CXCR-4 Is Expressed by Primary Macrophages and Supports CCR5-Independent Infection by Dual-Tropic but Not T-Tropic Isolates of Human Immunodeficiency Virus Type 1

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J Virol, January 1998, p. 772-777, Vol. 72, No. 1
0022-538X/98/$04.00+0
Copyright © 1998, American Society for Microbiology. All rights reserved.

CXCR-4 Is Expressed by Primary Macrophages and Supports CCR5-Independent Infection by Dual-Tropic but Not T-Tropic Isolates of Human Immunodeficiency Virus Type 1

Yanjie Yi,¹ Shalini Rana,¹ Julie D. Turner,² Nathan Gaddis,¹ and Ronald G. Collman¹^,^*

Divisions of Pulmonary and Critical Care¹ and Hematology-Oncology,² Department of Medicine, University of Pennsylvania School of Medicine, Philadelphia, Pennsylvania 19104

Received 20 August 1997/Accepted 1 October 1997

	ABSTRACT

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Primary macrophages are infected by macrophage (M)-tropic but not T-cell line (T)-tropic human immunodeficiency virus type1 (HIV-1) strains, and CCR5 and CXCR-4 are the principal cofactorsutilized for CD4-mediated entry by M-tropic and T-tropic isolates,respectively. Macrophages from individuals homozygous for an inactivatingmutation of CCR5 are resistant to prototype M-tropic strains thatdepend on CCR5 but are permissive for a dual-tropic isolate, 89.6,that can use both CCR5 and CXCR-4, as well as CCR2b, CCR3, andCCR8. Here we show that 89.6 entry into CCR5-deficient macrophagesis blocked by an anti-CXCR-4 antibody and by the CXCR-4-specificchemokine SDF but not by the ligands to CCR2b or CCR3. Reversetranscription-PCR demonstrated expression of CXCR-4 but not CCR3or CCR8 in macrophages, while CCR2b was variable. Macrophage surfaceexpression of CXCR-4 was confirmed by immunofluorescence stainingand flow cytometry. Thus, CXCR-4 is expressed by primary macrophagesand functions as a cofactor for entry by dual-tropic but not T-tropicHIV-1 isolates, and macrophage resistance to T-tropic strainsdoes not result from a lack of the T-tropic entry cofactor CXCR-4.Since CXCR-4 on macrophages can be used by some but not otherisolates, these results indicate that HIV-1 strains differ inhow they utilize chemokine receptors as cofactors for entry andthat the ability of a chemokine receptor to mediate HIV-1 entrydiffers, depending on the cell type in which it is expressed.

	TEXT

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Macrophage (M)-tropic human immunodeficiency virus type 1 (HIV-1) strains infect primary macrophages and lymphocytes but notCD4⁺ transformed cell lines, while T-cell line (T)-tropic HIV-1 strainsinfect lymphocytes and cell lines but not macrophages. The chemokinereceptors CCR5 and CXCR-4 are the principal cofactors that enableentry by M-tropic and T-tropic strains, respectively, when introducedalong with CD4 into otherwise nonpermissive cells (8, 17,19, 20, 22). Certain dual-tropic strains that infect macrophages,lymphocytes, and transformed cell lines can utilize both CXCR-4and CCR5 (19, 46). Target cell tropism is largely determinedat the level of virus entry and is encoded mainly by the HIV-1env gene (4, 34, 43). The reciprocal patterns of cofactoruse by M-tropic and T-tropic strains suggest a simple model forthe cellular determinants of tropism in which CCR5 would be expressedby macrophages, CXCR-4 would be expressed by transformed celllines, and both would be expressed by lymphocytes. Whether thisis accurate, however, remains to be determined.

Several molecules in addition to CCR5 and CXCR-4 also support entry by more restricted subsets of HIV-1 isolates. These includeCCR3, CCR2b, and a growing list of known or putative chemokinereceptors, such as CCR8 (also known as chemR1), the cytomegalovirusreceptor US28, and others (8, 15, 19, 38, 40). Mosthave been identified in heterologous transfection-based systems,however, and defining their role in the infection of native targetcells is critical for understanding HIV-1 pathogenesis and developingtherapeutic agents targeted at cofactor-mediated viral entry.

