. GRK5 is alsopredominantly associated with the membrane through interactionsbetween a positively charged domain located near its carboxylterminus and the negatively charged head groups of membrane lipids,including phosphatidylinositol-4,5-bisphosphate (PIP₂) (Pitcheret al., 1996). The binding of phospholipids also enhances theactivity of GRK5 by promoting its autophosphorylation (Kunapuliet al., 1994). Thus, five GRKs (1, 4, 5, 6, and 7) are locatedat the membrane and near the activated receptors, which they bindandphosphorylate.

The situation is more complex with regard to GRK2 and GRK3 because they do not undergo permanent lipid or isoprene modificationand are not constitutively associated with membranes. Rather,most of the cellular complement of these kinases is located inthe cytosol, and they undergo only transient recruitment to theplasma membrane after GPCR activation. Both these kinases possesspleckstrin homology domains, through which they bind to PIP₂ inthe plasma membrane (Fig. 1A) (Pitcher et al., 1995). However,translocation also requires G protein activation because GRK2and GRK3 must bind liberated G dimers to be recruitedto the membrane (Pitcher et al., 1992b). The importance of recruitmentof GRK2 in GPCR desensitization has been clearly demonstratedin vitro (Koch et al., 1993) and in vivo (Koch et al., 1995) usingthe isolated pleckstrin homology/G-binding domain ofGRK2 as an inhibitor to prevent the kinase from interacting withG subunits. This results in the receptors becoming poorlyphosphorylated, and thus desensitization is greatly diminished.

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Fig. 1. The regulation of GPCR desensitization by GRK2 and $beta$ -arrestins. A, receptor activation is followed by the recruitment of GRK2 by G to the receptor where it is anchored by phosphatidylinositol-4,5-bisphosphate and positioned to phosphorylate the C terminus of the receptor. GRK2 activity can be enhanced by its phosphorylation by protein kinase A (PKA), protein kinase C (PKC), and c-Src. Alternatively, GRK2 activity can be reduced by its phosphorylation by Erk1/2 or its binding to calcium/calmodulin (CaM). B, GRK2 can also inhibit receptor signaling by sequestering G_q to prevent its coupling to its effectors, such as PLC $beta$ . C. G_s-coupled receptors activate the effector adenylyl cyclase (AC) to generate the second messenger cAMP. After phosphorylation of the receptor by GRK, $beta$ -arrestin is recruited to the receptor, translocating PDE4 with it. This places the PDE4 on the membrane, the site of cAMP generation, thus allowing it to efficiently degrade cAMP to AMP and reduce signaling.

GRK2 and GRK3 have also been demonstrated to bind to the activated, GTP-bound form of the G_q subunit through domainslocated near the amino termini of the kinases, domains that showsignificant homology to the regulator of G protein signaling (RGS)family of proteins. Although RGS proteins are known to act aspotent GTPase accelerating proteins for a number of G protein $alpha$ subunits (Berman and Gilman, 1998), the RGS-like domains ofGRK2 and GRK3 enhance G_q GTPase activity only weakly (Carmanet al., 1999). However, this interaction greatly reduces G_qactivation of phospholipase C $beta$ after G_q-coupled receptor stimulationby a mechanism that is independent of desensitization of the receptors,because both a catalytically inactive mutant and an amino terminalfragment of GRK2 can inhibit inositol polyphosphate productionin cells (Carman et al., 1999; Sallese et al., 2000b). Thus, inaddition to their ability to phosphorylate GPCRs and mediate desensitization,GRK2 and GRK3 also are able to limit the extent of G_q-coupledreceptor signaling by sequestering G_q and preventing itscoupling to downstream effectors (Fig. 1B). It has also been hypothesizedthat the mere interaction of GRK2 and -3 with the GPCR, withoutthe requirement for receptor phosphorylation, could be sufficientto suppress signaling (Dhami et al., 2002; Freedman et al., 1997).

	Regulation of GRKs through Phosphorylation by Other Kinases

Top Introduction Receptor Phosphorylation... Regulation of GRKs through... Regulation of GRKs by... GRK Specificity for GPCRs:... Regulation of Arrestins during... Of Mice and MEFs:... Summary and Perspectives References

Several recent studies have shown that receptor phosphorylation by GRKs is modulated by the activity of other kinases thatdirectly phosphorylate the GRKs and alter a variety of their properties(Fig. 1A). The effects of a specific phosphorylation event aredetermined by what site becomes phosphorylated, which is dependenton the identity of the phosphorylating kinase. These effects includechanges in catalytic activity, protein binding affinity, and stabilityof the GRK protein. Most of these studies have focused on thephosphorylation of GRK2, but some have investigated the regulationofGRK5.

