Cooperation of the V1/V2 and V3 Domains of Human Immunodeficiency Virus Type 1 gp120 for Interaction with the CXCR4 Receptor

doi:10.1128/JVI.75.12.5457-5464.2001

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Journal of Virology, June 2001, p. 5457-5464, Vol. 75, No. 12
0022-538X/01/$04.00+0 DOI: 10.1128/JVI.75.12.5457-5464.2001
Copyright © 2001, American Society for Microbiology. All rights reserved.

Cooperation of the V1/V2 and V3 Domains of Human Immunodeficiency Virus Type 1 gp120 for Interaction with the CXCR4 Receptor

Béatrice Labrosse, Carole Treboute, Anne Brelot, and Marc Alizon^*

INSERM U.332, Institut Cochin de Génétique Moléculaire, 75014 Paris, France

Received 4 January 2001/Accepted 21 March 2001

	ABSTRACT

Top Abstract Introduction Materials and Methods Results Discussion References

Human immunodeficiency virus type 1 (HIV-1) entry is triggered by the interaction of the gp120 envelope glycoprotein witha cellular chemokine receptor, either CCR5 or CXCR4. We have identifieddifferent mutations in human CXCR4 that prevent efficient infectionby one HIV-1 strain (NDK) but not another (LAI) and sought todefine these strain-dependent effects at the gp120 level. Thelack of activity toward the NDK strain of the HHRH chimeric CXCR4in which the second extracellular loop (ECL2) derived from therat CXCR4 and of CXCR4 with mutations at an aspartic acid in ECL2(D193A and D193R) was apparently due to the sequence of the thirdvariable loop (V3) of gp120, more precisely, to its C-terminalpart. Indeed, substitution of the LAI V3 loop or only its C-terminalpart in the NDK gp 120 context was sufficient to restore usageof the HHRH, D193A, and D193R receptors. The same result was achievedupon mutation of a single lysine residue of the NDK V3 loop toalanine (K319A) but not to arginine (K319R). These results providea strong case for a direct interaction between the gp120 V3 loopand the ECL2 domain of CXCR4. By contrast, V3 substitutions hadno effect on the inability of NDK to infect cells via a mutantCXCR4 in which the amino-terminal extracellular domain (NT) isdeleted. In experiments with a set of chimeric NDK-LAI gp120s,the V1/V2 region from LAI gp120 was both necessary and sufficientfor usage of the NT-deleted CXCR4. Different variable domainsof gp120 can therefore cooperate for a functional interactionwithCXCR4.

	INTRODUCTION

Top Abstract Introduction Materials and Methods Results Discussion References

The envelope glycoproteins of human immunodeficiency virus type 1 (HIV-1) consist of trimeric complexes of a surface (gp120)and a transmembrane (gp41) subunit and mediate fusion of the viralenvelope with the target cell membrane (reviewed in references21, 37, and 57). To achieve this goal, the gp120-gp41 complexmust undergo conformation changes which are not yet understoodin their molecular details but are known to be triggered, in mostsituations, by the interaction of gp120 with two components ofthe cell membrane, CD4 and a chemokine receptor, either CCR5 orCXCR4 (reviewed in references 2, 18, and 44). These chemokinereceptors can therefore be viewed as CD4-associated coreceptorsfor HIV-1. Viral strains dependent on CCR5 or CXCR4 or capableof using either of them are termed R5, X4, and R5X4, respectively.While R5 strains can be isolated at all stages of HIV-1 infectionin vivo, R5X4 and X4 strains generally emerge at later stages,marked by a decline of the immune defenses (17, 38, 45).Several types of CCR5 and CXCR4 ligands can prevent the interactionwith gp120 and block HIV-1 infection (4, 15, 24, 39,49). To pursue this type of antiviral strategy, it is importantto gain a better understanding of the interaction of gp120 withchemokine coreceptors and of its consequences on the HIV-1 entryprocess. Among other means, this can be achieved by functionalstudies involving mutant forms of chemokine receptors and HIV-1envelopeproteins.

There is relatively limited information on how gp120 binds chemokine receptors. Elucidation of the crystal structure of thegp120 core (30) allowed definition of a CCR5-binding site formedby juxtaposition of residues from different conserved domains(43). It is not known if these conserved residues of gp120 alsoparticipate in the interaction with CXCR4. Regions of gp120 thatdisplay extreme genetic variation among HIV-1 strains, in particularthe third hypervariable loop (V3), seem to contribute in an importantway in the interaction of gp120 with the chemokine receptors.First, the CCR5-binding site seems to be masked by variable loopsV3 and V2 until gp120 has interacted with CD4 (43). Second,there was no detectable binding to CCR5 of a recombinant gp120with a V3 loop deletion (56). Finally, there are numerous observationsthat the primary sequence of the V3 and to a lesser extent theV1/V2 loops can determine the selectivity of HIV-1 strains forCCR5 or CXCR4 (13, 26, 27, 35, 47, 51); likewise,it determines biological properties, such as tropism for macrophagesor cell lines and ability to induce syncytia in infected cellcultures, which are largely dependent on coreceptor choice (reviewedin references 2 and 25). On the cellular side, the absenceof information on the spatial structure of chemokine receptorsis a major obstacle to determining their interaction with gp120.Indirect information was mainly gathered from functional studiesperformed with mutant forms of CXCR4 or CCR5. For both receptors,the amino-terminal domain (NT) and the second extracellular loop(ECL2) seem to play a critical role in the interaction with HIV-1,as evidenced by the effect of mutations or domain swapping withother chemokine receptors (reviewed in references 3 and 44).These effects often vary between HIV-1 strains, indicating a certainflexibility in theinteraction.

