A Second Target for the Peptoid Tat/Transactivation Response Element Inhibitor CGP64222: Inhibition of Human Immunodeficiency Virus Replication by Blocking CXC-Chemokine Receptor 4-Mediated Virus Entry

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Vol. 57, Issue 1, 116-124, January 2000

A Second Target for the Peptoid Tat/Transactivation Response Element Inhibitor CGP64222: Inhibition of Human Immunodeficiency Virus Replication by Blocking CXC-Chemokine Receptor 4-Mediated Virus Entry

Dirk Daelemans, Dominique Schols, Myriam Witvrouw, Christophe Pannecouque, Sigrid Hatse, Sonia van Dooren, François Hamy, Thomas Klimkait,¹ Erik de Clercq, and Anne-Mieke VanDamme

Rega Institute for Medical Research, Katholieke Universiteit Leuven, Leuven, Belgium (D.D., D.S., M.W., C.P., S.H., S. Van D., E. De C., A.-M.V.); and Novartis Pharmaceuticals, Pharma Research, Basel, Switzerland (F.H., T.K.)

	Abstract

Top Abstract Introduction Materials and Methods Results Discussion References

The peptoid CGP64222 has been previously demonstrated to inhibit the human immunodeficiency virus (HIV) Tat/transactivationresponse element complex formation. It has previously been shownthat CGP64222 selectively inhibits HIV-1 long terminal repeat-drivengene expression and HIV-1_LAV replication in lymphocytes. Here,we show that CGP64222 inhibits the replication of a wide rangeof laboratory strains of HIV-1 and HIV-2 in MT-4 cells. However,CGP64222 proved inactive in MT-4 cells against HIV-1 strains thatare resistant to the bicyclams. The bicyclams are known to specificallyinteract with CXC-chemokine receptor 4, the main coreceptor usedby T-tropic HIV strains to enter the cells. Mechanism of actionstudies revealed that CGP64222 can inhibit the HIV replicativecycle, also through a selective interaction with the CXC-chemokinereceptor 4coreceptor.

	Introduction

Top Abstract Introduction Materials and Methods Results Discussion References

The replication of human immunodeficiency virus (HIV) requires the function of Tat, one of the regulatory gene products encodedby HIV (Arya et al., 1985; Sodroski et al., 1985). Tat transactivatesexpression of all viral genes that depend on the long terminalrepeat (LTR) by increasing the rate of initiation and the processivityof transcription (Laspia et al., 1989; reviewed in Cullen, 1998).These activation events are mediated through the ability of Tatto interact with a cis-acting RNA sequence, the transactivationresponse element (TAR), located downstream of the transcriptionalinitiation site. Binding to TAR is mediated by a short, linearpeptide domain of Tat that is predominantly composed of basicamino acids. This interaction may be considered a suitable targetfor the chemotherapy of HIV infection, because an inhibitor ofthe Tat/TAR interaction may have the potential to keep the virusin its dormant state. We have previously reported that a basicpeptoid oligomer of nine residues, CGP64222 (Fig. 1), can effectivelycompete with Tat for binding to TAR. NMR spectroscopy indicatedthat CG64222 interacts with the TAR RNA in the region encompassingthe UCU bulge and the 2 bp on either side of the bulge. CGP64222induces a conformational change in TAR, and this change is mediatedby direct contacts between an N-Arg side chain from the compoundand G26 and U23 from TAR (Hamy et al., 1997). CGP64222 was alsoshown to block HIV-1_LAV replication in PBLs (Hamy et al., 1997).

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Fig. 1. Chemical structure of CGP64222.

Numerous publications over the past 2 years have demonstrated the importance of chemokine receptors for HIV entry into thecells. Chemokines are chemotactic cytokines, which are classifiedas CC or CXC, depending on the positioning of conserved cysteineresidues. The CXC-chemokine receptor 4 (CXCR4) mediates entryof T cell line-tropic (T-tropic) viruses, and this function canbe inhibited by stromal cell-derived factor-1 $alpha$ (SDF-1 $alpha$ ), the naturalligand of CXCR4 (Oberlin et al., 1996). The CC-chemokine receptorCCR5 mediates entry of macrophage-tropic (M-tropic) viruses (Alkhatibet al., 1996). Bicyclams have been established as highly selectiveanti-HIV agents (De Clercq et al., 1992) that specifically blockthe CXCR4 coreceptor (Schols et al., 1997a,b; Donzella et al.,1998). Other antagonists of CXCR4 are ALX40-4C, a polycationic,nonapeptide solely existing of arginine residues (Doranz et al.,1997), and T22, which is also a positively charged peptide containingarginine and lysine residues (Murakami et al., 1997).

Here, we demonstrate that the polycationic peptoid CGP64222, designed as a Tat inhibitor, can also block early events in HIV-1replication. In particular, this compound was shown to inhibitviral entry into the cells through blockade of the CXCR4coreceptor.

