Selective Interactions of Polyanions with Basic Surfaces on Human Immunodeficiency Virus Type 1 gp120

doi:10.1128/JVI.74.4.1948-1960.2000

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Journal of Virology, February 2000, p. 1948-1960, Vol. 74, No. 4
0022-538X/00/$04.00+0
Copyright © 2000, American Society for Microbiology. All rights reserved.

Selective Interactions of Polyanions with Basic Surfaces on Human Immunodeficiency Virus Type 1 gp120

Maxime Moulard,¹^, Hugues Lortat-Jacob,² Isabelle Mondor,¹ Guillaume Roca,¹ Richard Wyatt,³ Joseph Sodroski,³ Lu Zhao,⁴ William Olson,⁴ Peter D. Kwong,⁵ and Quentin J. Sattentau¹^,^*

Centre d'Immunologie de Marseille-Luminy, 13288 Marseille Cedex 9,¹ and Institut de Biologie Structurale, 38027 Grenoble Cedex 01,² France; Department of Cancer Immunology and AIDS, Dana-Farber Cancer Institute, Harvard Medical School, Boston, Massachusetts 02115³; Progenics Pharmaceuticals Inc., Tarrytown, New York 10591⁴; and Department of Biochemistry and Molecular Biophysics, College of Physicians and Surgeons, Columbia University, New York, New York 10032⁵

Received 25 June 1999/Accepted 17 November 1999

	ABSTRACT

Top Abstract Introduction Materials and Methods Results Discussion References

It is well established that the gp120 V3 loop of T-cell-line-adapted human immunodeficiency virus type 1 (HIV-1) binds bothcell-associated and soluble polyanions. Virus infectivity is increasedby interactions between HIV-1 and heparan sulfate proteoglycanson some cell types, and soluble polyanions such as heparin anddextran sulfate neutralize HIV-1 in vitro. However, the analysisof gp120-polyanion interactions has been limited to T-cell-line-adapted,CXCR4-using virus and virus-derived gp120, and the polyanion bindingability of gp120 regions other than the V3 loop has not been addressed.Here we demonstrate by monoclonal-antibody inhibition, labeledheparin binding, and surface plasmon resonance studies that asecond site, most probably corresponding to the newly defined,highly conserved coreceptor binding region on gp120, forms partof the polyanion binding surface. Consistent with the bindingof polyanions to the coreceptor binding surface, dextran sulfateinterfered with the gp120-CXCR4 association while having no detectableeffect on the gp120-CD4 interaction. The interaction between polyanionsand X4 or R5X4 gp120 was readily detectable, whereas weak or undetectablebinding was observed with R5 gp120. Analysis of mutated formsof X4 gp120 demonstrated that the V3 loop is the major determinantfor polyanion binding whereas other regions, including the V1/V2loop structure and the NH₂ and COOH termini, exert a more subtleinfluence. A molecular model of the electrostatic potential ofthe conserved coreceptor binding region confirmed that it is basicbut that the overall charge on this surface is dominated by theV3 loop. These results demonstrate a selective interaction ofgp120 with polyanions and suggest that the conserved coreceptorbinding surface may present a novel and conserved target for therapeuticintervention.

	INTRODUCTION

Top Abstract Introduction Materials and Methods Results Discussion References

A number of pathogenic microorganisms attach to cell surfaces via heparan sulfate proteoglycans (HSPG). Of these, severalviruses appear to use HSPG at a step prior to interaction withtheir specific receptors. Thus, herpes simplex virus (81), pseudorabiesvirus (27), human herpesvirus 7 (71), adeno-associated virus(76), dengue virus (10), and vaccinia virus (13) can allinteract with cell surface HSPG. The crystal structure of a complexformed by foot-and-mouth disease virus and heparin has recentlybeen determined (29). Human immunodeficiency virus type 1 (HIV-1)binds cell surface HSPG, and the type and quantity of HSPG ona given cell type modulate virus infectivity in vitro (50, 57,59, 65) and may influence viral tropism in vivo (83).

It is well established that HIV-1 can interact with soluble polyanions and cell surface HSPG via the gp120 V3 loop; polyanionssuch as dextran sulfate (DexS) compete with V3 loop-specific monoclonalantibodies (MAbs) for binding (3, 8, 32, 63, 65) butinterfere weakly or undetectably with soluble-gp120-CD4 binding(8, 33). Moreover, radioactively labeled heparin binds V3loop peptides and recombinant gp120 (3, 33), and variouspolyanions neutralize the infectivity of T-cell-line-adapted (TCLA)HIV-1 at low (micromolar) concentrations (2, 41, 48, 82).The V3 loop-HSPG association is thought to take place via electrostaticinteractions between the acidic sulfate groups on heparan sulfateand basic residues within the V3 loop. Indeed, some TCLA viruses,such as the HXBc2 molecular clone, have a V3 loop with a net chargeof +9 and a sequence motif of X-B-B-B-X-B-X-X-B-X (where X isa hydropathic residue and B is a basic residue), similar to themotifs described for other heparin-protein interactions (27).However, not all strains of HIV-1 have such basic V3 loops; thoseof CCR5-using (R5 [4]) viruses are substantially less basicthan those of CXCR4-using (X4 [4]) and dualtropic, CCR5- andCXCR4-using (R5X4 [4]) viruses (28, 42), and primary isolate(PI) X4 viruses tend to have less-basic V3 loops than TCLA X4viruses. The level of positive charge present on the gp120 surfacemay relate directly to coreceptor utilization, in that the exposedsurface of CXCR4 has been modeled as highly acidic whereas thatof CCR5 appears to be less so (17, 42). However, a recentstudy suggests that negatively charged moities, including acidicamino acids and sulfated tyrosine residues, may be important forbinding of gp120 to both CCR5 and CXCR4 (24).

The solution of the crystal structure of the gp120 core complexed with domains 1 and 2 of CD4 and an Fab fragment of a neutralizingMAb (44) has generated a great deal of information with respectto gp120-CD4 interactions (44, 90), gp120-coreceptor interactions(44, 64), and gp120-antibody interactions (88). Within thisstructure, the Fab fragment (17b) binds an epitope that comprisespart of the CD4-induced (CD4i) region, so called because it becomesmore accessible after CD4 binding (75, 77, 89). A comprehensivemutagenesis study based on the R5 gp120_YU2 has defined this regionas a coreceptor binding surface that is highly conserved amongHIV-1, HIV-2, and simian immunodeficiency virus isolates (64).It seems likely, based on experimental and structural evidence,that this surface is at least partially masked by the V1/V2 andV3 loops in the intact gp120-gp41 trimer, and CD4 binding displacesthese variable loops, revealing the conserved surface (44, 64,68, 75). The coreceptor binding site on gp120 most likelyconsists of both the V3 loop, which defines coreceptor specificity(12, 14, 37, 38), and the conserved surface, which mediatestight attachment to the coreceptor and the induction of conformationalchanges within the gp120 oligomer (38, 44, 64, 68). Onestriking aspect of the conserved coreceptor binding domain isits basic nature; seven basic amino acids are located within arelatively restricted surface on gp120_YU2 (64). We speculatedthat as a result of its positive charge and high degree of conservation,this surface might bind polyanions and be a potential target forattack by such molecules. Here we provide evidence, obtained byMAb inhibition studies and labeled-heparin binding and surfaceplasmon resonance (SPR) analyses, that the conserved coreceptorbinding surface in association with the V3 loop on X4 and R5X4gp120, but not R5 gp120, binds polyanions. Based on these dataand a molecular model of the electrostatic potential on this surfaceof gp120, we propose that HSPG binding probably takes place initiallyvia a selective and high-affinity interaction with the gp120 V3loop followed by a second, lower-affinity interaction with theconserved coreceptor binding surface. These interactions may haveimplications for HIV tropism and replication in vitro and in vivoand may allow for the development of inhibitors with therapeuticpotential.

