Multiple Active States and Oligomerization of CCR5 Revealed by Functional Properties of Monoclonal Antibodies

doi:10.1091/mbc.01-03-0129

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Originally published as MBC in Press, 10.1091/mbc.01-03-0129 on February 4, 2002

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Vol. 13, Issue 2, 723-737, February 2002

Multiple Active States and Oligomerization of CCR5 Revealed by Functional Properties of Monoclonal Antibodies

Cédric Blanpain,^* Jean-Marie Vanderwinden, Josef Cihak, Valérie Wittamer,^* Emmanuel Le Poul,^§ Hassan Issafras, Manfred Stangassinger, Gilbert Vassart,^*^¶ Stefano Marullo, Detlef Schlndorff,^# Marc Parmentier,^*^@^** and Matthias Mack^#

^*Institut de Recherche Interdisciplinaire en Biologie Humaine et Nucléaire, Laboratoire de Neurophysiologie, Service de Génétique Médicale, and ^@Laboratoire de Cytologie et Cancérologie Expérimentale, Université Libre de Bruxelles, B-1070 Brussels, Belgium; Institute for Animal Physiology, University of Munich, 80539 Munich, Germany; ^§Euroscreen s.a., B-1070 Brussels, Belgium; ^¶Département de Biologie Cellulaire, Institut Cochin de Génétique Moléculaire, 75014 Paris, France; and ^#Medizinische Poliklinik, University of Munich, 80336 Munich, Germany

Submitted March 21, 2001; Revised November 19, 2001; Accepted November 19, 2001
Monitoring Editor: Peter N. Devreotes

	ABSTRACT

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION CONCLUSION REFERENCES

CC-chemokine receptor 5 (CCR5) is the principal coreceptor for macrophage-tropic strains of human immunodeficiency virus type1 (HIV-1). We have generated a set of anti-CCR5 monoclonal antibodiesand characterized them in terms of epitope recognition, competitionwith chemokine binding, receptor activation and trafficking, andcoreceptor activity. MC-4, MC-5, and MC-7 mapped to the amino-terminaldomain, MC-1 to the second extracellular loop, and MC-6 to a conformationalepitope covering multiple extracellular domains. MC-1 and MC-6inhibited regulated on activation normal T cell expressed andsecreted (RANTES), macrophage inflammatory polypeptide-1 $beta$ , andEnv binding, whereas MC-5 inhibited macrophage inflammatory polypeptide-1 $beta$ and Env but not RANTES binding. MC-6 induced signaling in differentfunctional assays, suggesting that this monoclonal antibody stabilizesan active conformation of CCR5. Flow cytometry and real-time confocalmicroscopy showed that MC-1 promoted strong CCR5 endocytosis.MC-1 but not its monovalent isoforms induced an increase in thetransfer of energy between CCR5 molecules. Also, its monovalentisoforms bound efficiently, but did not internalize the receptor.In contrast, MC-4 did not prevent RANTES binding or subsequentsignaling, but inhibited its ability to promote CCR5 internalization.These results suggest the existence of multiple active conformationsof CCR5 and indicate that CCR5 oligomers are involved in an internalizationprocess that is distinct from that induced by the receptor'sagonists.

	INTRODUCTION

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION CONCLUSION REFERENCES

Chemokines constitute a large family of proteins that regulate leukocyte recruitment to sites of inflammation and coordinatetheir trafficking throughout the body. They mediate these functionsthrough the binding and activation of seven transmembrane domainG protein-coupled receptors (GPCRs) specifically expressed byvarious populations of leukocytes (Baggiolini, 1998; Murphy etal., 2000). CC-chemokine receptor 5 (CCR5) is a functional receptorfor the inflammatory CC-chemokines macrophage inflammatory polypeptide(MIP)-1 $alpha$ , MIP-1 $beta$ , regulated on activation normal T cell expressedand secreted (RANTES), monocyte chemotactic protein (MCP)-2, andMCP-4 (Samson et al., 1996a; Murphy et al., 2000). It is expressedon memory T lymphocytes, macrophages, dendritic cells, thymocytes,hematopoietic progenitors, and other cell populations (Murphyet al., 2000). CCR5 is thought to be involved in the recruitmentof leukocytes in a growing number of inflammatory diseases, suchas rheumatoid arthritis, multiple sclerosis, and asthma, and itplays a major role in acquired immunodeficiency syndrome pathogenesis(Berger et al., 1999; Gerard and Rollins, 2001). Cellular entryof human immunodeficiency virus (HIV) is initiated by the interactionbetween the gp120 subunit of the viral Env glycoprotein, CD4,and a coreceptor that belongs to the chemokine receptor family.CCR5 is the principal coreceptor for macrophage tropic (M-tropicor R5) HIV strains, which are responsible for viral transmissionand predominate during the asymptomatic phase of the disease.The essential role of CCR5 in HIV pathogenesis was demonstratedby the strong resistance toward HIV infection of individuals homozygousfor a nonfunctional allele (CCR5 $Delta$ 32) of the coreceptor gene (Liuet al., 1996; Samson et al., 1996b). These individuals have noobvious pathological phenotype, making CCR5 an attractive candidatefor therapeutic intervention. Agents proposed as potential viralentry blockers include chemokines or chemokine analogs, monoclonalantibodies (mAbs), and chemical antagonists (Moore and Stevenson,2000). The first described inhibitors of CCR5 coreceptor functionwere its natural ligands MIP-1 $alpha$ , MIP-1 $beta$ , and RANTES (Cocchi etal., 1995). Synthetic derivatives of natural chemokines, suchas amino-oxypentane (AOP)-RANTES were later shown to display enhancedHIV suppressive activities (Simmons et al., 1997). Two complementarymechanisms have been proposed to account for the ability of chemokinesto inhibit HIV infection. First, chemokines compete for gp120binding (Trkola et al., 1996). Second, agonists induce CCR5 internalization,resulting in a prolonged reduction of the coreceptor number atthe cell surface (Alkhatib et al., 1997; Amara et al., 1997; Macket al., 1998), a parameter found to be critical for HIV infection(Wu et al., 1997a). The relative contribution of these two mechanismsremains to be clarified in each case. The pronounced antiviralactivity of AOP-RANTES has been attributed to the efficient inductionof endocytosis and the inability of CCR5 to reaccumulate on thecell surface after removal of the ligand (Mack et al., 1998; Signoretet al., 2000). It has also been suggested that CCR5 endocytosisinduced by antibodies may account for HIV resistance of exposed-uninfectedindividuals (Lopalco et al., 2000).

Monoclonal antibodies blocking chemokine and gp120 binding to CCR5 have been described (Wu et al., 1997b; Hill et al., 1998;Lee et al., 1999; Olson et al., 1999), as well as a first setof chemical CCR5 antagonists (Baba et al., 1999) that are presentlyregarded as candidate therapeutic inhibitors of viral entry. However,from a theoretical point of view, compounds able to inhibit gp120binding and promote efficient and prolonged internalization ofCCR5, without triggering the intracellular signaling cascades,would constitute ideal antiviral agents. Monoclonal antibodiesinteracting with various epitopes of a receptor constitute interestingtools to study the relationship between stabilization of an "active"receptor conformation and the various consequences of this activation(G protein coupling, internalization). Moreover, the availabilityof dimeric or monomeric isoforms of the same monoclonal allowsfor determination of the contribution of receptor dimerizationin the studiedprocesses.

In this study, we have characterized a novel set of anti-CCR5 mAbs and have determined their functional properties. Theirepitopes were characterized by using a large panel of chimericand mutant receptors. We correlated these findings with the abilityof the mAbs to inhibit chemokine and/or gp120 binding, to modulateactivation of intracellular cascades, and to influence receptortrafficking.

