WO2003072766A1 - Anti-ccr5 antibody - Google Patents

Abstract

The invention is directed an anti-CCR5 antibody which comprises (i) two light chains, each light chain comprising the expression product of a plasmid designated pVK:HuPRO140-VK (ATCC Deposit Designation PTA-4097), and (ii) two heavy chains, each heavy chain comprising an expression product of either a plasmid designated pVg1:HuPRO140 HG2-VH (ATCC Deposit Designation PTA-4098) or a plasmid designated pVgl:HuPR0140 (mutB+D+I)-VH (ATCC Deposit Designation PTA-4099) or a fragment thereof which binds to CCR5 on the surface of a human cell.

Description

ANTI-CCR5 ANTIBODY

This application is a continuation-in-part of and claims - the priority of U.S. Application Serial No. 10/081,128, filed February 22, 2002, the contents of which are hereby incorporated by reference into this application .

Throughout this application, various publications are referenced by Arabic numerals. Full citations for these publications may be found at the end of the specification immediately preceding the claims. The disclosure of these publications is hereby incorporated by reference into this application to describe more fully the art to which this invention pertains.

Background of the Invention

Human immunodeficiency virus type 1 (HIV-l) induces viral-to-cell membrane fusion to gain entry into target cells (8, 15, 66). The first high-affinity interaction between the virion and the cell surface is the binding of the viral surface glycoprotein gpl20 to the CD4 antigen (13, 30, 41, 42). This in turn induces conformational changes in gpl20, which enable it to interact with one of several chemokine receptors (4, 5, 21, 36). The CC-chemokine receptor CCR5 is the major co-receptor for macrophage-tropic (R5) strains, and plays a crucial role in the sexual transmission of HIV- 1 (4, 5, 21, 36). T cell line-tropic (X4) viruses use CXCR4 to enter target cells, and usually, but not always, emerge late in disease progression or as a consequence of virus propagation in tissue culture (4, 5, 21, 36). Some primary HIV-1 isolates are dual-tropic (R5X4) since they can use both co-receptors, though not always with the same efficiency (11, 57) . Mutagenesis studies coupled with the resolution of the gpl20 core crystal structure demonstrated that the co-receptor- binding site on gpl20 comprises several conserved residues (32, 53, 65) .

It has been demonstrated that tyrosines and negatively charged residues in the amino-terminal domain (Nt) of CCR5 are essential for gpl20 binding to the coreceptor, and for HIV-1 fusion and entry (6, 18, 20, 22, 28, 31, 52, 54). Residues in the extracellular loops (ECL) 1-3 of CCR5 were dispensable for coreceptor function, yet the CCR5 inter-domain configuration had to be maintained for optimal viral fusion and entry (24) . This led to the conclusion either that gpl20 forms interactions with a diffuse surface on the ECLε, or that the Nt is maintained in a functional conformation by bonds with residues in the ECLs . Studies with chimeric co-receptors and anti-CCR5 monoclonal antibodies have also shown the importance of the extracellular loops for viral entry (5, 54, 64) .

Molecules that specifically bind to CCR5 and CXCR4 and block interactions with their ligands are a powerful tool to further probe the structure/function relationships of the co-receptors. Characterizing such compounds could also assist in designing effective therapeutic agents that target co-receptor-mediated steps of viral entry. Inhibitors of CCR5 or CXCR4 coreceptor function identified to date are diverse in nature and include small molecules, peptides, chemokines and their derivatives, and monoclonal antibodies (mAbs) . The mechanisms of action of the small molecules that block entry by interfering with CXCR4 co-receptor function are not well understood (17, 49, 55, 68) . One such inhibitor, the anionic small molecule AMD3100, depends on residues in ECL2 and the fourth trans-membrane (TM) domain of CXCR4 to inhibit viral entry, but it is not clear whether it does so by disrupting gpl20 binding to CXCR4 or post-binding steps leading to membrane fusion (16, 34, 55) . To date, no small molecules have been reported that specifically block CCR5-mediated HIV-1 entry. Inhibition of HIV-1 entry by chemokines is mediated by at least two distinct mechanisms: blockage of the gpl20/co-receptor interaction and internalization of the chemokine/receptor complex (3, 26, 59, 63) . The variant AOP-RANTES also inhibits recycling of CCR5 to the cell surface (40, 56) . Variants such as RANTES 9-68 and Met- RANTES only prevent the gpl20/CCR5 interaction and do not down-regulate CCR5 (67) . SDF-1 variants presumably act through a similar mechanism to block viral entry mediated by CXCR4 (12, 27, 39). Only one anti-CXCR4 mAb, 12G5, has been characterized for its anti-viral properties. The efficiency of 12G5 inhibition of viral entry has been reported to be both cell- and isolate- dependent (43, 58). This mAb binds to the ECL2 of CXCR4 , but the mechanism by which it inhibits entry is unknown (7) . Few of the anti-CCR5 mAbs characterized to date efficiently prevent HIV-1 entry (28, 64). Interestingly, mAbs whose epitopes lie in the Nt domain of CCR5 , which contains the gpl20-binding site, inhibit viral fusion and entry less efficiently than mAb 2D7 , whose epitope lies in ECL2. 2D7 also antagonizes CC- chemokine activity (64).

A panel of six murine mAbs, designated PA8 , PA9 , PA10, PA11, PA12 and PA14 have been isolated and characterized. All six mAbs specifically bound to CCR5⁺ cells but with different efficiencies that were cell type-dependent . Epitope mapping studies identified the residues that are important for mAb binding and also revealed information about the folding and interactions of the CCR5 extracellular domains. All mAbs inhibited HIV-1 fusion and entry, but there was no correlation between the ability of a mAb to inhibit fusion and entry and its ability to inhibit binding of gpl20/sCD4 to CCR5^* cells. Summary of the Invention:

This invention provides an anti-CCR5 antibody which comprises (i) two light chains, each light chain comprising the expression product of a plasmid designated pVK:HuPRO140-VK (ATCC Deposit Designation PTA-4097), and (ii) two heavy chains, each heavy chain comprising the expression product of either a plasmid designated pVgl :HuPRO140 HG2-VH (ATCC Deposit Designation PTA-4098) or a plasmid designated pVgl:HuPRO 140 (mut B+D+D-VH (ATCC Deposit Designation PTA-4099), or a fragment of such antibody, which binds to CCR5 on the surface of a human cell.

This invention also provides an anti-CCR5 antibody comprising two light chains, each chain comprising consecutive amino acids, the amino acid sequence of which is set forth in SEQ ID NO: 6, and two heavy chains, each heavy chain comprising consecutive amino acids, the amino acid sequence of which is set forth in SEQ ID NO: 9.

This invention also provides an anti-CCR5 antibody comprising two light chains, each chain comprising consecutive amino acids, the amino acid sequence of which is set forth in SEQ ID NO : 6 , and two heavy chains, each heavy chain comprising consecutive amino acids, the amino acid sequence of which is set forth in SEQ ID NO: 12.

This invention also provides an isolated nucleic acid encoding a polypeptide comprising consecutive amino acids, the amino acid sequence of which is set forth in SEQ ID NO: 6. In the subject embodiment, the nucleic acid comprises the sequence set forth in SEQ ID NO: 5.

This invention also provides an isolated nucleic acid encoding a polypeptide comprising consecutive amino acids, the amino acid sequence of which is set forth in SEQ ID NO: 9. In the subject embodiment, the nucleic acid comprises the sequence set forth in SEQ ID NO: 8.

This invention also provides an isolated nucleic acid encoding a polypeptide comprising consecutive amino acids, the amino acid sequence of which is set forth in SEQ ID NO: 12. In the subject embodiment, the nucleic acid comprises the sequence set forth in SEQ ID NO: 11.

This invention also provides a composition comprising at least one anti-CCR5 antibody, or a fragment thereof, as described above, together with a carrier.

This invention also provides a composition comprising the anti-CCR5 antibody, or a fragment thereof, having attached thereto a material such as a radioisotope, a toxin, polyethylene glycol, a cytotoxic agent and/or a detectable label .

This invention also provides a method of inhibiting infection of a CD4+ cell which comprises contacting the CD4+ cell with an antibody which comprises (i) two light chains, each light chain comprising the expression product of a plasmid designated pVK:HuPRO140-VK (ATCC Deposit Designation PTA-4097) , and (ii) two heavy chains, each heavy chain comprising the expression product of either a plasmid designated pVgl :HuPRO140 HG2-VH (ATCC Deposit Designation PTA- 4098) or a plasmid designated pVgl :HuPRO140 (mut B+D+D-VH (ATCC Deposit Designation PTA-4099), or a fragment of such antibody which binds to CCR5 on the surface of a CD4+ cell, in an amount and under conditions such that fusion of HIV-1 or an HIV-1- infected cell to the CD4+ cell is inhibited, thereby inhibiting HIV-1 infection of the CD4+ cell. This invention also provides a method of treating a subject afflicted with HIV-1 which comprises administering to the subject an effective HIV-1 treating dosage of an anti-CCR5 antibody comprising (i) two light chains, each light chain comprising the expression product of a plasmid designated pVK:HuPRO140-VK (ATCC Deposit Designation PTA-4097) , and (ii) two heavy chains, each heavy chain comprising the expression product of either a plasmid designated pVgl:HuPRO140 HG2-VH (ATCC Deposit Designation PTA- 4098) or a plasmid designated pVgl :HuPRO140 (mut B+D+D-VH (ATCC Deposit Designation PTA-4099), or a fragment of such antibody, which binds to CCR5 on the surface of a human cell, under conditions effective to treat the HIV-1-infected subject.

This invention also provides a method of preventing a subject from contracting an HIV-l infection which comprises administering to the subject an effective HIV-l infection-preventing dosage amount of an anti- CCR5 antibody comprising (i) two light chains, each light chain comprising the expression product of a plasmid designated pVK:HuPRO140-VK (ATCC Deposit Designation PTA-4097), and (ii) two heavy chains, each heavy chain comprising the expression product of either a plasmid designated pVgl :HuPRO140 HG2-VH (ATCC Deposit Designation PTA-4098) or a plasmid designated pVgl :HuPRO140 (mut B+D+D-VH (ATCC Deposit Designation PTA-4099) , or a fragment of such antibody, which binds to CCR5 on the surface of a human cell, under conditions effective to prevent the HIV-1, infection in the subject.

This invention also provides an anti-CCR5 antibody conjugate comprising an anti-CCR5 antibody which comprises (i) two light chains, each light chain comprising the expression product of a plasmid designated pVK: HuPRO140-VK (ATCC Deposit Designation PTA-4097), and (ii) two heavy chains, each heavy chain comprising the expression product of either a plasmid designated pVgl :HuPRO140 HG2-VH (ATCC Deposit Designation PTA-4098) or a plasmid designated pVgl :HuPRO140 (mut B+D+D-VH (ATCC Deposit Designation PTA-4099) , or a fragment of such antibody which binds to CCR5 on the surface of a human cell, conjugated to at least one polymer.

This invention also provides a method of inhibiting infection of a CCR5+ cell by HIV-1 comprising administering to a subject at risk of HIV-1 infection the above-described conjugate in an amount and under conditions effective to inhibit infection of CCR5+ cells of the subject by HIV-1.

This invention also provides a method of treating an HIV-1 infection in a subject comprising administering the above-described conjugate to an HIV-1- infected subject in an amount and under conditions effective to treat the subject's HIV-1 infection.

This invention also provides a transformed host cell comprising at least two vectors, at least one vector comprising a nucleic acid sequence encoding heavy chains of an anti-CCR5 antibody, and at least one vector comprising a nucleic acid sequence encoding light chains of the anti-CCR5 antibody, wherein the anti-CCR5 antibody comprises two heavy chains having the amino acid sequence set forth in SEQ ID NO : 9 , and two light chains having the amino acid sequence set forth in SEQ ID NO: 6.

This invention also provides a transformed host cell comprising at least two vectors, at least one vector comprising a nucleic acid sequence encoding heavy chains of an anti-CCR5 antibody, and at least one vector comprising a nucleic acid sequence encoding light chains of the anti-CCR5 antibody, wherein the anti-CCR5 antibody comprises two heavy chains having the amino acid sequence set forth in SEQ ID NO: 12 and two light chains having the amino acid sequence set forth in SEQ ID NO: 6.