Most of the cellular complement of GRK2 exists in a basally phosphorylated state that maintains it in an inactive conformationin the cytosol. This was first demonstrated when two chemicallydistinct fractions of GRK2 protein were purified by gel filtrationfrom Sf9 cell lysates (Pitcher et al., 1999). The more abundantfraction was shown to be phosphorylated at Ser670, within a confirmedphosphorylation consensus sequence for the extracellular signal-regulatedkinases, Erk1 and Erk2. Phosphorylation of Ser670 in GRK2 causesa dramatic reduction in both the activity of the kinase and itsability to bind G subunits (Fig. 1A) (Pitcher et al.,1999). In doing so, the ability of GRK2 to be targeted to theplasma membrane and to phosphorylate receptors is directly regulatedby the Erk1/2 mitogen-activated protein kinase (MAPK) cascade(Pitcher et al., 1999). Indeed, constitutively active or dominant-negativemutants of the Erk1/2 activating kinase MEK1, alter the abilityof GRK2 to phosphorylate ligand-occupied receptors in the expectedmanner: inhibition of Erk1/2 activation with dominant negativeMEK1 enhances receptor phosphorylation, whereas activation ofErk1/2 with constitutively active MEK1 reduces it (Pitcher etal., 1999).

Furthermore, it has been demonstrated that GRK2 and Erk1 rapidly associate in cells after activation of the $beta$ ₂ adrenergicreceptor. In vitro assays have shown that this is enhanced bythe presence of both agonist-occupied receptor molecules and Gsubunits (Elorza et al., 2000). Taken together, these observationssuggest that phosphorylation of GPCRs by GRK2 is a tightly regulatedmechanism in which dephosphorylated GRK2 is recruited to its siteof action at the plasma membrane after GPCR activation. Once incomplex with the receptor and G subunits, GRK2 bindsErk1 or Erk2 (Elorza et al., 2000) and becomes phosphorylatedon Ser670 (Pitcher et al., 1999), deactivating the GRK2 and promotingits release from the plasma membrane back into to the cytosol.Thus, phosphorylation by Erk1/2 maintains the majority of thecellular pool of GRK2 in an inhibited or "off" state, which becomesactive only during agonist activation of the GPCR but is thenrapidly returned to the inactive state after binding to receptorsand G subunits. However, for such a mechanism to work,it would also require a phosphatase to become activated shortlyafter GPCR activation to remove the inhibitory phosphate moietyfrom GRK2 and allow it to be recruited to the receptors and tophosphorylate them. The identity of this phosphatase has yet tobeelucidated.

GPCR-mediated production of the second messengers cAMP, diacylglycerol, and inositol-1,4,5-trisphosphate (IP₃), leads to theactivation of the second messenger-activated kinases: PKA by cAMP,PKC by diacylglycerol, and calcium/calmodulin-activated kinasesby IP₃-induced calcium mobilization. It has long been appreciatedthat two of these kinases, PKA and PKC, directly induce receptordesensitization by phosphorylating GPCRs (Benovic et al., 1985;Roth et al., 1991; Pitcher et al., 1992a). More recently, it hasbeen demonstrated that PKA and PKC can also affect the desensitizationof GPCRs by phosphorylating GRK2 and altering its activity (Fig.1A) (Winstel et al., 1996; Cong et al., 2001). The best studiedof these systems involves the specific enhancement by PKA of GRK2activity toward the G_s/adenylyl cyclase-coupled $beta$ ₂ adrenergicreceptor. The $beta$ ₂ adrenergic receptor indirectly binds to PKA byvirtue of its interaction with the PKA scaffolding protein A-kinaseanchoring protein 79 (AKAP79) (Fraser et al., 2000). When the $beta$ ₂ adrenergic receptor is stimulated, cellular levels of cyclicAMP increase and PKA becomes activated, resulting in enhancedreceptor phosphorylation. This is sensitive to both chemical andtransfectable inhibitors of PKA activity, and is also dependenton PKA being tethered to the receptor by AKAP79, because disruptionof this interaction also inhibits receptor phosphorylation (Fraseret al., 2000). However, the enhancement is not the direct resultof increased phosphorylation of the receptor by PKA, because thesame effect is observed with a $beta$ ₂ adrenergic receptor mutant thatis not a PKA substrate. Instead, PKA phosphorylates GRK2 at serine685, which increases its binding affinity for G dimersand thus promotes the recruitment of GRK2 to the plasma membraneand into a complex with its activated receptor substrates (Conget al., 2001). This mechanism seems to be specific for GPCRs thatbind AKAP79, although alternative mechanisms for tethering PKAto other GPCRs may exist. Furthermore, it cannot be assumed thattethering is necessary for PKA to phosphorylate GRK2 under allcircumstances.

A similar mechanism may also exist after the activation of PKC by G_q-coupled receptors. Stimulation of the G_q-coupled $alpha$ _1Badrenergic receptor causes GRK2 to become phosphorylated at asite within its carboxyl terminus, which may be the same sitephosphorylated by PKA. Similarly, GRK2 phosphorylation can alsobe induced when cells are treated with either calcium ionophoresor with phorbol esters, both of which potently activate PKC. Asis the case with phosphorylation by PKA, PKC phosphorylation increasesthe activity of GRK2 toward receptors but not soluble substrates.Moreover, treating cells with phorbol esters causes GRK2 to redistributefrom the cytosol to the plasma membrane (Chuang et al., 1995;Winstel et al., 1996), indicating that phosphorylation of GRK2by PKC enhances recruitment to the membrane rather than increasingthe specific activity of thekinase.