	MATERIALS AND METHODS

Top Abstract Introduction Materials and Methods Results Discussion References

Antisera, MAbs, and recombinant proteins. The anti-CD4 mouse MAb Q4120 (from H. Holmes and the MRC AIDS Reagent Project, Potters Bar, United Kingdom), which was previouslymapped to the first domain of CD4, competes with gp120 for CD4binding (35). Pooled HIV immune immunoglobulin (61) was obtainedfrom the AIDS Reagent Repository, National Institutes of Health(NIH), Bethesda, Md. The following HIV-1 gp120-specific MAbs ofhuman origin were used (their specificities are in parentheses):21h (CD4 binding site [CD4bs]), 19b (V3 loop) (53), 17b, and48d (CD4i epitope) (77) were from J. Robinson (University ofConnecticut), and 447-52D (V3 loop) (15, 31) was purchasedfrom Cellular Products Inc., Buffalo, N.Y. The chimpanzee anti-gp120-V2MAb C108G, prepared as previously described (86), was obtainedfrom S. Tilley, Public Health Research Institute, New York, N.Y.The anti-CD4bs (IgG1b12) (7) and anti-V3 loop (Loop 2) (18)monospecific antibodies were from D. Burton, Scripps ResearchInstitute, La Jolla, Calif. The human anti-gp120 MAb 2G12 (79,80) was from A. Trkola, Aaron Diamond AIDS Research Center,New York, N.Y. Murine MAb G3-136 (V2 specific) was from TannoxBiosystems Inc., Houston, Tex. and D. D. Ho (Aaron Diamond AIDSResearch Center), SC258 was from Abbott Laboratories, 9284 (V3specific) was from NEN Life Science Products (Le Blanc Mesnil,France), and 110.I (V3 specific) was from F. Traincard, InstitutPasteur, Paris, France. The D7324 antibody, specific for a conservedregion of the gp120 COOH terminus, was obtained from Aalto Bioreagents,Dublin, Ireland. Recombinant soluble CD4 (sCD4) prepared in Chinesehamster ovary (CHO) cells was prepared by R. Sweet, SmithKlineand Beecham (King of Prussia, Pa.) (16) and was obtained fromthe NIH AIDS Reagent Repository. Recombinant soluble gp120 (sgp120)IIIB (BH10), HxBc2, and MN were derived from X4 TCLA viruses,SF-2 is from an R5X4 TCLA virus, 89.6 and W61D are from R5X4 PIviruses, and Bal and JRFL are from R5 PI viruses (19). IIIB,MN, W61D, and SF2 were obtained from the MRC AIDS Reagent Project,and Bal was from R. Sweet, SmithKline and Beecham. The V3-deletedform of JRFL was prepared as previously described (78). Wild-type(WT) gp120_HXBc2 was derived from the IIIB X4 TCLA isolate of HIV-1,and mutants in which the COOH and NH₂ termini and the V1/V2 andV3 loops were deleted were prepared as previously described (89,91). sgp120 was prepared either from purified CHO cell supernatants(IIIB, SF-2, JRFL, and JRFL $Delta$ V3) or from Drosophila cells (MN,Bal, 89.6, HXBc2, and mutantsthereof).

Polyanion inhibition of MAb binding to monomeric gp120 detected by ELISA. DexS, dextran, chondroitin sulfate, heparin, pentosan sulfate (PS), and aurintricarboxylic acid (ATA) were obtained from Sigma-Aldrich(Saint Quentin Fallavier, France). The interaction between monomericrecombinant sgp120 and polyanions was measured by a sandwich enzyme-linkedimmunosorbent assay (ELISA). Ninety-six-well Maxisorp ELISA plates(Nunc; Polylabo, Strasbourg-Meinau, France) were coated overnightat 4°C with 50 µl of a 5-µg/ml solution of D7324 in carbonatebuffer (pH 8.5). Plates were washed twice in 25 mM Tris-HCl (pH8.0)-150 mM NaCl-0.05% Tween 20 (ELISA buffer [EB]), then saturatedwith 2% bovine serum albumin (BSA) in phosphate-buffered saline(PBS) for 1 h at room temperature (RT). After two washes withEB, sgp120 was captured for 3 h at RT. Plates were washed sixtimes and then incubated with 50 µl of one of the polyanions,at various concentrations, in PBS-2% BSA for 30 min at RT. EitherMAbs were added directly to the mixture or, in some experiments,the plates were washed twice before MAb addition. After incubationof plates for 1 h at RT followed by six washes, bound MAbs weredetected with either peroxidase-conjugated goat anti-mouse immunoglobulinG (IgG) (1/2,500; Immunotech, Marseille, France) or peroxidase-conjugatedgoat anti-human IgG (1/5,000) in PBS-2% BSA by incubation for1 h at RT. Detection was carried out with a Sigma Fast o-phenylenediaminedihydrochloride kit from Sigma-Aldrich in accordance with thesupplier's recommendations. For detection of polyanion inhibitionof MAb binding to gp120 complexed with sCD4, two methods wereused. In the first assay format, gp120 captured onto ELISA platesas described above was incubated with a 1-µg/ml solution of sCD4for 1 h at RT, and then the plates were washed before MAbs wereadded as in the original assay. In the second assay format, ELISAplates were coated with the anti-CD4 MAb L120 overnight at 4°C,then blocked with PBS-2% BSA for 1 h at RT. After two washes ofthe plates with EB, sCD4 was added at 1 µg/ml and the plates wereincubated for 3 h at RT. The plates were washed six times in EB,then incubated with sgp120 at 1 µg/ml for 3 h at RT. Followingsix washes of the plates with EB, polyanion diluted in PBS-2%BSA was added at various concentrations and the plates were incubatedfor 30 min at RT. MAbs were added, and the plates were incubatedfor 1 h at RT before detection of binding as describedabove.

Polyanion inhibition of MAb binding to HIV-1-infected cells. The T-cell line H9, obtained from M. Popovic and R. Gallo and supplied by the MRC AIDS Reagent Project, was grown in RPMI1640 supplemented with 10% fetal calf serum (FCS), H9 cells wereinfected with either the HIV-1 TCLA X4 molecular clone HX10 (obtainedfrom B. Hahn, University of Alabama $---$ Birmingham and A. Fisher,Royal Post Graduate Medical School, Hammersmith Hospital, London,United Kingdom) (25) or the HIV-1 TCLA X4 MN isolate (obtainedfrom R. Gallo via the NIH AIDS Repository) for 8 to 10 days. Atthis time postinfection there was no detectable CD4 remainingat the cell surface or syncytium formation in the culture, butstrong Env expression was detected using gp120-specific MAbs andflow cytometry (see below). The interaction of the polyanionswith the infected cells was detected indirectly by measuring inhibitionof MAb binding to cell surface Env. Infected H9 cells (4 × 10⁵) were washed with PBS-1% FCS-0.02% sodium azide (wash buffer[WB]) and resuspended in 50 µl of WB containing polyanions atthe appropriate concentration. After a 2-h incubation at 37°C,the cells were washed twice in WB and then incubated with MAbs.After a 1-h incubation with agitation at 4°C, the cells were washedtwice in WB and fixed overnight with 0.5% formaldehyde at 4°C.The cells were washed twice, and then a goat anti-human IgG-phycoerythrinconjugate (Immunotech) was added at a 1/100 dilution in WB. Aftera further 1-h incubation at 4°C with agitation, the cells werewashed twice, resuspended in 200 µl of WB, and analyzed by single-colorflow cytometry with a FACScan (Becton Dickinson, San Diego, Calif.)equipped with Lysis II software. Each datum point represents theacquisition of 10,000 events gated on side and forward light scatterand is the mean of data from triplicatesamples.