Here we took advantage of such strain-dependent effects of mutations in CXCR4 to address its interaction with HIV-1. Cellsexpressing ECL2 mutants or an NT-deleted form of CXCR4 could beinfected by HIV-1 strain LAI but not by HIV-1 strain NDK (6,8, 41). We found that the inability of the NDK strain touse the ECL2 mutants resulted from differences with the LAI strainin the level of the V3 loop, while the lack of infection via theNT-deleted CXCR4 was due to differences in the V1/V2 region. Theseresults suggest that the variable domains of gp120 can both contributeto the interaction withCXCR4.

	MATERIALS AND METHODS

Top Abstract Introduction Materials and Methods Results Discussion References

Cell lines and viruses. The CD4⁺ human astroglioma cell line U373MG-CD4, stably transfected with the Escherichia coli $beta$ -galactosidase gene (lacZ) undertranscriptional control of the HIV-1 long terminal repeat (LTR)(23), and derivatives stably expressing the human or rat CXCR4(31) have been described. U373MG-CD4 cells were cotransfectedwith the D193A or D193R human CXCR4 expression vectors (see below)and a vector allowing selection with puromycin. Individual cloneswere screened for their ability to fuse with cells expressingHIV-1 envelope proteins as described previously (42). Viralstocks of HIV-1 strains LAI (40), NDK (52), and 89.6 (16),as well as LAI and NDK derivatives with mutant env genes (seebelow), were produced by transient transfection of HeLa cellswith molecularly cloned proviruses. Stocks of HIV-1 strains GUN-1(48) (a gift from R. Weiss). OUA, and ATE (50) were supernatantsof acutely infected T cells. All infectious titers were determinedby scoring $beta$ -galactosidase-positive cells 24 h after infectionof LTRlacZ HeLa-P4 cells (14).

Plasmid vectors. All forms of CXCR4 were expressed from the cytomegalovirus immediate-early promoter. The vectors allowing expression of thewild-type (WT) human (H) and rat (R) CXCR4 (41), the HHRH andRRHR chimeras, and the $Delta$ 4-36 CXCR4 (8), D193A, and D193R humanCXCR4 mutants (6) have been described. All HIV-1 envelope proteins(Env) were expressed in an LAI provirus with a gag-pol deletion(46). The WT LAI Env and chimeric LAI-V3_NDK Env vectors havebeen described (32). The NDK Env vector (33) actually allowsexpression of a chimeric Env with gp120 and the gp41 ectodomainfrom NDK and the rest of gp41 from LAI (see Fig. 6A for the structureof the chimeric Env). A ClaI restriction site created in the V3-encodingregion of LAI env at nucleotide (nt) 6471 (provirus sequence)was used to derive the LAI-V3_LN and LAI-V3_NL constructs by ligatingSalI (nt 5320)-ClaI and ClaI-BamHI (nt 8068) PCR fragments amplifiedfrom LAI env or from LAI-V3_NDK env, respectively. Restrictionsites flanking V1/V2 (PstI, nt 6192, and SpeI, nt 6409) and V3(MluI, nt 6706, and SmaI, nt 6818) created in the LAI env geneallowed exchanges with PCR fragments amplified from the NDK env.Site-directed mutagenesis was performed on an NDK env subclonewith MluI and SmaI sites flanking V3 (32), allowing substitutionof mutant NDK V3 into either NDK or LAI Env expression vectors.For infection assays, LAI and NDK proviruses with V3 substitutions(LAI-V3_NDK and NDK-V3_LAI) have been described (41). All othermutant env were subcloned in an LAI provirus (40).

Infection assays. Infections of subconfluent U373MG-CD4 cells were performed in 12-well trays with approximately 10³ infectious units (I.U.) per well 24 h after transfection withWT or mutant CXCR4 expression vectors as described (41). Cellswere washed and fixed in 0.5% glutaraldehyde 48 h after infectionand stained for $beta$ -galactosidase activity with the X-Gal (5-bromo-4-chloro-3-indolyl- $beta$ -D-galactopyranoside)substrate as described previously (19). Blue-stained foci werescored under 20× magnification. Cell counts of >200 were obtainedby extrapolation from randomly selectedfields.

Cell fusion assays. Subconfluent monolayers of HeLa cells in six-well trays (~2 × 10⁵ cells per well) were transfected with Env expression vectorsby calcium phosphate precipitation. An equivalent amount of U373MG-CD4cells stably expressing WT or mutant human or rat CXCR4 freshlydetached by trypsinization was added 20 h after transfection.After overnight coculture, adherent cells were fixed in 0.5% glutaraldehydeand stained with X-Gal. Blue-stained foci were scored under 20×magnification.