Recently, a mutant allele of the CCR5 gene (ccr5 $Delta$ 32) was identified that encodes a truncated protein which is not expressedon the cell surface and cannot support HIV entry (16, 28,42). Individuals homozygous for ccr5 $Delta$ 32 are resistant to HIV-1infection, and lymphocytes and macrophages from these individualsare resistant to infection with M-tropic HIV-1 isolates (14,16, 28, 39, 42). Although resistance in vivo is incomplete(1), this nevertheless shows that CCR5 is the principal entrycofactor used in primary macrophages and lymphocytes by prototypeM-tropic strains and confirms the critical role of CCR5-dependentM-tropic strains in person-to-person HIV-1 transmission. The presenceof this naturally occurring CCR5 knockout model also offers theopportunity to examine pathways other than CCR5 that may be utilizedby certain viruses for entry into primary target cells.

HIV-1 89.6 is a dual-tropic primary isolate that infects both macrophages and some transformed cell lines (9) and can useboth CCR5 and CXCR-4 as cofactors for entry, as well as CCR3,CCR2b, and CCR8 (19, 39, 40). While primary macrophagesderived from ccr5 $Delta$ 32-homozygous individuals are resistant to infectionwith most M-tropic prototype HIV-1 isolates, we recently foundthat these cells were permissive for strain 89.6 (39). We havedemonstrated 89.6 replication in CCR5-deficient macrophages fromeach of six ccr5 $Delta$ 32-homozygous donors tested (data not shown).To address mechanisms of entry into macrophages in addition toCCR5, and to better understand how different HIV-1 strains utilizeentry cofactors in primary cells, we sought to identify the pathwayused by 89.6 for entry into CCR5-deficient macrophages.

CCR5-independent, CD4-dependent infection of primary macrophages. To be sure that infection of CCR5-deficient macrophages by strain 89.6 reflected a CD4-mediated entry pathway and not a distinctmechanism independent of CD4, we tested whether infection wouldbe inhibited by blocking CD4 (Fig. 1). The CCR5 genotypes of blooddonors were determined by PCR (39), and macrophages were isolatedfrom peripheral blood mononuclear cells by a stringent two-stepselective adherence procedure and maintained in culture as previouslydescribed (11, 39). After 1 week in culture, the macrophageswere infected overnight with equal amounts of cell-free virusstocks based on p24 antigen content, washed, and sampled periodicallyby enzyme-linked immunosorbent assay (Dupont, Wilmington, Del.)for p24 antigen production. Cells infected with 89.6 were incubatedfor 1 h prior to and throughout the infection with an anti-CD4monoclonal antibody (MAb), no. 19 (21), or with a control MAb,B33.1 (10).

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FIG. 1. HIV-1 replication in normal and CCR5-deficient macrophages. Monocytes were isolated from individuals homozygous for the wild-type CCR5 allele or ccr5 $Delta$ 32, plated at 2 × 10⁵ per well in 48-well plastic tissue culture plates, and allowed to differentiate into macrophages in vitro. After 7 days in culture they were infected overnight with 20 ng of p24 antigen of M-tropic (SF162 or ADA), T-tropic (NL43), or dual-tropic (89.6) strains. Cultures were then washed, and the supernatant was sampled periodically for p24 antigen. Cells infected with 89.6 were incubated for 1 h prior to and during infection with the anti-CD4 MAb no. 19 or the control MAb B33.1 (each at 10 µg/ml), which was then maintained in the medium throughout the experiment.

As shown in Fig. 1, 89.6 infection of both normal and CCR5-deficient macrophages was blocked by the anti-CD4 MAb but not bythe control MAb. Thus, infection of primary macrophages in theabsence of functional CCR5 requires CD4 and does not result froma fundamentally different, CD4-independent entry mechanism. Asexpected, the prototype M-tropic strain SF162 infected wild-typebut not CCR5-deficient macrophages (Fig. 1).

In addition to CCR5 and CXCR-4, 89.6 can also utilize the chemokine receptors CCR3, CCR2b, and CCR8 (also known as chemR1)for entry (19, 25, 40). We showed previously that macrophageslacking functional CCR5 were not permissive for the M-tropic strainYU-2, which can use both CCR3 and CCR5, suggesting that CCR3 wasnot involved in CCR5-independent entry (8, 39). Here we testedthe M-tropic strain ADA, which can use both CCR8 and CCR3 in additionto CCR5 (8, 40). ADA also failed to replicate in macrophageslacking functional CCR5 (Fig. 1). These results suggest that 89.6infection of CCR5-deficient macrophages is unlikely to resultfrom utilization of either CCR3 or CCR8.