DexS inhibition of gp120-CXCR4 interactions. The assay used to measure DexS inhibition of gp120-CXCR4 interactions was a modified version of a previously described method(50, 84). Briefly, sgp120 at 30 µg/ml that had or had notbeen preincubated with various concentrations of DexS for 30 minat RT was incubated with 10⁶ A3.01 cells (obtained from T. Folks, Centers for Disease Controland Prevention, Atlanta, Ga.) in a total volume of 50 µl for 1h at 37°C with agitation. Each sample was divided into five aliquots,one of which was incubated directly with Q4120 (2 µg/ml) and three(replicates) of which were incubated with 12G5 (5 µg/ml) in atotal volume of 50 µl for 1 h at 4°C with agitation. The fifthaliquot was washed twice in WB and incubated with either HIV immuneimmunoglobulin (100 µg/ml) or MAb 2G12 (10 µg/ml) for direct detectionof gp120 bound at the cell surface. The cells were subsequentlywashed in WB, and bound MAb was labeled with phycoerythrin-conjugatedgoat anti-mouse IgG (Immunotech) at a 1/200 dilution or a goatanti-human IgG-phycoerythrin conjugate (Immunotech) at a 1/100dilution for 1 h at 4°C with agitation. After the cells were washedin WB, bound antibody was detected by flow cytometric analysisas described above. Percent inhibition of Q4120 and 12G5 bindingwas calculated by using the equation 100 $-$ [(t $-$ c)/(m $-$ c) ×100], where t represents the signal for the test sample, c representsbackground staining in the absence of MAb, and m represents stainingin the absence of inhibitor (gp120). Percent reduction of inhibitionof 12G5 binding was calculated by taking the maximum inhibitionof 12G5 binding in the presence of sgp120 as 0% and no inhibitionof 12G5 binding in the absence of sgp120 as 100%. The absenceof a direct effect of DexS on the binding of MAbs Q4120 and 12G5was determined without sgp120, and, similarly, no effect of DexSon 2G12 binding to gp120 wasobserved.

DexS inhibition of HIV-1 infectivity. HIV-1 clones HXBc2 (TCLA X4) and JRCSF (PI R5) were obtained from J. Moore, Aaron Diamond AIDS Research Center, and the NIHAIDS Research and Reference Reagents Program, Bethesda, Md., respectively.Infectious stocks of these viruses were prepared by infectingperipheral blood lymphocytes (PBL) previously activated for 3days with phytohemagglutinin at 1 µg/ml and cultured in RPMI 1640supplemented with 10% heat-inactivated FCS and 40 IU of interleukin-2(growth medium [GM]). Approximately 100 50% tissue culture infectivedoses of each virus was preincubated with various concentrationsof DexS, in a total volume of 100 µl, for 1 h at 37°C in a U-bottomed96-well plate (Nunc). PBL at 5 × 10⁴/well in 100 µl of GM were added to the virus-DexS mixture, whichwas then incubated for a further 2 h at 37°C with agitation. Thecells were washed and resuspended in GM at 200 µl/well. After7 days of culture, during which the cells were maintained at 1× 10⁶ to 2 × 10⁶/ml, 100 µl of supernatant was harvested from each well and testedfor cell-free p24 activity as previously described (51). Resultsare expressed as medians of data for three replicate wells ± 1standard deviation. Chondroitin sulfate and dextran, used as negativecontrols, consistently failed to reduce infectivity of eithervirus at the same concentrations as those at which DexS was used(results notshown).

Binding of [³⁵S]heparin to gp120. To measure binding of ³⁵S-labeled heparin to gp120, we used a technique adapted from one described in reference 33. Briefly,³⁵S-labeled heparin (40 µg/ml, corresponding to approximately 6µCi) (Amersham Ltd., Little Chalfont, United Kingdom) was incubatedovernight at RT with WT sgp120, mutated forms thereof, or sgp120precomplexed for 1 h at RT with a fivefold molar excess of MAbin 25 mM Tris-HCl buffer, pH 7.5, at various concentrations intotal volumes of 90 µl. Three 30-µl aliquots of each incubationmixture were filtered through a reinforced nitrocellulose membranefilter (0.2-µm pore size; Cellulosensitrat BA 83; Schleicher andSchuell, Dassel, Germany) by using a 96-well micromanifold (Andermanand Co., Kingston, United Kingdom). The wells were washed twicein Tris-HCl buffer, and the filtered areas were excised and individuallyplaced in scintillation vials containing 200 µl of 2 M NaCl. Thevials were shaken for 1 h before addition of 4 ml of scintillationfluid (Ecoscint; Packard, Meriden, Conn.). ³⁵S radioactivity was then measured on a Beckman LS 6500 scintillationcounter. In some experiments, the specificity of the interactionwas determined by preincubation of the sgp120 with an excess ofunlabeled heparin prior to addition of the [³⁵S]heparin. Negative controls measured [³⁵S]heparin binding to the filter in the absence of any proteinor in the presence of MAbs such as 48d; similar levels of bindingwere obtained in bothcases.

Kinetic analysis of gp120-heparin interactions by SPR. Size-fractionated, biotinylated heparin was immobilized onto a streptavidin-coated Biacore B1 sensor chip at densities yielding65, 35 or 20 resonance units (RU) to determine the optimal concentrationfor sgp120 binding. WT or mutant sgp120 in Tris-buffered salinewas reacted with the sensor chip at flow rates of 5 to 15 µl/min.These initial studies demonstrated that a maximum density of 20to 25 RU of heparin was required to give a detectable signal butavoid the mass transport effect, and these densities were usedfor all subsequent kinetic studies. In a typical analysis, severalconcentrations of gp120 (see legend to Fig. 6) were injected ontothe heparin-coated surface at a flow rate of 15 µl/min for 6 min,after which the complexes were rinsed with buffer to analyze thedissociation phase. In other studies, the association phase wasallowed to proceed to equilibrium, which took 20 min. Subsequently,the heparin surface was regenerated with a 6-min pulse of Tris-bufferedsaline containing 1.0 M NaCl. Sets of sensorgrams were analyzedby global fitting of the data, using BIAevaluation 3.0software.