	MATERIALS AND METHODS

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION CONCLUSION REFERENCES

Generation of Monoclonal Antibodies against CCR5

BALB/c mice were immunized at 4-wk intervals by at least six intraperitoneal injections of Chinese hamster ovary (CHO) cellsstably transfected with CCR5. Four days after the last injection,the spleens were removed and the splenocytes fused with P3X63-Ag8plasmocytoma cells. Culture supernatants were screened by flowcytometry on CHO cells expressing CCR5, or CXCR4 as control. Inaddition to MC-1 (Mack et al., 1998) and MC-5 (Mack et al., 2000),three monoclonal antibodies (MC-4, MC-6, and MC-7) were obtainedthat specifically recognize CCR5 and do not cross-react with CHOcells overexpressing CCR1-4 or CXCR4. None of the mAbs stainedCCR5-deficient (CCR5 $Delta$ 32/ $Delta$ 32) peripheral blood mononuclear cells.Apart from the clone MC-5 (IgG-2a), all other clones were of IgG-1isotype.

Generation of Monovalent mAb Isoforms

A plasmid encoding an MC-1 single-chain fragment (ScFv-MC-1) was performed by reverse transcription on total RNA extractedfrom the $alpha$ CCR5 hybridoma MC-1 with random hexamers and the SuperScriptreverse transcriptase (Invitrogen, Paisley, United Kingdom). Thelight and heavy variable domains were cloned by polymerase chainreaction amplification with Pfu polymerase (Orlandi et al., 1989).As described previously, the two domains were joined by a linkercoding for (Gly₄Ser₁)₃ and a C-terminal tail encoding six histidineswas attached to facilitate purification. The single-chain fragmentwas expressed in the periplasmic space of Escherichia coli andpurified by Ni-NTA (QIAGEN S.A., Courtaboeuf, France) as described(Mack et al., 1995).

The F(ab) fragments were obtained by digesting MC-1, MC-4, and MC-6 mAbs (2 mg/ml each), respectively, for 2 h with 0.02 mg/ml,for 4 h with 0.02 mg/ml, and for 2 h with 0.1 mg/ml papain (Sigma,St. Louis, MO) in phosphate-buffered saline (PBS) containing 20mM EDTA and 20 mM cysteine (Sigma). After stopping the reactionwith 30 mM iodocetamide, the antibodies were dialyzed overnightagainst PBS. Fc fragments and undigested mAbs were removed withProtein A-Sepharose CL-4B (Pharmacia, Freiburg, Germany). Aliquotsof each digestion were checked by SDS-PAGE and Coomassie bluestaining. By using fluorescein isothiocyanate (FITC)-labeled secondaryantibodies specific for F(ab) fragments (Jackson Immunoresearch,West Grove, PA), similar mean channel fluorescence values wereobtained with F(ab) fragments and half-equimolar amounts of theparental monoclonal antibodies, indicating that the binding propertieswere not affected by the digestionprocedure.

CCR5 Constructs

All CCR5 constructs used in this study have been previously described (Lee et al., 1999; Samson et al., 1997; Blanpain etal., 1999a, 2000, 2001). The constructs were sequenced and subclonedinto the bicistronic expression vector pEFIN3 for the generationof stable cell lines as previously described (Samson et al., 1997).

Cell Culture and Expression of Mutant Receptors in CHO-K1 Cells

CHO-K1 cells stably expressing apoaequorin, G $alpha$ ₁₆ and wild-type or mutant CCR5 receptor (Blanpain et al., 1999b) were culturedin Ham's F-12 medium supplemented with 10% fetal calf serum (Invitrogen),100 U/ml penicillin, 100 µg/ml streptomycin (Invitrogen), 250µg/ml Zeocin (Invitrogen), and 400 µg/ml G418(Invitrogen).

Fluorescence-activated Cell Sorting (FACS) Analysis

Binding affinities of the different mAbs for CCR5 were determined by flow cytometry. CCR5-expressing CHO-K1 cells were incubatedwith mAbs for 30 min on ice, washed, stained with different anti-mouseIgG secondary antibodies conjugated with phycoerythrin (Sigma),FITC (Sigma), or Texas Red (Jackson Immunoresearch), and analyzedon a FACScan (BD Biosciences, Aalst, Belgium). The binding parameterswere determined by nonlinear regression using the PRISM software(GraphPad Software, San Diego,CA)

Epitopes were mapped by flow cytometry with a panel of ~70 CHO-K1 cell lines stably expressing chimeric and point mutant receptors(Samson et al., 1997; Lee et al., 1999; Blanpain et al., 1999a,2000). Cells were incubated for 30 min on ice with saturatingconcentrations of anti-CCR5 mAbs, washed, and stained with polyethylene(PE)-conjugated anti-mouse Ig antibody (Sigma). CHO-K1 cells expressingCCR2b were used as negativecontrol.

For endocytosis experiments, 5 × 10⁵ CHO cells expressing wtCCR5 were incubated for 30 min at 37°C with chemokines or mAbs.Cells were then placed on ice, incubated with 15 µg of MC-1 orMC-4 or their respective F(ab) fragments for 1 h, washed withcold PBS, and stained with FITC-conjugated anti-mouse Ig antibody(F313; DAKO, Hamburg, Germany). Cells were washed and analyzedon a FACSCalibur (BD Biosciences). For experiments with ScFv-MC-1,cells were incubated for 45 min with 3 µg/ml ScFv-MC-1, on iceor 37°C as indicated. Cells were washed twice with cold PBS andincubated with 4 µg/ml anti-His antibody (Dianova, Hamburg, Germany)for 45 min, on ice or at 37°C as indicated. Cells were washedagain with cold PBS and stained with PE-labeled rabbit antimouseF(ab)₂ (DAKO), and analyzed on a FACSCalibur with CellQuest software(BDBiosciences).

For inhibition of chemokine-induced CCR5 endocytosis by mAbs, CHO cells expressing CCR5 were incubated on ice with mediumor MC-4 or MC-4 F(ab) for 30 min. Cells were then incubated withRANTES or AOP-RANTES for 30 min at 37°C. The cells were washed,incubated with 15 µg/ml MC-4 or MC-4 F(ab) followed by FITC-conjugatedanti-mouse F(ab) Ig antibody(DAKO).

Binding Assays

Competition binding assays were performed with CCR5 expressing CHO-K1 cells as described (Blanpain et al., 1999a), by using0.08 nM ¹²⁵I-MIP-1 $beta$ or ¹²⁵I-RANTES (2000 Ci/mmol; Amersham plc, Little Chalfont, Buckinghamshire,United Kingdom) as tracer, variable concentrations of mAbs, and40,000 cells. Total binding was measured in the absence of competitorand nonspecific binding was measured in the presence of a 100-foldexcess of unlabeled chemokine. Soluble JRFL gp120 was iodinatedas described (Lee et al., 1999). Env binding assays were performedon CCR5-expressing CHO-K1 cells with ¹²⁵I-JRFL gp120 as tracer, in the presence of 100 nM sCD4 and competitors.Total binding was measured in the absence of competitor and nonspecificbinding was measured in the presence of a 100-fold excess of unlabeledgp120.

Aequorin-based Functional Assay

The functional response to chemokines and monoclonals was analyzed with an aequorin-based assay as described (Blanpain etal., 1999b). Inhibition of chemokine signaling by anti-CCR5 mAbswas analyzed with the same assay. mAbs were incubated for 30 minat room temperature with 50,000 CHO-K1 cells expressing CCR5 thenRANTES or MIP-1 $beta$ (1 nM final concentration) was added to the cellsuspension, and the luminescence was recorded for 30 s in a luminometer.Stimulation (100%) was defined as the response to 1 nM chemokinein the absence of mAbs, and 0% as the luminescence in the absenceof ligand. A chemokine dose-response curve was used as positivecontrol in eachexperiment.