	Materials and Methods

Top Abstract Introduction Materials and Methods Results Discussion References

Viruses, Cells and Drugs. The origins of the virus stock HIV-1 III_B and RF (Popovic et al., 1984) and HIV-1 NDK (Spire et al., 1989) were describedpreviously. The strains HIV-1 MN, the 3'-azido-2',3'-dideoxythymidine(AZT)-resistant HIV-1 strain RTMC (Larder and Kemp, 1989; a recombinant,AZT-resistant HIV-1 strain containing RT mutations D67N, K70R,T215F, and K219Q), HIV-2 ROD, and the HIV-1 M-tropic strains BaLand ADA were all obtained through the Medical Research CouncilAIDS reagent project (Herts, UK). The HIV-1 molecular clone NL4.3was obtained from the National Institute of Allergy and InfectiousDisease AIDS reagent program (Bethesda, MD). The HIV-1-resistantstrains NL4.3_AMD3100^R (Esté et al., 1998), NL4.3_AMD2763 (De Vreese et al., 1996),NL4.3_DS5000^R, and NL4.3_AR177^R (Esté et al., 1998) were obtained as described previously. HIV-1HE is a clinical isolate from a Belgian patient with AIDS. Allvirus stocks were prepared from the supernatants of infected MT-4cells except for the strains tested in peripheral blood lymphocytes(PBLs), which were cultured on donor lymphocytes. HL_tat cells(Felber et al., 1990) were maintained in Dulbecco's modified Eagle'smedium supplemented with 10% FCS; MT-4 cells, Jurkat_tat cells,Jurkat cells, and SUP-T1 cells (American Type Culture Collection,Rockville, MD) were grown and maintained in RPMI 1640 medium supplementedwith 10% FCS. PBLs from healthy donors were isolated by densitygradient centrifugation (Ficoll hypaque) and stimulated with phytohemagglutinin(1 µg/ml; Sigma Chemical Co., Bornem, Belgium) during 3 days at37°C. The activated cells (phytohemagglutinin-stimulated blasts)were washed three times with PBS and inoculated with virus asdescribed previously (Schols et al., 1997b).

Dextran sulfate was obtained from Sigma. AZT was synthesized by Christophe Pannecouque. AMD3100 and AMD2763 was kindly providedby Dr. G. Henson (AnorMED, Langley, British Columbia, Canada).Saquinavir was provided by N. Roberts (Roche Products, WelvynGarden City, UK). Ro5-3335 was synthesized by Wayne A. Spitzeand Frantz Victor at Lilly Research Laboratories (Indianapolis,IN). The anti-CXCR4 monoclonal antibodies (mAb; clones 12G5 and171) and the anti-CCR5 mAb (clone 2D7) were purchased from R andD Systems (Minneapolis, MN). The anti-CXCR4 mAb 2B11 was a kindgift of Dr. R. Förster and Dr. M. Lipp (Max Delbrück Center,Berlin-Buch,Germany).

Analysis of HIV-1 Transactivation. Tat-dependent and independent transactivation of HIV-1 was monitored as described previously (Daelemans et al., 1997). Forthe Tat-dependent transactivation, HL_tat cells were transfectedwith pHIVLacZ (Maio and Brown, 1988) or pCMV $beta$ (Berger et al.,1988) plasmid DNA. pHIVLacZ was obtained from the National Instituteof Allergy and Infectious Disease AIDS reagent program and containsthe LacZ gene driven by the HIV-1 LTR promoter, and pCMV $beta$ (Clontech,Palo Alto, CA) expresses the LacZ gene under control of the cytomegalovirus(CMV) immediate-early promoter. The compound Ro5-3335, previouslyreported as a specific HIV-1 LTR transactivation inhibitor (Hsuet al., 1991; Witvrouw et al., 1992), was used as reference compound.Additionally, Jurkat_tat cells were transfected with pHIVLuc plasmidDNA, which contains the luciferase reporter gene under controlof the HIV-1 LTR. pHIVLuc was obtained by ligating the KpnI/HindIIIHIV-1 LTR fragment from pHIVLacZ into the pGL3basic vector (Promega,Madison, WI). Ten million Jurkat cells were suspended in 200 µlof medium, and 15 µg of plasmid DNA was electroporated (260 V,1050 µF, and infinite resistance) into the cells. Two hundredthousand electroporated cells were incubated in the presence ofdifferent concentrations of test compound in 96-well plates. Forthe Tat-independent transactivation, Jurkat cells were transfectedwith pHIVLuc and stimulated with phorbol-12-myristate-13-acetate(PMA; 5 µM). In all transactivation assays, inhibition of transactivationwas measured by quantification of reporter gene activity 24 hafter transfection. $beta$ -Galactosidase reporter gene activity wasquantified with a colorimetric assay as described previously (Daelemanset al., 1997). Luciferase activity was measured by adding 100µl of luciferase reagent (LucLite; Packard) to the same volumeof cells according to the user's manual. The IC₅₀ value was calculatedas being the inhibitor concentration that reduces reporter geneexpression by 50%. Toxicity of the test compounds to the cellswas performed either through quantification of total protein contentaccording to the Bradford method (Bio-Rad, Hercules, CA) as describedpreviously (Daelemans et al., 1997) or a tetrazolium-based viabilityassay (Celltiter 96 assay;Promega).

In Vitro Integration Assay. The inhibition of the HIV integrase 3'-processing and DNA strand transfer was monitored as described previously (Cherepanovet al., 1997).

Reverse Transcriptase Assay. Inhibition of HIV RT activity was monitored in vitro in standard reverse transcriptase assays of cell culture supernatantsamples by incubating them with a standard RT reaction mixtureas described previously (Willey et al., 1988). Briefly, the compoundwas added at increasing concentrations to the RT reaction mixturebefore the addition of culture medium containing virus. RT-dependentextension to oligo(dT) on synthetic poly(A)⁺ RNA was determined by the in vitro incorporation of [³²P]dTTP into the synthesizedproduct.