No replication by the T-tropic strain NL43 (Fig. 1) or several other T-tropic isolates (data not shown) was seen in eitherwild-type or ccr5 $Delta$ 32-homozygous macrophages. Since T-tropic strainsreplicate efficiently in lymphocytes even in the absence of CCR5(14, 28, 39), this confirmed that our macrophage cultureswere not significantly contaminated with T cells and that 89.6replication did not result from infection of contaminating lymphocytes.The lack of NL43 replication in CCR5-deficient macrophages alsoindicates that the absence of functional CCR5 in macrophages doesnot lead to enhanced permissiveness for T-tropic HIV-1 strains.

Detection of chemokine receptor-specific RNA in macrophages. To determine which chemokine receptors used by 89.6 might be involved in entry independent of CCR5, we carried out reversetranscription-PCR (RT-PCR) on RNA from purified monocyte-derivedmacrophages with primers that detect CCR5, CXCR-4, CCR3, CCR2b,and CCR8 (chemR1), as well as CD4 (Fig. 2). RNA was extractedfrom 7-day-old macrophage cultures with TRIZOL-LS (GIBCO-BRL,Grand Island, N.Y.) and incubated with RNase-free DNase I (30min at 37°C in the presence of 5 mM MgCl₂) to eliminate any residualgenomic DNA, and DNase was inactivated by the addition of EDTA(5 mM) and heating (65°C for 10 min). rTth polymerase (Perkin-Elmer,Emeryville, Calif.) was used for both reverse transcription andPCR amplification as directed by the manufacturer, using specificantisense primers for reverse transcription and 45 cycles of PCRamplification. Sense (S) and antisense (A) primers used were asfollows: CCR5-S (5'-CGTCTCTCCCAGGAATCATCTTTAC-3') and CCR5-A (5'-TTGGTCCAACCTGTTAGAGCTACTG-3'),which yield a 356-bp CCR5 product; CXCR4-S (5'-GAACTTCCTATGCAAGGCAGTCC-3')and CXCR4-A (5'-CCATGATGTGCTGAAACTGGAAC-3'), which amplify a 304-bpCXCR-4 product; CD4-S (5'-GCAATTGCTAGTGTTCGGATTGA-3') and CD4-A(5'-GTCAGCTTTTCAACTGTAAAGGCG-3'), which yield a 347-bp CD4 product;CCR2-S (5'-GCGGAATCTTCTTCATCATCCTC-3') and CCR2-A (5'-CCTCTTCTTCTCGTTTCGACACC-3'),which yield a 338-bp CCR2b product; CCR3-S (5'-AGCTGGAGGCATTTCCACACTC-3')and CCR3-A (5'-TTCATGCAGCAGTGGGAGTAGG-3'), which yield a 311-bpCCR3 product; and CCR8-S (5'-TCCATGCCGTGTATGCCC-3') and CCR8-A(5'-CCACGTTGAATGGGACCC-3'), which yield a 363-bp CCR8 product.Specificity of the primers was confirmed with plasmid DNA, DNAextracts of human and nonhuman cells, and RNA extracts of cellsexpressing specific chemokine receptors (17), and the identityof RT-PCR products was also verified in selected experiments bySouthern blotting with specific internal oligonucleotide probes(data not shown).

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FIG. 2. RT-PCR detection of chemokine receptor expression in macrophages. RNA was extracted from 7-day-old macrophage cultures and subjected to reverse transcription and PCR amplification for CCR5, CXCR-4, CCR3, CCR8 (chemR1), and CCR2b, as well as CD4. Products were separated on agarose gels and stained with ethidium bromide. Macrophages from a CCR5 wild-type-homozygous donor are shown, and the same pattern was seen with cells from ccr5 $Delta$ 32-homozygous donors. Amplification was done following reverse transcription with (+) or without ( $-$ ) reverse transcription enzyme present. m, molecular size standards.

As expected, RT-PCR signals for CD4 and CCR5 were detected in macrophages (Fig. 2). Surprisingly, we also saw a strong signalfor CXCR-4. This was consistent among macrophages from multiplewild-type- and ccr5 $Delta$ 32-homozygous donors. We confirmed that thissignal represented RNA and not cellular DNA contamination, sinceno band was seen if reverse transcription was omitted prior toPCR (Fig. 2). In addition, the amplified band was verified asCXCR-4 by Southern blotting with a CXCR-4-specific internal oligonucleotideprobe (data not shown).