Electrostatic modeling of the gp120 trimer. To analyze the influence of V3 loop charge on the overall electrostatic potential of the conserved coreceptor binding surface,we carried out modeling, as described in reference 45, basedon the HXBc2 crystal structure of the monomeric gp120 core (44),in which optimization of quantifiable surface parameters was usedto model precisely the gp120 core structure. Variations in thestructure of the V3 loop were found to have little influence onthe contribution of the V3 electrostatic component to the overallelectrostatic potential (45). The models used here comprisea composite model of the MN V3 loop nuclear magnetic resonancestructure (9) grafted onto the HXBc2 gp120 core X-ray structure(44). For the gp120s derived from the HXBc2, 89.6, MN, and JRFLisolates, homology modeling was carried out by using the programPrISM (A.-S. Yang and B. Honig, Columbia University, unpublisheddata), thus adapting the initial composite model to the correctsequence for each gp120. Because of the large sizes of the trimericmodels, the electrostatic potentials were calculated with theprogram Delphi (55), using a 129-division grid, which correspondsto 1.2 Å per grid segment. Although small local deviations canbe observed as a result of the grid approximation used in thecalculation of the potential, the overall calculation is highlyaccurate (39).

	RESULTS

Top Abstract Introduction Materials and Methods Results Discussion References

Polyanions selectively inhibit binding of MAbs to the gp120 V3 loop and the CD4i epitopes. Previous studies have demonstrated that polyanions inhibit binding of MAbs to the V3 loop of TCLA X4 gp120. To investigatewhether polyanions are also able to interact with other regionsof gp120, we tested the ability of DexS, a well-characterizedpolyanion with relatively potent gp120 V3 loop binding activity,to interfere with the binding of a panel of gp120-specific MAbsin an ELISA. We initially chose to study gp120 derived from thefollowing viruses: MN, an X4 TCLA HIV-1 isolate, and JRFL, anR5 clone. Four MAbs that are known to react with both gp120s wereselected: 447-52D (specific for V3), IgG1b12 (specific for theCD4bs), and 17b and 48d (specific for CD4i). As shown in Fig.1, DexS at 12.3 µM, a dose previously demonstrated to inhibitsubstantially TCLA HIV-1 infectivity (see Fig. 4), reduced thebinding of MAbs 17b and 48d to gp120_MN by approximately 10- and30-fold, respectively, as determined by measuring the displacementof the antibody binding curves, but had only a very weak effecton their binding to gp120_JRFL. The binding of MAbs IgG1b12 and447-52D to both gp120s was unaffected by DexS, confirming dataof a previous study (65) demonstrating that the CD4bs and certainV3 loop epitopes are unaffected or only weakly affected by polyanions.To further dissect the effect of polyanions on MAb binding togp120, we tested the ability of DexS to interfere with the bindingof a number of MAbs to different epitopes on gp120_IIIB (TCLA X4)and gp120_JRFL. These MAbs were chosen because they bind neutralizingepitopes on monomeric gp120 that are well exposed on the virion-associatedtrimeric form of gp120 (52, 69). As shown in Table 1, substantialreductions in half-maximal (50%) MAb binding to IIIB gp120 wereseen for the V3 loop MAbs 9284 and 110.I (5- and 100-fold reductions,respectively) and the two CD4i MAbs 17b and 48d (50- and 37-fold,respectively). Moderate (8.6-fold) inhibition was observed forthe V2-specific MAb C108G, whereas inhibition of MAbs specificfor the CD4bs and the 2G12 epitopes was weak or absent. By contrast,little inhibition of binding of any MAb was observed for JRFL:only the V3 loop-specific MAb Loop 2 and the CD4i-specific MAbs17b and 48b demonstrated reductions in 50% binding (3.0, 1.8,and 2.4-fold, respectively). We evaluated the ability of DexSto interfere with binding of 17b and 48d to gp120 molecules withdifferent viral origins and coreceptor usages: gp120 BH10; MN(TCLA X4), SF2 (TCLA R5X4), 89.6, and W61D (PI R5X4); and JRFLand Bal (PI R5). DexS potently inhibited binding of 48d and 17bto gp120 BH10 (IIIB), MN, SF-2, 89.6, and W61D but had littleor no effect on IgG1b12 binding (Table 2). By contrast, DexShad more subtle effects on MAb binding to the R5 gp120 molecules.Inhibition of 48d and 17b binding to JRFL was very weak (maximum,2.4-fold), whereas inhibition of binding of the same MAbs to Balgp120 was intermediate (5- to 6-fold). Finally, we tested theabilities of other polyanions to interfere with the binding of17b and 48d to gp120. ATA, PS, and heparin are all anionic andhave been previously demonstrated to reduce HIV infectivity, whereasdextran (uncharged) and chondroitin sulfate (weakly anionic) donot. The spectrum of potency observed for inhibition of 17b bindingby the different polyanions was ATA > DexS > PS, with dextranand chondroitin sulfate failing to interfere with the bindingof any MAb (results not shown).

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FIG. 1. DexS inhibition of MAb binding to the conserved coreceptor binding site. Monomeric recombinant sgp120 derived from the MN or JRFL strain of HIV-1 was captured on the solid phase by an antibody to the conserved COOH terminus, then preincubated without ( $-$ ) or with (+) 12.3 µM DexS prior to addition of sequential dilutions of gp120 antibodies specific for the CD4bs (IgG1b12) (A), the V3 loop (447-52D) (B), and the CD4i epitopes 17b (C) and 48d (D). Detection of bound MAb was carried out by ELISA, and the results are presented as optical densities at 450 nm. Each datum point is the mean of values obtained from triplicate samples, and each experiment was repeated on at least three separate occasions.

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TABLE 1. DexS inhibition of MAb binding to gp120

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TABLE 2. DexS inhibition of MAb binding to gp120 molecules of different origins

Influence of sCD4 binding on DexS inhibition of CD4i-specific MAbs. To investigate whether the inability of polyanions to interfere with binding of 17b and 48d to gp120_JRFL was a result of maskingby the variable loops or an inappropriate conformation of theconserved coreceptor binding region in the absence of CD4, weattempted to inhibit the binding of these MAbs after sCD4 wascomplexed with gp120. The gp120_MN-sCD4 complex bound 17b, 48d,and a third CD4i-specific MAb, CG10, with higher affinity thandid MN gp120 alone, confirming the CD4-induced nature of theseepitopes (Table 3). By contrast, no significant alteration ofthe V3 loop-specific MAb 447-52D was observed, in accordance withthe constitutively well-exposed nature of this epitope. The additionof DexS at 12.3 µM reduced 48d binding similarly regardless ofwhether sCD4 was complexed (without sCD4 there was a 50-fold reduction,and with sCD4 there was a 43-fold reduction), whereas 17b bindingwas inhibited by approximately 4-fold more in the presence ofsCD4 (without sCD4 there was a 20-fold reduction, while with sCD4there was an 80-fold reduction). Thus, sCD4 appears to selectivelyincrease the accessibility of the polyanion binding site on MNgp120. Since CG10 is unable to react with gp120 in the absenceof CD4, we were unable to determine polyanion inhibition of thisMAb under these conditions. However, the potent inhibition ofCG10 binding to the CD4-gp120 complex is consistent with the dataobtained for 17b and 48d. The binding of CD4i-specific MAbs togp120_JRFL was increased from approximately 10-fold (17b) to >100-fold(CG10) in the presence of sCD4. However, the increased bindingof the CD4i-specific MAbs had little impact on the ability ofDexS to interfere with MAb binding to gp120_JRFL; no significantinhibition of binding of any of the CD4i-specific MAbs was observedunder any conditions. The inability of sCD4 complexing to facilitatethe binding of DexS to the conserved coreceptor binding site ongp120_JRFL implies that the lack of association is constitutiverather than conformational or cryptic.