Quantification of Exposed CXCR4 and CCR5. SUP-T1 cells, U87.CD4.CXCR4, or U87.CD4.CCR5 cells were incubated with either CGP64222, the bicyclam AMD3100, or PBS for 30min at 4°C before the cells were rinsed with PBS to remove unboundcompound. The anti-CXCR4 and anti-CCR5 mAbs were then added, andthe cells were washed and incubated with fluorescein isothiocyanate(FITC)-conjugated goat anti-mouse antibody (Caltag Labs, San Francisco,CA). Cells were analyzed by a FACScan flow cytometer (Becton-Dickinson).The percentage of inhibition of mAb binding in the presence ofdifferent concentrations of the compound was calculated usingthe mean fluorescence intensity (MFI) values, as previously described(Schols et al., 1997b).

The biotinylated human macrophage inflammatory protein-1 $alpha$ (MIP-1 $alpha$ ) fluorokine kits were purchased from R and D Systems. Thebinding of the biotinylated MIP-1 $alpha$ was performed according tothe protocol of the manufacturer. Briefly, U87.CD4.CCR5 cellswere incubated with CGP64222 for 30 min at 4°C, and then the stainingprotocol with biotinylated MIP-1 $alpha$ wasstarted.

Intracellular Calcium Flux Assay. Exponentially growing SUP-T1 cells or U87.CD4.CCR5 cells were loaded for 45 min at room temperature with the fluorescent calciumindicator Fluo-4-AM (Molecular Probes, Leiden, the Netherlands)at 4 µM in cell culture medium. Thereafter, the cells were washedtwice with calcium flux buffer (Hanks' balanced salt solutionwith 20 mM HEPES and 0.2% BSA, pH 7.4) and seeded onto a 96-wellblack-wall microplate (Costar, Cambridge, MA) at 3 × 10⁵ cells/well. After a 20-min preincubation of the cells with thetest compounds (CGP64222 or AMD3100) at the appropriate concentrations,the intracellular calcium flux in response to 5 ng/ml human recombinantSDF-1 $alpha$ or 2.5 ng/ml RANTES (regulated on activation normal T cellexpressed and secreted; PeproTech, Rocky Hill, NJ) was monitoredat 37°C as a function of time using a Fluorescent Imaging PlateReader (FLIPR, MolecularDevices).

Antiviral Replication Assays. The antiviral activities of the compounds were determined in MT-4 cells by measuring inhibition of virus-induced cytopathogenicity.Briefly, MT-4 cells were infected with virus at 100× the 50% cellculture infective dose/ml in the presence of various concentrationsof the test compound. The number of viable cells was determinedafter 5 days of incubation at 37°C, according to the 3-(4,5-dimethylthiazol-2-yl)-2,5-diphenyltetrazoliumbromide method described previously (Pauwels et al., 1988).

The inhibitory effect of the compounds on the replication of HIV-1 strain III_B in PBLs was monitored 7 days after infectionby quantification of HIV-1 p24 core antigen (Ag) using an enzyme-linkedimmunosorbent assay (ELISA; DuPont, Wilmington, DE). These experimentswere performed according to the ACTGDoDprotocol.

U87.CD4 Transfectants. Astroglioma U87.CD4 cells, stably transfected with CXCR4 or CCR5 (kindly provided by Nathaniel R. Landau, Aaron Diamond AIDSResearch Center, New York, NY), were cultured in Dulbecco's modifiedEagle's medium containing 10% FCS. The parental U87.CD4 cellsdo not express either CXCR4 or CCR5. CXCR4- or CCR5-transfectedcells were incubated with HIV-1 NL4.3 or HIV-1 BaL equivalentto 10³ pg of p24, and viral replication was measured 6 days later withthe p24 Ag ELISA.

Time-of-Addition Experiment in MT-4 Cells. MT-4 cells were infected with HIV-1 III_B at a multiplicity of infection of more than 1, and the test compounds were addedat different times (0, 1, 2, 3, 24 h) after infection, as describedpreviously (De Clercq et al., 1992). Viral p24 antigen productionwas determined 29 h post infection by p24 Ag ELISA.

Analysis of Inhibition of HIV-1 Viral DNA and Single-Spliced Viral RNA Production by Semiquantitative Polymerase Chain Reaction (PCR) in MT-4 cells. Two hundred thousand MT-4 cells were infected with HIV-1 III_B (multiplicity of infection, 0.5) and incubated with differentconcentrations of the test compound. Twenty-four hours after infection,cells were counted and washed once with RPMI 1640. DNA was extractedfrom 1 × 10⁵ cells (QIAamp Blood Kit; Qiagen, Studio City, CA), and PCR wasperformed in a total volume of 50 µl, mainly as described previously(Balzarini et al., 1992). The other half of the cells (1 × 10⁵) was used for RNA extraction via TRIZOL and cDNA synthesis usingthe RNA-PCR kit from Perkin-Elmer Cetus (Norwalk, CT). The PCRwas performed on 10 µl of cDNA in a total volume of 50 µl with10 mM Tris · HCl (pH 8.3), 50 mM KCl, 1.5 mM MgCl₂, 200 µM concentrationof dNTPs, 1 µM concentration of primers, and 1.25 U of AmpliTaqDNA polymerase (Perkin-Elmer Cetus). The primers used were KPNA,5'-AGAGTGGTGGTTGCTTCCTTCCACACAG-3' sense and upstream of the major5' splice donor (Neumann et al., 1994), and AV14, 5'-CTCTCTCGACGCAGGACTCGGCTTGCTGAA-3'antisense and downstream of the env splice acceptor, to amplifytwo fragments of 466 and 482 bp in the env region of HIV-1, onefragment of 665 bp in the vpr region, a 1053-bp fragment in thevif region, and a 1530-bp fragment in the tat region of HIV-1.As internal control, a 285-bp fragment of human $beta$ -actin RNA wasamplified using the $beta$ -Actin Primer Pair (Promega). Five microlitersof each PCR product were electrophoretically separated in a 6%acrylamide gel, and the DNA was stained with ethidium bromide.The HIV-specific bands of the inhibition experiments were comparedwith those obtained from a 2-fold dilution series of HIV-1 III_B-infectedMT-4 cells (obtained from the same experiment) diluted with mock-infectedMT-4 cells, and the $beta$ -actin bands of the inhibition experimentwere compared with those obtained from a 2-fold dilution seriesof HIV-1 III_B-infected MT-4 cells (from the same inhibition experiment)diluted withmedium.