In contrast to CXCR-4, neither CCR3 nor CCR8 (chemR1) yielded an RT-PCR signal in macrophages. Based on serial dilutions ofplasmid DNA, the primer pairs can detect 20 cDNA molecules forCCR8 and 2,000 cDNA molecules for CCR3 (data not shown). Whenamplification for CCR2b was done, no signal was seen in most macrophagecultures (data not shown), but it did give a positive band inapproximately one-third of the donors tested (Fig. 2). Based onserial dilutions of plasmid, the CCR2b primers can detect 200molecules of cDNA (data not shown). This occasional detectionof CCR2b suggests either that there is significant donor-to-donorvariability in CCR2b expression or that the level of expressionunder these culture conditions is low and just at the thresholdof detection. Thus, CXCR-4 is the only cofactor used by 89.6,other than CCR5, that was uniformly detected in these macrophagesby RT-PCR. There were no differences in patterns of cofactor expressiondetected by RT-PCR when macrophages from homozygous wild-typeand ccr5 $Delta$ 32 donors were compared (data not shown).

CXCR-4 is present on the surface of primary monocyte-derived macrophages. Expression of CXCR-4 RNA by primary macrophages was somewhat unexpected, since these cells are resistant to infection by CXCR-4-dependentT-tropic HIV-1 isolates. Therefore, to determine whether CXCR-4protein was present on the cell surface, we carried out immunofluorescencestaining with the anti-CXCR-4 MAb 12G5 (21). One-week-old culturedmacrophages were detached with EDTA (1 mM for 5 min) and gentlescraping, suspended in staining buffer (SB) (phosphate-bufferedsaline with 1 mg of bovine serum albumin/ml and 0.02% sodium azide),and incubated for 30 min with 5% rat serum and 5% rabbit serum.They were then stained for 30 min with murine MAbs diluted inSB, washed, and incubated for 30 min with fluorescein isothiocyanate-conjugatedgoat anti-mouse immunoglobulin G (Biosource, Camarillo, Calif.)diluted 1:200 in SB supplemented with 50% fetal bovine serum.The cells were washed again, fixed with 4% paraformaldehyde, andanalyzed by flow cytometry. All incubations were carried out at4°C. The MAbs used were as follows: 12G5 (6 µg/ml) to detect CXCR-4,no. 19 (10 µg/ml) to detect CD4, OKT3 (diluted 1:10) to stainT lymphocytes, and OKM1 (diluted 1:10) to stain macrophages. Amajor histocompatibility complex class I MAb was used as a positivecontrol (w6/32; 1:10 dilution of hybridoma supernatant), and anirrelevant MAb directed against HIV-1 gp120 (D47; 10 µg/ml) servedas a negative control that was isotype matched with 12G5 and no.19. OKT3 and OKM1 were obtained from Ortho Diagnostic Systems(Raritan, N.J.); 12G5, no. 19, and w6/32 (21, 35) were providedby J. Hoxie (University of Pennsylvania); and D47 (5) was providedby R. Doms (University of Pennsylvania). In parallel we examinedthe CD4⁺ T-cell line SUP-T1, which is highly permissive for CXCR-4-dependentstrains. As shown in Fig. 3, staining with OKM1 and OKT3 demonstratedhighly purified macrophages that were devoid of contaminatingT cells. This level of purity also indicates that our detectionof CXCR-4 in the macrophage cultures by RT-PCR was unlikely tobe the result of lymphocyte contamination.

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FIG. 3. Macrophage surface expression of CXCR-4 by flow cytometry. Seven-day-old cultures of monocyte-derived macrophages (MDM) were detached and stained with MAbs for major histocompatibility complex class I as a positive control (w6/32), a T-cell marker (OKT3), a macrophage marker (OKM1), CD4 (#19), and CXCR-4 (12G5). Cells were then analyzed by flow cytometry with a minimum of 10⁴ cells. Specific MAb profiles are indicated by the black histogram, and the negative control antibody is shown as the shaded histogram in each graph. Macrophages from a CCR5 wild-type-homozygous donor are shown and are representative of cells from six different donors. The same patterns were seen with cells from ccr5 $Delta$ 32-homozygous donors. The SUP-T1 cell line was stained in parallel.

