A Peptide Derived from Bee Venom-Secreted Phospholipase A2 Inhibits Replication of T-Cell Tropic HIV-1 Strains via Interaction with the CXCR4 Chemokine Receptor

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Vol. 60, Issue 2, 341-347, August 2001

A Peptide Derived from Bee Venom-Secreted Phospholipase A₂ Inhibits Replication of T-Cell Tropic HIV-1 Strains via Interaction with the CXCR4 Chemokine Receptor

David Fenard, Gerard Lambeau, Thomas Maurin, Jean-Claude Lefebvre, and Alain Doglio

Laboratoire de Virologie, Institut National de la Sante et de la Recherche Medicale U526, Faculté de Médecine, Nice, France (D.F., T.M., J.C.L., A.D.); and Institut de Pharmacologie Moléculaire et Cellulaire, Centre National de la Recherche Scientifique UPR411, Valbonne, France (G.L.)

	Abstract

Top Abstract Introduction Materials and Methods Results Discussion References

We have previously shown that secreted phospholipases A₂ (sPLA₂) from bee and snake venoms have potent anti-human immunodeficiencyvirus (HIV) activity (Fenard et al., 1999). These sPLA₂s blockHIV-1 entry into host cells through a mechanism linked to sPLA₂binding to cells. In this study, 12 synthetic peptides derivedfrom bee venom sPLA₂ (bvPLA₂) have been tested for inhibitionof HIV-1 infection. The p3bv peptide (amino acids 21 to 35 ofbvPLA₂) was found to inhibit the replication of T-lymphotropic(T-tropic) HIV-1 isolates (ID₅₀ = 2 µM) but was without effecton monocytotropic (M-tropic) HIV-1 isolates. p3bv was also foundcapable of preventing the cell-cell fusion process mediated byT-tropic HIV-1 envelope. Finally, p3bv can inhibit the bindingof radiolabeled stromal cell-derived factor (SDF)-1 $alpha$ , the naturalligand of CXCR4, and the binding of 12G5, an anti-CXCR4 monoclonalantibody. Taken together, these results indicate that p3bv blocksthe replication of T-tropic HIV-1 strains by interacting withCXCR4. Its mechanism of action however appears distinct from thatof bvPLA₂ because the latter inhibits replication of both T-tropicand M-tropic isolates and does not compete with SDF-1 $alpha$ and 12G5binding toCXCR4.

	Introduction

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HIV-1 isolates are known to display distinct cellular tropism. Most primary HIV-1 isolates, referred to as "M-tropic" HIV-1isolates, can infect human macrophages and primary T cells. Onthe other hand, laboratory-adapted HIV-1 isolates, known as "T-tropic",can infect primary and immortalized human T cells. Besides bindingto the CD4 receptor (Dalgleish et al., 1984), this tropism isdetermined at the level of virus entry by the use of a specificcoreceptor that belongs to the chemokine receptor family (Chanand Kim, 1998; Berger et al., 1999; Ross et al., 1999). The CCchemokine receptor (CCR) 5 is the major coreceptor for M-tropicHIV-1 strains, now referred to as R5 viruses (Alkhatib et al.,1996; Choe et al., 1996; Deng et al., 1996; Dragic et al., 1996).On the other hand, the CXC chemokine receptor (CXCR) 4 is themajor coreceptor for T-tropic HIV-1 strains, referred to as X4viruses (Feng et al., 1996). To a lesser extent, other membersof the chemokine receptor family, like CCR3, CCR2b, CCR8, arealso capable of mediating HIV entry into host cells (Berger etal., 1999; Ross et al., 1999). The chemokines and their derivativesthus form a potent class of HIV inhibitors and could be potentialtherapeutic agents (Howard et al., 1999). These factors are ableto compete with HIV-1 envelope glycoprotein (gp120) for bindingto the chemokine receptor and can also down-regulate their cognatereceptor (Chan and Kim, 1998; Berger et al., 1999; Ross et al.,1999). For instance, the CXC chemokine SDF-1 $alpha$ , which binds toCXCR4, specifically blocks the replication of X4 viruses (Bleulet al., 1996; Oberlin et al., 1996). Furthermore, various low-molecularweight compounds that bind to CXCR4 and inhibit HIV-1 replicationhave been identified. They include positively charged peptides(Doranz et al., 1997), the bicyclam compound AMD3100 (Schols etal., 1997), and T22, a strong anti-HIV peptide (Murakami et al.,1997b).