Guanosine-5'-O-(3-thio)triphosphate (GTP $gamma$ S) Binding Assay

Membranes of CHO-K1 cells expressing 20 µg/ml CCR5, prepared from cells treated or not with 100 ng/ml pertussis toxin for18 h, were incubated in 20 mM HEPES pH 7.4, 100 mM NaCl, 3 mMMgCl₂, 3 µM GDP, and 10 µg/ml saponin, with different concentrationsof RANTES or mAbs, in 96-well microplates (Basic FlashPlates;PerkinElmer Life Sciences, Boston, MA), for 15 min at room temperature.After addition of 0.1 nM [³⁵S]GTP $gamma$ S (Amersham plc), the microplates were shaken for 1 minand incubated further for 30 min at 30°C. The incubation was stoppedby centrifugation of the plates for 10 min at 800 × g and 4°C,and aspiration of the supernatant. Microplates were counted ina TopCount (Packard Instrument, Meriden, CT) for 1 min/well. NeitherRANTES nor mAbs effected [³⁵S]GTP $gamma$ S binding to membranes of CHO-K1 cells expressing otherrelated (CCR8) or unrelated (CRF₂) GPCRs. Functional parameterswere determined with the PRISM software (GraphPad Software) byusing nonlinear regression applied to a sigmoidal dose-responsemodel.

Inhibition of cAMP Accumulation

Inhibition of cAMP accumulation by chemokines and monoclonals was performed on CCR5-expressing cells spread on Petri dishes(25,000 cells/well) containing cultured overnight. Cells werepreincubated for 15 min in Krebs-Ringer-HEPES buffer and 1 mM3-isobutyl-1-methylxanthine (Calbiochem, San Diego, CA), and thenincubated for 20 min in the same medium supplemented with 5 µMforskolin and variable concentrations of RANTES or 10 µg/ml mAbs.The cAMP content was measured by enzyme-linked immunosorbent assay(cAMP-screen, CS100; Tropix, Bedford, MA) according to the procedurespecified by themanufacturer.

In Vivo Cellular Assays for Receptor Trafficking and Oligomerization

For confocal microscopy in living cells, clonal cell lines expressing CCR5-green fluorescent protein (GFP) were seeded on22-mm round glass coverslips, and grown for 18 h. Coverslips wererinsed in DMEM/F-12 and placed in the observation chamber (maintainedat 37°C) of an MRC 1024 confocal microscope (Bio-Rad, Hercules,CA) fitted on an Axiovert 100 inverted microscope (Zeiss, WelwynGarden City, United Kingdom) equipped with a Plan-Neofluar 40×/1.3oil immersion objective (Zeiss). The 488-nm excitation beam ofan Argon-Krypton laser and a 522-532-nm band-pass emission filterwere used for viewing enhanced green fluorescent protein (EGFP).The 568-nm excitation beam and a 605-632-nm band-pass emissionfilter were used for viewing transferrin AlexaFluor 564. The beampower was kept below 10% of maximal power to reduce photobleachingand phototoxicity. Pinhole was set to generate 1-µm-thick opticalsections. Fields of interest (512 × 512 pixels) were selectedvisually. Data were sequentially collected for each fluorochrome(approximate collection time 4 s), every 3 min for the indicatedtime. Cells expressing CCR5-GFP were incubated with 50 µg/ml AlexaFluor-Transferrin(Molecular Probes, Eugene, OR) alone or together with ligandsfor 15-45 min, and washed three times beforeviewing.

For induction of CCR5-GFP endocytosis, 10 µg/ml mAbs or 100 nM RANTES were added to the cells, and images were acquired every3 min for 45 min. For ScFv-MC-1 experiments, cells were firstincubated for 45 min with ScFv-MC-1, washed three times, incubatedwith anti-His (4 µg/ml) for 30 min, and images were collectedevery 3 min. No endocytosis was seen with control IgG or anti-Hisantibody. For inhibition of CCR5-GFP endocytosis, the cells werefirst incubated with 10 µg/ml mAbs for 45 min then with 100 nMRANTES, and frames were acquired every 3 min for 45min.

For determining the endocytic pathways, CCR5-GFP-expressing cells were incubated with 100 ng/ml pertussis toxin (Sigma) for18 h, 0.45 M sucrose for 1 h, 2.5 µg/ml filipin III (Sigma) for45 min, or 10 mM $beta$ -methyl-cyclodextrine (Sigma) for 45 min at37°C, and then tested for endocytosis in DMEM/F-12 containingtheinhibitor.

Arrestin translocation assays were performed by transfecting 100 ng of $beta$ -arrestin 2-EGFP (gift of Mark Scott, ICGM, Paris,France) into CCR5-expressing cells. The day after, cells wereanalyzed by confocal microscopy as described above after additionof RANTES ormAbs.

The bioluminescence resonance energy transfer (BRET) assay was performed as described by Angers et al. (2000). Briefly, humanizedRenilla luciferase (Packard Instrument) and the yellow variantof GFP (CLONTECH) were fused to the last C-terminal residue ofCCR5 and expressed in human embryonic kidney 293 cells. Fusionproteins were expressed at the plasma membrane and were internalizedupon agonist stimulation (as determined by FACS analysis). Instable clones expressing either wild-type CCR5 or the fusion proteinsRANTES and MIP-1 $beta$ resulted in the inhibition of forskolin-inducedcAMP production. Antibody-promoted changes of BRET ratio werecalculated by subtracting the basal BRET ratio, measured in theabsence of antibodies, from the BRET ratios observed in the presenceof the indicated antibodies. The details of the application ofthe BRET assay to CCR5 will be described elsewhere (Issafras,Bouvier, and Nerullo, unpublisheddata).

	RESULTS

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION CONCLUSION REFERENCES

Generation and Epitope Mapping of Anti-CCR5 mAbs

Mice were immunized with CHO cells expressing human CCR5. Five CCR5-specific mAbs (MC-1, MC-4, MC-5, MC-6, and MC-7) wereisolated and further characterized. Saturation binding experimentswere conducted using flow cytometry. All mAbs bound CCR5 withhigh affinity, with K_d values of 0.54 ± 0.25 (MC-1), 0.61 ± 0.24(MC-4), 0.35 ± 0.21 (MC-5), and 1.18 ± 0.28 µg/ml (MC-6; our unpublisheddata). All mAbs stained CCR5 on monocytic and lymphocytic populationsof freshly isolated human peripheral blood mononuclear cells,similarly to the reference antibody 2D7 (our unpublisheddata).

The contribution of extracellular domains of CCR5 to the epitopes was determined by testing a set of CHO-K1 cell lines stablyexpressing CCR5-CCR2b chimeras in FACS analysis. Two previouslymapped mAbs (3A9 and 2D7) were used as controls (Wu et al., 1997b).As shown in Table 1 and Figure 1, MC-4, MC-5, MC-7, and 3A9 recognizeepitopes located within the amino-terminal domain of CCR5. MC-1and 2D7 are specific for the second extracellular loop (ECL2)of CCR5 (Figure 1). MC-6 requires multiple CCR5 domains for recognition,including ECL1, ECL2, and the amino-terminal domain (Figure 1).