	Results

Top Abstract Introduction Materials and Methods Results Discussion References

Inhibition of HIV-1 Transactivation. The transactivation assay allowed us to quantify Tat-dependent HIV-1 LTR transactivation in HL_tat and Jurkat_tat cells aftertransient transfection with pHIVLacZ or pHIVLuc, respectively.Tat-independent transactivation of the HIV-1 LTR by PMA was alsomeasured in pHIVLuc-transfected Jurkat cells. After the Tat-dependentor independent transactivation of the HIV-1 LTR, the expressionof the reporter genes was increased up to 12-fold with respectto the nontransfected cells. Thus, these assays provide a sensitiveway to study HIV-1 LTR activity. The peptoid CGP64222, previouslyreported as an inhibitor of the Tat/TAR complex formation (Hamyet al., 1997), inhibited the Tat-dependent expression of the reportergene with an IC₅₀ value of 20 µg/ml in HL_tat cells (not shown)and an IC₅₀ value of 9.5 µg/ml in Jurkat_tat cells (Fig. 2A). CGP64222also inhibited the Tat-independent PMA-induced transactivationof the HIV-1 LTR in Jurkat cells with an IC₅₀ value of 13 µg/ml(Fig. 2B). Because a previous finding demonstrated an interactionof CGP64222 with TAR (Hamy et al., 1997), the Tat-independentanti-transactivation activity noted here is probably mediatedthrough interference with cellular activators binding to TAR.The compound was not able to inhibit reporter gene expressionin HeLa or Jurkat cells transiently transfected with a constructcontaining the reporter gene under the control of a Tat-independentCMV promoter (Fig. 2), thus proving the specificity of CGP64222interaction with the HIV LTR promoter. Up to the highest concentrationtested (50 µg/ml), CGP64222 was not cytotoxic as measured in parallelwith a tetrazolium-based viability assay.

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Fig. 2. Effect of CGP64222 on the expression of luciferase in the transactivation assay in Jurkat cells. Cytotoxicity was determined in parallel with a tetrazolium-based viability assay ( $black-down-triangle$ , $down-triangle$ ). Reporter gene activity was measured with a luciferase-dependent luminescence assay. Zero percent is the luminescence measured in untransfected cells, and 100% is the luminescence measured in transfected cells without the addition of drug. After Tat-dependent transactivation of the HIV-1 LTR, the expression of luciferase activity was increased up the 12-fold, whereas for the Tat-independent transactivation, the expression of luciferase was increased up to 6-fold. Experimental data are the average of two or three independent experiments, each performed in triplicate; error bars show the S.D. A, Jurkat_tat cells were transfected with pHIVLuc or with pCMVLuc, and the inhibition of the Tat-dependent (

) or the HIV-independent ( $black-square$ ) luciferase expression by CGP64222 was measured. B, Jurkat cells were transfected with pHIVLuc and stimulated with PMA. The inhibition of the Tat-independent LTR activation ( $open circle$ ) or the HIV-independent transcription (

) was measured via the luciferase reporter gene.

Effect on Integration and RT. Using the 3'-processing and DNA strand-transfer assays, CGP64222 was found not to interfere with the in vitro integrationup to concentrations of 100 µg/ml (W. Pluymers, unpublished data).Possible inhibition of the HIV-1 reverse transcriptase by CGP64222was examined using particle-associated enzyme. Virus isolatedfrom HUT/4-3 cultures, constitutively producing pNL4.3, was lysedand incubated in the presence of CGP64222 at concentrations upto 70 µg/ml. In quadruplicate tests, no significant dose-dependentinhibition of the reverse transcriptase reaction was found (notshown).

Antiviral Activity Spectrum. We assessed the ability of CGP64222-treated cells to support the replication of different HIV-1 and HIV-2 strains. CGP64222was examined for its inhibitory effect on the cytopathogenicityinduced by the HIV-1 strains III_B, NL4.3, RF, NDK, MN, RTMC, andHE (a clinical isolate) and the HIV-2 strain ROD. CGP64222 wasfound to inhibit HIV-1 III_B replication in MT-4 cells with anIC₅₀ value of 8.4 µg/ml, whereas it was not cytotoxic at a concentrationup to 125 µg/ml, resulting in a selectivity index of more than15 (Table 1). The anti-HIV activity of CGP64222 in MT-4 cellswas confirmed for a number of other HIV-1 strains, including theclinical isolate HE, the AZT-resistant strain RTMC, and the HIV-2strain ROD (IC₅₀ = 1.8-11.9 µg/ml; Table 1).