Secreted phospholipases A₂ (sPLA₂) form a structurally related family of enzymes that catalyze the hydrolysis of glycerophospholipidsto produce free fatty acids and lysophospholipids (Gelb et al.,1995; Dennis, 1997; Murakami et al., 1997a; Tischfield, 1997;Lambeau and Lazdunski, 1999; Valentin and Lambeau, 2000). A diversityof sPLA₂s has been purified from snake and insect venoms, andthese enzymes have been shown to exert a wide array of pharmacologicaleffects, including neurotoxicity and myotoxicity (Kini and Evans,1989). Recent studies have revealed that a diversity of sPLA₂sis also present in mammals (Cupillard et al., 1997; Ishizaki etal., 1999; Valentin et al., 1999a, 1999b, 2000; Gelb et al., 2000;Suzuki et al., 2000; Valentin and Lambeau, 2000), and these sPLA₂sare likely to be associated with various physiological and pathologicalprocesses, including host defense (Murakami et al., 1997a; Tischfield,1997; Lambeau and Lazdunski, 1999; Valentin and Lambeau, 2000).Furthermore, specific receptors for sPLA₂s have been identifiedsuggesting that these enzymes may also function as ligands (Lambeauand Lazdunski, 1999).

We have recently shown that several venom sPLA₂s are potent inhibitors of the replication of HIV-1 and HIV-2 (Fenard et al.,1999). For instance, bee venom sPLA₂ (bvPLA₂) is able to blockthe entry of both X4 and R5 viruses into host cells at nanomolarconcentrations (Fenard et al., 1999). The inhibition does notresult from a virucidal or cytotoxic effect but involves a morespecific mechanism linked to sPLA₂ binding to cells (Fenard etal., 1999). In this study, we have analyzed the inhibitory effectof several synthetic peptides derived from bvPLA₂ on HIV-1 replication.A peptide of 15 amino acids that corresponds to a surface-exposedloop of bvPLA₂ was found to display a potent anti-HIV-1 activityagainst T-tropic HIV-1 strains and can bind to CXCR4, the majorcoreceptor of these T-tropic HIV-1strains.

	Materials and Methods

Top Abstract Introduction Materials and Methods Results Discussion References

Plasmids and Reagents. Plasmids for HIV-1 (pNL.AD8, pYU2, pHXB2, pBRU-2) and pCMVtat were kindly provided by Drs. P. Charneau and N. Israel, respectively(Pasteur Institute, Paris, France). pHXB2-env was obtained fromDrs. Kathleen Page and Dan Littman through the National Institutesof Health AIDS Research & Reference Reagent Program (Rockville,MD). Peptides were synthesized by the Neosystem Laboratory (Strasbourg,France). pCa was synthesized and oxidized to allow the formationof a disulfide bond between cysteines 9 and 31. The 12G5 anti-CXCR4monoclonal antibody (mAb) was obtained from Dr. James Hoxie (NIHAIDS Research & Reference Reagent Program), 6H8 was from Dr. F.Arenzana-Deisdedos (Institut Pasteur), and anti-human human leukocyteantigen class I mAb (W6/32) was from DAKO (Glostrup, Denmark).Human recombinant SDF-1 $alpha$ was from PeproTech, Inc. (Rocky Hill,UK), and bvPLA₂ was prepared as described (Lambeau et al., 1989).