	RESULTS

Top Abstract Introduction Materials and Methods Results Discussion References

V3 loop and ECL2 substitutions. The HIV-1 coreceptor activity of different forms of CXCR4, i.e., their ability to allow infection of CD4⁺ cells, was tested in the human astroglioma cell line U373MG-CD4,which is naturally resistant to HIV-1 entry and to fusion withcells expressing the HIV-1 envelope proteins (23). Cells transfectedto express the human (H) or the rat (R) CXCR4 or the derived HHRHand RRHR chimeric receptors corresponding to reciprocal ECL2 substitutionscould be infected by the LAI HIV-1 strain, while infection bythe NDK HIV-1 strain was detected only for cells expressing humanCXCR4 or the RRHR chimera (Fig. 1). Previous studies have shownthat these different forms of CXCR4 were expressed at a similarlevel at the surface of transfected cells (6). In agreementwith our earlier observations (41), substitution of the NDKV3 loop in the LAI gp 120 context yielded a chimeric virus (LAI-V3_NDK)infectious for cells expressing the human but not the rat CXCR4,while the chimeric NDK-V3_LAI virus (NDK gp 120 with the V3 loopfrom LAI) could infect cells via the human or the rat CXCR4 (Fig.1). The V3 substitutions also modified the ability of LAI or NDKto infect cells via the chimeric forms of CXCR4, HHRH, and RRHR(Fig. 1). The efficiency of infection by the NDK-V3_LAI virus wasrelatively low whether cells expressed chimeric or wild-type receptors.This suggests that this V3 substitution impairs the function ofthe gp120-gp41 complex in a way that is independent of CXCR4.In these experiments, the NDK V3 loop determined a strict dependencefor receptors with the human CXCR4 ECL2, while the V3 loop ofLAI was required for usage of receptors with the rat CXCR4 ECL2and could confer this property on the gp120 of a genetically divergentstrain (LAI and NDK belong to clades B and D, respectively).

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FIG. 1. Infection of U373MG-CD4 cells expressing human or rat CXCR4 or the derived chimeric receptors HHRH and RRHR by HIV-1 strains LAI and NDK or derivatives with substitutions of the gp120 V3 loop. Cells were infected with approximately 1,000 I.U. per well (12-well plates) and stained with X-Gal after another 48 h. Blue-stained cells, representing HIV-1-infected cells, were scored in duplicate wells. Bars represent means of three independent transfections.

This analysis was refined by substituting the N-terminal or the C-terminal part of the V3 loop of LAI with the homologousregion from the NDK V3, yielding the LAI-V3_NL and LAI-V3_LN chimericEnvs, respectively (Fig. 2). Both forms of Env mediated HIV-1infection or syncytium formation with U373MG-CD4 cells expressinghuman CXCR4, but only the LAI-V3_NL Env allowed infection and fusionwhen cells expressed the rat CXCR4 (Fig. 3A and B). Sequence differencesin the distal part of the V3 loop therefore seem to account forthe phenotypic differences between LAI and NDK in usage of therat CXCR4 as a coreceptor.

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FIG. 2. Alignment of the amino acid sequence of gp120 V3 loops of NDK and LAI strains and derived mutants. Numbering is according to the NDK gp120 sequence (52).

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FIG. 3. Effect of V3 substitutions and mutations on usage of rat and human CXCR4. (A) Infections of U373MG-CD4 cells stably expressing human or rat CXCR4 were performed and scored as described in the legend to Fig. 1. (B) Syncytium formation assays between these cell lines and HeLa cells transfected with Env expression vectors with the indicated type of gp120. Cocultures were performed in six-well plates, and cells were stained with X-Gal after 24 h. Blue-stained foci representing syncytia were scored in duplicate wells. Bars represent means of three independent transfections.

Mutagenesis of NDK V3. A striking feature of the NDK V3 loop in its distal moiety is a cluster of four adjacent lysine residues (positions 316 to319), while only one lysine is found in the corresponding regionof the LAI V3 loop (Fig. 2). Each of these four lysine residuesof the NDK V3 was replaced with an alanine, and the resultingmutant V3 was inserted in the LAI gp120 context. The functionof these chimeric envelope proteins was tested in HIV-1 infection(Fig. 3A) and cell fusion (Fig. 3B) assays. The K317A and K318Amutations were apparently not compatible with these Env functions.The K316A mutation markedly reduced the efficiency of infectionand fusion with cells expressing human CXCR4 and did not seemto confer ability to use the rat CXCR4. In contrast, the K319Amutation was compatible with efficient infection or fusion withcells expressing the human CXCR4 and also with cells expressingthe rat CXCR4. When the lysine residue was replaced with an arginine(K319R), the corresponding chimeric LAI-V3_NDK gp120 could onlymediate HIV-1 infection and fusion with cells expressing humanCXCR4, not rat CXCR4. In the NDK gp120 context, the K319A andK319R mutations resulted in a complete loss of function in infectionassays (Fig. 3A) but not in syncytium formation assays (Fig. 3B).In that case, the K319A but not K319R mutation restored usageof the rat CXCR4 by the NDK gp120. The presence of a positivelycharged residue at a defined position in the V3 loop of gp120apparently explained why the NDK HIV-1 strain cannot functionallyinteract with the rat CXCR4. Why the mutant NDK Env can mediatecell-cell fusion but not HIV-1 infection has not been determined,but mutations in the V3 loop can reduce the stability of the gp120-gp41complex (55). This can result in gp120 shedding from virionsand loss of infectivity. But even unstable gp120-gp41 complexescan probably mediate syncytium formation, provided they reachthe cellsurface.