Like GRK2, GRK5 also undergoes phosphorylation by PKC at an undetermined site in the carboxyl terminal region. However, ratherthan translocating it to the plasma membrane, phosphorylationof GRK5 inhibits its activity toward both receptors and solublesubstrates (Pronin and Benovic, 1997). Thus the PKC-mediated phosphorylationof GRK2 and GRK5 result in opposite effects on their activity.In fact, GRK5 phosphorylation by PKC functions in a manner similarto that of GRK2 phosphorylation by Erk1/2: to inactivate the GRKin response to specific cell-signaling events after receptor activation.It will be interesting to see whether other mechanisms known toregulate GRK2 activity are also applicable to GRK5 and the otherGRKs and whether similarities or differences in their regulationhelp illuminate specific functions for each of thesekinases.

After stimulation of the $beta$ ₂ adrenergic receptor, GRK2 has also been shown to undergo phosphorylation at several tyrosine residuesby the nonreceptor tyrosine kinase c-Src (Sarnago et al., 1999).This phosphorylation is dependent on the ability of $beta$ -arrestinto bind to and recruit c-Src to the receptor, because mutantsof $beta$ -arrestin that fail to bind to c-Src or to the receptor inhibitthe phosphorylation of GRK2 (Penela et al., 2001). Furthermore,a catalytically inactive mutant of GRK2 fails to be phosphorylatedby c-Src (Penela et al., 2001), presumably because it blocks phosphorylationof the receptor and so inhibits $beta$ -arrestin/c-Srcrecruitment.

Tyrosine phosphorylation affects GRK2 activity in two ways. First, it rapidly and transiently increases GRK2 activity, enhancingphosphorylation of GPCR substrates and promoting more rapid receptordesensitization (Fig. 1A) (Sarnago et al., 1999). Second, thetyrosine phosphorylation of GRK2 promotes its degradation by theubiquitin/proteosome pathway (Penela et al., 1998, 2001). It shouldbe noted that phosphorylation is a vital initial step in the ubiquitinationand degradation of a number of proteins. Although it is not knownwhich of the many E3 ubiquitin ligases that are expressed in cellsis responsible for GRK2 ubiquitination, it should also be notedthat the $beta$ -arrestins are known to bind to one such ligase, Mdm2(Shenoy et al., 2001). Thus, it is tempting to speculate that $beta$ -arrestin may recruit both c-Src and an ubiquitin ligase intocomplex with GRK2 and the receptor and so supply both the proteinsnecessary to target GRK2 for degradation. Phosphorylation of GRK2by c-Src, then, seems to act as the initial event in a long-termfeedback loop that regulates GRK2 activity within the cell byreducing GRK2 protein levels. This supplies the cell with a mechanismthat allows it to alter its responsiveness to a wide variety ofreceptor ligands and is of particular interest because cellularlevels of GRK2 protein are positively and negatively regulatedin a number of pathologies (Ungerer et al., 1994; Lombardi etal., 2001). Whether this represents a normal mechanism used bycells to respond to a disease state or it is somehow pathogenic,possibly through dysregulation of receptors, remains to beclarified.

	Regulation of GRKs by Calcium Sensing Proteins

Top Introduction Receptor Phosphorylation... Regulation of GRKs through... Regulation of GRKs by... GRK Specificity for GPCRs:... Regulation of Arrestins during... Of Mice and MEFs:... Summary and Perspectives References

Calcium signaling is a common feature in all cell types and impacts many aspects of cell physiology, including GPCR signaling.Increases in the cytosolic concentration of calcium ions, eitherbecause of its release from intracellular stores or influx fromoutside the cell through calcium channels in the plasma membrane,results in the activation of a group of calcium-binding proteinsknown collectively as calcium sensor proteins (CSPs). A numberof CSPs are known to interact with and alter the activities ofGRKs (Sallese et al., 2000a). The best studied of these is recoverin,a CSP found predominantly in photoreceptor cells, where it functionsby binding to GRK1 and inhibiting its ability to phosphorylaterhodopsin (Chen et al., 1995; Klenchin et al., 1995). Becausebasal calcium levels in the cytosol of photoreceptors are high,it is believed that recoverin acts to "silence" GRK1 activityin the dark when the cells are not signaling and to relieve theinhibition after light stimulation when calcium levels are lowered,allowing GRK1 to phosphorylate rhodopsin and initiate desensitization.Several other recoverin-like CSPs also bind to and inhibit GRK1(De Castro et al., 1995; Sallese et al., 2000a). The specificfunctions of these interactions have yet to bedetermined.

The ubiquitously expressed calcium sensor calmodulin (CaM) inhibits the activity of all the GRKs except GRK1 (Fig. 1A) (Chuanget al., 1996). Calcium-bound calmodulin (Ca/CaM) binds to an amino-terminalregion common to GRK2, -3, -4, -5, and -6 (Pronin et al., 1997).In addition, Ca/CaM also binds to GRK2 and 5 through sites intheir carboxyl termini (Levay et al., 1998; Pronin et al., 1998).The relative sensitivity of the GRKs to CaM inhibition variesgreatly: GRK2 is the least sensitive (IC₅₀, ~2 µM), and GRK5 isthe most sensitive (IC₅₀, 40-50 nM) (Chuang et al., 1996; Proninet al., 1997). The mechanism of inhibition also varies betweenGRKs, because Ca/CaM directly inhibits GRK2 catalytic activitybut acts on GRK5 by inducing inhibitory autophosphorylation aswell as blocking membrane association and possibly also by interferingwith receptor recognition (Pronin et al., 1998). The functionalsignificance of these differences is not well studied, but itis likely that they allow cells to regulate GPCRs in a highlyspecific manner in response to fluctuations in intracellular calciumlevels.