This invention also provides a vector comprising a nucleic acid sequence encoding a heavy chain of an anti-CCR5 antibody, wherein the heavy chain comprises the amino acid sequence set forth in SEQ ID NO: 9.

This invention also provides a vector comprising a nucleic acid sequence encoding a heavy chain of an anti-CCR5 antibody, wherein the heavy chain comprises the amino acid sequence set forth in SEQ ID NO: 12.

This invention also provides a process for producing an anti-CCR5 antibody which comprises culturing a host cell containing therein (i) a plasmid designated pVK:HuPRO140-VK (ATCC Deposit Designation PTA-4097) , and (ii) either a plasmid designated pVgl :HuPRO140 HG2- VH (ATCC Deposit Designation PTA-4098) or a plasmid designated pVgl :HuPRO140 (mut B+D+D-VH (ATCC Deposit Designation PTA-4099) under conditions permitting the production of an antibody comprising two light chains encoded by the plasmid designated pVK:HuPRO140-VK (ATCC Deposit Designation

PTA-4097) and two heavy chains encoded either by the plasmid designated pVgl :HuPRO140 HG2-VH (ATCC Deposit Designation PTA-4098) or by the plasmid designated pVgl :HuPRO140 (mut B+D+D-VH (ATCC Deposit Designation PTA-4099) , so as to thereby produce an anti-CCR5 antibody. This invention also provides a process for producing an anti-CCR5 antibody which comprises a) transforming a host cell with (i) a plasmid designated pVK:HuPRO140-VK (ATCC Deposit Designation PTA-4097) and (ii) either a plasmid designated pVgl :HuPRO140 HG2-VH (ATCC Deposit Designation PTA-4098) or a plasmid designated pVgl :HuPRO140 (mut B+D+D-VH (ATCC Deposit Designation PTA-4099) , and b) culturing the transformed host cell under conditions permitting production of an antibody comprising two light chains encoded by the plasmid designated pVK:HuPRO140-VK (ATCC Deposit Designation PTA-4097) and two heavy chains encoded either by the plasmid designated pVgl :HuPRO140 HG2-VH (ATCC Deposit Designation PTA-4098) or by the plasmid designated pVglHuPRO140 (mut B+D+I) -VH (ATCC Deposit Designation PTA-4099) , so as to thereby produce an anti-CCR5 antibody.

This invention also provides a kit for use in a process of producing an anti-CCR5 antibody. The kit comprises a) a vector comprising a nucleic acid sequence encoding a light chain of an anti-CCR5 antibody, wherein the light chain comprises the amino acid sequence set forth in SEQ ID NO : 6 , and b) a vector comprising a nucleic acid sequence encoding a heavy chain of an anti-CCR5 antibody, wherein the heavy chain comprises the amino acid sequence set forth in SEQ ID NO : 9 , or a vector comprising a nucleic acid sequence encoding a heavy chain of an anti-CCR5 antibody, wherein the heavy chain comprises the amino acid sequence set forth in SEQ ID NO: 12.

Brief Description of the Figures:

Figure 1 :

Binding of anti-CCR5 monoclonal antibodies to CCR5 cells : Flow cytometry was used to detect CCR5 protein expression on the surface of L1.2-CCR5^* cells and freshly isolated, PHA/ IL-2 -stimulated PBMC. Cells were incubated with saturating concentrations of each mAb, which were detected with a PE-labeled anti -mouse IgG reporter antibody. Results from a representative experiment are shown. Results for each mAb are expressed both in mean fluorescence intensities (m.f.i.) and in % gated cells. Since PA8-PA12 and PA14 are all of the IgGi subclass, their m.f.i. are directly comparable. 2D7 is an IgG2a.

Figure 2:

CI values for different combinations of mAbs and viral inhibitors :

Experiments like those described in the legend of Fig. 7 were performed for different combinations of viral entry inhibitors. Anti-CCR5 mAbs were tested in combination with each other, CC- chemokines, and CD4-IgG2, which inhibits HIV-1 attachment to target cells. The PA11 and PA12 concentration range was 0-250 μg/ml; the 2D7 and PA14 concentration range was 0-25 μg/ml; the RANTES concentration range was 0-250 ng/ml; the CD4-IgG2 concentration range was 0-25 μg/ml. The concentrations of single-agents or their mixtures required to produce 50% and 90% inhibition of fusion or entry were quantitatively compared in a term known as the Combination Index (CI) . Figure 3 :

IC.._n values for inhibition of cell-cell fusion, viral entry and gpl20/sCD4 binding by anti-CCR5 mAbs :

For comparative purposes we have summarized the IC₅₀ values obtained in the different assays that the anti-CCR5 mAbs were tested in. IC₅₀ values were only calculated for mAbs that could inhibit >90% of fusion, entry or binding.

Figure 4 :

Epitope mapping of anti-CCR5 mAbs:

A two color staining protocol was used to assess binding of mAbs to mutant CCR5 proteins, tagged at the C-terminus with the HA peptide. HeLa cells expressing CCR5 point mutants were incubated with saturating concentrations of each mAb followed by detection with a PE-labeled anti-mouse IgG. Cell surface co-receptor expression was measured by double-staining of the cells with a FITC labeled anti -HA mAb. The four grids correspond to the four extracellular domains of CCR5. The first row of every grid indicates the amino acid sequence of the corresponding CCR5 extracellular domain (SEQ ID NOS: 1-4). Binding of anti-CCR5 mAbs to the alanine mutant of each residue is expressed as a percentage of binding to wild-type CCR5 , as described in Materials and Methods.

Figure 5 :

Inhibition of calcium mobilization into CCR5" cells by anti-CCR5 mAbs:

L1.2-CCR5^* cells were loaded with Indo-IAM and stimulated sequentially with an anti-CCR5 mAb or PBS, followed with RANTES (a) . Fluorescence changes were measured with a spectrofluorometer and the tracings are from a representative experiment . Calcium flux inhibition by PA14 and 2D7 was tested for a wide range of mAb concentrations (b) . Results are plotted as % inhibition of calcium influx = [1- (relative fluorescence in the presence of mAb ÷ relative fluorescence in the absence of mAb)] x 100%, and are means of values from three independent experiments .

Figure 6 :

Inhibition of CCR5 co-receptor function by anti- CCR5 mAbs:

Inhibition of cell-cell fusion by anti-CCR5 mAbs was tested in the RET assay (a) . 0-250μg/ml of PA8-PA12, or 0-25μg/ml of PA14 or 2D7 , were added to a mix of He a-Env_JR._FL ⁺ and PM1 cells, labeled with F18 and R18 respectively. Fluorescence RET was measured after 4h of incubation. Results are mean values from three independent experiments and are expressed as % inhibition of fusion = [1- (%

RET in the presence of mAb ÷ % RET in the absence of mAb)] x 100%. Inhibition of HIV-l entry by anti-CCR5 mAbs was tested in a single round of replication luciferase based entry assay (b) . U87- CD4⁺CCR5⁴ cells were infected with NLluc'env^" reporter virus carrying the JR-FL envelope in the presence of 0-250μg/ml of PA8-PA12, or 0-25μg/ml PA14 or 2D7. Luciferase activity (relative light units, r.l.u.) was measured in cell lysates 72h post-infection. Results are from a representative experiment and are expressed as % inhibition of entry = [1- (r.l.u. in the presence of mAb ÷ r.l.u. in the absence of mAb)] x 100%. Binding of biotinylated [b] gpl20, sCD4 and b-gpl20-CD4 complexes to L1.2-CCR5^* cells (c) . Strong binding is observed when gpl20 derived from the R5 virus HIV-l_JR._FL is complexed with an equimolar amount of sCD4. No binding is observed in the absence of sCD4 or for gpl20 derived from the X4 virus HIV-1 _m. Background binding to CCR5- LI .2 cells has been subtracted from all curves. Inhibition of gpl20/sCD4 binding to L1.2-CCR5^* cells was tested in the presence of varying concentrations of each antibody (d) . Cells were pre-incubated in 96-well plates with an anti-CCR5 mAb followed by an incubation with a saturating concentration of biotinylated gpl20/sCD4. Finally, binding of PE- labeled streptavidin to cells was measured using a fluorescence plate reader. Results are from a representative experiment and are expressed as % inhibition of gpl20/εCD4 binding = [1- (m.f.i. in the presence of mAb ÷ m.f.i. in the absence of mAb) ] x 100%.

Figure 7 :

Synergistic inhibition of cell-cell fusion by PA12 and 2D7 :

Dose-response curves were obtained for the mAbs used individually and in combination. 0-50μg/ml of PA12, 0-25μg/ml 2D7 , or a combination of the two in a 2:1 ratio, were added to a mix of HeLa-Env_JR._FL ^'' and PM1 cells, labeled with R18 and F18 respectively. Fluorescence RET was measured after 4 hours of incubation. Results are expressed as % inhibition of fusion and are the means of values from three independent experiments . Data were analyzed using the median effect principle, which can be written f = i/[l + (K/c)^m] (1) where f is the fraction affected/inhibited, c is concentration, K is the concentration of agent required to produce t-he median effect, and m is an e pirical coefficient describing the shape of the dose-response curve. Equation (1) is a generalized form of the equations describing Michaelis-Menton enzyme kinetics, Langmuir adsorption isotherms, and Henderson-Hasselbalch ionization equilibria, for which m = 1. In the present case, K is equal to the IC₅₀ value. K and m were determined by curve-fitting the dose-response curves and Equation (1) was rearranged to allow calculation of c for a given f. The best-fit parameters for K and c are 8.8μg/ml and 0.54 for PA12, 0.36μg/ml and 0.68 for 2D7 , and O.llμg/ml and 1.1 for their combination. These curves are plotted and indicate a reasonable goodness-of -fit between experiment and theory.

Figure 8 :

This figure shows the amino acid sequence of the light chain variable region of a humanized version of mouse anti-CCR5 antibody PA14 (SEQ ID NO: 6) and the nucleic acid sequence encoding the same (SEQ ID NO: 5) , in accordance with the invention. SEQ ID NO: 7 identifies the region of SEQ ID NO: 5 which codes for the amino acid sequence set forth in SEQ ID NO: 6. This light chain variable region is present in the antibodies designated herein as PRO 140 #1 and #2. The complementarity-determining regions ("CDRs") are underlined.

Figure 9 :

This figure shows the amino acid sequence of a first heavy chain variable region of a humanized version of mouse anti-CCR5 antibody PA14 (SEQ ID NO:9), and the nucleic acid sequence encoding the same (SEQ ID NO: 8), in accordance with the invention. SEQ ID NO: 10 identifies the region of SEQ ID NO: 8 that codes for the amino acid sequence set forth in SEQ ID NO : 9. This heavy chain variable region is present in the antibody designated herein as PRO 140 #2. The CDRs are underlined.

Figure 10:

This figure shows the amino acid sequence of a second heavy chain variable region of a humanized version of mouse humanized anti-CCR5 antibody PA14 (SEQ ID NO: 12) and the nucleic acid sequence encoding the same (SEQ ID NO: 11) in accordance with the invention. SEQ ID NO: 13 identifies the region of SEQ ID NO: 11 that codes for the amino acid sequence set forth in SEQ ID NO: 12. This heavy chain variable region is present in the antibody designated herein as PRO 140 #1. The CDRs are underlined.

Figure 11:

Single-Dose of humanized CCR5 antibody potently reduces viral loads in vivo:

SCID mice were reconstituted with normal human

PBMC and infected with HIV-1- When a viral steady state was reached, the animals were treated with a single 1 milligram i.p. dose of humanized CCR5 antibody (PRO 140) or isotype control antibody and monitored for plasma HIV RNA (Roche Amplicor Assay) .

Figure 12:

Sustained Reduction in Viral Load:

SCID mice were reconstituted with normal human PBMC and infected with HIV-1_JR._CEF. When a viral steady state was reached, the animals were treated i.p. with 0.1 mg doses of humanized CCR5 antibody (PRO140) every three days and monitored for plasma HIV RNA (Roche Amplicor Assay) . Figure 13 :

Demonstrates that there was no depletion of lymphocytes with the use of the CCR5 antibody (PRO 140) prepared in accordance with the invention.