Usage of ECL2 mutants. We have previously shown that a negatively charged aspartic acid residue (Asp193) in the ECL2 of the human CXCR4 was criticalfor a functional interaction with the NDK strain (6). The presenceof a neutral asparagine residue at the corresponding positionin the ECL2 of the rat CXCR4 could therefore explain its lackof coreceptor activity for NDK. We have tested the ability ofLAI and NDK gp120 with V3 loop substitutions or mutations at theLys319 residue to mediate infection of U373MG-CD4 cells stablyexpressing human CXCR4 with mutation of the Asp193 residue toalanine (D193A) (Fig. 4A). This mutant CXCR4 enabled infectionby the LAI and NDK-V3_LAI viruses, but not the NDK or LAI-V3_NDKvirus. Also, infection via the D193A receptor was markedly moreefficient for the LAI-V3_NL virus, in which the first part of theV3 loop derived from NDK and the second from LAI, than for theLAI-V3_LN virus. The distal moiety of the LAI V3 therefore seemedimportant for usage of human CXCR4 with the Asp193 mutation, likewisefor usage of the rat CXCR4 and HHRH chimera.

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FIG. 4. Effect of V3 substitutions and mutations on usage of human CXCR4 and the derived ECL2 mutants D193A and D193R. Infections (A) and syncytium formation assays (B) were performed and scored as described in the legend to Fig. 3.

Cells expressing the D193A mutant CXCR4 could be infected by a chimeric LAI-V3_NDK virus with the K319A but not K319R mutationin the NDK V3 loop (Fig. 4A). Similar results were obtained insyncytium formation assays performed with cells expressing thesedifferent HIV-1 envelope proteins and U373MG-CD4 cells stablyexpressing human CXCR4 with a D193A or D193R mutation (Fig. 4B).The latter CXCR4 mutant was used because it yielded clearer results.Indeed, cells expressing the D193A mutant were not completelyresistant to fusion mediated by the NDK or LAI-V3_NDK Env. If anegative charge at position 193 in ECL2 is important for function,it was not unexpected that substitution with a positively chargedresidue (D193R) would have a stronger effect than substitutionwith a neutral residue (D193A). In cell fusion assays, we couldalso monitor the effect of the K319A and K319R mutations in theNDK Env context (Fig. 4B). Again, the inability to use the D193Aor D193R mutant CXCR4 appeared to be related to the presence ofa positively charged residue at position 319 in the V3 loop ofthe NDKstrain.

Usage of NT-deleted CXCR4. The deletion of 32 of the 39 residues of the amino-terminal domain (NT) of CXCR4 is compatible with coreceptor activity forthe LAI HIV-1 strain (8). The efficiency of infection mediatedby this mutant ( $Delta$ 4-36) or the WT CXCR4 was in proportion of theirlevels of cell surface expression (8), suggesting that theNT domain of CXCR4 is dispensable for a functional interactionwith the gp120 of the LAI strain. Cells stably expressing the $Delta$ 4-36 CXCR4 could be infected by the HIV-1 strain 89.6 (R5X4)but were resistant to infection by the NDK (X4) and GUN-1 (R5X4)strains and almost resistant to infection by the primary X4 isolatesOUA and ATE (Fig. 5). Among this limited set of HIV-1 strains,there was no apparent correlation between the ability to use theNT-deleted CXCR4 and a strictly X4 or R5X4 phenotype, or withthe genetic subtype, since LAI, GUN-1, and 89.6 all belong toenv subtype B.

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FIG. 5. Effect of a deletion in the amino-terminal domain (NT) of CXCR4 on its coreceptor activity for different HIV-1 strains. Infections of U373MG-CD4 cells stably expressing human CXCR4 or the $Delta$ 4-36 mutant were performed in 12-well plates with approximately 2,000 I.U. per well. Cells were stained with X-Gal 48 h later, and blue-stained cells were scored in duplicate wells.