	GRK Specificity for GPCRs: Lessons from Genetically Altered Mice

Top Introduction Receptor Phosphorylation... Regulation of GRKs through... Regulation of GRKs by... GRK Specificity for GPCRs:... Regulation of Arrestins during... Of Mice and MEFs:... Summary and Perspectives References

It has been suggested that functional redundancy might exist between the seven isoforms of GRK, with there being little orno specificity, or that there may be some subtype specificityin phosphorylating different GPCR substrates. In fact, numerousstudies using heterologous expression of the different GRKs toidentify which GPCRs can act as their substrates have revealedexamples of both redundancy and specificity of GRK function. Forexample, GRKs exhibit redundancy with regard to the $beta$ ₂ adrenergicreceptor because it can be phosphorylated and desensitized byGRKs 2 through 6 (Benovic et al., 1989, 1991; Benovic and Gomez,1993; Premont et al., 1994, 1996). In contrast, the secretin andthe parathyroid hormone receptors can be phosphorylated and desensitizedonly by GRKs 2, 3, and 5 (Shetzline et al., 1998; Flannery andSpurney, 2001). Furthermore, although overexpression of eitherGRK2, -3, -4, -5, or -6 results in phosphorylation of the vasoactiveintestinal polypeptide type-1 receptor, only phosphorylation byGRKs 2, 3, or 5 actually leads to the receptors becoming desensitized(Shetzline et al., 2002).

With the recent generation of GRK transgenic and knockout mouse models, the true extent of specificity of function for theGRKs has now begun to be elucidated. Although these studies arestill in their infancy, with only a few receptors having beenexamined, the results so far show that defined roles for eachof the GRKs do exist (Tables 1 and 2). The following is a reviewof the results of the GRK transgenic and knockout models investigatedso far.

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TABLE 1
GRK and arrestin knockout mice phenotypes and target GPCRs
It is important to note that the phenotype of the knockout animals have been tested only by the stimulation of the listed GPCRs. The number of other GPCRs affected by the GRK and arrestin gene deletions is unknown. No phenotype indicates that stimulation of the listed GPCR was carried out and the response was not different from wild type animals.

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TABLE 2
In vivo specificity of GPCR regulation in GRK-overexpressing transgenic mice
GRK2 overexpression was targeted to either the heart or the vasculature. GRK4 gene polymorphism A142V was targeted to all tissues. All other GRK transgenic mice have targeted overexpression in the heart. No phenotype indicates that stimulation of the listed GPCR was carried out and the response was not different from wild-type animals

Genetically modified animals bearing targeted deletions of GRK1, GRK2, GRK3, GRK5, and GRK6 have been constructed to studythe roles of individual GRKs in various pathways of receptor signaling.In addition, mice with cardiac-specific overexpression of GRK2,GRK3, and GRK5 have been generated, and a mouse overexpressingGRK4 in all tissues has also beendeveloped.

GRK1 (rhodopsin kinase) knockout animals display an almost complete lack of light-induced phosphorylation of rhodopsin, resultingin a larger and more prolonged response of the retinal rod cellsto light (Table 1) (Chen et al., 1999). Similarly, the responseof the cone cells is also impaired, showing a recovery rate 30to 50 times slower than in wild-type mice (Lyubarsky et al., 2000).Furthermore, the absence of GRK1 resulted in morphological changesin the retina from light-dependent apoptosis of the rod cellsand the degeneration ofvision.

A GRK2 knockout animal has not been studied because they displayed embryonic lethality by gestational day 15.5. The embryosshowed pronounced hypoplasia of the ventricular myocardium, suggestingthat GRK2 plays an important role during embryogenesis and isessential in cardiac development (Jaber et al., 1996). Becauseablation of GRK2 is embryonically lethal, in vivo studies havebeen performed using the heterozygous GRK2 knockout mice [GRK2( $-$ /+)]instead. In studies of $beta$ -adrenergic signaling in the heart, GRK2( $-$ /+)mice showed enhanced cardiac contractile function compared withthe wild-type mice demonstrating that cardiac function can bemodulated by GRK2 activity (Table 1) (Rockman et al., 1998).To further decrease GRK2 activity in vivo, the GRK2( $-$ /+) micewere crossed with a transgenic mouse with targeted myocardialoverexpression of a GRK2 inhibitor fragment, $beta$ ARKct. The resultof this cross is a further lowering of GRK2 activity in cardiactissues and a subsequent enhancement of cardiac contractilityin comparison with the GRK2( $-$ /+) mouse (Rockman et al., 1998).The biochemical analysis of the hearts of the hybrid mice showeddecreased receptor phosphorylation and enhanced $beta$ -adrenergic signaling.Conversely, the targeted overexpression of GRK2 in the myocardium(Koch et al., 1995) or in vascular smooth muscle (Eckhart et al.,2002) resulted in an attenuation of agonist-stimulated cardiaccontractility or vasodilation, respectively (Table 2). This seriesof experimental data clearly demonstrate in vivo that GRK2 servesto modulate $beta$ -adrenergic signaling in the heart andvasculature.