Cell Culture. P4 cells are HeLa CD4⁺ cells in which transactivation by HIV-1 Tat protein induces expression of the Escherichia coli Lac Zgene from the HIV-1 long terminal repeat (Charneau et al., 1994).P4-CCR5 cells are P4 cells expressing the CCR5 receptor (Fenardet al., 1999). These cells and the human embryonic kidney 293cells (ATCC, CRL-1573) were cultured in Dulbecco's modified Eagle'smedium (Invitrogen, Carlsbad, CA) supplemented with 7% fetal bovineserum (Biomedia, Boussens, France). CEM is a CD4⁺ T-cell line obtained from NIH AIDS Research & Reference ReagentProgram. These cells were cultured in RPMI 1640 medium (Invitrogen)supplemented with 10% fetal bovineserum.

HIV-1 Infection Assays. HIV-1_ADA, HIV-1_YU2, HIV-1_HXB2, and HIV-1_BRU were produced after transfection of the respective plasmids pNL.AD8, pYU2, pHXB2,and pBRU-2 in 293 cells using a Ca²⁺ phosphate mammalian transfection kit (Stratagene, Strasbourg,France). Three days after transfection, supernatants were collected,centrifuged (1500g, 15 min), and stored at $-$ 80°C. High-titer viralstocks of HIV-1_BRU were prepared as previously described (Fenardet al., 1999). Viral stocks were evaluated for HIV-1 viral capsidprotein content using an enzyme-linked immunosorbent assay kit(Organon Teknica, Fresnel, France). Single rounds of viral replicationwere performed as previously described (Fenard et al., 1999).Briefly, P4-CCR5 cells, seeded in 24-well plates, were infectedwith HIV-1 (100 ng of p24) in the presence or absence of variouseffectors for 8 h, then the incubation medium was replaced withfresh medium containing 50 µM 3'-azido-3'-deoxythymidine (AZT;Sigma-Aldrich, St. Quentin Fallavier, France). Two days later,cells were lysed, and 98 $beta$ -galactosidase ( $beta$ -gal) activity wasmeasured and used as an index of HIV-1 replication. For syncytiumformation assay, 293 cells were cotransfected with pHXB2-env andpCMVtat and mixed 1 day later with P4 cells (3:1 ratio) in thepresence or absence of effectors. After 48 h of coculture, cellswere lysed and the level of $beta$ -gal activity was used as an indexof cell-cell fusion. Time-of-addition experiments of p3bv wereperformed as previously described (Fenard et al., 1999). Briefly,p3bv was added at different times before or after infection ofP4-CCR5 cells with HIV-1_BRU (up to 8 h), and cells were then processedas described above for single round infectionassay.

Binding Experiments. SDF-1 $alpha$ -binding experiments were performed in 500 µl of binding buffer (RPMI 1640 medium, 0.1% bovine serum albumin) containing2 × 10⁵ CEM cells, 50 pM ¹²⁵I-SDF-1 $alpha$ (PerkinElmer Life Science Products, Courtaboeuf, France),and various concentrations of unlabeled SDF-1 $alpha$ or peptides. After1 h at 25°C, incubations were layered on 500 µl of fetal bovineserum, centrifuged for 3 min at 10,000g, and analyzed for radioactivityassociated with cell pellets. Nonspecific ¹²⁵I-SDF-1 $alpha$ binding was determined in the presence of 200 nM unlabeledSDF-1 $alpha$ . For cytometric analysis, 10⁶ CEM cells were incubated in 200 µl of phosphate-buffered salineat 4°C for 30 min in the presence or absence of effectors, andmAbs (5 µg/ml) were then added for another 30-min incubation period.After two washes, cells were incubated at 4°C with fluoresceinisothiocyanate (FITC)-conjugated secondary antibody (DAKO) for30 min. Cells were washed, resuspended in phosphate-buffered salineand 4% formaldehyde, and analyzed for fluorescence using a FACScanflow cytometer (Becton-Dickinson, Franklin Lakes, NJ). Bindingcompetition studies with radiolabeled sPLA₂s were performed aspreviously described (Fenard et al., 1999).