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TABLE 3. Effect of sCD4 treatment on DexS inhibition of MAb binding

Polyanions inhibit the binding of MAbs 17b and 48d to oligomeric, functional X4 gp120. Soluble, monomeric gp120 is a useful tool for analyzing a variety of interactions but does not fully represent the behaviorof the oligomeric, functional form of the glycoprotein. We thereforeattempted to establish whether the binding of polyanions to oligomeric,mature X4 gp120 interfered with the binding of MAbs to the CD4iepitope. For this we used H9 cells infected with the HIV-1_MN isolate.Different MAbs were titrated onto cells that had or had not beenpretreated with DexS or ATA. As can be seen in Fig. 2, low concentrationsof DexS (<100 nM) inhibited the binding of 17b and 48d to thecells by >50%. Interestingly, the CD4bs-specific MAb IgG1b12 wasalso partially inhibited by DexS, suggesting the occurrence ofeither polyanion interference with the CD4bs on oligomeric asopposed to monomeric gp120 or DexS-induced dissociation of gp120from gp41 as has been previously reported (6). The latter explanationseems unlikely to account entirely for the IgG1b12 inhibition,however, since 447-52D binding was only weakly inhibited by DexSat all concentrations tested whereas gp120 dissociation wouldaffect both epitopes in the same way. ATA was also a potent inhibitorof 17b binding but had little effect on IgG1b12 binding at theconcentrations used (Fig. 2B). Since ATA does not induce significantgp120 dissociation (unpublished results), this result is consistentwith a direct effect of anionic compounds on MAb binding to CD4iepitopes. Levels of CD4i and CD4bs MAb inhibition similar to thoseobtained in this experiment were observed for cells infected withHIV-1_HX10 (results not shown).

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FIG. 2. Inhibition of MAb binding to oligomeric Env expressed on the surface of HIV-1_MN-infected cells. Cells were preincubated with various concentrations of DexS (A) or ATA (B) before being washed, and gp120-specific MAbs were added. Bound MAb was detected by indirect immunofluorescence and flow cytometry, and the results are expressed as percent inhibition of MAb binding relative to the positive (no inhibitor) and negative (no MAb) controls. Each datum point is the mean of values for triplicate samples.

DexS interferes with gp120-CXCR4 interactions. We showed previously that the binding of TCLA X4 gp120 to CD4⁺ CXCR4⁺ cells inhibited the binding of the CXCR4-specific MAb 12G5, demonstratinga CD4-dependent interaction between gp120 and CXCR4 (49, 84).The observation that DexS could associate with the V3 loop andconserved chemokine binding surface of gp120 implied that polyanionswould interfere with gp120-coreceptor interactions. To test this,we attempted to block the inhibition of CXCR4-specific MAb bindingby sgp120 at the surface of CD4⁺ CXCR4⁺ cells by pretreating the sgp120 with polyanions prior to incubationwith the cells. The attachment of sgp120 to CD4 was monitoredindirectly by measuring the inhibition of binding of a CD4 MAb(Q4120) that competes with gp120 for CD4 binding (49, 84).Incubation of the cells with gp120_MN inhibited 12G5 binding byapproximately 35% (data not shown). Increasing concentrationsof DexS reduced the inhibition of CXCR4 MAb 12G5 binding to thecells to a maximum of about 80% at 6.6 µM, suggesting that thepolyanion was interfering with the gp120-CXCR4 interaction (Fig.3A). We excluded the possibility of any effects of DexS on thebinding of gp120 to CD4 by demonstrating that Q4120 inhibitionwas essentially complete at all concentrations of DexS used, andwe eliminated the possibility that DexS inhibited the bindingof 12G5 or Q4120 to CXCR4 and CD4, respectively, by preincubatingthe cells and MAbs directly with DexS in the absence of gp120(Fig. 3B).

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FIG. 3. DexS inhibition of gp120-CXCR4 interactions. (A) A3.01 (CD4⁺ CXCR4⁺) T cells were preincubated with various concentrations of DexS prior to the addition of HIV-1_MN gp120. The CXCR4-specific MAb 12G5 or the CD4-specific MAb Q4120 was subsequently added. (B) A3.01 cells were preincubated with DexS prior to addition of MAb 12G5 or Q4120. Bound MAb was detected by indirect immunofluorescence and flow cytometry, and the results are expressed as percent inhibition of MAb binding relative to the positive (no inhibitor) and negative (no MAb) controls. Each datum point is the mean of values obtained from triplicate samples.

Selective inhibition of X4 virus infectivity by DexS. To determine whether the ability of polyanions to selectively bind basic gp120 molecules correlated with inhibition of viralinfectivity, we tested the effect of DexS on the infection ofactivated PBL by HIV-1_HXBc2 (X4 TCLA) and HIV-1_JRCSF (R5 PI).Equivalent infectious doses of each virus were preincubated withvarious concentrations of DexS and then incubated with phytohemagglutinin-activatedPBL for 2 h. The cells were subsequently washed thoroughly, toprevent inhibition of viral infectivity at steps subsequent tovirus binding and entry, and cultured for 7 days. Infectivitywas assayed by detection of cell-free HIV-1 p24. Figure 4 showsthat the HXBc2 titer was reduced in a dose-dependent manner from0.66 ng/ml in the absence of DexS to 0.15 ng/ml in the presenceof 37.5 nM DexS (a 77% reduction in infectivity), whereas thetiter of JRCSF remained constant, at about 0.7 ng/ml, regardlessof the presence of DexS. Thus, X4 HIV-1 appears to be considerablymore susceptible to DexS inhibition than is R5 HIV-1, coordinatewith the results of polyanion binding to gp120 (see below).

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FIG. 4. Inhibition of HIV-1 infectivity by DexS. HIV-1_HXBc2 and HIV-1_JRCSF were preincubated for 1 h at 37°C with the concentrations of DexS shown, then added to activated PBL for a further 1 h. After being washed, the cells were cultured for 7 days, and then the production of virus was measured by detection of cell-free viral p24 in the supernatant. The results, expressed as picograms of p24 per milliliter, were calculated from the optical densities at 492 nm. Each bar represents the mean of values for three replicate wells, and the error bars indicate ± 1 standard deviation.