Overexpression of either GRK2 or -3 in cultured cells results in an agonist-stimulated increase in both $alpha$ _1B-adrenergic ( $alpha$ _1B-AR)(Diviani et al., 1996) and $beta$ -AR (Benovic et al., 1991) phosphorylationand desensitization. To investigate whether both GRK2 and -3 affectin vivo function of the $alpha$ _1B-AR, transgenic mice were generatedwith concomitant cardiac overexpression of $alpha$ _1B-AR and either GRK2or -3. Interestingly, overexpression of GRK2 had no effect onthe $alpha$ _1B-AR-mediated cardiac phenotype; however, overexpressionof GRK3 completely attenuated cardiac $alpha$ _1B-AR signaling (Table2) (Eckhart et al., 2000). Thus, although $alpha$ _1B-AR shows no invitro specificity for either GRK2 or -3, GRK3 is the relevantGRK for desensitizing the $alpha$ _1B-AR in the heart. As described previously,myocardial overexpression of GRK2 leads to attenuation of $beta$ -ARsignaling. In contrast, overexpression of GRK3 resulted in completelynormal $beta$ -AR signaling, having no effect on the $beta$ -AR-mediated cardiacresponses (Iaccarino et al., 1998). Analysis of the in vivo functionof other GPCRs in the GRK3 cardiac overexpression model revealedthat angiotensin II type 1 receptor function is unaltered, whereasthrombin signaling is attenuated (Table 2) (Iaccarino et al.,1998), again indicating that GRKs show substrate specificity evenwhen expressed within the same tissuetype.

In olfactory epithelium, GRK2 is virtually absent but GRK3 is expressed to a high degree. Consistent with in vitro data suggestingthe involvement of GRK3 in olfactory signal transduction, deletionof the GRK3 gene results in the complete lack of fast odorant-induceddesensitization of second messenger production in cilia preparations(Table 1) (Peppel et al., 1997). Interestingly, despite the extensivesimilarity to GRK2, GRK3 gene deletion does not alter embryonicand postnatal development. Further physiological studies on theGRK3 knockout mouse [GRK3( $-$ / $-$ )] have determined a role for GRK3in airway responses. Agonist stimulation of cholinergic muscarinicreceptors in GRK3( $-$ / $-$ ) animals resulted in an enhanced airwayresponse compared with wild-type mice, as well as a baroreflexpotentiation of heart rate (Table 1) (Walker et al., 1999). Thus,in vivo, GRK3 displays a physiological specificity for the desensitizationof odorant and muscarinicreceptors.

Because the GRK4 gene locus has been linked to hypertension, a transgenic mouse overexpressing GRK4 in all tissues was constructedto explore the in vivo role of GRK4 in hypertension and in desensitizationof the D1 dopaminergic receptor (D1R) (Felder et al., 2002). Inessential hypertension there is a defective coupling of the renalD1R with its effector that results in impaired urinary sodiumexcretion. The naturally occurring polymorphism A142V in GRK4has increased kinase activity toward the D1R relative to wild-typeGRK4. Transgenic mice carrying this polymorphism displayed a hypertensivephenotype, whereas wild-type GRK4 transgenic mice did not (Table2). Furthermore, whereas D1R agonists normally increase urinarysodium excretion, this effect was impaired in GRK4(A142V) transgenicmice (Felder et al., 2002). Thus, the increased phosphorylationof the D1R by GRK4 results in impaired signal transduction thatmay ultimately lead to the pathogenesis ofhypertension.

In addition to GRK2, GRK5 is also highly expressed in heart supporting a role for this kinase in the regulation of cardiacfunctions. Transgenic mice overexpressing GRK5 in a cardiac specificmanner show a marked enhancement of $beta$ -AR desensitization (Table2) (Rockman et al., 1996). Furthermore, contractility in responseto $beta$ -agonists is attenuated, yet, the response to angiotensinII remains unchanged (Rockman et al., 1996). To further investigatethe role of GRK5 in vivo, GRK5 gene deletion mice were generated.The GRK5 knockout mice [GRK5( $-$ / $-$ )] displayed no differences indopamine agonist-induced locomotor responses compared with wild-typeanimals, as well as in serotonin 5-HT1A induced hyperthermic responses(Gainetdinov et al., 1999). However, classic cholinergic muscarinicreceptor responses such as hypothermia and hypoactivity were enhancedin GRK5( $-$ / $-$ ) mice (Table 1) (Gainetdinov et al., 1999). Biochemicalassays also demonstrated a lack of muscarinic receptor desensitizationin the knockout animals. Thus, in vivo, GRK5 targets the $beta$ -adrenergicreceptors and muscarinic receptors but not the angiotensin II,dopamine, and serotoninreceptors.