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Table 1. Epitope mapping of anti-CCR5 mAbs

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Figure 1. Immunostaining of CCR5-CCR2b chimeras and CCR5 point mutants with anti-CCR5 mAbs. CCR5-CCR2b chimeras are coded according to the origin of the N-terminal domain (first digit), and of the three extracellular loops (last three digits): 5555 and 2222 represent CCR5 and CCR2b, respectively; 2555 represents a chimeric receptor containing the amino-terminal domain of CCR2b and the three extracellular loops of CCR5. CCR5 point mutants are designated by the nature of their amino acid substitution. CHO-K1 cells stably expressing these constructs were stained with saturating concentrations of the different anti-CCR5 mAbs and phycoerythrin-conjugated anti-mouse IgG, and analyzed by FACS. Fluorescence histograms are shown together with the background fluorescence obtained for cells expressing CCR2b.

Specific residues involved in the epitopes of MC-4, MC-5, and MC-7 were determined with amino-terminal truncations and alaninesubstitution mutants of CCR5 (Table 1). The first three residuesof CCR5 are essential for the MC-5 epitope and MC-5 was the onlymAb able to recognize CCR5 in Western blotting, suggesting thatits epitope is linear (Oppermann et al., 1999; Mack et al., 2000).Alanine scanning mutants demonstrated that the MC-7 epitope includesS7-P8 and Y10-D11 (Table 1). The MC-4 epitope was mapped moredistally in the CCR5 amino terminus (residues 14-17 and E18).MC-1 and MC-6, like 2D7, were not affected by mutations in CCR5N terminus (Table 1).

Chimeras and point mutants involving ECL2 were used to specify the epitopes of MC-1 and MC-6 (Table 1). MC-1 and 2D7 recognizedthe first part of ECL2. MC-6 binding was affected by replacementof both the first and the second halves of ECL2, and by the pointsubstitutions K171A and E172A (but not R168A) in the first partof ECL2 (Figure 1 and Table 1). Other point mutations known toaffect the conformation of the extracellular domains of CCR5,such as C178R (that disrupts the disulfide bond linking ECL1 andECL2; Blanpain et al., 1999b, 2000), reduced or prevented bindingof MC-1, MC-6, and 2D7, but had little effects on other mAbs.The other point mutants tested had no effects on mAbrecognition.

MC-6 Binding to CCR5 Promotes G protein Activation but not Calcium Mobilization

Using CCR5-expressing CHO cells, we examined the ability of the different mAbs (at the concentration of 10 µg/ml) to promote[³⁵S]GTP $gamma$ S binding to membranes. RANTES promoted a marked and dose-dependentincrease in [³⁵S]GTP $gamma$ S binding, with an EC₅₀ value of 2.3 nM (Figure 2A). Amongthe mAbs tested, only MC-6, but not its F(ab) fragment, induceda significant increase in GTP $gamma$ S binding to membranes of CCR5-expressingcells (Figure 2B; our unpublished data). This effect was blockedby pertussis toxin pretreatment (our unpublished data). Noteworthy,MC-1 had no effect in this assay, although it promoted receptorinternalization, as shown below. Neither RANTES nor MC-1 nor anyother mAb increased GTP $gamma$ S binding to membranes of cells expressingother receptors (our unpublished data). MC-6, but not its F(ab)fragment, was also able to inhibit cAMP accumulation in CCR5-expressingCHO-K1 cells with an efficacy similar to that found in the GTP $gamma$ Sassay (Figure 2C).

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Figure 2. CCR5 activation by the multidomain mAb MC-6. Effect of different concentrations of RANTES (A) and anti-CCR5 mAbs at 10 µg/ml (B) on the binding of [³⁵S]GTP $gamma$ S to membranes of CHO-K1 cells expressing human CCR5. Data are presented as raw cpm values (A) or normalized (B) to basal (0%) and maximal [³⁵S]GTP $gamma$ S binding in response to RANTES (100%). These experiments were repeated four times with similar results. All data points were analyzed in triplicates (error bars: SEM). (C) Inhibition of forskolin-stimulated cAMP accumulation. CHO-K1 cells expressing CCR5 were incubated for 20 min with 5 µM forskolin and RANTES or the various mAbs, and cAMP was measured by enzyme-linked immunosorbent assay. The results were normalized for basal (0%, in the presence of forskolin only) and maximal response (100%, cAMP levels obtained with a saturating concentration of RANTES). The experiments were performed in triplicate (error bars: SEM), and the figure represents a typical experiment out of two performed independently.

We also investigated whether the mAbs could induce intracellular calcium release by using an aequorin-based assay. None ofthe mAbs, including MC-6, were able to promote calcium signalingin CCR5-expressing cells, whereas RANTES induced a robust responsecharacterized by an EC₅₀ value of 2.5 nM (our unpublisheddata).

mAbs Differently Antagonize the Function of RANTES, MIP-1 $beta$ , and gp120 onto CCR5

We next investigated the ability of the mAbs to compete for ¹²⁵I-MIP-1 $beta$ or ¹²⁵I-RANTES binding to CCR5. As shown in Figure 3A, MC-1 and MC-6inhibited both MIP-1 $beta$ and RANTES binding with an IC₅₀ value <1µg/ml. MC-4 and control IgG did not compete for chemokine binding.MC-5 competed partially for MIP-1 $beta$ binding but competed very poorlyfor RANTES binding up to concentrations of 10 µg/ml. We furthertested whether these mAbs prevent CCR5 activation by chemokines.In agreement with the binding data, MC-1, MC-5, and MC-6 inhibitedcalcium mobilization induced by 1 nM MIP-1 $beta$ , in a concentration-dependentmanner (Figure 3B). MC-1 and MC-6, but not MC-5, inhibited calciumsignaling in response to 1 nM RANTES. MC-4 and control IgG hadno effect.

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Figure 3. Inhibition of MIP-1 $beta$ , RANTES, and HIV Env binding and receptor activation. (A) Different concentrations of anti-CCR5 mAbs ( $black-square$ , 0 µg/ml;

, 0.1 µg/ml;

, 1 µg/ml;

, 10 µg/ml) were tested for their ability to compete with binding of ¹²⁵I-MIP-1 $beta$ or ¹²⁵I-RANTES to CHO cells expressing CCR5. Results were normalized for nonspecific binding (0%) and specific binding in the absence of competitor (100%). (B) mAb-mediated inhibition of functional responses to MIP-1 $beta$ and RANTES in cell lines coexpressing CCR5 and apoaequorin. Cells were preincubated for 30 min with mAbs then MIP-1 $beta$ or 1 nM RANTES was added, and luminescence was recorded for 30 s. Results were normalized for the chemokine response in the absence of antibodies (100%) and the basal luminescence of the cells (0%). (C) Influence of mAbs on the binding of ¹²⁵I-gp120 derived from the macrophage-tropic HIV-1 strain JRFL to CCR5-expressing CHO-K1 cells, in the presence of 100nM sCD4. Results were normalized for nonspecific binding (0%) and specific binding in the absence of competitor (100%). All experiments were repeated at least twice with similar results. All points were performed in triplicates (error bars: SEM).

We and others have shown that chemokines and HIV Env bind overlapping but distinct CCR5 domains (Rucker et al., 1996; Wu etal., 1997b; Farzan et al., 1998; Blanpain et al., 1999a). We thereforetested the ability of our mAbs to compete for the binding of ¹²⁵I-JRFL-gp120 to CCR5. MC-1, MC-5, MC-6, and the reference mAb2D7 efficiently inhibited JRFL-gp120 binding in the presence ofsoluble CD4 (Figure 3C). Neither control isotype IgG nor MC-4inhibited Env binding up to concentrations of 10 µg/ml.