CXCR-4 staining of macrophages with MAb 12G5 revealed a population with a single peak that was clearly positive compared withthe control MAb (Fig. 3). This was confirmed with macrophagesfrom six donors and verified with two isotype-matched negativecontrol MAbs (data not shown). Background fluorescence after stainingwith the negative control antibody was generally higher in macrophagesthan in SUP-T1 cells, as described previously (10). Nevertheless,the mean channel fluorescence for 12G5 in macrophages from sixdonors was consistently twice that of the negative control MAb(mean ± standard error of the mean, 28.3 ± 3.8 for 12G5 comparedwith 14.4 ± 2.3 for the control MAb). This contrasts with SUP-T1cells, for which the 12G5 mean channel fluorescence was considerablyhigher than that of the negative control MAb (118 ± 24 for 12G5versus 6.99 ± 1.02 for the control). With a stringent cutoff todetermine positive staining (a fluorescence level greater than99% of the cells stained with the isotype-matched negative controlMAb), (11.3 ± 2.6)% of macrophages were positive for CXCR-4 (range,5.3 to 23.3%) compared to (85.3 ± 5.3)% of SUP-T1 cells. Thus,fluorescence-activated cell sorter analysis revealed CXCR-4 onthe surface of primary macrophages, although the level of expressionwas low compared to that of transformed cell lines. The same patternof staining for CXCR-4, CD4, and other markers was seen with macrophagesderived from CCR5 wild-type- and ccr5 $Delta$ 32-homozygous individuals(data not shown).

Entry into macrophages lacking CCR5 is inhibited by blocking CXCR-4. Because these studies revealed both CXCR-4 gene expression and protein on the surface of macrophages but no CCR3 or CCR8 andinconsistent CCR2b expression, we next examined whether CCR5-independententry into macrophages could be inhibited by agents directed againstCXCR-4 or other potential cofactors. Entry was determined by PCRdetection of viral DNA with primers directed at early reversetranscription products. One-week-old cultures of macrophages wereinfected as described above with the M-tropic strain SF162, theT-tropic strain NL43, and the dual-tropic isolate 89.6, usingDNase-treated (50 U/ml for 30 min at room temperature) cell-freevirus stocks. To test for blocking, cells were incubated for 1h prior to and throughout the infection with the anti-CXCR-4 MAb12G5, the anti-CD4 MAb no. 19, or the control MAb B33.1 (all at10 µg/ml) or with specific chemokines (Peprotech, Rocky Hill,N.J.). The chemokines MCP-1, MCP-3, and eotaxin were used at 1µg/ml and SDF was used at 2.5 µg/ml (2, 24, 33). Two daysafter infection the cells were lysed and amplified with primersthat detect conserved regions of the HIV-1 long terminal repeat(LTR), followed by Southern blotting. The LTR primers, PCR amplificationconditions, and Southern blotting protocol have been describedpreviously (19).

In agreement with the replication data shown in Fig. 1, SF162 entered wild-type macrophages but not CCR5-deficient macrophageswhile 89.6 entered both normal and CCR5-deficient macrophages(Fig. 4). The T-tropic strain NL43 failed to generate viral DNAin either wild-type or CCR5-deficient macrophages (Fig. 4), whichindicates that NL43 is blocked in macrophages at an early stageof infection, consistent with entry. This also confirms that theabsence of functional CCR5 in macrophages does not result in enhancedentry by T-tropic isolates. Entry by both 89.6 and SF162 was blockedby the anti-CD4 antibody but not by a control antibody (Fig. 4),which is also consistent with the infection experiments and showsthat the PCR signals reflect actual infection and not DNA carryoverin the virus inoculum. In agreement with this, no band was seenif virus stocks were heat inactivated before infection (data notshown).