The V3 loop sequence had no apparent role in the ability of LAI to use the NT-deleted form of CXCR4, since cells expressingthe $Delta$ 4-36 mutant could be infected with similar efficiency bythe LAI and NDK-V3_LAI viruses and were equally resistant to infectionby the NDK and LAI-V3_NDK viruses (Fig. B). We sought to determinewhether a defined region of gp120 (or the gp41 ectodomain) wasresponsible for the ability of the LAI strain to use the NT-deletedform of CXCR4, likewise V3 for the ECL2 mutants. We tested theability of a set of LAI/NDK chimeric Envs (Fig. 6A) to mediateHIV-1 infection of U373MG-CD4 cells stably expressing either WTor $Delta$ 4-36 CXCR4 (Fig. 6B). Results with the LAI-(C1-C2)_NDK chimerashowed that the region of LAI gp120 which is N-terminal to V3,i.e., the C1 and C2 conserved domains and the interventing V1/V2variable loops, was required for usage of the NT-deleted CXCR4.Replacing the C1 or C2 domain of LAI gp120 with the correspondingNDK domain (LAI-C1_NDK and LAI-C2_NDK, respectively) reduced theefficiency of infection of cells expressing $Delta$ 4-36 CXCR4 but didnot abolish it. In contrast, there was no detectable infectionof these cells when the V1/V2 region of LAI gp120 was absent,for example, with the LAI-(C1-V1V2)_NDK or the LAI-(V1V2)_NDK chimera.We next found that substitution of the V1/V2 region from LAI intothe NDK gp120 context (NDK-V1V2_LAI chimera) was sufficient torestore detectable infection of cells expressing the $Delta$ 4-36 CXCR4.The V1/V2 region of the LAI gp120 was both necessary and sufficientto confer usage of the NT-deleted CXCR4 in the genetically distantcontext of the NDK gp120. Other regions of gp120 or the gp41 ectodomainapparently had no role in the phenotype difference between LAIand NDK.

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FIG. 6. Effect of exchanges between the envelope proteins of LAI and NDK on usage of the NT-deleted CXCR4. (A) Schematic organization of chimeric env genes, with restriction sites created to allow substitutions. m.a., membrane anchor domain of gp41. (B) Infections of cells stably expressing human CXCR4 or the $Delta$ 4-36 mutant with LAI or NDK virus or recombinant LAI viruses bearing the indicated env gene, performed and scored as in Fig. 5.

	DISCUSSION

Top Abstract Introduction Materials and Methods Results Discussion References

Mutations or substitutions in the extracellular domains of the CCR5 and CXCR4 chemokine receptors can reduce or abolish theirHIV-1 coreceptor activity, that is, their ability to mediate HIV-1entry in CD4⁺ cells. The effects of such mutations can be very different indifferent HIV-1 strains, suggesting that not all gp120 envelopeglycoproteins have the same requirements for a functional interactionwith their coreceptors. This may represent an obstacle to antiviralapproaches but can also be a source of information on the gp120-coreceptorinteraction. Here we have used two CXCR4-dependent (X4) HIV-1strains, LAI and NDK, that have relatively divergent gp120s anddisplay clear-cut phenotypic differences in usage of certain formsof CXCR4. The NDK strain cannot infect CD4⁺ cells via (i) the rat CXCR4 (41), (ii) the HHRH chimeric humanCXCR4, in which the second extracellular loop (ECL2) derives fromthe rat CXCR4 (8), (iii) human CXCR4 with mutations at position193 in ECL2 (D193A or D193R) (6), or (iv) human CXCR4 withan almost complete deletion of the amino-terminal extracellulardomain (NT) (7). These four types of CXCR4 were functionalcoreceptors for the LAI strain. We had already observed that theability to use the rat CXCR4 as a coreceptor could be conferredon NDK by replacing the third variable loop (V3) with the homologousregion of LAI gp120 (41). Here we found that this V3 substitutionwas also sufficient to allow usage of the HHRH chimeric receptorand the D193A and D193R CXCR4 mutants, but not the NT-deletedCXCR4. It confirmed the importance of the V3 loop of gp120 fora functional interaction with CXCR4 and showed that other domainsof gp120 contribute to thisinteraction.

The role of the V3 loop was further studied by exchanging fragments of V3 between the gp120 of LAI and NDK and by site-directedmutagenesis in the NDK V3 loop. In the LAI gp120 context, onlythe C-terminal part of V3 appeared to be necessary for infectionof cells via the rat CXCR4, the HHRH chimera, and the D193A andD193R mutants. The importance of the C-terminal part of V3 forusage of CXCR4 is in agreement with a recent study based on chimericgp120 derived from X4 and R5 HIV-1 strains (27). The usage ofthese three types of mutant CXCR4 coreceptors was restored bythe mutation of a lysine residue of the NDK V3 loop to alanine(K319A) but not to arginine (K319R). These results were consistentwith some form of interaction between the V3 loop of the NDK gp120and the ECL2 domain of CXCR4. The LAI V3 loop could have differentrequirements for its interaction with ECL2; in particular, itcould be independent of the Asp193 residue. Alternatively, theLAI V3 loop could allow an interaction with CXCR4 that is totallyindependent of the ECL2 domain. We consider the second possibilityless likely, given the negative effect of other ECL2 mutationson HIV-1 infection (6, 7) and its blocking by reagents targetingthe ECL2 domain of CXCR4, such as the AMD3100 bicyclam (31)and the 12G5 monoclonal antibody (8).

There is evidence for the accumulation of basic amino acids in the V3 loop of X4 HIV-1 strains (20, 29). These positivelycharged residues could allow electrostatic interactions with thenegatively charged residues of CXCR4 that are apparently involvedin HIV-1 coreceptor activity and located in the NT or ECL2 domain(10, 11, 28, 54). In line with this view, it could beproposed that contact between the Lys319 residue of the NDK V3loop and the Asp193 residue of ECL2 is critical for a functionalinteraction of gp120 and CXCR4. However, for the effect of theK319A mutation to fit with this model, one also has to envisionthat the basic residue Lys319 in the NDK V3 loop is detrimentalto the interaction with CXCR4 in the absence of a negatively chargedAsp193 residue in ECL2, which is the case for the rat CXCR4 (Ser).Alternatively, the K319A mutation could indirectly affect thestructure of the NDK V3 loop, allowing it to cope with mutationsat the Asp193 residue, likewise the LAI V3loop.