Bivalent, but not Monovalent MC-1, Promotes CCR5 Endocytosis

The ability of our mAbs to induce CCR5 internalization in CHO-K1 cells was investigated. As shown in Figure 4A, MC-1 induceda dose-dependent down-modulation of the cell surface receptor.As measured by FACS analysis, 5 µg/ml MC-1 induced a 50% decreaseof cell surface CCR5, similar to the level of down-modulationobtained with 100 nM RANTES (Figure 4, A and B). No significantendocytosis was seen when cells were incubated on ice with MC-1(our unpublished data). Incubation of cells at 37°C with MC-4or MC-5 had no effect (Figure 4A; our unpublished data). Inductionof internalization by MC-1 was also found in lymphocyte and monocytepopulations expressing CCR5 naturally. Given the lower expressionlevel of the receptor in these cells, the phenomenon was howeverless demonstrative than in CHO cells (our unpublished data).

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Figure 4. MC-1 mAb induces CCR5 endocytosis in CHO cells. CHO cells expressing CCR5 were incubated with MC-1 ( $black-square$ ]), MC-4 (

) (A), or RANTES ( $black-square$ ) (B) for 30 min at 37°C. Cell surface CCR5 was detected by flow cytometry with a saturating concentration of the same mAbs or MC-4 for RANTES-induced CCR5 down-modulation. Results were normalized for the fluorescence of unstimulated cells (100%) and for the background fluorescence (0%). All experiments were repeated at least twice with similar results.

Because MC-1 promoted CCR5 endocytosis without triggering detectable signaling, we investigated whether MC-1 or RANTES couldinduce different routes of receptor endocytosis. CHO-K1 cellsexpressing high levels of a CCR5-GFP chimeric protein were generated.This chimeric receptor was activated by chemokines with a concentration-responsecurve similar to wtCCR5 (our unpublished data). In the absenceof ligands, cells expressing CCR5-GFP showed intense fluorescenceat the cell surface, although a significant proportion of thefusion protein was localized intracellularly (Figure 5A). Thisfraction of labeling likely corresponds partly to biosyntheticcompartments, such as endoplasmic reticulum and Golgi complex,but also to endosomal compartments. Indeed, the early endosomemarker AlexaFluor 594-Transferrin colocalized with intracellularCCR5-GFP, even in the absence of ligands (Figure 5A), and recycledefficiently from this endosomal compartment to the cell surface(our unpublished data). Addition of 100 nM RANTES to these cellsinduced a profound subcellular redistribution of the fluorescence(Figure 5, B-E, and Video 1). Shortly after agonist addition,a local enhancement of membrane-associated fluorescence was observed,possibly resulting from receptor clustering. Ruffling of membraneswas also apparent as a consequence of receptor signaling and cytoskeletalrearrangements. After 10-15 min, CCR5-GFP was internalized intoendocytic vesicles that progressively fused with larger endosomalcompartments. In contrast to endocytosis mediated by RANTES, thesubcellular redistribution of CCR5-GFP induced by MC-1 occurredin a very different manner in terms of morphology and time course(Figure 5, F-J, and Video 2). Immediately after 10 µg/ml MC-1addition, enhancement of cell surface fluorescence was observed,but soon thereafter, a large number of small intracellular vesicleswas formed, which did not fuse further with endosomes (Figure5G). MC-5, MC-6, and isotype control IgG were unable to induceCCR5-GFP endocytosis (our unpublished data).

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Figure 5. Down-modulation of cell surface CCR5-GFP by RANTES and MC-1. (A) CHO-K1 cells expressing CCR5-GFP (green) were incubated with AlexaFluor-Transferrin (red) for 30 min, washed twice with media, and analyzed by confocal microscopy for colocalization (yellow). Dynamics of CCR5-GFP was measured after stimulation of the cells by RANTES or MC-1 mAb. The cells were exposed to 100 nM RANTES or 10 µg/ml MC-1 in DMEM/F-12 medium at 37°C, under confocal microscopy. Images were acquired every 3 min for 45 min. CCR5-GFP distribution is shown 0, 15, 30 and 45 min after addition of RANTES (B-E) or MC-1 (F-I). This session is representative of at least five similar experiments. Bar, 5 µm. Videos of the experiments described in this figure are available in the online version of this article.

To investigate further in vivo the involvement of oligomers in the endocytosis process mediated by MC-1, we took advantageof a new biophysical assay based on BRET, which allows to monitorthe interaction between two fusion proteins (Angers et al., 2000).Addition of 10 µg/ml MC-1 produced a robust increase of the BRETsignal (Figure 6A) in 293T cells coexpressing CCR5-luc and CCR5-YFP,with kinetics similar to that found for CCR5-GFP endocytosis (ourunpublished data). Neither MC-4, MC-5, MC-6 (Figure 6A), nor controlIgG (our unpublished data) induced changes in the BRET signal.These results indicate that MC-1 induces a profound change inthe physical proximity between two or more CCR5 molecules.

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Figure 6. Receptor oligomerization are involved in MC-1-induced CCR5 endocytosis. (A) 293T cells expressing CCR5-luc and CCR5-YFP were incubated with coelenterazine, and the luminescence and the fluorescence signals were quantified before and after the addition of the indicated mAb. The BRET ratio was defined as [(emission at 485 nm ± 20)/(emission at 530 nm ± 25)] $-$ [(emission at 485 nm ± 20)/(emission at 530 nm ± 25)] for CCR5-luc expressed alone in the same experiments. Variation in BRET signal compared with baseline (addition of buffer alone) after 10 min of incubation with antibodies is displayed. All experiments were repeated at least twice with similar results. All points were performed in triplicates (error bars: SEM). (B) CHO cells expressing CCR5 were incubated with 3 µg/ml ScFv-MC-1 for 45 min at 4 or 37°C, washed twice with cold PBS, and incubated with anti-His at 4 or 37°C as indicated. Surface expression of CCR5 was measured by flow cytometry with PE-labeled anti-mouse antibody. Fluorescence was normalized for cells incubated with ScFv MC-1 and anti-His both at 4°C (100%), and for background fluorescence (0%). (C-H) Confocal microscopy. Cells expressing CCR5-GFP were incubated with 10 µg/ml ScFv-MC-1 at 37°C and are shown before (C) and 45 min after the incubation (D). Cells were then washed three times with buffer (E) and incubated with an anti-polyhistidine antibody (anti-His, 4 µg/ml) for 45 min (F). Videos of the experiment described in this figure are available in the online version of this article. Anti-His antibody alone did not result in CCR5-GFP endocytosis after 45 min of observation (G and H). All experiments were at least repeated twice with similar results.

We also investigated the functional properties of monovalent versions of MC-1 by flow cytometry and confocal microscopy. Botha single chain fragment of MC-1 (ScFv-MC-1) tagged with poly-histidineand a purified F(ab) fragment of MC-1 continued to bind CCR5 withhigh affinity (our unpublished data). CCR5 internalization promotedby ScFv-MC-1 was quantified by FACS analysis. CCR5 surface expressionof cells incubated on ice with both ScFv-MC-1 and anti-His mAbwas used as control (100% fluorescence). As shown in Figure 6B,the incubation of cells with ScFv-MC-1 at 37°C followed by anti-Hison ice did not significantly reduce surface expression of CCR5,indicating that monovalent MC-1 could not induce CCR5 down-modulation.However, when scFv-MC-1 and anti-His mAb were both incubated at37°C, CCR5 surface fluorescence decreased by 50%, indicating thatcross-linking of scFv-MC-1 can restore the effect of the parentaldivalent antibody. Confocal microscopy was used to visualize theendocytosis of CCR5 with various combinations of the monovalentScFv-MC-1 and cross-linking secondary antibodies. Neither monovalentScFv-MC-1 nor MC-1 F(ab) was able to induce significant internalizationof CCR5-GFP (Figure 6, C and D; our unpublished data). We theninduced cross-linkage of the ScFv-MC-1 with anti-His mAb, aftera 45-min preincubation with 10 µg/ml ScFv-MC-1 alone. This partiallyrestored the effect on CCR5 endocytosis (Figure 6, E and F, andVideo 3), whereas anti-His alone had no effect (Figure 6, G andH). In addition, the two monovalent isoforms of MC-1, MC-1 F(ab)and MC-1 ScFv, did not induce significant changes in the BRETsignal (Figure 6A). Taken together, these results demonstratethat the bridging property of divalent antibodies is necessaryfor inducing CCR5internalization.