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FIG. 4. Inhibition of HIV-1 entry into normal and CCR5-deficient macrophages. Macrophages were isolated from individuals homozygous for the wild-type CCR5 allele (w/w) or the ccr5 $Delta$ 32 allele ( $Delta$ / $Delta$ ). After 7 days in culture they were infected with 20 ng of p24 antigen of the dual-tropic isolate 89.6, the T-tropic strain NL43, or the M-tropic strain SF162. The indicated wells were incubated for 1 h prior to and throughout the infection with the anti-CD4 MAb no. 19 (#19), the anti-CXCR-4 MAb 12G5, or the control antibody B33.1 or with SDF, MCP-1 and MCP-3, or eotaxin. Three days after infection the cells were lysed and subjected to PCR amplification with primers that detect conserved regions of the HIV-1 LTR, followed by Southern blotting. Infections were done in duplicate and amplified in independent PCR reactions, both of which are shown. Amplification with $beta$ -globin primers showed a positive signal in all wells (data not shown). HIV plasmid DNA was used as a positive control (+) for amplification. Data are representative of replicate experiments with cells from three ccr5 $Delta$ 32-homozygous donors.

We then determined whether CCR5-independent entry into macrophages would be inhibited by agents that target specific chemokinereceptors. MAb 12G5 has been shown to block CXCR-4-mediated entryof some HIV-1 and HIV-2 strains, including 89.6 (21, 47).SDF, the chemokine ligand for CXCR-4, also blocks CXCR-4-mediatedentry by 89.6 and other isolates (2, 33). We also examinedMCP-1 and MCP-3, which are the ligands for CCR2b, and eotaxin,which is the ligand for CCR3 and can block CCR3-mediated infection(24). As shown in Fig. 4, entry of 89.6 into CCR5-deficientmacrophages was inhibited by both 12G5 and SDF. Thus, specifictargeting of CXCR-4 prevented CCR5-independent infection of macrophagesby strain 89.6, and this indicates that CXCR-4 is the cofactorutilized by 89.6 for CD4-mediated entry into these cells. In contrast,no evidence was seen to suggest a role for CCR2 or CCR3, sinceneither MCP-1 and MCP-3 nor eotaxin blocked infection (Fig. 4).As expected, neither SDF nor 12G5 blocked infection of macrophagesexpressing wild-type CCR5, indicating that the inhibition seenin ccr5 $Delta$ 32-homozygous macrophages did not result from a nonspecificeffect of the chemokine or antibody on macrophages (Fig. 4).

Significance of CXCR-4-mediated infection of macrophages. The discovery that distinct entry cofactors are used by M-tropic and T-tropic HIV-1 variants initially suggested that tropismcould be easily explained by cell-specific distribution of CXCR-4on lymphocytes and transformed cell lines but not macrophagesand of CCR5 on primary macrophages and lymphocytes but not transformedcell lines. In this report, however, we show that tropism patternsare not explained by this simple paradigm, since the inabilityof T-tropic strains to enter and infect primary macrophages doesnot result from an absence of CXCR-4 on these target cells. Inaddition, because T-tropic strains use CXCR-4 on transformed cellsbut not on macrophages, our data also indicate that the abilityof a cofactor to support HIV-1 entry can vary markedly, dependingon the cellular context in which it is expressed. Furthermore,since CXCR-4 expressed on macrophages supports entry of 89.6 butnot T-tropic isolates, these results show that HIV-1 strains differin the way they utilize this cofactor.

The reason(s) that macrophage CXCR-4 supports entry of 89.6 but not T-tropic strains may offer important clues about the functionof these molecules or their interaction with other componentsof the cell surface. One straightforward explanation might relateto levels of expression in different cell types, combined withstrain differences in the efficiency of receptor and coreceptorutilization. Macrophages express low levels of CD4 compared tothose of other CD4-positive cell types, and our data show thatlevels of CXCR-4 immunofluorescence are also low compared withthose of T-cell lines. Recently, CD4 levels were found to havedistinct effects on entry by different HIV-1 isolates, such thatT-cell line-adapted T-tropic strains could utilize CXCR-4 in thepresence of low CD4 levels while primary T-tropic isolates requiredhigher CD4 levels (27). It is possible that in the presenceof low CD4 levels on macrophages, low levels of CXCR-4 can beused by a dual-tropic strain like 89.6 but not by T-tropic strains.A related explanation we initially considered was that a stoichiometricinteraction between CD4 and the chemokine receptor might be neededfor entry. Since CD4 levels in macrophages are low, the presenceof CCR5 might leave insufficient CD4 available to associate withthe small amount of CXCR-4 present. However, our finding thatT-tropic strains also failed to enter macrophages from ccr5 $Delta$ 32-homozygousdonors argues against this possibility.