The V3 loop sequence had no apparent role in the ability of the LAI strain to infect cells via an NT-deleted form of CXCR4.This property was apparently linked to the first variable loopsV1/V2 of the gp120, which suggested their role in the functionalinteraction of gp120 with CXCR4. This is in apparent contradictionto the observed binding to CXCR4 of a recombinant gp120 deletedin the V1/V2 region (36). Two types of explanations can be proposed.First, the monomeric gp120 used in direct binding assays may behavedifferently from the trimeric gp120 complexed to gp41 involvedin functional assays. Second, the V1/V2 region could have a minorrole in terms of binding of gp120 to CXCR4, as it can be physicallymeasured but still be important for a correct positioning andhence a functional interaction. In the case of the NDK gp120,it can be postulated either that the V1/V2 region directly interactswith the NT region of CXCR4 or that it has no role in the interactionwith CXCR4. We lack experimental evidence to sort out these possibilities,but the former is indirectly supported by several reports involvingthe V1 or V2 region of gp120 in the tropism of different HIV-1strains for T-cell lines and hence their adaptation to the CXCR4coreceptor (1, 5, 9, 22). More recently, substitutionof either the V1/V2 or the V3 region from a dualtropic strain(R5X4) in the context of a macrophage-tropic (R5) strain was foundsufficient to confer ability to utilize the CXCR4 coreceptor (12).It can therefore be proposed that the V1/V2 and V3 variable loopsof gp120 cooperate for interaction with the extracellular loopsof CXCR4 (LAI strain) or with the loops and NT domain (NDKstrain).

An important issue that could not be addresed in this study is the possible contribution to the interaction with CXCR4 ofthe conserved gp120 residues forming the putative CCR5 bindingsite (43). Does this site contribute to the interaction withCXCR4, particularly in R5X4 strains, or is it dispensable, particularlyfor strictly X4 strains? These questions will probably be answeredby functional assays with a set of gp120 mutants. More generally,it can be wondered if the ability of CCR5 or CXCR4 $---$ and otherchemokine receptors in certain experimental conditions $---$ to mediateHIV-1 entry is due only to their ability to bind gp120, itselfdependent on the structure of their extracellular domains, oris also dependent on other features, for example, the colocalizationof chemokine receptors with CD4 (53) or their monomeric versusdimeric status (34).

Differences in the interaction of HIV-1 strains with CXCR4 could represent an obstacle to the development of CXCR4 ligandsas antiviral agents. The NT domain of CXCR4 contains a high affinitybinding site for the SDF-1 chemokine, but signaling requires bindingto a conformational site formed by residues of the extracellularloops and membrane-spanning domains (7). Natural or syntheticCXCR4 ligands binding to the NT domain of CXCR4 may have limitedantiviral efficacy for HIV-1 strains such as LAI and 89.6. Onthe other hand, ligands targeting the extracellular loops of CXCR4could have a broader spectrum of antiviral activity but be morelikely to interfere with the natural signaling function. Thisshould be kept in view for the selection or design of inhibitorsof the CXCR4coreceptor.

	ACKNOWLEDGMENTS

We thank F. Letourneur (ICGM) for assistance with DNAsequencing.

This work was supported by the Agence Nationale de Recherche sur leSIDA.

	FOOTNOTES

^* Corresponding author. Mailing address: INSERM U.332, Institut Cochin de Génétique Moléculaire, 22 rue Méchain, 75014 Paris,France. Phone: 33-1-40 51 64 86. Fax: 33-1-40 51 64 54. E-mail:alizon{at}cochin.inserm.fr.

REFERENCES

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References

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6. Brelot, A., N. Heveker, K. Adema, M. J. Hosie, B. Willett, and M. Alizon. 1999. Effect of mutations in the second extracellular loop of CXCR4 on its utilization by human and feline immunodeficiency viruses. J. Virol. 73:2576-2586[Abstract/Free Full Text].

7. Brelot, A., N. Heveker, M. Montes, and M. Alizon. 2000. Identification of residues of CXCR4 critical for human immunodeficiency virus coreceptor and chemokine receptor activities. J. Biol. Chem. 275:23736-23744[Abstract/Free Full Text].

8. Brelot, A., N. Heveker, O. Pleskoff, N. Sol, and M. Alizon. 1997. Role of the first and third extracellular domains of CXCR-4 in human immunodeficiency virus coreceptor activity. J. Virol. 71:4744-4751[Abstract].

9. Carrillo, A., and L. Ratner. 1996. Human immunodeficiency virus type 1 tropism for T-lymphoid cell lines: role of the V3 loop and C4 envelope determinants. J. Virol. 70:1301-1309[Medline].

10. Chabot, D. J., H. Chen, D. S. Dimitrov, and C. C. Broder. 2000. N-linked glucosylation of CXCR4 masks coreceptor function for CCR5-dependent human immunodeficiency virus type 1 isolates. J. Virol. 74:4404-4413[Abstract/Free Full Text].