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TABLE 1
Inhibitory effect of CGP64222 on the replication of several HIV strains in MT-4 cells
Data are averages of two or three experiments, each performed in triplicate.

Table 1 also shows the effect of CGP64222 on the replication of NL4.3-derived strains selected for their resistance to binding/fusioninhibitors. CGP64222 inhibited the replication of viruses resistantto DS5000 and AR177, two binding inhibitors, with an IC₅₀ value5.9 and 14.5 µg/ml, respectively. However, CGP64222, at a concentrationof 50 µg/ml, did not suppress the replication of viruses maderesistant to the bicyclam derivatives AMD2763 and AMD3100 (Table1).

CGP64222 Dose-Dependently Inhibits Binding of CXCR4-Specific mAbs. Because HIV-1 strains resistant to the bicyclams (which are CXCR4-specific antagonists) also showed resistance to CGP64222,the interaction of CGP64222 with CXCR4 was further investigated.The mAbs 12G5, 171, and 2B11 react specifically with the humanCXCR4 protein and recognize this receptor on many T cell lines,such as the SUP-T1 T cell line (Endres et al., 1996). The 12G5mAb (Labrosse et al., 1998) and 171 mAb mainly bind to the secondloop of CXCR4, whereas 2B11 mAb (Förster et al., 1998) interactswith the first 63 amino-terminal amino acid residues of CXCR4.CGP64222 showed a clear dose-dependent inhibition of the interactionof the antibodies 12G5 and 171 with the CXCR4 receptor on SUP-T1cells, although relatively high concentrations of inhibitor wererequired. At 50 µg/ml (36 µM), CGP64222 inhibited by 30 and 51%the binding of the 12G5 mAb (not shown) to CXCR4 and of the mAb171 to CXCR4, respectively (Fig. 3C), whereas no effect was seenon the binding of the mAb 2B11 to the receptor at this concentration(Fig. 3F). The interference of CGP64222 with mAb binding to CXCR4is a result of direct binding of CGP64222 to CXCR4, because theexperiments were performed in a way that unbound CGP64222 waswashed away before binding of the mAb to CXCR4 was measured. Incomparison, AMD3100 at 8 ng/ml inhibited the binding of the mAb12G5 to CXCR4 by 80%, which is in agreement with previous data(Schols et al., 1997b). In addition, AMD3100 (D. Schols, unpublisheddata) or SDF-1 $alpha$ (Förster et al., 1998) had no effect on the bindingof the 2B11 mAb to CXCR4.

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Fig. 3. Inhibition of the binding of the anti-CXCR4 mAb (171) to SUPT1 cells (left) and no inhibition of the binding of the anti-CXCR4 mAb (2B11) to SUPT1 cells (right) in the presence of CGP64222 (50 µg/ml; C and F). A and D, an isotype control mAb was used as negative control. B and E, the specific anti-CXCR4 mAb was used as positive control. The percentage of positive cells and the MFI values are indicated in each histogram. The percentage of inhibition can be calculated by comparing the MFI in presence of CGP64222 with the MFI of the positive control.

To investigate the specificity of the interaction of CGP64222 with CXCR4, competition of the binding of anti-CCR5 mAb 2D7to U87.CD4 cells expressing CCR5 and of the binding of the anti-CXCR4mAb 171 to U87.CD4 cells expressing CXCR4 was investigated (Fig.4). At 50 µg/ml, CGP64222 did not inhibit the binding of 2D7 mAbto the CCR5 coreceptor (Fig. 4, F and G), whereas we could detect38% inhibition of 171 mAb binding to U87.CD4 cells expressingthe CXCR4 coreceptor (Fig. 4, B and C). The known CXCR4 antagonistAMD3100 completely blocked the binding of the 171 mAb to CXCR4on U87.CD4.CXCR4 cells, whereas it had no effect on the interactionof the 2D7 mAb with CCR5 (Fig. 4, D and H).

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Fig. 4. Inhibition of the binding of the anti-CXCR4 mAb (171) to U87.CD4.CXCR4 cells (left) and no inhibition of the binding of the anti-CCR5 mAb (2D7) to U87.CD4.CCR5 cells (right) in the presence of CGP64222 (50 µg/ml; C and G) and AMD3100 (200 ng/ml; D and H). A and E, an isotype control mAb was used as negative control. B and F, the specific anti-CXCR4 mAb or anti-CCR5 mAb was used as positive control. The percentage of positive cells and the MFI values are indicated in each histogram. The percentage of inhibition can be calculated by comparing the MFI in presence of CGP64222 with the MFI of the positive control.

In addition, CGP64222 did not inhibit the binding of biotinylated MIP-1 $alpha$ to U87.CD4.CCR5 cells, whereas as control, the anti-humanMIP-1 $alpha$ blocking antibody included in the fluorokine kit almostcompletely blocked the binding of the biotinylated MIP-1 $alpha$ (Fig.5)

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Fig. 5. Lack of inhibition of the binding of biotinylated MIP-1 $alpha$ to U87.CD4.CCR5 cells in the presence of CGP64222 (50 µg/ml; D). A, only the avidin-FITC was added as negative control. B, the biotinylated MIP-1 $alpha$ and avidin-FITC were added as positive control. D, the biotinylated MIP-1 $alpha$ and avidin-FITC were added in the presence of CGP64222 (50 µg/ml), C, the biotinylated MIP-1 $alpha$ and avidin-FITC were added in the presence of the blocking antibody. The percentage of positive cells and MFI values are indicated in each histogram. The percentage of inhibition can be calculated by comparing the MFI in presence of CGP64222 with the MFI of the positive control.