Figure 14 :

Humanized CCR5 Antibody (PRO140) Potently Blocks CCR5-mediated HIV-1 Cell-Cell Fusion. Murine CCR5 antibody was humanized using the method of complementarity-determining region (CDR) grafting and framework substitutions. Humanized CCR5 antibodies (PRO 140 #1 and PRO 140 #2) were expressed in Sp2/0 cells, purified by protein A chromatography and tested for the ability to block replication of HIV-1_JR._F env-mediated membrane fusion as described (Litwin, et al . , J, Virol.,

70 :6437, 1996) .

Figure 15 :

Humanized CCR5 Antibody (PRO 140) Mediates Potent, Subtype-Independent Inhibition of HIV-1. CCR5 Antibodies (Pro 140 #1 and #2) according to the invention were tested for the ability to block replication of wild-type HIV-1 in peripheral blood mononuclear cells (PBMCs) as described (Trkola et al . , J. Virol., 72:396, 1998). The extent of viral replication was measured by assaying the p24 antigen content of 7-day PBMC culture supernatants .

Figure 16 :

This figure provides a map of plasmid pVK-HuPRO140 encoding the light plasmid chain variable region shown in Figure 8 as well as the human Kappa constant regions as described in Co et al . , J. Immunol., 148:1149, 1992. Figure 17 :

This figure provides a map of plasmid pVg4 -

HuPR0140 HG2 encoding the heavy chain variable region shown in Figure 9 as well as the human heavy chain constant regions, CHI, hinge, CH2 , and CH3 , of human IgG4 as described in Co et al, Supra.

Figure 18 :

This figure provides a map of plasmid pVg4 - HuPRO140 (mut B+D+I) encoding the heavy chain variable region shown in Figure 10 as well as the human heavy chain constant regions, CHI, hinge, CH2 , and CH3 , of human IgG4 as described in Co et al , Supra.

Figure 19

Hu PRO140 Blocks HIV-1 But Not RANTES Signaling

PRO140 antibodies according to the invention were tested for the ability to block RANTES-induced calcium mobilization in L1.2-CCR5 cells (Olson, et al . , J.Virol., 72:396, 1998). This figure shows that a humanized CCR5 antibody (huPRO140) blocks HIV-1 but not RANTES signaling.

Detailed Description of the invention:

The plasmids designated as HuPRO140-VK, HuPRO140 (mut+B+D+I) -VH, and HuPRO140 HG2-VH, which are referred to in figures 16, 18, and 17 as pVK-HuPRO140 , pVg4 - HUPRO140 (mut B+D+I) and pVg4 -HuPRO140 HG2 , respectively, were deposited with the American Type Culture Collection, Manassas, Va . , U.S.A. 20108 on February 22, 2002, under ATCC Accession Nos. PTA 4097, PTA 4099 and PTA 4098 respectively. These deposits were made pursuant to the provisions of the Budapest Treaty on the International Recognition of the Deposit of Microorganisms for the Purpose of Patent Procedure (Budapest Treaty) .

This invention provides a composition for inhibiting HIV-1 infection comprising at least two compounds in synergistically effective amounts for inhibiting HIV-1 infection, wherein at least one of the compounds prevents with the productive interaction between HIV-1 and an HIV-1 fusion co-receptor.

As used herein, "composition" means a mixture. The compositions include but are not limited to those suitable for oral, rectal, intravaginal , topical, nasal, opthalmic, or parenteral administration to a subject. As used herein, "parenteral" includes but is not limited to subcutaneous, intravenous, intramuscular, or intrasternal injections or infusion techniques .

As used herein, "HIV-l" means the human immunodeficiency virus type-1. HIV-1 includes but is not limited to extracellular virus particles and the forms of HIV-1 found in HIV-1 infected cells.

As used herein, "HIV-1 infection" means the introduction of HIV-1 genetic information into a target cell, such as by fusion of the target cell membrane with HIV-1 or an HIV-1 envelope glycoprotein⁴ cell. The target cell may be a bodily cell of a subject. In the preferred embodiment, the target cell is a bodily cell from a human subject.

As used herein, "inhibiting HIV-1 infection" means the reduction of the amount of HIV-1 genetic information introduced into a target cell population as compared to the amount that would be introduced without said composition.

As used herein, "compound" means a molecular entity, including but not limited to peptides, polypeptides, and other organic or inorganic molecules and combinations thereof .

As used herein, " synergistically effective" means that the combined effect of the compounds when used in combination is greater than their additive effects when used individually.

As used herein, "productive interaction" means that the interaction of HIV-1 and the HIV-1 co-receptor would lead to the fusion of said HIV-1 or HIV-1 envelope glycoprotein" cell and the membrane bearing the co-receptor .

As used herein, "prevents the productive interaction" means that the amount of interaction is reduced as compared to the amount that would occur without the compound. The interactions may be prevented by masking or altering interactive regions on the co-receptor or HIV-1 or by altering the expression, aggregation, conformation, or association state of the co-receptor. As used herein, "HIV-1 fusion co-receptor" means a cellular receptor that mediates fusion between the target cell expressing the receptor and HIV-1 or an HIV-l envelope glycoprotein^* cell. HIV-1 fusion coreceptors include but are not limited to CCR5, CXCR4 and other chemokine receptors .

This invention also provides a composition which inhibits fusion of HIV-1 or an HIV-1 envelope glycoprotein^* cell to a target cell, comprising at least two compounds in εynergistically effective amounts for inhibiting fusion of HIV-1 or an HIV-1 envelope glycoprotein^* cell to a target cell, wherein at least one of the compounds prevents the productive interaction between HIV-l and an HIV-1 fusion coreceptor .

As used herein, "fusion" means the joining or union of the lipid bilayer membranes found on mammalian cells or viruses such as HIV-1. This process is distinguished from the attachment of HIV-1 to a target cell. Attachment is mediated by the binding of the HIV-1 exterior glycoprotein to the human CD4 receptor, which is not a fusion co-receptor.

As used herein, "inhibits" means that the amount is reduced as compared with the amount that would occur without the composition.

As used herein, "target cell" means a cell capable of being infected by or fusing with HIV-1 or HIV-1 infected cells.

As used herein, "chemokine" means a cytokine that can stimulate leukocyte movement. They may be characterized as either cys-cys or cys-X-cys depending on whether the two amino terminal cysteine residues are immediately adjacent or separated by one amino acid. It includes but is not limited to RANTES, MlP-lα, MlP-lβ, SDF-1 or another chemokine which blocks HIV-1 infection.

In one embodiment of the above compositions, the coreceptor is a chemokine receptor. In the preferred embodiment of the above compositions, the chemokine receptor is CCR5 or CXCR4. Several other chemokine and related receptors are known to function as HIV coreceptors including but not limited to CCR2 , CCR3 , CCR8, STRL33, GPR-15, CX3CR1 and APJ (69) .

As used herein, "chemokine receptor" means a member of a homologous family of seven-transmembrane spanning cell surface proteins that bind chemokines.

As used herein, "CCR5" is a chemokine receptor which binds members of the C-C group of chemokines and whose amino acid sequence comprises that provided in Genbank Accession Number 1705896 and related polymorphic variants .

As used herein, " CXCR4 " is a chemokine receptor which binds members of the C-X-C group of chemokines and whose amino acid sequence comprises that provided in Genbank Accession Number 400654 and related polymorphic variants .

In one embodiment of the above compositions, at least one of the compounds is a nonpeptidyl molecule. In one embodiment, the nonpeptidyl molecule is the bicyclam compound AMD3100. (16).

As used herein, "nonpeptidyl molecule" means a molecule that does not consist in its entirety of a linear sequence of amino acids linked by peptide bonds. A nonpeptidyl molecule may, however, contain one or ore peptide bonds.

In one embodiment of the above compositions, at least one of the compounds is an antibody. In one embodiment, the antibody is a monoclonal antibody. In another embodiment, the antibody is a anti -chemokine receptor antibody. In one embodiment, the antibody is an anti- CXCR4 antibody. In a further embodiment, the anti CXCR4 antibody is 12G5. (43) . In a preferred embodiment, the antibody is an anti-CCR5 antibody. The anti-CCR5 antibody includes but is not limited to PA8 , PA9, PA10, PA11, PA12, PA14 and 2D7. In this composition the compounds are in an appropriate ratio. The ratio ranges from 1 : 1 to 1000:1.

The monoclonal antibodies PA8 , PA9 , PA10, PA11, PA12 and PA14 were deposited pursuant to and in satisfaction of, the requirements of the Budapest Treaty on the International Recognition of the Deposit of Microorganisms for the Purposes of Patent Procedure with the American Type Culture Collection (ATCC) , 10801 University Boulevard, Manassas, Virginia 20110-2209 on December 2, 1998 under the following Accession Nos.: ATCC Accession No. HB-12605 (PA8), ATCC Accession No. HB-12606 (PA9) , ATCC Accession No.HB-12607 (PA10) , ATCC Accession No. HB-12608 (Pll) , ATCC Accession No. HB- 12609 (PA12) ATCC Accession No. HB-12610 (PA14) .

In another embodiment of the above compositions, two or more of the compounds are antibodies. In one embodiment of the invention, the antibodies include but are not limited to PA8 , PA9 , PA10, PA11, PA12, PA14 and 2D7. In this composition the antibodies are in an appropriate ratio. The ratio ranges from 1:1 to 50:1.

As used herein, "antibody" means an immunoglobulin molecule comprising two heavy chains and two light chains and which recognizes an antigen. The immunoglobulin molecule may derive from any of the commonly known classes, including but not limited to IgA, secretory IgA, IgG and IgM. IgG subclasses are also well known to those in the art and include but are not limited to human IgGi, IgG2 , IgG3 and IgG4. It includes, by way of example, both naturally occurring and non-naturally occurring antibodies. Specifically, "antibody" includes polyclonal and monoclonal antibodies, and monovalent and divalent fragments thereof. Furthermore, "antibody" includes chimeric antibodies, wholly synthetic antibodies, single chain antibodies, and fragments thereof. Optionally, an antibody can be labeled with a detectable marker. Detectable markers include, for example, radioactive or fluorescent markers. The antibody may be a human or nonhuman antibody. The nonhuman antibody may be humanized by recombinant methods to reduce its immunogenicity in man. Methods for humanizing antibodies are known to those skilled in the art.

As used herein, "monoclonal antibody," also designated as mAb, is used to describe antibody molecules whose primary sequences are essentially identical and which exhibit the same antigenic specificity. Monoclonal antibodies may be produced by hybridoma, recombinant, transgenic or other techniques known to one skilled in the art .

As used herein, "anti-chemokine receptor antibody" means an antibody which recognizes and binds to an epitope on a chemokine receptor. As used herein, "anti-CCR5 antibody" means a monoclonal antibody which recognizes and binds to an epitope on the CCR5 chemokine receptor.

As used herein, "appropriate ratio" means mass or molar ratios wherein the compounds are synergistically effective .

In one embodiment of the above compositions, at least one compound is a chemokine or chemokine derivative. The chemokines include but are not limited to RANTES, MlP-lα, MlP-lβ, SDF-1 or a combination thereof. In this composition, the compounds are in an appropriate ratio. The chemokine derivatives include but are not limited to Met-RANTES, AOP-RANTES, RANTES 9-68, or a combination thereof.

As used herein, "chemokine derivative" means a chemically modified chemokine. The chemical modifications include but are not limited to amino acid substitutions, additions or deletions, non-peptidyl additions or oxidations. One skilled in the art will be able to make such derivatives.

In another embodiment of the above compositions, at least one compound is an antibody and at least one compound is a chemokine or chemokine derivative. In this composition, the compounds are in an appropriate ratio. The ratio ranges from 100:1 to 1000:1.

In another embodiment of the above compositions, at least one compound binds to the gp41 subunit of the HIV-1 envelope glycoprotein. In one embodiment, at least one compound is the T-20 peptide inhibitor of HIV-1 entry (70) .

In another embodiment of the above compositions, at least one of the compounds inhibits the attachment of HIV-l to a target cell. In one embodiment, at least one compound binds CD4. In one embodiment, at least one compound is an HIV-1 envelope glycoprotein. In one embodiment, at least one compound is an anti-CD4 antibody. In one embodiment, at least one compound binds to the HIV-1 envelope glyoprotein. In one embodiment, at least one compound is an antibody to the HIV-l envelope glycoprotein. In one embodiment, at least one compound is a CD4 -based protein. In one embodiment, at least one compound is CD4-IgG2.