Alternatively, CXCR-4 may be expressed in macrophages in a form different from that in lymphocytes and cell lines, resultingin utilization by some but not other isolates. Studies with chimericchemokine receptors have shown that individual HIV-1 strains interactdifferently with cofactors and that isolates rely on distinctalthough somewhat overlapping domains of the cofactors (30,36, 37, 41). It is possible, therefore, that on the surfaceof primary macrophages there are molecules associated with CXCR-4that interfere with its ability to function as a cofactor forT-tropic but not dual-tropic strains or that differences betweenmacrophages and other cells in glycosylation or other posttranslationalmodifications of CXCR-4 might affect its ability to mediate entryby some but not other strains. Supporting this possibility, theanti-CXCR-4 MAb 12G5 is able to block infection by some HIV-1strains in a manner that is both strain specific and dependenton the cell in which the cofactor is expressed (31).

While there clearly exists a general association between tropism and cofactor selectivity, these results show that cofactorutilization in heterologous cells does not necessarily predictuse in primary cell targets. Others have also identified exceptionswhere cofactor selectivity does not predict tropism (7, 18).Similarly, although the finding of CXCR-4 expression by primarymacrophages contrasts with the host range of CXCR-4-dependentT-tropic HIV-1 strains, it is consistent with several previousreports of CXCR-4 expression in monocytes or macrophages (3,29, 31) and calcium currents induced by SDF (33). Our studyextends those observations to show that CXCR-4 is expressed onmacrophages in a form that is functional as a cofactor for entryfor some HIV-1 isolates.

In addition to CCR5 and CXCR-4, some HIV-1 isolates can use a growing list of other known or putative chemokine receptorsfor entry in heterologous systems. A critical question is whichof them are involved in infection of primary cells that are relevantin vivo. CCR3 can be used by many M-tropic strains and mediatesinfection of microglia (24). In agreement with other reports(12), we found no evidence for CCR3 expression or cofactor functionin monocyte-derived macrophages. Similarly, strain 89.6 can useCCR8 (40) but we found no evidence for expression or entry cofactorfunction in these cultures. In contrast, CCR2b is well describedin macrophages (13, 44), yet we found variable and inconsistentexpression and no evidence that it was involved in CCR5-independentmacrophage infection by an isolate that uses CCR2b in transfection-basedsystems. A likely explanation is that expression levels vary underdifferent culture conditions and in these cultures there wereextremely low levels that were just at or below the thresholdof detection by RT-PCR and were insufficient to support entry.It is also possible that CCR2b utilization in heterologous systemsmay not predict entry function in primary target cells, similarto our findings involving T-tropic isolates and CXCR-4 in macrophages.

T-tropic strains were blocked in our macrophage cultures at an early stage of infection, prior to the generation of initialreverse transcription products. This points to a defect in entry,which is similar to results reported by most other laboratoriesand is supported by direct evidence that env genes derived fromM-tropic but not T-tropic strains can mediate fusion with macrophagecell membranes (4, 34). However, HIV-1 host cell tropismis relative, rather than absolute, and low-level replication inmacrophages by T-tropic strains may occasionally be seen (11).In addition, some groups have reported fusion and/or entry byT-tropic strains in macrophages despite their failure to replicate(26, 45). Our finding that CXCR-4 is present on macrophagesmay provide a means of reconciling these results. Since thereare clearly steps subsequent to entry at which replication ofeven CCR5-dependent HIV-1 and simian immunodeficiency virus strainsmay be restricted in macrophages (6, 23, 32), there maybe conditions under which CXCR-4 does mediate entry by T-tropicstrains into macrophages, but downstream events then lead to restrictedreplication.

	ACKNOWLEDGMENTS

We thank J. Hoxie, R. Smyth, D. Kolson, S. Isaacs, and G. Besson for valuable discussions and critical reading of the manuscript.We also thank the blood donors who generously provided cells;J. Hoxie, R. Doms, R. Horuk, and J. Hesselgesser for MAbs andother reagents; and C. Woods for M-CSF.

This work was supported by grants AI-35502, NS-27405, and HL-58004 from the National Institutes of Health.

	FOOTNOTES

^* Corresponding author. Mailing address: 522 Johnson Pavilion, University of Pennsylvania School of Medicine, 36th and HamiltonWalk, Philadelphia, PA 19104-6060. Phone: (215) 898-0913. Fax:(215) 662-2947. E-mail: collmanr{at}mail.med.upenn.edu.

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