These results suggest that the CGP64222 clearly interacts with the second extracellular loop (ECL2) of the CXCR4 receptorbut not with the amino-terminal end of CXCR4. Also, CGP64222 isnot able to block 2D7 mAb binding to CCR5 or biotinylated MIP-1 $alpha$ toCCR5.

Inhibition of SDF-1 $alpha$ -Triggered Calcium Flux. On binding of SDF-1 $alpha$ to its receptor CXCR4 or on binding of RANTES to the CCR5 receptor, a transient intracellular calciumflux can be measured. Inhibition of chemokine binding can be quantifiedby a reduction in calcium flux. Figure 6 shows a dose-dependentinhibition of SDF-1 $alpha$ -mediated intracellular calcium flux by CGP64222,whereas no inhibition of RANTES-induced calcium flux was observedwith CGP64222 (Fig. 6B) at a concentration (50 µg/ml) that blockedthe SDF-1 $alpha$ -mediated signaling through CXCR4. These data indicatethat like AMD3100, CGP64222 acts as a CXCR4 antagonist.

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Fig. 6. A, concentration-dependent reduction of SDF-1 $alpha$ -induced intracellular calcium flux by CGP64222 in SUP-T1 cells. SUP-T1 cells were preincubated with CGP64222 at 0, 2, 10, and 50 µg/ml or with AMD3100 at 1 µg/ml. The cells were then stimulated with 5 ng/ml SDF-1 $alpha$ . The transient increase in fluorescence is a measure for the transient increase in intracellular calcium concentration on binding of the chemokine (SDF-1 $alpha$ ) to its receptor (CXCR4). The control represents the response of the cells elicited by 5 ng/ml SDF-1 $alpha$ in the absence of any antagonist. Each curve shows the average of four wells. B, U87.CD4.CCR5 cells were preincubated with CGP64222 at 50 µg/ml. The cells were stimulated with 2.5 ng/ml RANTES. The transient increase in fluorescence is a measure for the increase in intracellular calcium concentration on binding of RANTES to its CCR5 receptor. The control represents the response of the cells elicited by chemokine in the absence of any antagonist.

Anti-HIV activity of CGP64222 in U87.CD4 transfectants. To confirm the interaction of CGP64222 with the CXCR4 receptor, the anti-HIV activity of the peptoid was tested in the astrogliomaU87 cell line stably expressing CD4 and CXCR4 or CD4 and CCR5(Deng et al., 1997). The T-tropic NL4.3 wild-type virus was usedfor infection of U87.CD4.CXCR4 cells (and was not able to infectthe U87.CD4.CCR5 cells), and the M-tropic HIV-1 BaL strain wasused for infection of U87.CD4.CCR5 cells (and does not replicatein the U87.CD4.CXCR4 cells; Schols et al., 1998). As controls,SDF-1 $alpha$ and RANTES were used. SDF-1 $alpha$ and RANTES, which are naturalligands for CXCR4 and CCR5, respectively, are inhibitory to thereplication of the T-tropic and M-tropic virus, respectively.Table 2 shows the anti-HIV effect of CGP64222 in U87.CD4-transfectedcells. The peptoid was found to inhibit NL4.3 replication in U87.CD4.CXCR4cells at an IC₅₀ value of 1.1 µg/ml, whereas it did not inhibitthe replication of HIV-1 BaL in U87.CD4.CCR5 cells. The Tat antagonistRo5-3335 (Hsu et al., 1991; Witvrouw et al., 1992) was able toinhibit both NL4.3 and BaL replication in the U87.CD4 transfectedcells with an IC₅₀ value varying between 0.5 and 1.8 µg/ml (Table2).

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TABLE 2
Anti-HIV activity of CGP64222, SDF-1 $alpha$ , RANTES, and Ro5-3335 in U87.CD4 cells transfected with CXCR4 or CCR5
Virus yield was monitored in the cell-free supernatant from U87.CD4 transfected cells 6 days after infection using a viral p24 antigen ELISA.

Stage of Interaction with HIV Replicative Cycle in MT-4 Cells. To pinpoint at which stage the peptoid actually interacts with the HIV replicative cycle in MT-4 cells, a time-of-additionexperiment was carried out (Fig. 7). The cells were infected athigh virus multiplicity (multiplicity of infection, 1), and thecompounds were added every hour after infection during 24 hours.Depending on the stage at which a specific compound would act,and influenced by the intracellular metabolism and concentration,the addition of a given compound could be postponed for t hourswithout loss of activity. Dextran sulfate (100 µg/ml), which actsat the virus adsorption step (Baba et al., 1988; Mitsuya et al.,1988), must be added together with the virus (t = 0) to be active.For AZT (0.5 µg/ml), which, after its intracellular phosphorylation,acts at the RT step (Huang et al., 1990), the addition to thecells could be delayed for up to 5 h (t = 5) after infection.The protease inhibitor saquinavir (2 µg/ml), which interacts witha late event in the virus cycle (assembly of mature virions; Dreyeret al., 1989), is still effective if added as late as 21 h afterinfection (t = 21). Like dextran sulfate, the peptoid CGP64222(150 µg/ml) has to be added together with the virus (t = 0) tobe active against viral replication in MT-4 cells (Fig. 7). Thisindicates that CGP64222 must interact with an early stage of theviral replicative cycle in MT-4 cells.