In another embodiment of the above compositions, at least one compound is an antibody and at least one compound binds to an HIV-l envelope glycoprotein. In one embodiment, the compound is a CD4 -based protein. In one embodiment, the compound is CD4-IgG2. In this composition, the compounds are in an appropriate ratio. The ratio ranges from 1:1 to 10:1.

As used herein, "attachment" means the process that is mediated by the binding of the HIV-1 envelope glycoprotein to the human CD4 receptor, which is not a fusion co-receptor.

As used herein, " CD4 " means the mature, native, membrane-bound CD4 protein comprising a cytoplasmic domain, a hydrophobic transmembrane domain, and an extracellular domain which binds to the HIV-1 gpl20 envelope glycoprotein.

As used herein, "HIV-1 envelope glycoprotein" means the HIV-1 encoded protein which comprises the gpl20 surface protein, the gp4l transmembrane protein and oligomers and precursors thereof.

As used herein, "CD4 -based protein" means any protein comprising at least one sequence of amino acid residues corresponding to that portion of CD4 which is required for CD4 to form a complex with the HIV-1 gpl20 envelope glycoprotein . As used herein, "CD4-IgG2" means a heterotetrameric CD4 -human IgG2 fusion protein encoded by the expression vectors deposited under ATCC Accession Numbers 75193 and 75194.

In one embodiment of the above compositions at least one of the compounds comprises a polypeptide which binds to a CCR5 epitope. In one embodiment, the epitope is located in the N-terminus, one of the three extracellular loop regions or a combination thereof. In one embodiment, the epitope is located in the N- terminus . The epitope can comprise N13 and Y15 in the N-terminus. The epitope can comprise comprises Q4 in the N-terminus. In another embodiment, the epitope includes residues in the N-terminus and second extracellular loop. The epitope can comprise D2 , Y3 , Q4,S7, P8 and N13 in the N-terminus and Y176 and T177 in the second extracellular ^' loop. The epitope can comprise D2 , Y3 , Q4 , P8 and N13 in the N-terminus and Y176 and T177 in the second extracellular loop. The epitope can comprise D2 in the N-terminus and R168 and Y176 in the second extracellular loop. In one embodiment, the epitope is located in the second extra cellular loop. The epitope can comprise Q170 and K171 in the second extracellular loop. The epitope can comprise Q170 and E172 in the second extra cellular loop.

As used herein, the following standard abbreviations are used throughout the specification to indicate specific amino acids:

A=ala=alanine R=arg=arginine

N=asn=asparagine D=asp=aspartic acid

C=cys=cysteine Q=gln--glutamine

E=glu--glutamic acid G=gly=glycine

H=his=histidine l=ile=isoleucine

L=leu=leucine K=lys=lysine M=met=methionine F=phe=phenylalanine P=pro=proline S--ser=serine

T=thr=threonine W=trp--tryptophan γ=tyr=tyrosine V=val=valine

As used herein, "polypeptide" means two or more amino acids linked by a peptide bond.

As used herein, "epitope" means a portion of a molecule or molecules that forms a surface for binding antibodies or other compounds. The epitope may comprise contiguous or noncontiguous amino acids, carbohydrate or other nonpeptidyl moitieε or oligomer-specific surfaces .

As used herein, "N-terminus" means the sequence of amino acids spanning the initiating methionine and the first transmembrane region.

As used herein, "second extra cellular loop" means the sequence of amino acids that span the fourth and fifth transmembrane regions and are presented on the surface .

In one embodiment of the above compositions at least one of the compounds comprises a light chain of an antibody. In another embodiment of the above compositions at least one of the compounds co priseε a heavy chain of an antibody. In another embodiment of the above compositions at least one of the compounds comprises the Fab portion of an antibody. In another embodiment of the above compositions at least one of the compounds comprises the variable domain of an antibody. In another embodiment, the antibody is produced as a single polypeptide or "single chain" antibody which comprises the heavy and light chain variable domains genetically linked via an intervening sequence of amino acids . -In another embodiment of the above compositions at least one of the compounds comprises one or more CDR portions of an antibody.

As used herein, "heavy chain" means the larger polypeptide of an antibody molecule compoεed of one variable domain (VH) and three or four constant domains (CHI, CH2, CH3, and CH4 ) , or fragments thereof.

As used herein, "light chain" means the smaller polypeptide of an antibody molecule composed of one variable domain (VL) and one constant domain (CL) , or fragments thereof.

As used herein, "Fab" means a monovalent antigen binding fragment of an immunoglobulin that consists of one light chain and part of a heavy chain. It can be obtained by brief papain digestion or by recombinant methods .

As used herein, "F(ab')2 fragment" means a bivalent antigen binding fragment of an immunoglobulin that consists of both light chains and part of both heavy chains. It cen be obtained by brief pepsin digestion or recombinant methods .

As used herein, "CDR" or "complementarity determining region" means a highly variable sequence of amino acids in the variable domain of an antibody.

This invention provides the above compositions and a pharmaceutically acceptable carrier. Pharmaceutically acceptable carriers are well known to those skilled in the art. Such pharmaceutically acceptable carriers may include but are not limited to aqueous or non-aqueous solutionε, suspensions, and emulsions. Examples of non-aqueous solvents are propylene glycol, polyethylene glycol, vegetable oils such as olive oil, and injectable organic esterε such as ethyl oleate . Aqueous carriers include water, alcoholic/aqueous solutions, emulsions or suspensions, saline and buffered media. Parenteral vehicles include sodium chloride solution, Ringer's dextrose, dextrose and sodium chloride, lactated Ringer's or fixed oils. Intravenous vehicles include fluid and nutrient replenishers , electrolyte replenisherε such as those based on Ringer's dextrose, and the like. Preservatives and other additives may also be present, such as, for example, antimicrobials, antioxidants , chelating agents, inert gases and the like.

This invention provides a method of treating a subject afflicted with HIV-1 which comprises administering to the subject an effective dose of the above compositions.

As used herein, "subject" means any animal or artificially modified animal capable of becoming HIV- infected. Artificially modified animals include, but are not limited to, SCID mice with human immune systems. The animals include but are not limited to mice, rats, dogs, guinea pigs, ferrets, rabbits, and primates. In the preferred embodiment, the subject is a human .

As used herein, "treating" means either slowing, stopping or reversing the progression of an HIV-1 disorder. In the preferred embodiment, "treating" means reversing the progression to the point of eliminating the disorder. As used herein, "treating" also means the reduction of the number of viral infections, reduction of the number of infectious viral particles, reduction of the number of virally infected cells, or the amelioration of symptoms associated with HIV-l. Aε used herein, "afflicted with HIV-1" means that the subject has at least one cell which has been infected by HIV-1.

As used herein, "adminiεtering" may be effected or performed uεing any of the methods known to one skilled in the art. The methods may comprise intravenous, intramuscular or subcutaneouε means.

The dose of the composition of the invention will vary depending on the subject and upon the particular route of administration used. Doεageε can range from 0.1 to 100,000 μg/kg. Baεed upon the compoεition, the dose can be delivered continuously, such as by continuous pump, or at periodic intervals. For example, on one or more separate occasions. Desired time intervals of multiple doses of a particular composition can be determined without undue experimentation by one skilled in the art .

As used herein, "effective dose" means an amount in sufficient quantities to either treat the subject or prevent the subject from becoming HIV-1 infected. A person of ordinary skill in the art can perform simple titration experiments to determine what amount is required to treat the subject.

This invention provides a method of preventing a εubject from contracting HIV-l which compriεeε administering to the subject an effective dose of the above compositions .

As used herein, "contracting HIV-1" means becoming infected with HIV-1, whose genetic information replicates in and/or incorporates into the host cells. This invention provides an anti-CCR5 monoclonal antibody. The antibody includes but iε not limited to the following: PA8. (ATCC Acceεεion No. HB-12605) , PA9

(ATCC Accession No. HB-12606), PA10 (ATCC Accession No. HB-12607) , PA11 (ATCC Accession No. HB-12608), PA12

(ATCC Accession No. HB-12609) , and PA14 (ATCC Accession No. HB-12610) .

This invention provides humanized forms of the above antibodies .

As used herein, "humanized" describes antibodies wherein some, most or all of the amino acids outside the CDR regions are replaced with corresponding amino acids derived from human immunoglobulin molecules. In one embodiment of the humanized forms of the antibodies, some, most or all of the amino acids outside the CDR regions have been replaced with amino acids from human immunoglobulin molecules but where some, most or all amino acids within one or more CDR regions are unchanged. Small additions, deletions, insertions, substitutionε or modificationε of amino acids are permissible as long as they would not abrogate the ability of the antibody to bind a given antigen. Suitable human immunoglobulin molecules would include IgGi, IgG2, IgG3 , IgG4 , IgA and IgM molecules. A "humanized" antibody would retain a similar antigenic specificity as the original antibody, i.e., in the present invention, the ability to bind CCR5.

One skilled in the art would know how to make the humanized antibodies of the subject invention. Various publications, several of which are hereby incorporated by reference into thiε application, also describe how to make humanized antibodies. For example, the methods described in United States Patent No. 4,816,567 (71) comprise the production of- chimeric antibodies having a variable region of one antibody and a constant region of another antibody.

United States Patent No. 5,225,539 (72) describes another approach for the production of a humanized antibody. This patent deεcribeε the use of recombinant DNA technology to produce a humanized antibody wherein the CDRs of a variable region of one immunoglobulin are replaced with the CDRs from an immunoglobulin with a different specificity such that the humanized antibody would recognize the desired target but would not be recognized in a significant way by the human subject's immune system. Specifically, site directed mutagenesis is used to graft the CDRs onto the framework.

Other approaches for humanizing an antibody are described in United States Patent Nos. 5,585,089 (73) and 5,693,761 (74) and WO 90/07861 which describe methods for producing humanized immunoglobulins. These have one or more CDRs and possible additional amino acids from a donor immunoglobulin and a framework region from an accepting human immunoglobulin. These patents describe a method to increase the affinity of an antibody for the desired antigen. Some amino acidε in the framework are chosen to be the same as the amino acidε at those positions in the donor rather than in the acceptor. Specifically, these patents describe the preparation of a humanized antibody that binds to a receptor by combining the CDRs of a mouse monoclonal antibody with human immunoglobulin framework and constant regions. Human framework regions can be chosen to maximize homology with the mouse sequence. A computer model can be used to identify amino acids in the framework region which are likely to interact with the CDRs or the specific antigen and then mouse amino acidε can be used at these positions to create the humanized antibody. The above patents 5,585,089 and 5,693,761, and WO 90/07861 (75) also propose four posεible criteria which may uεed in designing the humanized antibodies. The first proposal was that for an acceptor, use a framework from a particular human immunoglobulin that is unusually homologous to the donor immunoglobulin to be humanized, or use a consensus framework from many human antibodies . The second proposal was that if an amino acid in the framework of the human immunoglobulin is unusual and the donor amino acid at that position is typical for human εequences, then the donor amino acid rather than the acceptor may be selected. The third proposal was that in the positions immediately adjacent to the 3 CDRs in the humanized immunoglobulin chain, the donor amino acid rather than the acceptor amino acid may be selected. The fourth proposal was to use the donor amino acid reside at the framework positions at which the amino acid is predicted to have a side chain atom within 3A of the CDRs in a three dimensional model of the antibody and is predicted to be capable of interacting with the CDRs. The above methodε are merely illuεtrative of some of the methods that one εkilled in the art could employ to make humanized antibodieε. The affinity and/or specificity of the binding of the humanized antibody may be increased using methods of directed evolution as described in Wu et al . (1999) J. Mol. Biol. 284:151 and U.S. Patents Nos. 6,165,793; 6,365,408 and 6,413,774.

In an embodiment of the invention the humanized form of the antibody comprises a light chain variable amino acid sequence aε set forth in SEQ ID NO: 6. In another embodiment, the antibody comprises a heavy chain variable amino acid sequence as set forth in SEQ ID NO: 9. In a further embodiment, the antibody may comprise the heavy chain -variable amino acid sequence as set forth in SEQ ID NO: 12.