Down-Regulation Experiments. Experiments were performed as previously described (Tilton et al., 2000). Briefly, CEM cells (10⁶ cells/ml) were incubated at 37°C in RPMI 1640 medium supplementedwith 5% fetal calf serum in the presence of SDF-1 $alpha$ (10 nM) orp3bv (20 µM). At different times after the addition of effectors,cells were chilled on ice and stained with mAbs against CXCR4(6H8 and 12G5 mAbs) or isotype-matched control IgG, followed byFITC-conjugated goat anti-mouse IgG. Cell-associated fluorescencewas analyzed with a FACScan flowcytometer.

	Results

Top Abstract Introduction Materials and Methods Results Discussion References

Antiviral Activities of bvPLA₂-Derived Peptides. The three-dimensional crystal structure of bvPLA₂ has been obtained at a very high resolution, and this structure revealsseveral domains of homology with other sPLA₂s and a rigid networkof disulfide bonds that stabilizes the tertiary structure (Scottet al., 1990; Fig. 1A). Twelve overlapping synthetic peptidescovering the entire bvPLA₂ sequence were first designed (Fig.1B) and analyzed for their antiviral activity in a single roundinfection assay using P4-CCR5 cells infected with R5 (HIV-1_ADA)or X4 (HIV-1_BRU) HIV-1 viruses. Among these peptides, the p3bvpeptide (residues 21-35) was found to have antiviral activityagainst HIV-1_BRU but was without effect on HIV-1_ADA replication(Fig. 1B). The effect of p3bv appears specific because all otherbvPLA₂ peptides were without significant anti-HIV-1 activity (Fig.1B). As shown in Fig. 2A, the ID₅₀ value of X4 HIV-1 virus replication(HIV-1 _BRU and HIV-1_HXB2) for p3bv concentrations is close to2 µM, and replication of these X4 viruses is fully inhibited above10 µM. The lack of effect of p3bv on the replication of R5 HIV-1viruses was also confirmed using HIV-1_ADA and HIV-1_YU2 (Fig. 2A).

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Fig. 1. Inhibition of HIV-1 replication by various synthetic peptides derived from bvPLA₂. A, amino acid sequence of bvPLA₂ (Scott et al., 1990

). Numbers in parentheses indicate the positions of cysteines involved in disulfide bonds. *, active site histidine; $black-square$ , residues involved in the coordination of Ca²⁺ cofactor. B, P4-CCR5 cells were infected for a single round of viral replication with HIV-1_BRU or HIV-1_ADA in the absence or presence of the different synthetic peptides (20 µM). The level of viral replication was determined 2 days later by $beta$ -gal assay. Maximal viral replication (100%) was measured in the absence of any peptide. Each value represents the mean of at least three independent experiments with S.D. less than 10%.

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Fig. 2. Effects of p3bv on M- and T-tropic HIV-1 infections (A) and cell-cell fusion (B). A, P4-CCR5 cells were infected with different HIV-1 strains in the presence of different concentrations of p3bv. HIV-1_ADA and HIV-1_YU2 were used as prototypes of M-tropic HIV-1 strains (R5 viruses), HIV-1_BRU and HIV-1_HXB2 were used as prototypes of T-tropic HIV-1 strains (X4 viruses). The level of viral replication was determined 2 days later by $beta$ -gal assay. Maximal viral replication (100%) was measured in the absence of peptide. B, the syncytia formation was analyzed using 293 cells cotransfected with the plasmids coding for HIV-1_HXB2 gp120 and HIV-1 Tat protein. The next day, the 293-transfected cells were mixed with P4 cells in the absence or presence of various concentrations of the p3bv peptide, and the level of cell-cell fusion was estimated 48 h later by a $beta$ -gal assay, as described under Materials and Methods. Results are representative of two independent experiments with S.D. less than 10%.