11. Chabot, D. J., P. F. Zhang, G. V. Quinnan, and C. C. Broder. 1999. Mutagenesis of CXCR4 identifies important domains for human immunodeficiency virus type 1 X4 isolate envelope-mediated membrane fusion and virus entry and reveals cryptic coreceptor activity for R5 isolates. J. Virol. 73:6598-6609[Abstract/Free Full Text].

12. Cho, M. W., M. K. Lee, M. C. Carney, J. F. Berson, R. W. Doms, and M. A. Martin. 1998. Identification of determinants on a dualtropic human immunodeficiency virus type 1 envelope glycoprotein that confer usage of CXCR4. J. Virol. 72:2509-2515[Abstract/Free Full Text].

13. Choe, H., M. Farzan, Y. Sun, N. Sullivan, B. Rollins, P. D. Ponath, L. Wu, C. R. Mackay, G. LaRosa, W. Newman, N. Gerard, C. Gerard, and J. Sodroski. 1996. The beta-chemokine receptors CCR3 and CCR5 facilitate infection by primary HIV-1 isolates. Cell 85:1135-1148[CrossRef][Medline].

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17. Connor, R. I., K. E. Sheridan, D. Ceradini, S. Choe, and N. R. Landau. 1997. Change in coreceptor use coreceptor use correlates with disease progression in HIV-1-infected individuals. J. Exp. Med. 185:621-628[Abstract/Free Full Text].

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20. Fouchier, R. A., M. Groenink, N. A. Kootstra, M. Tersmette, H. G. Huisman, F. Miedema, and H. Schuitemaker. 1992. Phenotype-associated sequence variation in the third variable domain of the human immunodeficiency virus type 1 gp120 molecule. J. Virol. 66:3183-3187[Abstract/Free Full Text].

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23. Harrington, R. D., and A. P. Geballe. 1993. Cofactor requirement for human immunodeficiency virus type 1 entry into a CD4-expressing human cell line. J. Virol. 67:5939-5947[Abstract/Free Full Text].

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28. Kajumo, F., D. A. Thompson, Y. Guo, and T. Dragic. 2000. Entry of R5X4 and X4 human immunodeficiency virus type 1 strains is mediated by negatively charged and tyrosine residues in the amino-terminal domain and the second extracellular loop of CXCR4. Virology 271:240-247[CrossRef][Medline].