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Fig. 7. Time-of-addition experiment. MT-4 cells were infected with HIV-1 III_B at multiplicity of infection of more than 1, and the test compounds were added at different times post infection. Viral p24 Ag production was determined 29 h after infection.

We then further analyzed the inhibition by CGP64222 of viral DNA and single-spliced viral RNA production in MT-4 cells. Ifinhibition by CGP64222 is mediated exclusively by interferencewith the Tat/TAR interaction, we should see no inhibition of newviral DNA formation by reverse transcription (RT) after virusentry, whereas there should be inhibition of viral RNA production.Tat inhibition would result in diminished levels of HIV-1 specificsingle-spliced RNA levels as the result of interference with transactivation.To test this hypothesis, we analyzed viral DNA formation and viralsingle-spliced RNA production in MT-4 cells at 24 h after infectionusing a semiquantative PCR assay. Inhibition of HIV-1 III_B replicationby increasing concentrations of CGP64222 was correlated with adecrease in new viral DNA formation (Fig. 8). There was a dose-dependentdecrease in proviral DNA production that was not due to toxicity,because $beta$ -actin RNA formation was not impaired. In a parallelexperiment, the RT inhibitor AZT showed a dose-dependent inhibitionof viral DNA formation, whereas the protease inhibitor saquinavirhad no effect on viral DNA formation (not shown). In fact, AZTinhibited both viral DNA and single-spliced viral RNA production(Fig. 8), with the latter being a direct result of the inhibitionof proviral DNA synthesis. CGP64222 also inhibited viral RNA synthesis,but this seems to be completely secondary to inhibition of proviralDNA production (as observed for AZT). We could not detect anyadditional inhibitory effect with CGP64222 on viral RNA productionas a result of inhibition of transactivation.

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Fig. 8. Inhibition of viral DNA and RNA formation as measured by PCR after infection with HIV-1 III_B. Acutely infected MT-4 cells were cultured in the absence (0) or in the presence of different concentrations of compound before infection. $-$ , Mock-infected MT-4 cells. $beta$ -actin RNA production was measured as control for toxicity of the test compounds. For RNA, only the major 482-bp fragment in the env region of HIV-1 is shown. HIV-1 III_B RNA and DNA PCR products were loaded together in a single slot of the polyacrylamide gel (top). $beta$ -Actin RNA-PCR products were loaded on a separate gel (bottom). There is a dose-dependent inhibition of viral DNA synthesis and, hence, viral RNA production in the presence of the RT inhibitor AZT. CGP64222 is inhibiting the viral DNA synthesis, and no additional effect on viral RNA production could be detected.

Inhibition of M-Tropic HIV Strains in PBLs. The effect of CGP64222 on virus production in acutely infected PBLs with the M-tropic HIV-1 strains BaL and ADA was examined.HIV-1 BaL is assumed to exclusively use CCR5 as coreceptor, andADA uses mainly CCR5 (eventually, CCR2b and CCR3; Alkhatib etal., 1996). CGP64222 inhibited the replication of the HIV-1 strainsBaL and ADA with an IC₅₀ value of 1.2 and 0.7 µg/ml, respectively,and in the absence of cytotoxicity (CC₅₀ > 50 µg/ml; Table 3).

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TABLE 3
Inhibitory effect of CGP64222 on the replication of M-tropic HIV-1 strains in PBLs
Data are averages of two separate experiments.

	Discussion

Top Abstract Introduction Materials and Methods Results Discussion References

The search for drugs that can block the transactivation of HIV started several years ago (reviewed in Daelemans et al., 1999).In a recent report, a peptoidic compound, CGP64222, that was ableto effectively compete with Tat for binding to TAR RNA was described(Hamy et al., 1997). We also showed here that CGP64222 is inhibitingTat-dependent as well as Tat-independent transactivation of theHIV-1 LTR promoter, whereas it has no effect on the CMV controlpromoter. This confirms our previous data (Hamy et al., 1997)that the peptoid is specifically interacting with the HIV-1 LTRpromoter. In vitro experiments previously showed that this interactionis with the TAR RNA. Our results suggest that CGP64222 not onlyinhibits Tat/TAR binding but also inhibits promoter activity inthe absence of Tat, most probably through interference with cellularactivators.