A second set of peptides related to p3bv was then designed (Fig. 3A). Since p3bv contains two cysteines, this peptide possiblyforms a dimer, and thereby interferes with HIV-1 replication.To address this possibility, we designed a new peptide calledp3bvS in which the two cysteines are replaced by serines. Thispeptide has the same antiviral activity as p3bv (Fig. 3B), indicatingthat p3bv presumably acts as a monomer to inhibit HIV-1 replication.We next designed three small peptides of nine residues, correspondingto the N-terminal (p3bv1), middle (p3bv2), and C-terminal (p3bv3)part of p3bv (Fig. 3A). Of these three peptides, p3bv1 that containsthe N-terminal sequence of p3bv (residues 21-29) displays thestrongest antiviral activity (ID₅₀ = 8 µM, data not shown), indicatingthat the N-terminal sequence of p3bv is crucially involved inantiviral activity (Fig. 3B). Since the N-terminal sequence ofp3bv is in close vicinity to the Ca²⁺-binding loop of bvPLA₂ (Scott et al., 1990

), we designed a largerpeptide called pCa (residues 6-35; Fig. 3A) that, in additionto p3bv, contains residues forming the Ca²⁺-binding domain of bvPLA₂ (Scott et al., 1990

). Furthermore, sincethe Ca²⁺-binding loop of bvPLA₂ contains a disulfide bond that links thecysteines 9 and 31 (Fig. 1A), we synthesized both oxidized (pCa)and reduced (pCa.r) forms of this peptide and assayed them forHIV-1 inhibition. As shown in Fig. 3B, only pCa.r is able to inhibitHIV-1_BRU replication, indicating that pCa has to be reduced toacquire an active conformation. pCa.r was found to inhibit theviral replication with an ID₅₀ value of 4 µM (data not shown).This value is very similar to that measured for p3bv, suggestingthat the 15 N-terminal residues composing the Ca²⁺-loop of bvPLA₂ do not play a critical role in the antiviral activity.

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Fig. 3. Antiviral effects of the peptides derived from p3bv. A, amino acid sequence and position of the different peptides. The disulfide bond between cysteines 9 and 31 in pCa peptide is indicated by a plain. Numbers in parentheses indicate the position of each peptide within the bvPLA₂ sequence. B, anti-HIV-1 effects of the peptides shown in A. P4-CCR5 cells were infected with HIV-1_BRU in the absence or presence of peptide (20 µM) for a single round of replication as indicated in the legend to Fig. 1. pCa.r was obtained after a treatment at 56°C during 30 min in the presence of 50 mM dithiothreitol. Each value represents the mean of at least three independent experiments with S.D. less than 10%.

p3bv Prevents Cell-Cell Fusion and Acts Early during the Viral Cycle. The possible effect of p3bv on the inhibition of fusion between viral and cellular membranes was evaluated using syncytiumformation assay. As shown in Fig. 2B, p3bv inhibits the cell-cellfusion process between 293 cells expressing a viral envelope proteinfrom an X4 virus (HIV-1_HXB2) and P4 cells. Interestingly, theconcentrations of p3bv that inhibit the fusion process are verysimilar to those required for inhibition of infection, both phenomenashowing identical ID₅₀ values of 2 µM (Fig. 2B). Conversely, p8bv,devoid of antiviral activity (Fig. 1B), is unable to prevent theformation of syncytia (data not shown), indicating a specificeffect of p3bv on the cell-cell fusion process. This result alsoindicates that p3bv may act in an early step during the viralcycle by preventing the fusion between viral and cell membranes.This view was confirmed by time-of-addition experiments indicatingthat p3bv acts early during the HIV-1 cycle with a half-time effectof about 1.5 h (data notshown).