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1.	Andeweg, A. C., P. Leeflang, A. D. Osterhaus, and M. L. Bosch. 1993. Both the V2 and V3 regions of the human immunodeficiency virus type 1 surface glycoprotein functionally interact with other envelope regions in syncytium formation. J. Virol. 67:3232-3239[Abstract/Free Full Text].
2.	Berger, E. A., P. M. Murphy, and J. M. Farber. 1999. Chemokine receptors as HIV-1 coreceptors: roles in viral entry, tropism, and disease. Annu. Rev. Immunol. 17:657-700[CrossRef][Medline].
3.	Berson, J. F., and R. W. Doms. 1998. Structure-function studies of the HIV-1 coreceptors. Semin. Immunol. 10:237-248[CrossRef][Medline].
4.	Bleul, C. C., M. Farzan, H. Choe, C. Parolin, I. Clark-Lewis, J. Sodroski, and T. A. Springer. 1996. The lymphocyte chemoattractant SDF-1 is a ligand for LESTR/fusin and blocks HIV-1 entry. Nature 382:829-833[CrossRef][Medline].
5.	Boyd, M. T., G. R. Simpson, A. J. Cann, M. A. Johnson, and R. A. Weiss. 1993. A single amino acid substitution in the V1 loop of human immunodeficiency virus type 1 gp120 alters cellular tropism. J. Virol. 67:3649-3652[Abstract/Free Full Text].
6.	Brelot, A., N. Heveker, K. Adema, M. J. Hosie, B. Willett, and M. Alizon. 1999. Effect of mutations in the second extracellular loop of CXCR4 on its utilization by human and feline immunodeficiency viruses. J. Virol. 73:2576-2586[Abstract/Free Full Text].
7.	Brelot, A., N. Heveker, M. Montes, and M. Alizon. 2000. Identification of residues of CXCR4 critical for human immunodeficiency virus coreceptor and chemokine receptor activities. J. Biol. Chem. 275:23736-23744[Abstract/Free Full Text].
8.	Brelot, A., N. Heveker, O. Pleskoff, N. Sol, and M. Alizon. 1997. Role of the first and third extracellular domains of CXCR-4 in human immunodeficiency virus coreceptor activity. J. Virol. 71:4744-4751[Abstract].
9.	Carrillo, A., and L. Ratner. 1996. Human immunodeficiency virus type 1 tropism for T-lymphoid cell lines: role of the V3 loop and C4 envelope determinants. J. Virol. 70:1301-1309[Medline].
10.	Chabot, D. J., H. Chen, D. S. Dimitrov, and C. C. Broder. 2000. N-linked glucosylation of CXCR4 masks coreceptor function for CCR5-dependent human immunodeficiency virus type 1 isolates. J. Virol. 74:4404-4413[Abstract/Free Full Text].
11.	Chabot, D. J., P. F. Zhang, G. V. Quinnan, and C. C. Broder. 1999. Mutagenesis of CXCR4 identifies important domains for human immunodeficiency virus type 1 X4 isolate envelope-mediated membrane fusion and virus entry and reveals cryptic coreceptor activity for R5 isolates. J. Virol. 73:6598-6609[Abstract/Free Full Text].
12.	Cho, M. W., M. K. Lee, M. C. Carney, J. F. Berson, R. W. Doms, and M. A. Martin. 1998. Identification of determinants on a dualtropic human immunodeficiency virus type 1 envelope glycoprotein that confer usage of CXCR4. J. Virol. 72:2509-2515[Abstract/Free Full Text].
13.	Choe, H., M. Farzan, Y. Sun, N. Sullivan, B. Rollins, P. D. Ponath, L. Wu, C. R. Mackay, G. LaRosa, W. Newman, N. Gerard, C. Gerard, and J. Sodroski. 1996. The beta-chemokine receptors CCR3 and CCR5 facilitate infection by primary HIV-1 isolates. Cell 85:1135-1148[CrossRef][Medline].
14.	Clavel, F., and P. Charneau. 1994. Fusion from without directed by human immunodeficiency virus particles. J. Virol. 68:1179-1185[Abstract/Free Full Text].
15.	Cocchi, F., A. L. DeVico, A. Garzino-Demo, A. Cara, R. C. Gallo, and P. Lusso. 1996. The V3 domain of the HIV-1 gp120 envelope glycoprotein is critical for chemokine-mediated blockade of infection. Nat. Med. 2:1244-1247[CrossRef][Medline].
16.	Collman, R. 1992. Human immunodeficiency virus type 1 tropism for human macrophages. Pathobiology 60:213-218[CrossRef][Medline].
17.	Connor, R. I., K. E. Sheridan, D. Ceradini, S. Choe, and N. R. Landau. 1997. Change in coreceptor use coreceptor use correlates with disease progression in HIV-1-infected individuals. J. Exp. Med. 185:621-628[Abstract/Free Full Text].
18.	Dimitrov, D. S., X. Xiao, D. J. Chabot, and C. C. Broder. 1998. HIV coreceptors. J. Membr. Biol. 166:75-90[CrossRef][Medline].
19.	Dragic, T., U. Hazan, and M. Alizon. 1995. Detection of cell fusion mediated by the envelopes of human retroviruses by transactivation of a reporter gene. Methods Mol. Genet. 7:218-236[CrossRef].
20.	Fouchier, R. A., M. Groenink, N. A. Kootstra, M. Tersmette, H. G. Huisman, F. Miedema, and H. Schuitemaker. 1992. Phenotype-associated sequence variation in the third variable domain of the human immunodeficiency virus type 1 gp120 molecule. J. Virol. 66:3183-3187[Abstract/Free Full Text].
21.	Freed, E. O., and M. A. Martin. 1995. The role of human immunodeficiency virus type 1 envelope glycoproteins in virus infection. J. Biol. Chem. 270:23883-23886[Free Full Text].
22.	Groenink, M., R. A. Fouchier, S. Broersen, C. H. Baker, M. Koot, A. B. van't Wout, H. G. Huisman, F. Miedema, M. Tersmette, and H. Schuitemaker. 1993. Relation of phenotype evolution of HIV-1 to envelope V2 configuration. Science 260:1513-1516[Abstract/Free Full Text].
23.	Harrington, R. D., and A. P. Geballe. 1993. Cofactor requirement for human immunodeficiency virus type 1 entry into a CD4-expressing human cell line. J. Virol. 67:5939-5947[Abstract/Free Full Text].
24.	Heveker, N., M. Montes, L. Germeroth, A. Amara, A. Trautmann, M. Alizon, and J. Schneider-Mergener. 1998. Dissociation of the signalling and antiviral properties of SDF-1-derived small peptides. Curr. Biol. 8:369-376[CrossRef][Medline].
25.	Hoffman, T. L., and R. W. Doms. 1999. HIV-1 envelope determinants for cell tropism and chemokine receptor use. Mol. Membr. Biol. 16:57-65[CrossRef][Medline].
26.	Hoffman, T. L., E. B. Stephens, O. Narayan, and R. W. Doms. 1998. HIV type 1 envelope determinants for use of the CCR2b, CCR3, STRL33, and APJ coreceptors. Proc. Natl. Acad. Sci. USA 95:11360-11365[Abstract/Free Full Text].
27.	Hung, C. S., N. Vander Heyden, and L. Ratner. 1999. Analysis of the critical domain in the V3 loop of human immunodeficiency virus type 1 gp120 involved in CCR5 utilization. J. Virol. 73:8216-8226[Abstract/Free Full Text].
28.	Kajumo, F., D. A. Thompson, Y. Guo, and T. Dragic. 2000. Entry of R5X4 and X4 human immunodeficiency virus type 1 strains is mediated by negatively charged and tyrosine residues in the amino-terminal domain and the second extracellular loop of CXCR4. Virology 271:240-247[CrossRef][Medline].
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