In another embodiment, the humanized antibody comprises the light chain variable amino acid sequence as set forth in SEQ ID NO: 6, and the heavy chain variable amino acid sequence as εet forth in SEQ ID NO: 9. Alternatively, the antibody may comprise the light chain variable amino acid sequence as set forth in SEQ ID NO: 6 and the heavy chain variable amino acid sequence as set forth in SEQ ID NO: 12.

The variable regions of the humanized antibody may be linked to at least a portion of an immunoglobulin constant region of a human immunoglobulin. In one embodiment, the humanized antibody contains both light chain and heavy chain constant regions. The heavy chain constant region usually includes CHI, hinge, CH2 , CH3 and sometimes, CH4 region. In one embodiment, the constant regions of the humanized antibody are of the human IgG4 isotype .

This invention provides isolated nucleic acid molecules encoding theεe anti-CCR5 monoclonal antibodies or their humanized versions. The nucleic acid molecule can be RNA, DNA or cDNA. In one embodiment, the nucleic acid molecule encodes the light chain. In one embodiment, the nucleic acid molecule encodes the heavy chain. In one embodiment, the nucleic acid encodes both the heavy and light chains. In one embodiment, one or more nucleic acid moleculeε encode the Fab portion. In one embodiment, one or more nucleic acid molecules encode CDR portions. In one embodiment, the nucleic acid molecule encodes the variable domain. In another embodiment, the nucleic acid molecule encodes the variable domain and one or more constant domains. Preferably, analogs of exemplified humanized anti-CC_R5 antibodies differ from exemplified humanized anti-CCR5 antibodies by conservative amino acid substitutions. For purposes of classifying amino acid substitutions as conservative or non-conservative, amino acidε may be grouped as follows: Group I (hydrophobic side chains): met, ala, val, leu, ile,- Group II (neutral hydrophilic side chains): cys, ser, thr; Group III (acidic side chains) : asp, glu; Group IV (basic side chains) : asn, gin, his, lyε, arg; Group V (residues influencing chain orientation): gly, pro; and Group VI (aromatic side chains): trp, tyr, phe. Conservative subεtitutionε involve substitutionε between amino acids in the same class. Non-conservative εubstitutions constitute exchanging a member of one of these classes for a member of another .

Analogs of humanized anti-CCR5 antibodies show subεtantial amino acid sequence identity with humanized PRO 140 #1 or humanized PRO 140 #2, exemplified herein. Heavy and light chain variable regions of analogs are encoded by nucleic acid sequences that hybridize with the nucleic acids encoding the heavy or light chain variable regions of humanized PRO 140 #1, or humanized PRO 140 #2, or degenerate forms thereof, under stringent conditions.

Due to the degeneracy of the genetic code, a variety of nucleic acid sequenceε encode the humanized anti-CCR5 antibody of the present invention. In certain embodiments, the antibody is encoded by a nucleic acid molecule that is highly homologous to the foregoing nucleic acid molecules. Preferably the homologous nucleic acid molecule comprises a nucleotide sequence that is at least about 90% identical to the nucleotide sequence provided herein. More preferably, the nucleotide sequence is at least about 95% identical, at leaεt about 97% identical, at least about 98% identical, or at least about 99% identical to the nucleotide sequence provided herein. The homology can be calculated using various, publicly available software tools well known to one of ordinary skill in the art. Exemplary tools include the BLAST system available from the webεite of the National Center for Biotechnology Information (NCBI) at the National Inεtitutes of Health.

One method of identifying highly homologous nucleotide sequenceε is via nucleic acid hybridization. Thus the invention also includes humanized CCR5 antibodieε having the CCR5-binding propertieε and other functional propertieε deεcribed herein, which are encoded by nucleic acid molecules that hybridize under high stringency conditions to the foregoing nucleic acid molecules. Identification of related sequenceε can alεo be achieved using polymerase chain reaction (PCR) and other amplification techniques suitable for cloning related nucleic acid εequenceε . Preferably, PCR primers are selected to amplify portions of a nucleic acid sequence of interest, such as a CDR.

The term "high stringency conditions" as used herein refers to parameters with which the art iε familiar. Nucleic acid hybridization parameters may be found in references that compile such methods, e.g., Molecular Cloning: A Laboratory Manual, J. Sambrook, et al . , eds., Second Edition, Cold Spring Harbor Laboratory Press, Cold Spring Harbor, New York, 1989, or Current Protocols in Molecular Biology, F.M. Ausubel, et al . , eds., John Wiley & Sons, Inc., New York. One example of high stringency conditions is hybridization at 65 degrees Centigrade in hybridization buffer (3.5X SSC, 0.02% Ficoll, 0.02% polyvinyl pyrrolidone, 0.02% Bovine Serum Albumin, 2.5mM NaH₂P0₄ (pi17), 0.5% SDS, 2mM EDTA) . SSC is 0.15M sodium chloride/0.015M sodium citrate, pH7 ; SDS is sodium dodecyl sulphate; and EDTA is ethylenediaminetetracetic acid. After hybridization, a membrane upon which the nucleic acid is transferred is waεhed, for example, in 2X SSC at room temperature and then at 0.1-0.5X SSC/0.1X SDS at temperatures up to 68 degrees Centigrade.

The nucleic acid sequenceε are expressed in hosts after the sequences have been operably linked to (i.e., positioned to ensure the functioning of) an expression control sequence. These expresεion vectors are typically replicable in the host organismε, either aε epiεomeε or aε an integral part of the hoεt chromosomal DNA. Commonly, expression vectors will contain selection markers, e.g., tetracycline or neomycin, to permit detection of those cells transformed with the desired DNA sequenceε (see, e.g., U.S. Patent No. 4,704,362 which is incorporated herein by reference) .

E. coli is one prokaryotic host useful particularly for cloning the DNA sequences of the present invention. Other microbial hosts suitable for use include bacilli, such as Bacillus subtiluε, and other enterobacteriaccae, such as Salmonella, Serratia, and various Pseudomonaε species. In these prokaryotic hosts, one can also make expression vectors, which will typically contain expression control sequences compatible with the host cell (e.g., an origin of replication) . In addition, any number of a variety of well-known promoters will be present, such as the lactose promoter system, a tryptophan (trp) promoter system, a beta.-lactamase promoter system, or a promoter system from phage lambda. The promoters will typically control expreεsion, optionally with an operator sequence, and have ribosome binding site sequences and the like, for initiating ^' and completing transcription and translation.

Other microbes, such as yeaεt, may also be useful for expresεion. Saccharomyces is a preferred host, with εuitable vectors having expresεion control sequences, such as promoters, including 3 -phosphoglycerate kinase or other glycolytic enzymes and an origin of replication, termination sequenceε and the like as desired.

In addition to microorganismε , mammalian tissue cell culture may also be used to express and produce the polypeptides of the present invention (see, Winnacker, "From Genes to Clones,", VCH Publisherε, New York, New York (1987) ) . Eukaryotic cells are actually preferred, because a number of suitable host cell lines capable of εecreting intact immunoglobulinε have been developed in the art, and include the CHO cell lines, various COS cell lines, HeLa cells, preferably myeloma cell lines, etc. and transformed B cells or hybridomas. Expression vectors for theεe cells can include expression control sequences, such as an origin of replication, a promoter, an enhancer (Queen, et al . , Immunol. Rev., 89, 49-68 (1986) which is incorporated herein by reference), and necessary processing information siteε, εuch as riboεome binding sites, RNA splice sites, polyadenylation sites and transcriptional terminator sequences. Preferred expresεion control εequenceε are promoterε derived from immunoglobulin genes, SV40, Adenoviruε, cytomegalovirus, Bovine Papilloma Virus, and the like.

The^' vectorε containing the DNA segments of interest (e.g., the heavy and light chain encoding sequences and expresεion control sequences) can be transferred into the host cell by well-known methods, which vary depending on the type of cellular host. For example, calcium chloride transfection is commonly utilized for prokaryotic cells, whereaε calcium phosphate treatment or electroporation may be used for other cellular hosts (see generally, Maniatiε et al . , Molecular Cloning: A Laboratory Manual, Cold Spring Harbor Press (1982) which is incorporated herein by reference) .

Once expressed, the whole antibodies, their dimers, individual light and heavy chains, or other immunoglobulin forms of the present invention, can be purified according to standard procedures of the art, including ammonium sulfate precipitation, affinity columns, column chromatography, gel electrophoresis and the like (see generally, R. Scopes, "Protein Purification", Springer-

Verlag, New York (1982)). Substantially pure immunoglobulins of at least about 90 to 95% homogeneity are preferred, and 98 to 99% or more homogeneity most preferred, for pharmaceutical uses. Once purified, partially or to homogeneity as desired, the polypeptides may then be used therapeutically (including extracorporeally) or in developing and performing asεay procedures, immunofluorescent εtainingε and the like (see generally, Immunological Methods, Vols. I and II, Lefkovits and Pernis, eds., Academic Press, New York, New York (1979 and 1981)) .

For diagnostic or detection purposes, the antibodies may either be labeled or unlabeled. Unlabeled antibodies can be uεed in combination with other labeled antibodies (second antibodies) that are reactive with the humanized antibody, such as antibodies specific for human immunoglobulin constant regions. Alternatively, the antibodies can be directly labeled. A wide variety of labels can be employed, such as radionuclides, fluors, enzymes, enzyme substrates, enzyme cofactors, enzyme inhibitors, ligands ⁽particularly haptens) , etc. Numerous types of immunoassays are available and are well known to those skilled in the art for detection of CCR5 -expressing cells or detection of CCR5 modulation on cells capable of expressing CCR5.

The present invention also provides antibody fragment- polymer conjugates having an effective size or molecular weight that confers an increase in serum half-life, an increase in mean residence time in circulation (MRT) and/or a decrease in serum clearance rate over underivatized antibody fragments.

The antibody fragment -polymer conjugateε of the invention can be made by derivatizing the desired antibody fragment with an inert polymer. It will be appreciated that any inert polymer which provides the conjugate with the desired apparent size or which has the selected actual molecular weight is suitable for use in constructing the antibody fragment -polymer conjugates of the invention.

Many inert polymers are suitable for use in pharmaceuticalε . See, e.g., Davis et al . , Biomedical Polymers: Polymeric Materials and Pharmaceuticals for Biomedical Use, pp. 441-451 (1980). In all embodiments of the invention, a non-protinaceous polymer is used. The nonprotinaceous polymer ordinarily iε a hydrophilic synthetic polymer, i.e., a polymer not otherwiεe found in nature. However, polymerε which exist in nature and are produced by recombinant or in vitro methods are also useful, aε are polymers which are isolated from native sources. Hydrophilic polyvinyl polymerε fall within the scope of this invention, e.g., polyvinylalcohol and polyvinvypyrrolidone. Particularly useful are polyalkylene ethers such as polyethylene glycol (PEG) ; polyoxyalklyenes such as polyoxyethylene, polyoxypropylene and block copolymers of polyoxyethylene and polyoxypropylene (Pluronicε) ; polymethacrylates; carbomers; branched or unbranched polysaccharideε which compriεe the saccharide monomerε D-mannoεe, D- and L-galactoεe, fucoεe, fructose, D- xyloεe, L-arabinose, D-glucuronic acid, εialic acid, D- galacturonic acid, D-mannuronic acid (e.g., polymannuronic acid, or alginic acid), D-glucoεamine, D-galactoεamine , D-glucose and neuraminic acid including homopolysaccharideε and heteropolyεaccharideε such as lactose, amylopectin, starch, hydroxyethyl starch, amylose, dextran sulfate, dextran, dextrinε, glycogen, or the polyεaccharide subunit of acid mucopolyεaccharides , e.g., hyaluronic acid, polymerε of εugar alcoholε such as polysorbitol and polymannitol , heparin or heparon. The polymer prior to croεε-linking need not be, but preferably iε, water εoluble but the final conjugate muεt be water εoluble. Preferably, the conjugate exhibits a water solubility of at least about 0.01 mg/ml and more preferably at least about 0.1 mg/ml, and still more preferably at least about l mg/ml. In addition the polymer should not be highly immunogenic in the conjugate form, nor should it possess viscosity that iε incompatible with intraveneous infuεion or injection if the conjugate iε intended to be adminiεtered by εuch routes.