Inhibition of SDF-1 $alpha$ and 12G5 mAb Binding to CXCR4 by p3bv. Since p3bv specifically inhibits the replication of X4 viruses and yet has no effect on the replication of R5 viruses, itwas possible that this peptide interacts with CXCR4, the majorcoreceptor of X4 viruses. This possibility was addressed by firstanalyzing the inhibitory effect of p3bv on the binding of ¹²⁵I-SDF-1 $alpha$ to CXCR4. Specific SDF-1 $alpha$ binding was observed in CEMcells, and unlabeled SDF-1 $alpha$ was found to inhibit the binding of¹²⁵I-SDF-1 $alpha$ with a high affinity of 6 nM (Fig. 4A), similar to thatpreviously measured for the interaction of ¹²⁵I-SDF-1 $alpha$ to the CXCR4 receptor (Crump et al., 1997). Interestingly,p3bv was also able to inhibit the binding of ¹²⁵I-SDF-1 $alpha$ with a K_0.5 value close to 2 µM (Fig. 4A), indicatingthat p3bv binds to CXCR4 receptors. This result appeared in markedcontrast with bvPLA₂, which was unable to inhibit the bindingof ¹²⁵I-SDF-1 $alpha$ (Fig. 4A) even at concentrations up to 10 µM. Furthermore,competition binding experiments between radiolabeled sPLA₂ (Fenardet al., 1999) and unlabeled peptide (up to 10 µM) indicate thatp3bv does not compete with sPLA₂ binding (data not shown). Thisresult suggests that the binding sites of p3bv and sPLA₂ are distinct.To further demonstrate that p3bv binds to CXCR4, we analyzed theeffects of this peptide on the binding of 12G5, a mAb specificfor CXCR4. The binding of 12G5, as measured by FACS analysis,was completely inhibited by p3bv (Fig. 4B), confirming that p3bvbinds to CXCR4 receptors. The effect of p3bv on 12G5 antibodyis specific, since it does not prevent the binding of W6/32, amAb known to recognize the human leukocyte antigen class I surfaceantigen (Fig. 4B). Finally, the binding of 12G5 is also inhibitedby pCa.r, which has antiviral activity, but not by the oxidizedform of pCa and by the p8bv peptide, which has no effect on HIV-1infection (Figs. 3 and 4B). A possible effect of p3bv on the down-regulationof CXCR4 was analyzed by flow cytometry using two mAbs (6H8 and12G5) that recognize different surface-exposed epitopes of CXCR4.6H8 mAb is known to be specific for the N terminus of CXCR4 (Tiltonet al., 2000) and shows only borderline interference with SDF-1 $alpha$ or p3bv binding (Fig. 5; Tilton et al. 2000). On the other hand,both ligands compete with 12G5 mAb. As shown in Fig. 5, p3bv doesnot induce CXCR4 down-regulation since, in the presence of a saturatingamount of this peptide, the surface expression of CXCR4 is notmodified when detected with 6H8 mAb. On the contrary, SDF-1 promotesa rapid down-regulation of CXCR4 (Fig. 5). Taken together, theseresults suggest that the p3bv peptide specifically interacts withCXCR4, but does not promote its down-regulation, and that thisinteraction is responsible for the inhibition of X4 HIV-1 strains.

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Fig. 4. Effects of p3bv and bvPLA₂ on binding of ¹²⁵I-SDF-1 $alpha$ and 12G5 mAb to CXCR4. A, inhibition of ¹²⁵I-SDF-1 $alpha$ binding to CEM cells by p3bv and bvPLA₂. CEM cells (4 × 10⁵ cells/ml) were incubated with iodinated SDF-1 $alpha$ (50 pM) in the absence or presence of various concentrations of unlabeled SDF-1 $alpha$ , p3bv, or bvPLA₂. After 1 h, incubations were layered onto a cushion of fetal bovine serum, centrifuged, and the radioactivity associated with cellular pellets was counted. B, inhibition of 12G5 binding to CXCR4. CEM cells (5 × 10⁶ cells/ml) were incubated for 45 min at 4°C in the absence or presence of each peptide (20 µM) or SDF-1 (250 nM). The monoclonal antibodies 12G5 or W6/32 (5 µg/ml) were then added for 30 min. After several washes, the binding of antibodies was detected using an FITC-conjugated secondary antibody. The percentage of positive cells was determined using a FACS scan analyzer. Results are representative of three different experiments with S.D. less than 10%.