MC-1 Induces CCR5 Endocytosis via a Clathrin-independent but Caveolae-dependent Pathway

To investigate the mechanisms implicated in the endocytosis induced by MC-1, we treated cells with drugs blocking differentpathways of GPCR internalization. As shown in Figure 7, A andB, pertussis toxin did not prevent endocytosis induced by MC-1,whereas it inhibited strongly the endocytosis mediated by RANTES(Figure 7, C and D). Hypertonic sucrose severely decreased RANTES-inducedinternalization (Figure 7, E and F), whereas this treatment hadno effect on the ability of MC-1 to promote CCR5 endocytosis (Figure7, G and H). Two cholesterol-depleting agents, $beta$ -methyl-cyclodextrineand filipin, inhibited almost completely the endocytosis mediatedby both RANTES and MC-1 (Figure 7, I-L; our unpublished data).We also used a living cells assay to study the recruitment dependenceof the $beta$ -arrestin after RANTES or MC-1 binding to CCR5. RANTESinduced, within a minute, a robust translocation of $beta$ -arrestin-GFPfrom the cytosol to the plasma membrane in CCR5-expressing cells(Figure 7, M and N, and Video 4). In contrast, no subcellularredistribution of $beta$ -arrestin-GFP was seen after the addition ofMC-1 (Figure 7, O and P, and Video 5). These results demonstratethat MC-1 promotes CCR5 endocytosis via an arrestin- and clathrin-independentpathway, but that this pathway is highly dependent on the integrityof cholesterol-rich microdomains.

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Figure 7. MC-1 induces CCR5 endocytosis by an arrestin and clathrin-independent, caveolae-dependent pathway. (A-L). CHO-K1 cells expressing CCR5-GFP were incubated for 18 h with 100 ng/ml pertussis toxin 100 (A-D) or for 1 h with 0.45 M sucrose (E-H), or or 2.5 µg/ml filipin (I-L) for 1 h at 37°C. Cells were then stimulated with 100 nM RANTES (A, B, E, F, I, and J) or 10 µg/ml MC-1 (C, D, G, H, K, and L), and the dynamics of CCR5-GFP was recorded by confocal microscopy. Responses are shown before (A, C, E, G, I, and K) and 30 min after (B, D, F, H, J, and L) ligand addition. (M-P). CHO-K1 cells stably expressing CCR5 were transfected with $beta$ -arrestin-GFP; 24 h after transfection, subcellular redistribution of $beta$ -arrestin-GFP was analyzed by confocal microscopy. The cells were exposed to 100 nM RANTES (M and N) or 10 µg/ml MC-1 (O and P). Images were acquired every 15 s for 10 min. Responses are shown before (M and O), and 2 min (N) or 10 min (P) after ligand addition. Videos of the dynamics of $beta$ -arrestin-GFP trafficking in response to RANTES stimulation, as described in this figure, are available in the online version of this article. All experiments were repeated at least twice with similar results. Bar, 20 µm.

MC-4 Inhibits CCR5 Endocytosis

We also investigated whether mAbs could inhibit CCR5 internalization mediated by chemokines. Cells were preincubated withmAbs then with chemokines at 37°C, and surface expression of CCR5was measured by flow cytometry. MC-4 inhibited RANTES-inducedCCR5 endocytosis by >75% (Figure 8A). As described, AOP-RANTESwas more potent than RANTES in mediating CCR5 internalization(Figure 8B). In the presence of 10 µg/ml MC-4, a 10-fold higherconcentration of AOP-RANTES was required to induce 50% receptordown-modulation (Figure 8B). MC-4 F(ab) also inhibited CCR5 endocytosisalthough less efficiently than bivalent antibodies (Figure 8,A and B). Real-time confocal microscopy was used to study theeffect of MC-4 on the dynamics of CCR5-GFP trafficking. As describedabove, MC-4 alone had no effect on receptor localization (Figure8, C and D). When cells were stimulated with 100 nM RANTES inthe presence of MC-4, enhancement of membrane fluorescence andruffling were observed (Figure 8, E-G, and Video 6), as in theabsence of MC-4. However, no subsequent internalization occurred,and membrane ruffling could be observed during the 45-min observationperiod (Figure 8G). Isotype control IgG had no effect on CCR5-GFPlocalization (Figure 8, H and I) or RANTES-induced internalization(Figure 8J).

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Figure 8. MC-4 inhibits CCR5 endocytosis mediated by chemokines. (A and B) CHO-K1 cells expressing CCR5 were preincubated with medium ( $black-square$ ), 10 µg/ml MC-4 (

), or MC-4 F(ab) ( $triangle$ ) for 30 min on ice and then incubated with RANTES (A) or AOP-RANTES (B) for 30 min at 37°C. Surface expression of CCR5 was measured by flow cytometry with the antibody MC-4 or MC-4 F(ab) (15 µg/ml, on ice) and FITC-conjugated secondary antibodies. Fluorescence was normalized as 100% in the absence of chemokines and 0% for background fluorescence. All experiments were repeated at least three times with similar results. Cells expressing CCR5-GFP are shown before (C), and 30 min (D) after MC-4 addition (10 µg/ml) at 37°C. Cells were then stimulated with 100 nM RANTES, and the subsequent dynamics of CCR5-GFP was recorded every 3 min by confocal microscopy. Responses are shown 15 (E), 30 (F), and 45 min (H) after RANTES addition. Arrows point to agonist-stimulated receptor patches. Arrowheads point to remaining cell surface CCR5-GFP after 45 min of RANTES stimulation. This session is representative of at least four similar experiments. Videos of the dynamics of CCR5-GFP trafficking in response to RANTES stimulation, as described in this figure, are available in the online version of this article. CCR5-GFP-expressing cells did not show differences in cell surface receptor levels before (H) and 30 min after control Ig addition (I), and did not inhibit the ability of RANTES to induce CCR5 endocytosis after 45 min of observation (J).

	DISCUSSION

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION CONCLUSION REFERENCES

mAbs Recognizing the Second Extracellular Loop of CCR5 Antagonize Chemokine Binding

We have characterized five anti-CCR5 mAbs in terms of epitope mapping, inhibition of HIV Env binding and chemokine function,and investigated their ability to activate CCR5 and modulate itsintracellular trafficking. On the basis of their recognition ofvarious CCR5-CCR2b chimeras, these mAbs could be classified intothree groups. The epitopes of MC-4, MC-5, and MC-7 are locatedin the amino-terminal domain, that of MC-1 within ECL2, whereasthat of MC-6 involves multiple extracellular domains. MC-5 recognizesa linear epitope including the first two residues, that of MC-7includes Y10 and D11. These are clearly two dominant epitopes,recognized also by a number of other mAbs (Wu et al., 1997b; Hillet al., 1998; Lee et al., 1999; Olson et al., 1999). ECL2, thelongest extracellular loop of CCR5, also contains dominant epitopes.Both MC-1 and 2D7 mapped to the first part of ECL2 but recognizedifferent epitopes. MC-6 binding, like most multidomain mAbs,was highly dependent on K171 andE172.