In one embodiment, the polymer contains only a single group which is reactive. This helpε to avoid cross- linking of protein molecules. However it is within the scope of the invention to maximize reaction conditions to reduce cross- linking, or to purify the reaction products through gel filtration or ion-exchange chromatography to recover substantially homogeneous derivatives. In other embodiments the polymer contains two or more reactive groups for the purpose of linking multiple antibody fragments to the polymer backbone. Again, gel filtration or ion-exchange chromatography can be used to recover the desired derivative in substantially homogeneous form.

The molecular weight of the polymer can range up to about 500,000 D and preferably is at least about 20,000 D, or at least about 30,000 D, or at least about 40,000 D. The molecular weight chosen can depend upon the effective size of the conjugate to be achieved, the nature (e.g., structure such as linear or branched) of the polymer and the degree of derivitization, i.e., the number of polymer molecules per antibody fragment, and the polymer attachment site or sites on the antibody fragment .

The polymer can be covalently linked to the antibody fragment through a multifunctional crosεlinking agent which reacts with the polymer and one or more amino acid residues of the antibody fragment to be linked. However, it is also within the scope of the invention to directly crosslink the polymer by reacting a derivatized polymer with the antibody fragment, or vice versa .

The covalent crosεlinking εite on the antibody fragment includeε the N-terminal amino group and epsilon amino groups found on lysine residues, as well other amino, imino, carboxyl, sulfhydryl, hydroxyl or other hydrophilic groups. The polymer may be covalently bonded directly to the antibody fragment without the use of a multifunctional (ordinarily bifunctional) crosslinking agent, as described in U.S. Patent No. 6,458,355.

The degree of substitution with such a polymer will vary depending upon the number of reactive sites on the antibody fragment, the molecular weight, hydrophilicity and other characteristics of the polymer, and the particular antibody fragment derivitization sites chosen. In general, the conjugate contains from 1 to about 10 polymer molecules, but greater numbers of polymer molecules attached to the antibody fragments of the invention are also contemplated. The desired amount of derivitization iε eaεily achieved by uεing an experimental matrix in which the time, temperature and other reaction conditions are varied to change the degree of substitution, after which the level of polymer substitution of the conjugates is determined by εize excluεion chromatography or other meanε known in the art .

Functionalized PEG polymerε to modify the antibody fragments of the invention are available from Shearwater Polymers, Inc. (Huntsville, Ala.). Such commercially available PEG derivatives include, but are not limited to, amino-PEG, PEG amino acid esters, PEG- hydrazide, PEG-thiol, PEG-succinate, carboxymethylated PEG, PEG-propionic acid, PEG amino acidε, PEG succinimidyl succinate, PEG succinimidyl propionate, succinimidyl ester of carboxymethylated PEG, succinimidyl carbonate of PEG, succinimidyl esters of amino acid PEGs, PEG-oxycarbonyli idazole, PEG- nitrophenyl carbonate, PEG treεylate, PEG-glycidyl ether, PEG-aldehyde , PEG-vinylεulfone, PEG-maleimide, PEG-orthopyridyl-diεulfide, heterofunctional PEGs, PEG vinyl derivatives, PEG εilanes and PEG phospholides . The reaction conditions for coupling these PEG derivatives will vary depending on the protein, the desired degree of PEGylation and the PEG derivative utilized. Some factors involved in the choice of PEG derivatives include: the desired point of attachment (such as lysine or cysteine R-groups) , hydrolytic stability and reactivity of the derivatives, stability, toxicity and antigenicity of the linkage, suitability for analyεiε, etc. Specific instructions for the use of any particular derivative are available from the manufacturer. The conjugates of this invention are separated from the unreacted starting materials by gel filtration or ion exchange HPLC.

The anti-CCR5 antibody or fragments thereof may be used in combination with one or more additional anti-viral agents selected from the group consisting of nonnucleoside reverεe transcriptase inhibitors (NNRTIs) , a nucleoside reverse transcriptase inhibitor, an HIV-1 protease inhibitor, a viral entry inhibitor and combinations thereof.

The known NNRTI compounds that may be used in the composition of the present invention include but are not limited to efavirenz, UC-781, HBY 097, nevirapine

(ll-cyclopropyl-5 , 11 , -dihydro-4 -methyl-6H-dipyrido [3,2- b:2'3'-] [1,4] diazepin-6-one) , delavirdine

( (Rescriptor™; Pharmacia Upjohn) (piperazine, l-[3-[(l- methyl -ethyl) amino] -2-pyridinyl] -4- [ [5-

[ (methysulfonyl) amino] -lH-indol-2-yl] carbonyl] - , monomethaneεulfonate) , SJ-3366 ( 1- (3 -cyclopenten-1- yl) methyl -6- (3 , 5-dimethylbenzoyl) -5-ethyl -2 ,4- pyrimidinedione) , MKC-442 (6 -benzyl-1- (ethoxymethyl) -5- iεopropyluracil) , GW420867x (S-3 ethyl-6-fluro-4 - iεopropoxycarbonyl-3 , 4 -dihydro-quinoxalin-2 (1H) -one; Glaxo), HI-443 (N' - [2- (2-thiophene) ethyl] -N' - [2- (5- bromopyridyl) ] -thiourea) , and the like.

The nucleoεide reverεe transcriptase inhibitors that may be used in the composition in combination with at least one anti-CCR5 antibody or fragment thereof of the preεent invention include but are not limited to abacavir (Ziagen™, GlaxoSmithKline) ( (IS, cis) -4- [2- amino-6- (cyclopropylamino) -9H-purin-9-yl] -2- cyclopentene-1-methanol sulfate (salt) ) , lamivudine ⁽Epivir™, GlaxoSmthKline) ( (2R, cis) -4-amino-l- (2- hydroxymethyl-l,3-oxathiolan-5-yl) - (1H) -pyrimidin-2- one) , zidovudine (Retrovir™; GlaxoSmithKline) (3'azido- 3 ' -deoxythymidine) , stavudine (Zerit; Bristol-Myers Squibb) (2 ', 3 ' -didehydro-3 ' deoxythymidine) , zacitabine

(Hivid™; Roche Laboratories) (4 -amino-l-beta-D2 ' , 3 ' - dideoxyribofuranosyl-2- (1H) -pyrimidone) , didanosine, and the like.

The HIV-1 protease inhibitors that may be uεed in the composition in combination with anti-CCR5 antibody or fragments thereof of the present invention include but are not limited to lopinavir ( IS- [IR* , (R*) , 3R* , 4R*] ] -N- 4 - [ [ (2 , 6-dimethyphenoxy) acetyl] amino] -3 -hydroxy- 5- phenyl-l- (phenylmethyl) entyl] tetrahydro-alpha- (l- methylethyl) -2-oxol (2H) -pyrimidineacetamide) , saquinavir (N- tert-butyl -decahydro-2- [2 (R) -hydroxy-4- phenyl-3 (S) - [ [N- (2-quinolylcarbonyl ) -L- aεparaginyl] amino] butyl] - (4aS, 8aS) -iεoquinoline- (3S) - carboxamide) , nelfinavir meεylate ( [3S-

[2 (2S*, 3S*) ,3a,4β, 8aβ] ] -N- ( 1 , 1-dimethyetyl ) ecahydro- 2 [2 -hydroxy-3- [ (3 -hydroxy- 2 -methylbenzoyl) amino] -4-

(phenylthio) butyl] -3-isoquinolinecarboxamide mono- methane εulfonate) , indinavir sulfate

(([1(1S,2R),5(S))] -2,3,5-trideoxy-N- (2 , 3 -dihydro-2- hydroxy-lH-inden-1-yl) -5- [2- [ [ (1, 1- dimethylethyl) amino] carbonyl] -4- (3-pyridinylmethyl) -1- piperazinyl] -2- (phenylmethyl) -D-erythropentonamide sulfate (1:1) salt), amprenavir ( (3S) -tetrahydro-3- furyl N- [ (1S,2R) -3- (4-amino-W- isobutylbenzeneεulfonamido) -l-benzyl-2- hydroxypropyl] carbamate) , ritonavir ( (10-Hydroxy-2- methyl-5- (l-methylethyl) -1- [2- (1-methylethyl) -4- thiazolyl] -3, 6-dioxo-8, 11-biε (phenylmethyl) -2, 4, 7, 12- tetraazatridecan-13-oic acid, 5-thiazolylmethyl ester, [5S-(5R*, 8R*, 10R*, 11R*)]), and the like. HIV-l fusion or viral entry inhibitors that may be used in combination with the anti-CCR5 antibody or fragments thereof of the present invention include PRO 542 (Progenies Pharmaceuticals, Inc., Tarrytown, NY), T-20 (Trimeriε, Inc., Durham, NC) (US Patent Nos 5,464,933; 6,133,418; 6,020,459), T-1249 (US Patent No 6,345,568; 6,258,782), and the like.

For combination therapy, the anti-CCR5 antibody or fragment thereof of the present invention may be provided to the εubject prior to, εubεequent to, or concurrently with one or more conventional antiviral agents .

This invention will be better understood from the Experimental Details which follow. However, one skilled in the art will readily appreciate that the specific methods and resultε diεcuεsed are merely illustrative of the invention as described more fully in the claims which follow thereafter. Experimental Details:

Example 1

A. Materials and Methods

1 ) Reagents

MAb 2D7 was purchased from Pharmingen (San Diego, CA) and CC- and CXC-chemokines were obtained from R&D Syεtemε (Minneapolis, MN) . CD4-IgG2 (1), soluble (s) CD4 (2) and recombinant HIV-1_JR._FL gpl20 , were produced by Progenies Pharmaceuticals, Inc. (59).

2) Isolation and purification of anti-CCR5 mAbs L1.2-CCR5^* cells (63) were incubated for 16h in the presence of 5mM sodium butyrate, which activates tranεcription from the cytomegaloviruε (CMV) promoter that controls CCR5 expression, resulting in a 10-fold increase in cell εurface co-receptor density. Female Balb/c mice were immunized intraperitoneally with 10⁷ L1.2-CCR5^* cells at 3-week intervals, and administered an intravenous boost of 10⁷ LI .2-CCR5^* cells three days prior to εplenectomy. Splenocytes were fused with the Sp2/0 cell line. In a primary εcreen, εupernatants from ten thousand hybridoma cultures were tested; one hundred and twenty of these inhibited HIV-1 envelope- mediated fusion between PM1 cells (10) , which naturally expresε CCR5 and CD4 , and HeLa-Env_JR._FL ^* cells in a resonance energy transfer (RET) asεay, as previously described (19, 38) . Hybridomas that produced the most potently inhibitory supernatants and that also stained CCR5^* cells were sub-cloned by limiting dilution. Ascites fluidε were prepared by Harlan Bioproducts for Science, Inc. ( Indianapoliε , IN) from Balb/c mice that were injected with hybridomas producing the anti-CCR5 mAbs PA8, PA9 , PA10, PA11, PA12 and PA14. The mAbs were individually purified to >95% homogeneity by precipitation with ammonium sulfate followed by protein-A chromatography. All mAbs were resuspended in phosphate buffered saline (PBS) at a final concentration of 5mg/ml .

3 ) Fluorescence activated cell sorting (FACS) analysis and epitope mapping of anti-CCR5 mAbs Flow cytometry was used to detect cell-surface reactivity of mAbs PA8-PA12 and PA14 with CCR5. Sodium butyrate treated L1.2-CCR5* cells (10⁶) were incubated with 0.25μg of antibody, for 20min at 4°C in 0.1% sodium azide (NaN₃) in 50 μl of Dulbecco's PBS (DPBS) . The CCR5 mAb 2D7 was used as a positive control, a non-specific murine IgGi was used aε a negative control. The cellε were spun down, washed and incubated with phycoerythrin (PE) -labeled goat anti -mouse IgG (Caltag, Burlingame, CA) diluted 1:100, under the same conditions as the first antibody incubation. Finally, cells were analyzed by flow cytometry. PBMC were isolated and stimulated as previously deεcribed (60) and εtained uεing similar methods .