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Fig. 5. Effect of p3bv on the down-regulation of CXCR4. CEM cells were incubated at 37°C in RPMI 1640 medium supplemented with 5% fetal calf serum in the presence of 10 nM SDF-1 $alpha$ (filled symbols) or 20 µM p3bv (open symbols) for the indicated times. Cell surface-exposed CXCR4 was detected with mAb 12G5 (circles) or mAb 6H8 (squares). mAb 6H8, but not mAb 12G5, recognizes the NH₂ terminus of CXCR4 and shows only borderline interference with SDF-1 $alpha$ binding. Cells were then stained using FITC-conjugated goat anti-mouse IgG and detected with a FACScan flow cytometer. The percentage of CXCR4 surface expression was calculated from the relative fluorescence intensity. Results are representative of at least three independent determinations.

	Discussion

Top Abstract Introduction Materials and Methods Results Discussion References

Various peptides and small molecules have been previously described for their ability to block HIV replication through bindingto CXCR4 (Doranz et al., 1997; Murakami et al., 1997b; Scholset al., 1997). These molecules act by inhibiting the binding ofgp120 to CXCR4 or by down-regulating the expression of CXCR4.We describe here a novel peptide called p3bv, which inhibits HIV-1replication through binding to CXCR4 with an ID₅₀ value closeto 2 µM. Furthermore, we show that p3bv does not induce down-regulationof CXCR4. This result indicates that p3bv probably blocks HIV-1replication by preventing the interaction between CXCR4 and viralcomponents (i.e., the HIV-1 envelopeprotein).

The p3bv peptide is derived from bvPLA₂, which was previously described as a very potent inhibitor of replication of variousHIV-1 isolates (Fenard et al., 1999). However, p3bv appears asa weaker inhibitor than bvPLA₂, since the ID₅₀ value of bvPLA₂is close to 0.6 nM (Fenard et al., 1999). The relatively weakID₅₀ value of p3bv does not appear to result from rapid uptakeor degradation of the peptide, since pretreatment of cells withp3bv for up to 6 h before virus addition results in similar levelsof HIV-1 inhibition compared with experiments performed withoutpretreatment (data not shown). This result also confirms thatp3bv does not induce down-regulation ofCXCR4.

Unexpectedly, we found that p3bv behaves differently than bvPLA₂. Indeed, p3bv can only inhibit the replication of X4 viruses,whereas bvPLA₂ is able to inhibit both X4 and R5 viruses (Fenardet al., 1999). Furthermore, p3bv inhibits cell-cell fusion (Fig.2), whereas bvPLA₂ was previously shown to be unable to inhibitcell-cell fusion under similar experimental conditions (Fenardet al., 1999). Finally, as monitored by the interaction of SDF-1 $alpha$ and 12G5 antibody with CXCR4, p3bv appears to be a ligand forCXCR4 (Fig. 4). This result appears in marked contrast with bvPLA₂,which is unable to inhibit the binding of SDF-1 $alpha$ (Fig. 4A) and12G5 (data not shown) even at high concentrations up to 10 µM.Taken together, these differences suggest that the mechanismsof HIV inhibition by bvPLA₂ and p3bv are distinct. Alternatively,these discrepancies suggest that the mechanism of HIV-1 inhibitionby bvPLA₂ is a complex process involving multiple steps that cannotbe solely explained by the binding of p3bv to the CXCR4coreceptor.

In our previous study, we have shown that the mechanism of antiviral activity by bvPLA₂ is presumably linked to a high-affinitybinding of the sPLA₂ to host cells (K_0,5 = 0.08 nM) (Fenard etal., 1999). Our above results indicate that bvPLA₂ has no affinityfor CXCR4, and thus this receptor is probably not the primarycellular target of bvPLA₂. CXCR4, however, appears to bind p3bvderived from bvPLA₂, and this binding is most likely explainedby the HIV-1 inhibitory effect of this peptide. This suggeststhat within the bvPLA₂, the p3bv region does not have the sameconformation as that of the synthetic p3bv peptide. This hypothesisis supported in part by the fact that the reduced, but not oxidized,form of pCa inhibits HIV-1 infection and binding to CXCR4, illustratingthe importance of the conformation of the p3bv region (Figs. 3and 4).