Binding of [³⁵S]heparin to WT and mutated forms of sgp120. The inhibition of CD4i-specific MAb binding to sgp120 by polyanions may be the result of direct competition for MAb bindingto the epitope cluster or of indirect effects, such as stericinhibition resulting from polyanion attachment to the V3 loopor polyanion-induced conformational changes in the MAb epitopes.In an attempt to discriminate between these different possibilities,we measured the binding of ³⁵S-labeled heparin to WT and mutated forms of sgp120 lacking theV3 loop. Initial experiments established that [³⁵S]heparin bound X4 sgp120 in a dose-dependent and saturable mannerand that unlabeled heparin could efficiently compete with thelabeled heparin for binding sites (results not shown). Incubationof WT HXBc2 with [³⁵S]heparin under the above-described conditions resulted in a signal-to-noiseratio of about 40-fold (Fig. 5A). Deletion of the V3 loop resultedin a dramatic decrease in heparin binding (~12-fold). By contrast,gp120_JRFLbound [³⁵S]heparin only weakly (about twice the background level), anddeletion of the V3 loop resulted in a reduction of [³⁵S]heparin binding to close to background levels. These data suggestthat the V3 loop of X4 gp120 is an important determinant of polyanionbinding but imply that other regions also contribute, albeit toa lesser extent. To address which other regions of X4 gp120 mightbe implicated in polyanion binding, we tested gp120_HXBc2 moleculeswith more-substantial deletions and attempted to inhibit [³⁵S]heparin binding with MAb 48d, which is specific for the CD4iepitope. In this experiment, the level of [³⁵S]heparin binding to WT gp120_HXBc2 was about ninefold higher thanthe background (Fig. 5B). Preincubation of WT gp120_HXBc2 with48d resulted in a modest but significant decrease in [³⁵S]heparin binding. Deletion of the NH₂ and COOH termini and theV1/V2 loop structure (HXBc2_82C5V1V2) resulted ina similarly small decrease in [³⁵S]heparin binding, and preincubation of this mutant with MAb 48dreduced the signal further. An additional deletion of the V3 loop(HXBc2_82C5V1V2V3) dramatically reduced [³⁵S]heparin binding, and preincubation of this mutant with 48d furtherreduced binding to background levels. These data suggest thatthe COOH and NH₂ termini and the V1/V2 loops of HXBc2 gp120 contributeminimally to the attachment of polyanions whereas the V3 loopis the major determinant. Moreover, the inhibition by MAb 48dof [³⁵S]heparin binding to all three forms of gp120 (WT, HXBc2_82C5V1V2,and HXBc2_82C5V1V2V3) is consistent with [³⁵S]heparin interaction with the conserved chemokine receptor bindingsurface.

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FIG. 5. Direct binding of [³⁵S]heparin to immobilized gp120. gp120 and mutated forms thereof were incubated with [³⁵S]heparin before being blotted onto a nitrocellulose membrane. The radioactivity in bound material was determined with a scintillation counter, and results are expressed as counts per minute. (A) Binding of [³⁵S]heparin to 400 nM gp120_HXBc2, gp120_JRFL, and V3 loop deletion mutants thereof. (B) Binding of [³⁵S]heparin to 170 nM gp120_HXBc2, and mutants thereof, precomplexed (or not) with a molar excess of MAb 48d. The background value for [³⁵S]heparin represents binding to the filter in the absence of protein. Each bar represent the mean of values for triplicate samples, and the error bars represent ± 1 standard deviation.

Analysis of the gp120-heparin interaction by SPR. The results obtained in the labeled heparin binding studies suggest that the affinity of heparin for monomeric sgp120 dependson the conservation of the V3 loop and is strongly influencedby the V3 loop charge. However, the binding of soluble polyanionsto sgp120 in solution is a poor imitation of the physiologicalinteraction between cell membrane-anchored HSPG and gp120. Thus,we adopted a more physiologically relevant system in which heparinis coupled to the solid phase and sgp120 binding is analyzed bySPR. Not only does this system better represent HSPG presentationat the cell surface, but the multimerization of the heparin-bindingsites may increase the avidity for sgp120 if binding occurs atmore than one site. Injection of a range of concentrations (upto 45 nM) of X4 sgp120_HXBc2 over a sensor chip coated with nomore than 20 to 25 RU of size-fractionated heparin gave typicalsensorgrams (Fig. 6A). Higher densities of heparin were not usedon the sensor chip because they gave rise to a mass transporteffect that precluded precise kinetic analyses. Preliminary evaluationof the sensorgrams by linear transformation of the primary dataindicated that the binding was complex and did not follow singleexponential curves. Kinetic analyses were therefore performedby numerical integration, which allows fitting of the data tocomplex interaction models. Simultaneous fitting to all curves(including both association and dissociation phases), a procedurewhich improves the robustness of the fitting procedure (54),was carried out by using the Biaeval 3.0 software. Our data couldnot be fitted to single one-to-one binding as indicated above,and such a model returned a $chi$ ² value (which describes the closeness of the fit) of 4.25. Thereare several possible explanations for a value of this magnitude(some of which are inherent to the technology itself [43]),but it is likely that this reflects the existence of a complexbinding process (see below). To analyze the gp120-heparin interactionin more detail, we generated data under conditions in which theassociation phase was allowed to proceed to equilibrium. Equilibriumwas reached after 20 min (data not shown), and these data wereanalyzed to provide an affinity value independently of the kineticaspect of the binding (Fig. 6B). The overall equilibrium constantwas 220 nM, a value considerably lower than the K_d (10 nM) previouslydetermined by direct binding of [³⁵S]heparin to MN gp120 (33). However, these previously performedexperiments were carried out in the absence of salt, whereas allof our binding buffers contained a physiological concentrationof NaCl (0.15 M), an important point for electrostatic-based interactions(heparin-gp120 binding is completely inhibited by 1 M NaCl, andthis concentration was used to regenerate the chip after eachgp120 injection). The stochiometry of the binding indicated thaton average, 4.4 gp120 molecules bind each heparin chain.

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FIG. 6. SPR analysis of X4-derived gp120-heparin interactions: overlay of sensorgrams showing binding of WT and mutated forms of gp120_HXBc2 to immobilized heparin. sgp120 (used at concentrations of [from top to bottom] 45, 30, 22.5, 15, and 11.5 nM) was injected for 6 min over a heparin-activated surface at a flow rate of 15 µl/min to analyze the association phase, after which running buffer alone was injected to analyze the dissociation phase. (A) Binding curves for wild-type gp120_HXBc2. (B) Scatchard plot of the equilibrium binding data directly measured on the sensorgrams after a 25-min period of interaction. (C) Binding curves for gp120_HXBc2, alone or preincubated with a 10-fold molar excess of MAb 50-23, 48d, or both (from top to bottom). (D) Maximum responses measured at the end of the association phases shown in panel C. (E and F) Binding curves for gp120_{HXBc282C5V1V2} (E) and gp120_{HXBc282C5V1V2V3} (F) injected at (from top to bottom) 90, 60, 45, and 30 nM over the heparin surface.

In view of the data presented above (Fig. 1, 2, and 4) which suggest the existence of two distinct heparin binding domainswithin the gp120 molecule (the V3 loop and the CD4i region), weinvestigated the possibility that our data could be describedby a more complex binding model such as the bivalent analyte model.Using this model, the fitting procedure returned a $chi$ ² value of 1.5, demonstrating that this model described our datawell. The first gp120-heparin binding event was thus characterizedby a relatively high on rate, k_on1 = 2.7 × 10⁵ M¹ s¹, and by a rapid dissociation rate constant, k_off1 = 0.147 s¹, resulting in an affinity of K_d = k_off1/k_on1 = 550 nM. A secondbinding event, whose dissociation constant, k_off2, was 1.58 ×10³ s¹, further stabilized the complex, yielding the observed affinity.To add support to the existence of two heparin binding sites ongp120, we investigated the effect of prebinding MAbs to sgp120before reaction with immobilized heparin. In this assay, 45 nmolof gp120 was preincubated with 450 nmol of MAb 50-23 (V3 loop)or MAb 48d (CD4i), either alone or in combination, and then injectedover the heparin surface. The results (Fig. 6C) show that a complexmade up of gp120 and an anti-V3-loop MAb was still able to bindheparin, supporting the existence of a binding site outside ofthe 50-23 MAb epitope. Prebinding MAb 48d strongly inhibited thegp120-heparin interaction, consistent with the results obtainedin [³⁵S]heparin-gp120 binding studies (Fig. 5B). Finally, a complexof both MAbs with gp120 reduced the heparin-gp120 interactionto close to background levels. The total responses (in RU) atthe end of the injections are shown in Fig. 6D. The percentageinhibition caused by MAbs could not be ascertained because theSPR signal is sensitive to mass, and the responses were obtainedfrom different gp120-MAb complexes. However, it is clear froma visual inspection that occupation of both the V3 loop and theCD4i region is required to produce almost complete (>90%) inhibitionof gp120-heparinbinding.