GRK-mediated phosphorylation of the chemokine receptor CXCR4 has been shown to be important in the regulation of the CXCL12(stromal cell-derived factor 1)-stimulated CXCR4 signaling (Orsiniet al., 1999). To understand the role and specificity of GRKsin the chemotactic response generated by the activation of CXCR4,lymphocytes derived from GRK5 and GRK6 knockout animals were stimulatedwith CXCL12 and their ability to undergo chemotaxis was measured(Fong et al., 2002). Whereas there was no difference in the chemotacticactivity between GRK5 knockout lymphocytes and those derived fromwild-type mice, lymphocytes from GRK6-deficient animals were strikinglyimpaired in their ability to respond to CXCL12 (Table 1). Thus,GRK6 is specifically required for the in vivo phosphorylationof the CXCR4, which allows lymphocytes to respond correctly tothe chemotactic agent (Fong et al., 2002).

The evidence collected to date from cellular studies and genetically altered mice suggests that there is GRK specificity forparticular GPCRs. That is, all GPCRs are not regulated equivalentlyby all the GRKs expressed in a cell, and many GPCRs seem to befunctionally paired with a particular GRK. Further research incellular and mouse models will be required to delineate fullythe GRK specificity forGPCRs.

	Regulation of Arrestins during Desensitization

Top Introduction Receptor Phosphorylation... Regulation of GRKs through... Regulation of GRKs by... GRK Specificity for GPCRs:... Regulation of Arrestins during... Of Mice and MEFs:... Summary and Perspectives References

Several reports have described how the activities of the arrestins are regulated through post-translational modification andinteractions with accessory proteins. However, the majority ofthese interactions are concerned with the regulation of arrestinswhile functioning as adaptors during receptor internalization(for reviews, see Krupnick and Benovic, 1998; Ferguson, 2001;Claing et al., 2002; Perry and Lefkowitz, 2002) and have littleor no effect on their ability to desensitize receptors. For instance,phosphorylation of $beta$ -arrestin 1 (arrestin 2) on serine 412 bythe Erk1/2 kinases does not affect its ability to bind to anddesensitize the $beta$ ₂ adrenergic receptor (Lin et al., 1999). However,phosphorylation at this site does considerably reduce the internalizationof the receptor, because it inhibits the binding of clathrin to $beta$ -arrestin 1, which prevents the accumulation of receptors inclathrin-coated pits (Lin et al., 1997). However, one examplehas been described in which phosphorylation of an arrestin doesalter its ability to desensitize a receptor. In the Drosophilamelanogaster visual system, arrestin 2 (the major arrestin foundin D. melanogaster photoreceptor cells and most homologous tomammalian $beta$ -arrestin 2) binds to and desensitizes light-activatedrhodopsin molecules. Only unphosphorylated D. melanogaster arrestin2 is capable of binding rhodopsin, and its subsequent phosphorylationby calcium/calmodulin-dependent kinase II releases arrestin 2from rhodopsin (Alloway et al., 2000; Kiselev et al., 2000). BecauseD. melanogaster rhodopsin is a G_q-coupled receptor, activationby light stimulates the production of the second messengers IP₃and diacylglycerol and the release of calcium ions from intracellularstores. This results in a rapid activation of Ca/CaM-dependentkinase II and phosphorylation of arrestin 2. Thus, very soon afterrhodopsin becomes activated and desensitized by binding arrestin2, Ca/CaM-dependent kinase II phosphorylates the arrestin 2 andit dissociates from rhodopsin, allowing the photoreceptors toresensitize. This tightly regulated mechanism of rapid activation,desensitization, and resensitization ensures that the photoreceptorscan be repeatedly stimulated with light and not become permanentlydesensitized, a necessary adaptation for the correct functionof any highly responsive sensorysystem.

To allow a resensitized receptor to instigate further signaling, second messenger molecules that were synthesized (or mobilized,in the case of calcium ions) during previous rounds of signalingmust be removed from the cell. In the D. melanogaster visual system,this requires the return of calcium ions to the endoplasmic reticulumor to the extracellular milieu and the degradation of IP₃ anddiacylglycerol. In the case of G_s-coupled receptors, such as the $beta$ ₂AR, cAMP must be degraded to AMP by phosphodiesterase enzymes(Houslay, 2001). Until recently, the mechanisms that are responsiblefor degrading second messengers were thought to function independentlyof receptor desensitization. However, it has now been shown that,at least for the G_s-coupled $beta$ ₂AR, the $beta$ -arrestins form a linkbetween the two processes because they interact with the PDE4family of phosphodiesterases (Fig. 1C) (Perry et al., 2002). After $beta$ ₂ adrenergic receptor activation, the $beta$ -arrestins are recruitedto and desensitize the receptor molecules, translocating PDE4swith them to the plasma membrane. Because the plasma membraneis the site of cyclic AMP production by adenylyl cyclase enzymes,this results in both a reduction in the rate of synthesis of cyclicAMP (because the desensitized receptors can no longer couple aswell to G_s) and an increase in the rate of its degradation bythe higher levels of PDE4 activity present on the membrane (Perryet al., 2002). In this manner, the $beta$ -arrestins both desensitizethe receptors and facilitate the quenching of signaling by aidingin the degradation of second messenger molecules. It will be veryinteresting to see whether this paradigm extends beyond PDEs andG_s-coupled receptors to other second messenger degrading enzymes,such as those that eliminate diacylglycerol and IP₃ after G_q-coupledreceptorstimulation.