Numerous studies have highlighted the importance of CCR5 amino terminus and ECL2 to chemokine binding and HIV coreceptor function(Rucker et al., 1996; Samson et al., 1997; Farzan et al., 1998).ECL2 is particularly important for chemokine binding and selectivity,whereas the N terminus plays the dominant role for the gp120-CCR5interaction. In line with these observations, mAbs such as 539,531, and 2D7, recognizing ECL2 epitopes inhibit efficiently chemokinebinding and signaling, as well as HIV entry (Lee et al., 1999).Our present results are consistent with these previous observations.Both the ECL2 mAb MC-1 and the multidomain mAb MC-6, which relyon ECL2 among other domains, efficiently inhibited binding ofRANTES, MIP-1 $beta$ , and Env to CCR5, as well as the functional responseto chemokines. The N-terminal mAb MC-5 inhibited binding of MIP-1 $beta$ and gp120, but had no effect on RANTES binding and signaling,whereas MC-4 had no effect. The differential inhibition of MIP-1 $beta$ and RANTES function by MC-5 provides further evidence that CCR5ligands may use different extracellular residues for high-affinitybinding.

Partial Activation of CCR5 by a Conformation-sensitive Multidomain mAb

Chemokine receptors are coupled to heterotrimeric G proteins belonging to both pertussis toxin-sensitive G_i and pertussistoxin-insensitive G_q families. They regulate in turn a numberof intracellular cascades, including inhibition of cAMP production,intracellular Ca²⁺ release, and activation of phosphatidylinositol 3-kinase andmitogen-activated protein kinases. These cascades mediate thebiological effects of chemokines, such as chemotaxis and/or increaseof integrin adhesiveness (Sanchez-Madrid and del Pozo, 1999).Activation of GPCRs upon ligand binding is believed to involvethe reorganization of the transmembrane helix bundle, unmaskingintracellular domains that interact with G proteins, and triggeringtheir activation (Wess, 1997). Like chemokines, mAbs might also,by binding to CCR5, modify the equilibrium between its inactiveand active states, and either trigger signaling cascades, or preventtheiractivation.

mAbs directed at GPCRs and displaying agonist activities are rare, and were not reported so far for CCR5. However, an anti-CCR2bmAb was shown to activate this receptor in B cells (Frade et al.,1997). Our mAbs were tested in three functional assays. We showedthat the multidomain mAb MC-6 induced CCR5 activation in GTP $gamma$ Sand cAMP accumulation assays. MC-6 was however unable to promoteintracellular calcium release, whereas chemokines were equallyefficient in all three assays. This discrepancy suggests thatMC-6 and chemokines stabilize different active conformations ofCCR5, coupling differently to intracellular signaling cascades.Differential coupling of a receptor to G proteins according toligands has been proposed for CXCR2 (Hall et al., 1999). The conformationalepitope of MC-6 includes multiple CCR5 domains involved in chemokinebinding, which might explain why MC-6 promotes at least some ofthe conformational changes required for receptor activation. Theabsence of modification of BRET signal after bivalent MC-6 additionwould suggest that the oligomerization state of the receptor isnot modified in this process. Because the MC-6 F(ab) fragmenthas no signaling properties, it remains however possible thatbivalent monoclonals modify the conformation of preexisting dimerswithout changing the distance between the BRET donor (luciferase)and the BRET acceptor (yellowGFP).

mAb-induced Internalization of CCR5 Oligomers Involves an Arrestin-independent Caveolae-dependent Pathway

A molecule that would trigger efficient CCR5 internalization without activating intracellular signaling cascades would haveobvious advantages in terms of therapeutic usefulness as an HIVentry blocker. MC-1, although unable to activate the receptorin a number of bioassays, induced CCR5-GFP internalization. Theredistribution dynamics was however strikingly different to thatpromoted by chemokines, because CCR5-GFP-containing vesicles formedmore rapidly but did not fuse with each other nor with largerendosomal structures. On the other hand, CCR5 activation by theMC-6 mAb did not induce CCR5-GFP endocytosis, demonstrating thatG protein activation and receptor internalization can be totallydissociated. In the classical model of receptor desensitization,binding of a ligand to its receptor leads to G protein activation,after the recruitment of regulatory proteins that mediate phosphorylationof the receptor (G protein-coupled receptor kinases), inhibitionof signaling (arrestins), and ultimately its clathrin-mediatedendocytosis (adaptor-related protein complex AP-2, dynamin) (Lefkowitz,1998). However, recent experimental evidence has shown that receptoractivation and internalization can be dissociated. First, a numberof mutant receptors are unable to signal, but internalize normally,whereas other mutants do not internalize despite normal signalingcapacity (Cheung et al., 1990; Hunyady et al., 1994; Bennett etal., 2000). Second, morphine, an agonist of the µ-opioid receptor,does not induce endocytosis, whereas the receptor is internalizedwell in response to other ligands (Keith et al., 1996). An antagonistof the CCK receptor mediating endocytosis has also been described(Roettger et al., 1997). Finally, constitutive activity of GPCRmutants does not necessarily result in enhanced basal phosphorylationand internalization (Mhaouty-Kodja et al., 1999; Thomas et al.,2000). These observations led to the suggestion that receptorsmay exist in multiple active (and inactive) conformational states,each corresponding to a specific range of functional properties(Thomas et al., 2000). In this context, it is conceivable thatdifferent mAbs may stabilize preferentially one of these usuallytransient conformations. MC-6 would stabilize a signaling statusof CCR5, whereas MC-1 stabilizes a conformation triggeringinternalization.

The use of monovalent and bivalent forms of MC-1 allowed us to investigate whether this internalization-prone conformationinvolves oligomeric structures. The two monovalent versions ofMC-1 continued to bind specifically CCR5 but could no longer mediateinternalization of the receptor, whereas cross-linking by a secondaryantibody partially rescued the ability of the single-chain Fvfragment to induce receptor endocytosis. This partial restorationmight be due to the fact that cross-linking of the monovalentforms of MC-1 by anti-His antibodies does not necessarily restorethe original geometry of the bivalent monoclonal. Moreover, BRETanalysis demonstrated that bivalent MC-1, but not its monovalentforms, modifies the interaction between CCR5polypeptides.

For many membrane receptor families, such as growth factor or cytokine receptors, dimerization is necessary both for signaltransduction and endocytosis. Although GPCRs were until recentlybelieved to operate as monomers, experimental evidence now suggeststhat homo- or heterodimerization occurs, and is sometimes necessaryfor normal receptor trafficking and function (Hebert and Bouvier,1998). Using biophysical approaches, several groups have observedconstitutive homo- or heterodimerization of GPCRs in living cells(Angers et al., 2000; Overton and Blumer, 2000; Rocheville etal., 2000a,b; McVey et al., 2001; Kroeger et al., 2001). For some,but not all receptors, a change in the energy transfer level wasobserved after ligand addition. As stated in these studies, modificationsof fluorescent resonance energy transfer or BRET signals do notallow to distinguish clearly between the de novo association ofreceptor subunits, and the conformation change of preexistingdimers, modifying the relative distance between the two probes.Homodimerization ( $alpha$ -factor receptor) and heterodimerization ofreceptors (dopamine D₂ and somatostatin SST₅, SST₁, and SST₅, $beta$ ₂ adrenergic and opioid OP₁, bradykinin B₂, and angiotensin AT₁)have been shown to affect their signaling and internalizationproperties (AbdAlla et al., 2000; Yesilaltay and Jenness, 2000;Overton and Blumer, 2000; Roche-ville et al., 2000a,b; Jordanet al., 2001).

CCR5 homodimerization has been described, as well as heterodimerization with CCR2b (Benkirane et al., 1997; Mellado et al.,1999; Rodriguez-Frade et al., 1999). However, whether this processis regulated by ligand binding or necessary for any of the CCR5functions has not been conclusively demonstrated so far. We provideherein the evidence that bridging CCR5 polypeptides by bivalentantibodies is necessary for the induction of internalization byMC-1, and modification of energy transfer in BRET assays. Thesedata demonstrate the involvement of oligomers in the MC-1-inducedinternalization process. However, they do not allow discriminationbetween the de novo association of monomeric CCR5, aggregationof preexisting CCR5 dimers, or structural reorganization of theseconstitutivedimers.