In this study, we also found that CGP64222 indeed is a potent inhibitor of the replication of various HIV-1 laboratory strainsand clinical isolates and of HIV-2 (Table 1). The compound retainedfull activity against an AZT-resistant HIV-1 strain. An intriguingobservation, however, was that CGP64222 was inactive against HIVstrains resistant to bicyclams (Table 1), suggesting that inMT-4 cells CGP64222 and bicyclams might be acting on the sametarget. Bicyclams have recently been shown to be selective antagonistsof the CXCR4 coreceptor (Schols et al., 1997a; Donzella et al.,1998). Numerous publications over the past 2 years have demonstratedthe importance of chemokine receptors for HIV entry. The followingobservations further confirmed the hypothesis of a common targetfor CGP64222 and the bicyclams. On the one hand, CGP64222 interferedin a dose-dependent manner with the binding of specific anti-CXCR4mAbs to the second loop of the CXCR4-coreceptor on SUPT-1 T cells(Fig. 3). However, it did not block the binding of a specificmAb binding to the amino-terminal end of CXCR4 and the bindingof the CCR5 mAb 2D7 to the CCR5 coreceptor (Fig. 4). CGP64222does not appear to interact directly with CCR5 because it doesnot inhibit the binding of biotinylated MIP-1 $alpha$ or 2D7 mAb to theCCR5 receptor (Fig. 5). These results suggest that CGP64222 specificallybinds to the second extracellular loop of CXCR4 in vitro, as hasalso been demonstrated for AMD3100 (Labrosse et al., 1998). Theinhibitory potency against the anti-CXCR4 mAb binding was morethan 1000-fold lower than that of the bicyclam AMD3100. This differentialeffect could be due to the fact that the anti-CXCR4 mAbs are bindingtoward a slightly different epitope than CGP64222. However, thisdifferential activity can also be explained by the fact that thepeptoid has an IC₅₀ value between 1 and 10 µg/ml against T-tropicHIV strains in MT-4 cells, whereas the AMD3100 IC₅₀ value is 1000-foldmore active (1-10 ng/ml; Schols et al., 1997a). Second, in calciumflux experiments, CGP64222 proved to inhibit functionally andspecifically the binding of SDF-1 $alpha$ to the CXCR4 receptor (Fig.6). Third, the fact that HIV replication in U87.CD4.CXCR4 cells,but not in U87.CD4.CCR5 cells, is inhibited by CGP64222 demonstratesthat this compound specifically interferes with the CXCR4 receptor(Table 3). Furthermore, in the time-of-addition experiments inMT-4 cells, we could clearly show that CGP64222 interacts withan early event in the viral replication cycle (Fig. 7). Becausethe compound was equally active against the NL4.3_DS5000^R and the NL4.3_AR177^R, strains made resistant to the binding inhibitors DS5000 or AR177,compared with the NL4.3 wild-type strain, we can exclude thatthe compound behaves as a pure virus binding inhibitor. In addition,CGP64222 inhibited the viral DNA production in MT-4 cells, confirmingthat the peptoid interacts with HIV replication at a stage beforeor coinciding with RT (Fig. 8). No additional inhibitory effecton viral RNA production in MT-4 cells could be found because theproduction of single-spliced viral RNA was inhibited in a similarway as for the RT inhibitor AZT. Therefore, all the data are consistentwith an activity of the peptoid at the virus/cell fusion processmediated through the CXCR4 coreceptor binding in MT-4cells.

MT-4 cells are human T lymphotropic virus-1-transformed human T cells that express the human T lymphotropic virus-1 Tax transactivator,which is also able to induce the HIV LTR promoter. Therefore,in these cells, HIV transactivation inhibitors are very difficultto monitor, but all other inhibitory effects on viral replicationcan be evaluated. Our data in MT-4 cells therefore suggest thatCGP64222, previously shown to be able to block the Tat/TAR interaction,is also capable of interacting with the virus-cell binding processthrough inhibition of the CXCR4 coreceptor and that this targetis the only operational target for the anti-HIV activity of CGP64222in MT-4 cells. However, in PBLs, the peptoid interferes with thereplication of both T-tropic viruses (HIV-1_LAV; Hamy et al., 1997),which use the CXCR4 coreceptor, and M-tropic viruses (BaL), whichuse the CCR5 coreceptor (Table 3). These latter results suggestthat in PBLs, besides the CXCR4 coreceptor target, the peptoidis still capable of inhibiting viral replication through a postentryevent, most likely the Tat/TAR interaction. This differentialeffect seen with CGP64222 in MT-4 cells and PBLs reflects thecell type specificity of Tat inhibitors, as previously demonstratedfor other Tat antagonists (Witvrouw et al., 1992).

In conclusion, our findings indicate that CGP64222, an inhibitor of the Tat/TAR interaction, also shows inhibitory activityagainst HIV replication through interference with virus entryconsequent to blocking CXCR4 coreceptorbinding.

	Acknowledgments

We thank Cindy Heens, Kristien Erven, and Sandra Claes for excellent technical assistance and Wim Pluymers and Zeger Debyserfor performing the integrationassays.

	Footnotes

Received April 27, 1999; Accepted August 20, 1999

¹ Current address: Institute for Medical Mikrobiology, University of Basle, Petersplatz 10 CH-4003 Basle,Switzerland.

This work was supported by grants from the Belgian Nationaal Fonds voor Wetenschappelijk Onderzoek (G.3304.96), the GeconcerteerdeOnderzoeksacties (GOA 95/5), and the Biomedical Research Programmeof the European Union (EU Biomed. 2 grant BMH4-CT-95-1634). D.D.acknowledges a fellowship from the Flemish Institute supportingScientific-Technological Research in Industry(IWT).

Send reprint requests to: Dr. Dirk Daelemans, Rega Institute for Medical Research, Minderbroedersstraat 10, B-3000 Leuven, Belgium. E-mail: Dirk.Daelemans{at}uz.kuleuven.ac.be

	Abbreviations

HIV, human immunodeficiency virus; CMV, cytomegalovirus; LTR, long terminal repeat; FITC, fluorescein isothiocyanate; mAb, monoclonal antibody; MFI, mean fluorescence intensity; M-tropic, macrophage-tropic; PBL, peripheral blood lymphocyte; PCR, polymerase chain reaction; PMA, phorbol-12-myristate-13-acetate; RANTES, regulated on activation normal T cell expressed and secreted; AZT, 3'-azido-2',3'-dideoxythymidine; Ag, antigen; ELISA, enzyme-linked immunosorbent assay; RT, reverse transcription; SDF-1 $alpha$ , stromal cell-derived factor-1 $alpha$ ; TAR, transactivation responsive element; T-tropic, T cell line-tropic; CXCR4, CXC-chemokine receptor 4; MIP-1 $alpha$ , macrophage inflammatory protein 1 $alpha$ .

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