	Of Mice and MEFs: Revealing Specificity for GPCRs and the Arrestins

Top Introduction Receptor Phosphorylation... Regulation of GRKs through... Regulation of GRKs by... GRK Specificity for GPCRs:... Regulation of Arrestins during... Of Mice and MEFs:... Summary and Perspectives References

Until genetic knockout mouse strains lacking expression of specific arrestins became available the first, and best, evidencethat the different arrestin isoforms might be used preferentiallyby different receptors came from a study that compared in vitrothe ability of purified visual arrestin, $beta$ -arrestin 1, and $beta$ -arrestin2 (arrestins 1, 2, and 3) to desensitize rhodopsin and the $beta$ ₂adrenergic receptor (Attramadal et al., 1992). This study confirmeda high degree of specificity for visual arrestin by rhodopsinthat had already been suspected based on the highly restrictedand overlapping expression patterns of the two molecules (Wildenet al., 1986). However, it also suggested that the two $beta$ -arrestinsmight be functionally redundant because they showed identicaldesensitizing activity toward the $beta$ ₂ adrenergic receptor (Attramadalet al., 1992). Later efforts that used heterologous expressionand antisense RNA "knock-down" methods also failed to identifyany receptor preferences between $beta$ -arrestin 1 and 2 (Mundell etal., 1999).

Unlike arrestin, $beta$ -arrestin 1 and 2 are ubiquitous; hence, their GPCR specificities cannot be inferred from their expressionpatterns (Attramadal et al., 1992). To define the physiologicalroles of $beta$ -arrestin 1 and 2 in the regulation of GPCRs, knockoutmouse models were generated. Both knockout animals have neithergross abnormalities nor an overt phenotype (Conner et al., 1997;Bohn et al., 1999). When challenged with various stimuli, however,physiological differences with their wild-type littermates becomeapparent. When increasing concentrations of the $beta$ -agonist isoproterenolwere infused into the heart of the $beta$ -arrestin 1 knockout mouse,the resulting cardiac ejection fraction was significantly greaterthan in the wild-type mouse (Table 1) (Conner et al., 1997).This result suggested that there is enhanced $beta$ -adrenergic signalingin mice lacking $beta$ -arrestin 1 and consequently that $beta$ -arrestin1 is important for in vivo $beta$ -ARdesensitization.

To date, the $beta$ -arrestin 2 knockout animals have been used to study the in vivo desensitization of the opioid and chemokineCXCR4 receptors (Table 1). In the $beta$ -arrestin 2 knockout mice,the analgesic effects of morphine were potentiated and prolongedcompared with the wild type. Using specific antagonists for thedifferent isoforms of the opioid receptor, the effect was localizedto the impaired desensitization of the µ-opioid receptor (Bohnet al., 1999). Interestingly, the $beta$ -arrestin 2 knockout mice didnot develop tolerance to morphine but did develop dependence (Bohnet al., 2000). This suggests that the phenomena of desensitizationand tolerance are closely linked, whereas dependence occurs bya different mechanism. The chemotactic responses to CXCL12 mediatedthrough the CXCR4 receptors were markedly impaired in lymphocytesderived from $beta$ -arrestin 2 deficient mice, similar to the phenotypeobserved in GRK6 knockout lymphocytes (Fong et al., 2002). Thus,for desensitization of the CXCR4 receptor to occur in vivo, itwould seem to need to be first phosphorylated by GRK6 and thento bind $beta$ -arrestin 2. It will be of great interest in future studiesto compare the physiological responses of the $beta$ -arrestin 1 and2 knockout mice to the same stimulus and to thus determine theselectivity of either $beta$ -arrestin for a specific GPCR.

There is a limitation in studying the overall effects of $beta$ -arrestin in the knockout mice generated, because only one of thetwo ubiquitous $beta$ -arrestins was eliminated. The ideal experimentalmodel in which to analyze the roles of $beta$ -arrestin and the selectivityof $beta$ -arrestin 1 and 2 for particular GPCRs would be one that lacksboth $beta$ -arrestins. Unfortunately, $beta$ -arrestin 1 and 2 double knockoutmice could not be obtained because they displayed embryonic lethality.This hurdle was overcome by generating mouse embryonic fibroblastsfrom embryos that lack $beta$ -arrestin 1 or 2, or both (Kohout et al.,2001). These cells were then used to carefully dissect the rolesof $beta$ -arrestin 1 and 2 in the desensitization of various GPCRs.Experiments showed that desensitization of the $beta$ ₂-adrenergic andthe AT_1A receptors is impaired in cells lacking one or the otherof the $beta$ -arrestins and severely impaired in cells lacking both $beta$ -arrestins. However, there is no appreciable difference between $beta$ -arrestins 1 and 2 in their ability to desensitize these receptors(Kohout et al., 2001). This is in sharp contrast to the individualabilities of $beta$ -arrestins 1 and 2 to mediate sequestration of the $beta$ ₂ adrenergic receptor, because $beta$ -arrestin 2 is dramatically moreefficient than $beta$ -arrestin 1 (Kohout et al., 2001). However, similarexperiments analyzing the sequestration of the AT_1A receptor showedthat both $beta$ -arrestins are equally capable of mediating its internalization.Interestingly, the protease-activated receptor 1 (PAR1) does notdesensitize in the absence of $beta$ -arrestin 1 but has a normal desensitizationprofile in the absence of $beta$ -arrestin 2 (Paing et al., 2002). Hence, $beta$ -arrestin 1 seems to be the major regulator of PAR1 desensitization.This is the first example of a $beta$ -arrestin differentially regulatingGPCR desensitization. These data suggest that the ability of aparticular $beta$ -arrestin to either desensitize or sequester a GPCRis receptor-specific.