MC-1-mediated CCR5 internalization involves a pathway independent of arrestin and clathrin, but dependent on cholesterol-richcaveolae. Two recent studies reported that CCR5 could be foundin membrane raft microdomains and this subcellular localizationmay contribute to the ability of CCR5 to mediate chemotaxis andto support HIV infection (Manes et al., 1999, 2000). The pathwayof MC-1-induced endocytosis contrasts with the internalizationprocess promoted by chemokine agonists, which is arrestin andclathrin dependent. Whether the dimerization or oligomerizationstate of CCR5 is also involved in the chemokine-induced internalizationpathway will require furtherinvestigation.

To the best of our knowledge, MC-1 is the first mAb able to promote endocytosis of a native G protein-coupled receptor. Internalizationof tagged receptors (human muscarinic M1 and thyrotropin-releasinghormone receptors) has however been reported after incubationwith antibodies directed against the tags (Petrou et al., 1997;Tolbert and Lameh, 1998).

mAb Binding to CCR5 N Terminus Prevents Internalization without Preventing Chemokine-induced Signaling

MC-4 was able to potently and specifically inhibit endocytosis mediated by RANTES and AOP-RANTES, without preventing intracellularsignaling. Instead, persistent ruffling of the plasma membranewas seen in confocal microscopy, demonstrating prolonged activationof the receptor. Recently, a mAb (CCR5-02), mapping to the sameN-terminal epitope of CCR5 as MC-4 was found to inhibit HIV infection.This effect was attributed to receptor dimerization (Vila-Coroet al., 2000). Interestingly, antibodies directed against theamino-terminal domain of the bradykinin B₂ receptor, which isinvolved in dimerization, have been shown to reduce receptor internalizationinduced by bradykinin (AbdAlla et al., 1999). The inhibition ofCCR5 endocytosis by MC-4 is probably not related to the stateof CCR5 oligomerization because MC-4 did not induce changes inBRET signal, and its monovalent version was also able to inhibitCCR5 endocytosis. Therefore, this effect probably results fromthe stabilization of a particular conformation of thereceptor.

	CONCLUSION

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION CONCLUSION REFERENCES

We have characterized five mAbs that recognize CCR5 expressed on primary cells. They map to distinct epitopes, including theN-terminal segment (MC-4, MC-5, MC-7), the second extracellularloop (MC-1), or both (and other) domains (MC-6). Many of theseantibodies exhibit functional properties (partial activation ofCCR5 signaling pathways, stimulation of internalization withoutsignaling, inhibition of internalization without impairing signaling)that together suggest the existence of multiple active conformationstates of CCR5. The differential properties of monovalent anddivalent forms of the MC-1 antibody on both endocytosis and bioluminescenceenergy transfer also indicate that the endocytic pathway activatedby this antibody involves CCR5 oligomers. Finally, some of themonoclonal antibodies have interesting properties that might beused in different fields. The MC-1 mAb, which competes for gp120binding and promotes efficient internalization of the receptorwithout triggering intracellular signaling, might constitute thebasis for the development of anti-HIV therapeutic agents. OthermAbs, which appear to stabilize active conformations or dimers,might also be useful as tools to purify and crystallize activestates of CCR5 for structuralstudies.

	ACKNOWLEDGMENTS

Expert technical assistance was provided by M.J. Simons, H. Nguyen Tran, M.E. Decobecq, and T. Rupp. This work was supportedby a grant from the Deutsche Forschungsgemeinschaft (SFB 464),the Actions de Recherche Concertées of the Communauté Françaisede Belgique, the French Agence Nationale de Recherche sur le SIDA,the Center de Recherche Interuniversitaire en Vaccinologie, theBelgian program on Interuniversity Poles of attraction initiatedby the Belgian State, Prime Minister's Office, Science PolicyProgramming, the BIOMED and BIOTECH program of the European Community(grants BIO4-CT98-0543 and BMH4-CT98-2343), the Fonds de la RechercheScientifique Médicale of Belgium, Télévie and the FondationMédicale Reine Elisabeth to M.P. The scientific responsibilityis assumed by the authors. C.B. is Aspirant, and J.M.V. is ChercheurQualifié, of the Belgian Fonds National de la Recherche Scientifique.V.W. is recipient of a First fellowship of the Région Wallonne.We thank Amanda Proudfoot for kindly providing RANTES, Robin Offordand Brigitte Dufour for the synthesis of AOP-RANTES, Mark Scottfor providing $beta$ -arrestin-2-GFP, and the AIDS Research and ReferenceReagent Program for providing soluble CD4 and the 2D7 anti-CCR5mAb.

	FOOTNOTES

^** Corresponding author. E-mail address: mparment{at}ulb.ac.be.

Online version of this article contains video material for Figures 5-8. Online version available at www.molbiolcell.org.

Article published online ahead of print. Mol. Biol. Cell 10.1091/mbc.01-03-0129. Article and publication date are at www.molbiolcell.org/cgi/10.1091/mbc.01-03-0129.

REFERENCES

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
CONCLUSION
REFERENCES

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				C. Ji, J. Zhang, M. Dioszegi, S. Chiu, E. Rao, A. deRosier, N. Cammack, M. Brandt, and S. Sankuratri CCR5 Small-Molecule Antagonists and Monoclonal Antibodies Exert Potent Synergistic Antiviral Effects by Cobinding to the Receptor Mol. Pharmacol., July 1, 2007; 72(1): 18 - 28. [Abstract] [Full Text] [PDF]

				A. Gupta, F. M. Decaillot, I. Gomes, O. Tkalych, A. S. Heimann, E. S. Ferro, and L. A. Devi Conformation State-sensitive Antibodies to G-protein-coupled Receptors J. Biol. Chem., February 23, 2007; 282(8): 5116 - 5124. [Abstract] [Full Text] [PDF]

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				C. Govaerts, A. Bondue, J.-Y. Springael, M. Olivella, X. Deupi, E. Le Poul, S. J. Wodak, M. Parmentier, L. Pardo, and C. Blanpain Activation of CCR5 by Chemokines Involves an Aromatic Cluster between Transmembrane Helices 2 and 3 J. Biol. Chem., January 10, 2003; 278(3): 1892 - 1903. [Abstract] [Full Text] [PDF]

				M. Chelli and M. Alizon Rescue of HIV-1 Receptor Function through Cooperation between Different Forms of the CCR5 Chemokine Receptor J. Biol. Chem., October 11, 2002; 277(42): 39388 - 39396. [Abstract] [Full Text] [PDF]

				B. J. Willett, C. A. Cannon, and M. J. Hosie Upregulation of Surface Feline CXCR4 Expression following Ectopic Expression of CCR5: Implications for Studies of the Cell Tropism of Feline Immunodeficiency Virus J. Virol., September 15, 2002; 76(18): 9242 - 9252. [Abstract] [Full Text] [PDF]

				H. Issafras, S. Angers, S. Bulenger, C. Blanpain, M. Parmentier, C. Labbe-Jullie, M. Bouvier, and S. Marullo Constitutive Agonist-independent CCR5 Oligomerization and Antibody-mediated Clustering Occurring at Physiological Levels of Receptors J. Biol. Chem., September 13, 2002; 277(38): 34666 - 34673. [Abstract] [Full Text] [PDF]

				C. Watters Video Views and Reviews CBE Life Sci Educ, March 1, 2002; 1(1): 6 - 7. [Full Text] [PDF]