A similar procedure was used for epitope mapping of the anti-CCR5 mAbε . A panel of seventy CCR5 point mutants has been described (20, 24, 52) . The coding sequenceε of theεe proteinε are εub-cloned into the pcDNA3.1 vector (Stratagene) from which tranεcription can be driven by a 5 ' T7 -polymerase promoter. The CCR5 mutants carry a 9-residue hemaglutinin (HA) tag at the C- terminuε for detection of protein in cell lysates or by flow cytometry. HeLa cells (2xl0⁶) were incubated for 5h with 20μg/ml lipofectin and an equal amount of wild- type or mutant CCR5-expreεsing plasmid in OPTI-MEM (Life Technologies, Gaitherεburg, MD) . The cells were then infected for 12h with 2xl0⁷ p.f.u. of vTF7 (23) to booεt CCR5 expreεsion, detached with 2mM ethylenediamine tetracetic acid (EDTA) in PBS and washed once with binding buffer (1% BSA, 0.05% NaN₃ in DPBS) . Cells (lxlO⁶) were surface labeled with mAbs as deεcribed in the previous paragraph, washed once with the incubation buffer and resuspended in 1ml of lx FACSlyse in water (Becton Dickinson) for 30min at room temperature, to permeabilize the cell membranes. The cells were then spun down, washed with the incubation buffer and incubated for lh at 37°C with 4μg/ml of a fluorescein isothiocyanate (FITC) -labeled mouse anti-HA mAb (BabCo, Richmond, CA) for intracellular labeling. Finally, cells were washed once with binding buffer and once with DPBS, resuspended in 1% formaldehyde in PBS and analyzed by flow cytometry. The extent of binding of a mAb to mutant CCR5 was determined by the equation (mutant CCR5 PE m.f.i. / wt CCR5 PE m.f.i.) / (mutant CCR5 FITC m.f.i. / wt CCR5 FITC m.f.i.) xl00%. This normalizeε mAb binding for mutant co-receptor expreεsion levels.

4) gpl20/sCD4-binding assay gpl20 was biotinylated using NHS-biotin (Pierce, Rockford, IL) according to the manufacturer's instructions, and uncoupled biotin was removed by diaf iltration. Sodium butyrate-treated L1.2-CCR5^* cells were incubated with varying dilutions of an equimolar mixture of sCD4 and biotinylated gpl20, or 1.25μg/ml of sCD4 and 2.5μg/ml of biotinylated gpl20 in the presence of varying concentrations of anti-CCR5 mAbs PA8-PA12, PA14, 2D7 or a non-specific murine IgGi, for lh at room temperature in 0.1% NaN₃ in DPBS. Cells were washed with the incubation buffer and incubated with streptavidin- PE (Becton Dickinson) diluted 1:50, for lh at room temperature. Finally, cells were washed with binding buffer and analyzed using a fluorescence plate reader (Perspective Biosystems, Framingha , MA) .

5 ) Inhibition of envelope-mediated cell-cell fusion and HIV-1 entry by anti-CCR5 mAbs

HIV-1 envelope-mediated fusion between HeLa-Env_JR._FLι ⁺ and PM1 cellε waε detected using the RET assay. Equal numbers (2xl0⁴) of fluorescein octadecyl eεter (F18) - labeled envelope-expressing cells and octadecyl rhodamine (R18) -labeled PM1 cellε were plated in 96- well plateε in 15% fetal calf serum in DPBS and incubated for 4h at 37°C in the presence of varying concentrationε of the anti-CCR5 mAbs, PA8-PA12, PA14 , 2D7 or a non-specific murine IgGi. Fluorescence RET was measured with a Cytofluor plate-reader (PerSeptive Biosyεtemε) and % RET waε determined as previously described (38) .

NLluc⁺env^" viruses complemented in trans by envelope glycoproteins from JR-FL or Gun-1 were produced as previously described (20) . U87MG-CD4^*CCR5⁺ cells (14) were infected with chimeric, reporter viruses containing 50-100ng/ml p24 in the presence of varying concentrations of the individual mAbs. After 2h at 37°C, viruε-containing media were replaced by freεh, mAb- containing media. Freεh media, without antibodieε, were added again after 12 hours. After a total of 72h, lOOμl of lysiε buffer (Promega) were added to the cells and luciferase activity (r.l.u.) was measured as deεcribed (20) . The % inhibition of HIV-l infection iε defined aε [1- (r.l.u in the presence of antibody / r.l.u in the absence of antibody)] x 100%.

6) Calcium signaling assays

The fluorochrome Indo-IAM (Molecular Probes, Eugene, OR) waε added to sodium butyrate treated L1.2-CCR5^* cells at a final concentration of 5μM. After incubation at 37°C for 30min, the cells were washed once and resuspended in Hank's buffered saline. Cellε (10⁶) were stimulated sequentially with an anti-CCR5 mAb or PBS, followed 60s later with RANTES. MAbε PA8-PA12 and PA14 were uεed at a concentration of lOOμg/ml, 2D7 at 20μg/ml and RANTES at 250ng/ml. Calcium flux inhibition by PA14 and 2D7 was also tested for a wide range of mAb concentrations, ranging from 0-100μg/ml. Intracellular calcium levelε were monitored using a Perkin-Elmer LS- 50S fluorescence spectrophotometer by measuring the ratio of fluorescence emiεsions at 402nm (bound dye) and 486nm (free dye) following excitation at 358nm.

B. Results and Discussion

1) Isolating anti-CCR5 monoclonal antibodies PA8 , PA9, PA10, PA11, PA12 and PA14

It waε found that pep ideε corresponding to the extracellular domainε of CCR5 are inefficient at raiεing specific, high-titer antibody responses against the native, cell surface receptor (50) . Balb/C mice were immunized, therefore, with L1.2-CCR5" cells and hybridoma culture supernatants were tested for their ability to inhibit JR-FL envelope-mediated membrane fusion with CD4^*CCR5^* PM1 cellε in the RET assay (19, 38) . Even though well over a hundred supernatantε inhibited cell-cell fuεion by >50%, only εix deεignated PA8, PA9 , PA10, PA11, PA12 and PA14 εpecifically and intensely stained L1.2-CCR5^* but not the parental LI .2 cells, as demonstrated by flow cytometry (data not shown) . Based on previous experience, it was assumed that the other mAbs capable of inhibiting cell-cell fusion were probably directed against cell surface adhesion molecules such as LFA-1 (37) . Hybridomas PA8-PA12 and PA14 were determined by isotyping ELISA (Cappell, Durham, NC) to secrete IgGi mAbs. Asciteε fluidε were prepared from Balb/C mice that were injected with the six hybridomas and the IgGi fractions were purified. PA8 , PA9 , PA11, PA12 and PA14 exhibited distinct isoelectric focuεεing profileε, whereaε PA10 had a very εimilar profile to that of PA9 and therefore may be a εecond iεolate of the εame mAb (data not εhown) .

2) MAb binding to CCR5+ cells

None of the purified anti-CCR5 mAbs stained the parental LI .2 cell line (data not shown). However, mAbs PA9-PA12 and PA14 stained >90%, and PA8 stained -70%, of L1.2-CCR5^* cells as determined by flow cytometry, showing they recognized CCR5 (Figure 1) . The anti-CCR5 mAb 2D7, which was a positive control in our experiments, alεo stained >90% of L1.2-CCR5^* cells. PA8- PA12 and PA14 are all IgGi, and react equally well with a goat anti -mouse IgG, whereas 2D7 is an IgG2a and may react differently with the reporter antibody. Only mean fluorescence intensitieε (m.f.i.) measured with mAbs PA8-PA12 and PA14 therefore are directly comparable. The rank order of mean fluorescence intensities (m.f.i.) was PA12- PA11> (2D7=) PA14- PA10- PA9> PA8. The difference between PA12 m.f.i. and PA8 m.f.i. was three-fold. Differences in staining intensity between PA8 and the other mAbs remained constant over a wide range of concentrations (data not shown) and probably do not correspond to differences in mAb affinities for CCR5. This implies that PA8 interacts only with a εubεet of CCR5 moleculeε preεent on the surface of L1.2-CCR5^* cellε.

Compared with L1.2-CCR5+ cells, mitogen-stimulated PBMC exhibited different patterns of staining by the anti- CCR5 mAbε. 2D7 and PA14 εtained >20%, PAH and PA12 εtained -10%, PA8 , PA9 and PA10 εtained <5% of PBMC (Figure 1) . The mean fluoreεcence intensities of the stained PBMC were about ten- fold lower than those obtained with L1.2-CCR5^* cellε for each mAb; their rank order was (2D7>) PA14> PA12- PA11- PA10- PA9- PA8. Again, this differed somewhat from the order of reactivities observed on CCR5 transfectants . The difference between PA9 m.f.i. and PA14 m.f.i. waε εeven-fold. Other groupε have observed similar differences in the ability of anti-CCR5 mAbs to stain stable, CCR5^* cell lineε versus PBMC (28) . This may be due to cell-εpecific differences in CCR5 conformation, post-tranεlational modification or oligomerization. Alternatively, association with other cell surface molecules may differ between cells. Since an obvious choice for such a molecule would be the CD4 cell surface antigen, which is abεent from L1.2-CCR5⁴ cells and present on PBMCs, we also tested the ability PA8- PA12, PA14 and 2D7 to stain HeLa cells transiently expressing CCR5 alone or with CD4. No differences were observed in the ability of any of the mAbs to stain cell surface CCR5 in the presence of CD4 (data not εhown) . If there iε an aεεociation between theεe two proteins, it doeε not involve epitopeε recognized by the anti-CCR5 mAbs available to u . Alternatively, an aεεociation between CCR5 and CD4 might only occur on primary lymphocyteε .

3) Epitope mapping of the mAbε uεing CCR5 alanine mutantε None of the antibodies were able to detect reduced and denatured CCR5 protein by Western blotting indicating that they recognize conformationally εenεitive epitopeε

(data not εhown) . MAb epitope mapping studies were performed using a panel of seventy alanine point mutantε of residues in the Nt and ECLs of CCR5. HeLa cells were lipofected with mutant or wild type CCR5 coding sequences appended with C-terminal HA tags, and infected with vTF7 (23) to boost co-receptor expresεion. The cellε were then incubated with the anti-CCR5 mAbs and their binding waε revealed by a PE- labeled goat anti-mouεe IgG. A εecond, intracellular εtain waε performed with a FITC-labeled anti-HA mAb

(BabCo) . This internal control allowed us to directly normalize staining by the anti-CCR5 mAbs for mutant coreceptor expression levels on the cell surface. Hence, mAb binding to each mutant is expressed as a percentage of binding to wild-type CCR5 (Figure 4) .

Certain point mutationε reduced the binding of all of the antibodieε to CCR5 by >50%. In general, PA8-PA12 were the most affected, PA14 and 2D7 the least affected by this clasε of mutantε, which included the cysteine pair C101A and C178A, the Nt mutantε Y10A, D11A, K25A, the ECL1 mutant D95A, the ECL2 mutantε K171A/E172A, Q188A, K191A/N192A, and the ECL3 mutants F263A and F264A (Fig. 1). One interpretation is that these residues are not part of the mAb epitopes per se, but that changing them to alanines causes conformational perturbationε that have a common effect on binding of all mAbs. We asεumed that if a mutation lowered binding of an individual mAb by >75%, and did not also lower binding of most of the other antibodies, the residue waε probably a direct contributor to the epitope recognized by the mAb. Uεing these stringent guidelineε, it was concluded that the seven anti-CCR5 mAbs recognize overlapping but distinct epitopes (Figure 4) . MAb PA8 binding to CCR5 depended on N13 and Y15 in the Nt . MAb PA9 and PA10 required D2 , Y3 , Q4 , P8 and N13 in the Nt , and Y176 and T177 in ECL2. MAb PA9 also required S7 in the Nt . MAb PA11 and PA12 binding depended on Q4 in the Nt . PA14 required D2 in the Nt , and R168 and Y176 in ECL2. Finally, mAb 2D7 required Q170 and K171/E172 in ECL2 in order to bind to CCR5.