The mutant gp120_HXBc2NCV1V2 gave binding curves different from those obtained with the intact molecule; theydid not fit any obvious model of ligand-receptor binding, probablyas a result of mass transport (Fig. 6E). Although we were unableto determine an affinity constant for this molecule, visual inspectionof the curves clearly reveals significant heparin binding. Themutant gp120_{HXBc2NCV1V2V3}, from which the V3 loophad been further deleted, did not show any significant heparinbinding activity under the conditions used (Fig. 6F), consistentwith the idea that the V3 loop is the primary high-affinity bindingsite on gp120. Increasing the density of heparin on the sensorchip resulted in detectable but weak gp120_{HXBc2NCV1V2V3}binding (results not shown), confirming weak polyanion bindingactivity in the absence of the V3 loop. We next used the samebinding assay to compare the heparin binding activities of twoR5X4-derived sgp120s, 89.6 and W61D. Results show that gp120_89.6(Fig. 7A), but not gp120_W61D (Fig. 7B), interacts significantlywith the low-density immobilized heparin. These data suggest thatthe V3 loop charge alone may not be sufficient to explain theheparin binding activity, since these two gp120s differ by onlyone unit of charge (89.6 = +7 and W61D = +6). It is likely thatthe other parameters, such as the conformation of the V3 loopand the charge of regions outside of the V3 loop, also influenceheparin binding. Finally, R5 gp120_JRFL, which was analyzed underthe same experimental conditions of low heparin density, did notshow significant binding activity (Fig. 7C), and deletion of theV3 loop did not obviously modify this activity (Fig. 7D). Weakbinding of R5 gp120_JRFL was detected when the protein was injectedover a higher-density immobilized heparin, consistent with a very-low-affinityinteraction (data not shown).

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FIG. 7. SPR analysis of R5X4- and R5-derived gp120-heparin interactions: overlay of sensorgrams showing binding of gp120 to immobilized heparin. (A and B) Binding curves for R5X4 gp120_89.6 (A) and R5X4 gp120_W61D (B) injected at (from top to bottom) 60, 45, 30, 22.5, and 15 nM. (C and D) Binding curves for wild-type R5 gp120_JRFL (C) and V3 loop-deleted gp120_JRFL (D) injected at (from top to bottom) 90, 60, 45, and 30 nM over the heparin surface. Binding conditions were similar to those described in the legend to Fig. 6. S, seconds.

Electrostatic potential of the conserved coreceptor binding surface and the V3 loop. To better understand the interactions taking place between gp120 and polyanions, we prepared models representing the electrostaticpotential on the chemokine receptor binding surface based on therecently published gp120 core structure. The gp120 cores weremodeled as a trimer in a companion paper (45) to give a betterindication of the overall charge on this surface, and the V3 loopsof gp120 molecules of various origins, modeled as described inthat paper (45), were superimposed on the gp120 core structureto illustrate the influence of this loop on the electrostaticpotential. Figure 8 shows models oriented with the coreceptorbinding surface facing out from the page. The top panel representsthe electrostatic potential of the gp120_{HXBc2NCV1V2V3}core. The coreceptor binding surface is weakly basic (basic isrepresented by blue, acidic is represented by red, and neutralis represented by white). Subtle differences are, however, evidentin the degree of positivity; the coreceptor binding surface onthe gp120 core of HXBc2 is slightly more basic than those of theother gp120s. The middle panel of Fig. 8 represents the electrostaticpotential on models of the V3 loops derived from primary env sequencesof the viruses MN (X4), HXBc2 (X4), 89.6 (R5X4), and JRFL (R5).The HXBc2, MN, and 89.6 V3 loops are highly basic (+9, +8, and+7 charge, respectively), whereas the JRFL V3 loop is relativelyweakly basic (+4). The lower panel of Fig. 8 illustrates the overallcharge of the coreceptor binding surface with the V3 loop modeledonto the gp120 core. It is clear from these models that the V3loop charge dominates the electrostatic potential. The spatialoverlap of the V3 loop and the conserved coreceptor binding surfaceobserved in the electrostatic model is consistent with the sulfatedchains of polyanionic molecules being able to bind both sites.

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FIG. 8. Modeling of the electrostatic potential for the coreceptor binding surface of the gp120 trimer. The molecular models of the gp120 trimer shown here are orientated with the trimer axis perpendicular to the page, showing the conserved surfaces of the HIV-1 clones HXBc2, MN, 89.6, and JRFL. The top panels show the gp120 core, the middle panels show the V3 loop, and the bottom panels show the V3 loop integrated into the gp120 core. These models are depicted in a C $alpha$ worm representation (left column) and an electrostatic surface representation (other four columns). The C $alpha$ worm representations for the different strains are essentially indistinguishable: the one corresponding to the HXBc2 sequence is shown with the core colored rust brown and the V3 loop colored green. The electrostatic potentials were calculated with the program Delphi and are depicted at the solvent-accessible surface, which is colored according to the local electrostatic potential, ranging from dark blue (most positive, corresponding to 10 kT/e) to red (most negative). The figure was prepared with the program GRASP (56).

	DISCUSSION

Top Abstract Introduction Materials and Methods Results Discussion References

In this study we have demonstrated by several different techniques that polyanions interact with the V3 loop and the newlycharacterized conserved coreceptor binding surface on gp120 ina manner dependent on viral origin and coreceptor usage. Thus,the monomeric X4 and R5X4 gp120 molecules tested here bind polyanionsstrongly whereas R5 gp120 binds polyanions relatively weakly (gp120_Bal)or not at all (gp120_JRFL). Most of this variation comes from changesin the charge and structure of the V3 loop, but variability inthe conserved coreceptor binding surface, which displays someinterisolate differences in electrostatic potential (Fig. 8 andresults not shown), may also influence polyanion binding. Thedata that we have obtained from kinetic and MAb inhibition studiesof gp120-heparin binding strongly suggest a phenomenon based onan initial high-affinity association via the V3 loop followedby weaker binding via a second site, most probably the conservedcoreceptor binding region. Although we do not have unequivocalevidence of a direct interaction between polyanions and the conservedcoreceptor binding surface, the data presented here provide astrong case for this. Thus, (i) polyanions potently inhibit theattachment of MAbs specific for the conserved coreceptor bindingsurface and regions of the V3 loop but, with the exception ofone V2 loop-specific MAb, have little or no effect on MAbs toother exposed regions of gp120; (ii) CD4i-specific and V3 loop-specificMAbs inhibit the heparin-gp120 interaction in an additive manner;(iii) heparin binds mutants of gp120 from which the NH₂ and COOHtermini and the variable loops V1, V2, and V3 have been deleted,and the CD4i MAb 48d interferes with the binding of heparin tothis mutant; and (iv) weak binding of heparin to gp120_HXBc2V3,gp120_JRFLV3, and gp120_{HXBc282C5V1V2V3} canbe observed under the appropriateconditions.