The crystal structure of bvPLA₂ indicates that the most active part of the p3bv peptide (i.e., the p3bv1 peptide) is locatedwithin a surface loop that is likely to be conformationally flexible.This surface loop is close to the interfacial recognition surface,membrane lipids (Scott et al., 1990), and also to the residuesthat have been involved in the binding of bvPLA₂ to rat brainN-type sPLA₂ receptors (Nicolas et al., 1997). Since the high-affinitysPLA₂ binding sites found in HIV-1 host cells appear related torat brain N-type sPLA₂ receptors (Fenard et al., 1999), it ispossible that bvPLA₂ first binds to its primary target throughresidues that are close to the p3bv1 peptide loop and then conformationalchanges occur, allowing the sPLA₂ to interact with other cellularor viral targets. In particular, this primary binding may changethe conformation of the p3bv1 region, which in turn can interactwith the CXCR4 receptor. Another possibility could be that thebvPLA₂ is internalized and degraded after its high-affinity bindingto host cells and that this degradation generates bvPLA₂-derivedpeptides, such as the p3bv peptide. Interestingly, a region thatis very similar to p3bv has been identified as a specific epitopefor T cells after immunization with bvPLA₂ (Mori et al., 1993).

In conclusion, here we describe a novel peptide called p3bv that is derived from bvPLA₂ and inhibits T-tropic, but not M-tropicHIV-1, through its binding to CXCR4. Our results, however, suggestthat the mechanisms of HIV inhibition by the p3bv peptide areprobably different from the original bvPLA₂ complete protein.Comparisons of the antiviral properties of p3bv with those ofbvPLA₂ suggest that the mechanism of inhibition of HIV-1 by bvPLA2is a more complex process, which may involve several steps andvarious bvPLA₂ domains distinct from p3bv that can act separatelyor in concert to inhibit entry of X4 and R5 viruses into hostcells. Finally, the recent identification of a novel human sPLA₂that belongs to group III sPLA₂s and displays a significant homologywith bvPLA₂, in particular in the p3bv peptide region (Valentinet al., 2000), suggests a role of this type of sPLA₂ in HIV infection.Whether this human sPLA₂ has an antiviral activity similar tobvPLA₂ will be particularly interesting to analyze in thefuture.

	Acknowledgments

We are very grateful to Professor M. Lazdunski for a critical review of this manuscript and very fruitful discussions. Wethank P. Rochet for expert technical assistance. We are also gratefulto P. Charneau, N. Israel, the NIH AIDS Research and ReferenceReagent Program for the generous gifts of the various plasmidsand cell lines, and Y. Chvatchko for providing us with a firstset of bvPLA₂ peptides. Special thanks are also due to Dr. FernandoArenzana-Seisdedos for supplying the 6H8antibody.

	Footnotes

Received November 28, 2000; Accepted May 4, 2001

This work was supported by the Centre National de la Recherche Scientifique, the BV Foundation Limited, the Association pourla Recherche sur le Cancer, and the Ministère de la DéfenseNationale (Grant DGA-DRET 96/096). D. Fenard is a recipient ofa grant from Sidaction (Paris,France).

Dr. Alain Doglio, Laboratoire de Virologie, INSERM U526, Faculté de Médecine, Avenue de Valombrose, 06107 Nice Cedex 2, France. E-mail: doglio{at}unice.fr

	Abbreviations

HIV, human immunodeficiency virus; CCR, CC chemokine receptor; CXCR, CXC chemokine receptor; gp120, HIV-1 envelope glycoprotein; pCa.r, reduced form of pCa; sPLA₂, secreted phospholipase A₂; bvPLA₂, bee venom sPLA₂; AIDS, acquired immunodeficiency syndrome; mAb, monoclonal antibody; $beta$ -gal, $beta$ -galactosidase; FITC, fluorescein isothiocyanate; FACS, fluorescence-activated cell sorter; SDF, stromal cell-derived factor; T-tropic, T-lymphotropic; M-tropic, monocytotropic.

	References

Top Abstract Introduction Materials and Methods Results Discussion References

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