	Summary and Perspectives

Top Introduction Receptor Phosphorylation... Regulation of GRKs through... Regulation of GRKs by... GRK Specificity for GPCRs:... Regulation of Arrestins during... Of Mice and MEFs:... Summary and Perspectives References

Our understanding of the mechanisms involved in the regulation of GPCR desensitization has developed considerably over thepast decade. The complexity of regulation of GPCR desensitizationis now known to far exceed the simple model of GPCR phosphorylationby GRKs followed by arrestin binding and uncoupling of G proteinsignaling. GRK activities are not simply triggered by agonist-occupiedreceptors; rather, they are extensively regulated by a plethoraof interactions with and modifications by other proteins. Similarly, $beta$ -arrestins not only serve to physically interdict signaling tothe G protein but also further enhance GPCR desensitization bytranslocating cytosolic proteins such as PDEs and c-Src to thereceptor. Once at the membrane, PDEs and c-Src can turn off signalingat its source by degradating cAMP or by phosphorylating GRK2 toenhance its activity toward the receptor,respectively.

One of the most intriguing questions in GPCR desensitization is why the family of GRKs comprises seven members and the familyof arrestins has four members. Are the enzymatic activities ofthe various GRKs redundant or is there substrate specificity foreach one? Do the arrestins translocate to and subserve desensitizationequally well for all GPCRs or do they have specialized functions?Recent observations in transgenic mouse models, as well as knockoutmice and cells derived from knockout mice, have clearly indicatedthat such specificity does exist for both GRKs and arrestins.For example, in vivo signaling of the $alpha$ _1B-AR in the heart wasattenuated by the overexpression of GRK3 but not GRK2. In contrast,in the same cardiac-specific transgenic mouse models, GRK2 overexpressionattenuates AT₁R function, whereas GRK3 overexpression is ineffective.An even more illustrative example of differential regulation byGRK2 and 3 is their different roles in embryonic development.Whereas GRK2 knockout mice display embryonic lethality by gestationalday 15, GRK3 knockout mice live normally to maturity. It is evidentthat despite their structural and regulatory similarities, GRK2and GRK3 cannot substitute for one another. Indeed, it is likelythat GRK4, -5, -6, and -7, which are even more divergent in structureand in vitro substrate specificity from GRK2 and -3, have verydifferent in vivo modes of action and receptor specificity. Theeffects of $beta$ -arrestins 1 and 2 on the function of a specific GPCRhave not been compared in an in vivo setting. However, it is quitepossible that such differences will be found, as has been thecase with the GRKs, because studies in mouse embryonic fibroblastsderived from the $beta$ -arrestin knockout animals have shown, for example,that the PAR1 receptor can only be desensitized by $beta$ -arrestin1 and that $beta$ -arrestin 2 cannot substitute for thisfunction.

The regulation of GRKs and arrestins in GPCR desensitization process remains an exciting and vibrant field of investigation.Because more research is carried out in genetically altered mice,our appreciation of the distinctions between the members of theGRK and arrestin families will certainlyincrease.

	Acknowledgments

We thank Dr. Stephen J. Perry for valuable discussions and D. Addison and J. Turnbough for excellent secretarialassistance.

	Footnotes

Received September 9, 2002; Accepted October 16, 2002

This work was supported in part by National Institutes of Health Grant HL16037. R.J.L. is an Investigator of the Howard HughesMedicalInstitute.

Address correspondence to: Robert J. Lefkowitz, The Howard Hughes Medical Institute, Dept. of Medicine and Biochemistry, Duke University Medical Center, Research Dr., Box 3821, Carl Bldg., Rm. 468, Durham, NC 27710. E-mail: lefko001{at}receptor-biol.duke.edu

	Abbreviations

GPCR, G protein-coupled receptor; GRK, G protein-coupled receptor kinase; PKA, protein kinases A; PKC, protein kinase C; PIP₂, phosphatidylinositol-4,5-bisphosphate; RGS, regulator of G protein signaling; Erk, extracellular signal-regulated kinase; IP₃, inositol-1,4,5-trisphosphate; CSP, calcium sensor protein; CaM, calmodulin; AR, adrenergic receptor; PDE, phosphodiesterase; PAR1, protease-activated receptor 1.

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MINIREVIEW Regulation of G Protein-Coupled Receptor Kinases and Arrestins During Receptor Desensitization

MINIREVIEW

Regulation of G Protein-Coupled Receptor Kinases and Arrestins During Receptor Desensitization