The molecular model of the electrostatic potential on the coreceptor-binding face of gp120 shows that the basic nature ofthe combined V3 loop-conserved coreceptor binding surface is dominatedby the V3 loop charge. Although the models presented here andin reference 45 are of low resolution, it is clear that relativelylong-chain sulfated polysaccharides such as heparin would be capableof spanning the V3 loop and the conserved coreceptor binding surface,which exhibit considerable spatial overlap. Moreover, severalmolecules of gp120 could bind a single heparin chain. V3 loopcharge and conformation (12, 14, 60, 73, 85), in associationwith the variable loops V1 and V2 (11, 46, 67, 72), determinecoreceptor usage and viral tropism in vitro. It seems likely,based on our current understanding of HIV-1 attachment to receptor-bearingcells, that polyanion binding to gp120 parallels, at least tosome extent, the interaction between gp120 and its coreceptors.Binding of gp120 to the appropriate coreceptor is thought to takeplace initially via the V3 loop, an interaction that determinescoreceptor-gp120 specificity (12, 14, 38, 92), followedby exposure and binding of the conserved coreceptor binding region(64, 78, 87). The importance of electrostatic interactionsin the gp120-coreceptor association is underscored by a seriesof studies that demonstrate a reduction in gp120-CCR5 bindingand coreceptor function in virus infectivity and fusion assaysfollowing substitution of acidic or potentially sulfated aminoacids in the amino terminus of CCR5 (21, 23, 24, 62).However, interactions other than those mediated by the chemokinereceptor NH₂ terminus are also required for virus fusion to befully activated, such as those based around the second extracellularloops of CCR5 (20) and CXCR4 (5).

There is no direct evidence for HIV-1 adaptation to HSPG use in vivo; the evolution of the V3 loop toward a more basic structureappears to come from adaptation to CXCR4 usage (70). However,adaptation of HIV-1 to replicate in T-cell lines in vitro maybe driven, at least in part, by increased interaction betweenthe V3 loop and cell surface HSPG, since human T-lymphotropicleukemia virus type 1-immortalized T-cell lines such as H9, MT-2,and c8166 that have been used routinely to isolate, propogate,and phenotype viruses from infected individuals express largeamounts of surface HSPG (57). Indeed, this may help to explainwhy viruses passaged only in primary cells such as activated CD4⁺ T cells and macrophages, which express only small amounts ofHSPG (40, 57, 58), do not have V3 loops with net positivecharges greater than +5 or +6 whereas viruses passaged in immortalizedcell lines that express high levels of HSPG frequently have verybasic V3 loops with net positive charges of +8 and +9 (28, 42).In the present study, analysis of X4 gp120 was carried out withTCLA virus-derived clones. Clearly, further studies of PI X4 virus-derivedsgp120 will have to be done as this becomes available. However,the finding that the R5X4 PI gp120 89.6 binds heparin impliesthat PI X4 virus sgp120 will have a similarphenotype.

Although HIV-1 may use HSPG as a low-affinity attachment receptor, allowing the virus to scan the cell surface for specificentry receptors (34, 83), the biological implications of gp120binding to HSPG are unclear, since the principal target cellsfor HIV-1 in vivo, CD4⁺ T cells and macrophages, have little HSPG on their surfaces.Nevertheless, even low levels of HSPG influence the efficiencyof viral attachment and therefore entry and so may have importantconsequences for infectivity and cellular tropism in vivo. A selectiveability of X4 and R5X4 viruses to attach to these cells via HSPGmay give these viruses an advantage over R5 viruses that are potentiallyless able to do so. Other cell types that carry large amountsof HSPG are endothelial and epithelial cells (50), and certaintissues, such as the liver, are very rich in HSPG expression (66).These cell and tissue types are considered to be nonpermissivefor HIV infection, but one potential consequence of HSPG expressionmay be the preferential trapping of X4 and R5X4 viruses onto theirsurfaces, leading to selective exhaustion of these viral phenotypesin vivo (83). Such a phenomenon may help to explain the preferentialtransmission and early dominance of R5 viruses over R5X4 and X4viruses invivo.

Our observation that polyanions bind recombinant, monomeric sgp120 was reproduced with oligomeric, gp41-associated forms ofX4 gp120 expressed on HIV-1-infected cells, suggesting that themonomeric form may represent to some extent the functional heterotrimericform of gp120. However, it is very likely that the trimeric formwill have a greater avidity for membrane HSPG complexes. Experimentalevidence supporting this comes from a study by Roderiquez et al.(65), who demonstrated that whereas no binding of monomericTCLA X4 gp120 to cell surface HSPG was detectable, oligomericTCLA X4 gp140 derived from the same isolate bound specifically.Thus, the 220 nM affinity constant observed for monomeric sgp120_HXBc2binding to immobilized heparin may be of high avidity when multipleinteractions of this type take place on the surface of a virion.This idea is consistent with the predicted occupation of fouror five molecules of gp120 by one heparin chain under our experimentalconditions. Moreover, although we observed only a weak associationbetween soluble or immobilized polyanions and monomeric R5 sgp120,the interaction with oligomeric gp120, either soluble or virionassociated, could be stronger, as predicted by the electrostaticproperties of the gp120 trimer. Future studies will need to addressthe kinetics of binding of oligomeric gp140 or whole virus particlesto immobilized heparin or membraneHSPG.

The use of polyanionic compounds such as DexS as anti-HIV therapeutic agents systemically has not had obvious success in clinicaltrials, since there has been no obvious benefit to the patients(1, 26), adsorption has been considered poor (47), andsome toxicity has been observed (26). However, other studiesare more optimistic with regard to the use of polyanionic compoundsas anti-HIV and antiviral therapeutic agents either systemically(30, 36) or locally (74). One reason for the failure ofthese molecules in vivo may be their weak neutralization activityfor R5 viruses (Fig. 4), the viral phenotype associated with HIV-1transmission and early infection. Another is that HIV variantsresistant to DexS inhibition are rapidly generated in vitro, suggestingthat similar events would occur in vivo (22). However, the findingthat the basic and highly conserved coreceptor binding regioninteracts with polyanions and the recent availability of the gp120core crystal structure may allow for novel strategies in the rationaldevelopment of small-molecule inhibitors of X4 and perhaps R5HIV-1 infection based on electrostatic interactions withgp120.

	ACKNOWLEDGMENTS

We thank H. Holmes and the MRC AIDS Reagent Repository for supplying reagents and D. Burton, J. Robinson, J. Gershoni, G.Denisova, and S. Zolla-Pazner for kind gifts of monoclonalantibodies.

This study was supported by the Centre National de la Recherche Scientifique, the Institut National de la Santé et la RechercheMédicale, the Agence Nationale de Recherches sur le SIDA, theFondation pour la Recherche Médicale (SIDACTION), and the EuropeanCommunity Biomed II shared cost action "Antibody Mediated Enhancementand Neutralization of Lentivirus Infections: Role in Immune Pathogenesisand Vaccine Development." P.D.K. was a recipient of a BurroughsWellcome career development award, and M.M. was the recipientof a Philipps FoundationFellowship.

	FOOTNOTES

^* Corresponding author. Present address: Imperial College of Science, Technology and Medicine, Jefferiss Research Trust Laboratories,Norfolk Pl., London W2 1PG, England. Phone: 44-171 886 1539. Fax:44-171 886 6645. E-mail: quentin.sattentau{at}pathology.oxford.ac.uk.

Present address: Department of Immunology, The Scripps Research Institute, La Jolla, CA92037.

REFERENCES

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References

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