) Chemokine signaling in the presence of anti-CCR5 mAbs Chemokine receptor-binding agents can be antagonists or, more rarely, agoniεts of receptor-mediated intracellular signaling. Alternatively, they could have no effect on εignaling. CCR5 is able to bind three CC- chemokines, RANTES, MlP-lα and MlP-lβ, and transduce a εignal that modulateε cytoεolic calcium levelε. We therefore teεted the agonist/antagonist activity of various concentrations of mAbs PA8-PA12, PA14 and 2D7. Changes in intracellular calcium concentrationε, (Ca^2*)i, were measured in Indo-1- loaded L1.2-CCR5^* cells. None of the mAbs stimulated a change in (Ca²⁺)i, indicating that they are not agonistε for CCR5. PA8- PA12 were also unable to inhibit Ca^2* fluxes induced by RANTES (Fig.5A and data not shown), even at concentrations as high as lOOμg/ml, showing they are not antagonists either. These concentrations provide saturating binding of the mAbs to L1.2-CCR5^* cells, as shown by flow cytometry and the gpl20/CCR5 binding aεsay (Fig. 6D and data not shown) . MAbs PA14 and 2D7, however, blocked calcium mobilization induced by RANTES, although with different potencies (Fig.5A, 5B) . The IC₅₀ for PA14 calcium influx inhibition was 50μg/ml, which was approximately 8-fold higher than the IC₅₀ for 2D7 (Fig. 5B) . RANTES-, MlP-lα- and MlP-lβ-induced calcium fluxes were each inhibited by similar concentrations of PA14 (data not shown) . None of the mAbε affected SDF-1- induced calcium mobilization in L1.2-CCR5^* cellε, which endogenously express CXCR4 (data not shown) . Finally, neither mAbs nor CC-chemokines affected cytosolic calcium levels in parental LI .2 cells (data not shown) .

5) Inhibition of CCR5 co-receptor function by the mAbs

MAbs PA8-PA12 and PA14 were initially selected on the basiε of their ability to inhibit HIV-1 envelope- mediated cell -cell fusion. This activity was confirmed and quantified for the purified mAbε. As expected, all six mAbε, aε well aε mAb 2D7, blocked fusion between CD4^*CCR5^* PM1 cells and HeLa-Env_JR__FL ^* cells in the RET aεεay. The rank order of potency waε 2D7- PA14> PA12> PA11> PA10- PA9- PA8 (Fig. 6A) . IC₅₀ values for PA14 and 2D7 were 1.7μg/ml and 1.6μg/ml reεpectively, for PA11 and PA12 theεe were 25.5μg/ml and lO.Oμg/ml respectively (Figure 3) . PA8 , PA9 and PA10 inhibited fusion by only 10-15% at 300μg/ml. None of the mAbs affected fusion between PM1 cells and HeLa-Env-^^* cells, which expresε the full length envelope protein from an X4 viruε (data not εhown) .

The ability of the different anti-CCR5 mAbs to inhibit entry of a prototypic R5 virus, JR-FL, and a R5X4 virus, Gun-1, in a single-round of replication, luciferase-based entry assay was also tested. The rank order of potency in the entry assay was similar to the one determined in the cell-cell fusion aεεay (Fig. 6B) . A >50% inhibition of JR-FL or Gun-1 entry with PA8-PA11 waε unable to be obtained. The IC₅₀ value for PA12 waε 2.5 μg/ml. However, inhibition of entry by >60% with this mAb waε unable to be obtained. The IC₅₀ valueε for PA14 and 2D7 inhibition of JR-FL entry were determined to be 0.024 and 0.026 μg/ml respectively (Figure 3), and were 60 -fold lower then thoεe obtained in the fuεion aεεay. Entry of dual-tropic Gun-1 was 2-3-fold more sensitive to inhibition by anti-CCR5 mAbs than JR- FL entry (data not shown) .

Anti-co-receptor mAbε might inhibit envelope-mediated fusion either by directly affecting the gpl20/CCR5 interaction or by impeding post -binding steps involved in the formation of an active fusion complex. To determine the mechanism of inhibition of viral fusion and entry by PA8-PA12 and PA14 , the ability of the different mAbs to block the gpl20/CCR5 interaction waε tested. For this an asεay that detectε binding to L1.2- CCR5^* cellε of biotinylated HIV-l_JR._Flj gpl20 complexed with εCD4 was uεed. No binding of biotinylated gpl20 waε obεerved in the abεence of sCD4 or CCR5 , or when HIV-1-_j._j gpl20 was used (Fig. 6C) .

With the exception of PA8 , all mAbs abrogated gpl20/sCD4 binding to L1.2-CCR5^* (Fig. 6D) . Inhibition by PA8 saturated at -40%, which concurs with flow cytometry data (Figure 1) in suggeεting that thiε mAb binds only to a subset of CCR5 molecules on L1.2-CCR5^* cellε. MAbs PA9, PA10, PA11 and PA12 inhibited binding with IC₅₀ values of 0.24, 0.13, 0.33, 0.24 μg/ml respectively (Figure 3). Surprisingly, mAbs PA14 and 2D7 were the two least efficient inhibitors of gpl20/εCD4 binding, with IC₅₀ valueε of 1.58 and 1.38 μg/ml reεpectively (Figure 3) . Therefore, there was no correlation between the ability of a mAb to inhibit gpl20/CD4/CCR5-mediated membrane fusion and entry and its ability to block gpl20/sCD4 binding to the coreceptor .

6 ) Synergistic inhibition of HIV-1 fusion by combinations of anti-CCR5 mAbε and other viral entry inhibitorε

Co-receptor-specific agents may act at multiple stages of the entry procesε and exhibit non-additive effectε when uεed in combination. From a clinical perspective, it is important to determine the interactions of co- receptor-specific drug candidates with endogenous chemokines, which may afford some level of protection against diεease progression. CCR5 mAbs were therefore tested in combination with each other or with RANTES, or with CD4-IgG2, which binds to HIV-1 gpl20 to inhibit attachment to target cells. Dose-response curves were obtained for the agents used individually and in combination in viral fusion and entry assays. Data were analyzed using the median effect principle (9) . The concentrations of εingle-agentε or their mixtureε required to produce a given effect were quantitatively compared in a term known as the Combination Index (CI) . A CI value greater than 1 indicates antagonism, CI - 1 indicates an additive effect, and CI < 1 indicateε a εynergiεtic effect wherein the presence of one agent enhances the effect of another.

Combinationε of PA12 and 2D7 were the most potently synergistic, with CI valueε ranging between 0.02 and 0.29, depending on the ratio of the antibodies (Fig. 7 and Figure 2) . The degree of synergy is known to vary with the stoichiometry of the agents. The viral entry and fusion assays were generally consistent in identifying mAb combinations that are highly synergistic, PA12 and 2D7; moderately synergistic, PA12 and PA14; additive, PA11 and PA12; and weakly antagonistic, PA14 and 2D7. The lack of synergy between PA14 and 2D7 is not surpriεing given that theεe mAbε crosε-compete for binding to CCR5^* cells as determined by flow cytometry (data not shown) . The observation of an additive effect of PA11 and PA12 may be an indication that these mAbε bind to εlightly different epitopeε in CCR5 , while sharing a dependency on residue Q4 in the Nt .

The ability of mAbs PA12, PA14 and 2D7 to synergize with RANTES in blocking cell-cell fusion was also tested. PA12 and RANTES combinations exhibited moderate εynergy (Figure 2) . PA14 and 2D7 exhibited no synergy with RANTES, which is consiεtent with these mAbs being inhibitory of RANTES binding and signaling (Fig. 5A, 5B) . Finally, we tested synergy between mAbε PA12, PA14, 2D7 and CD4-IgG2, which interactε with gpl20. We obεerved moderate synergy between PA12 and CD4-IgG2 but no εynergy between PA14 or 2D7 and CD4-IgG2 (Figure 2) .

Experimental Discussion

Six murine anti-CCR5 IgGi mAbε were isolated and characterized. Whereas PA8 , PA9 , PA11, PA12 and PA14 are distinct molecular species, PA9 and PA10 are indistinguishable by the analyses and therefore are probably the same mAb. All of the mAbs that were isolated recognize complex conformational epitopes, as iε often the case with mAbε raised against native, cell surface proteins. Epitope mapping was performed for all mAbs using a panel of CCR5 alanine point mutants. Residues that affected binding of all mAbs similarly were assumed to cause conformational perturbations in the co-receptor and not to constitute part of the mAb epitopeε. Only two such residues, Y10 and Dll, have been shown to affect HIV-1 entry (20, 52) . The PA8 , PA11 and PA12 epitopes are located exclusively in the Nt domain. Consistent with this result, PA8 waε able to bind a biotinylated Nt peptide, containing reεidueε D2 through R31, in an ELISA (data not shown) . However, PAll and PA12, whose binding strongly depended only on Q4 , did not bind the Nt peptide in εolution (data not εhown) . One poεεibility iε that the Nt peptide doeε not assume the proper conformation for recognition by PAll and PA12, whereas PA8 binding may be lesε conformation- dependent. Alternatively, PAll and PA12 might interact with reεidues that we have not mutated, or form weak bonds with amino acidε located in other domains of CCR5 , or bind peptide backbone atoms whose presentation may be unchanged by mutagenesis. Antibodies PA9 , PA10 and PA14 recognized epitopeε that included reεidueε in both the Nt and ECL2 domainε of CCR5 , whereaε the 2D7 epitope waε located excluεively in ECL2.

The PA14 epitope comprises both D2 in the Nt and R168 in ECL2 indicating that these two residues are proximal to one another within the context of a mAb footprint . They may even directly interact with one another through their opposite charges.

MAbε PA8-PA12 and PA14 stained CCR5^* cells with different intensitieε and in a cell type-dependent manner. All mAbs except PA8 stained >90% L1.2-CCR5^* cells, the highest mean fluorescence intensity being observed with PAll and PA12. However, PA14 and 2D7 stained the highest percentage of PBMC and also yielded the highest mean fluorescence intensitieε on theεe cellε. Hill et al . (28) have recently characterized a panel of anti-CCR5 mAbs that similarly stained transfected cells, but only two of eight stained PBMC, and none stained primary monocytes. A low affinity for CCR5 probably accounted for the non-reactivity of two of the mAbs with primary cells, but this was unlikely to be the explanation for^' the failure of the other four to react. In our mAb panel, we observe the most intense staining of PBMC by mAbs 2D7 and PA14 that have epitopes located entirely or partially in the first ten residueε of ECL2. Hill et al . report, however, that mAbs specific for the Nt and ECL1 εtain PBMCε, while mAbs to ECL2 and ECL3 do not stain PBMC, so a conεistent pattern of reactivity has not been identified. One explanation for cell type-specific staining by mAbs would be that activated PBMCs (and monocytes) secrete CC-chemokineε that bind to cell εurface CCR5 , masking some mAb epitopeε. However, one would expect thiε to be eεpecially true for PA14 and 2D7 , which are antagoniεtε of chemokine-induced calcium mobilization and presumably compete with CC-chemokines for binding to CCR5. Yet theεe mAbε εtain PBMC the moεt intenεely. Alternatively, differential CCR5 epitope exposure may reflect cell type-εpecific receptor oligomerization, aεsociation with other cell-surface moleculeε, or different poεt-translational modifications such as glycosylation. We have εhown that differenceε in mAb binding probably do not reflect cell type-specific differences in CD4/CCR5 interactions.

MAbs PA8-PA12 did not inhibit CC-chemokine induced calcium mobilization in CCR5^* cells, nor did they mediate εignaling through CCR5. MAbε 2D7 and PA14 were inhibitorε of CC-chemokine induced calcium mobilization, but 2D7 waε almoεt an order of magnitude more potent than PA14. This may be because the PA14 epitope overlaps less with the CC-chemokine binding domain on CCR5 than the 2D7 epitope. All of the mAbs also blocked HIV-1 entry and envelope-mediated membrane fuεion, but inhibition of cell-cell fuεion required in εome caεeε almoεt two orders of magnitude more antibody than what was needed to block viral entry. Presumably, more gpl20/CD4/CCR5 interactions as well as interactions between adhesion molecules are established and act cooperatively during cell-cell fusion, compared to virus-cell fusion, making it more difficult to inhibit. This is commonly obεerved with antibodieε to LFA-1 or to the HIV-1 envelope glycoprotein (45, 51) . PA8, PA9 and PA10 were unable to block cell -cell fusion by >15% and viral entry by >40%, even at the highest antibody concentrations. However, >90% inhibition of fusion could be attained with PAll, PA12 and PA14 , and >90% inhibition of entry could be attained with PA14. The moεt potent of the six mAbs in blocking fusion and entry waε PA14 , which was as effective aε 2D7. Surpriεingly, PA14 and 2D7 were among the leaεt potent inhibitors of gpl20/sCD4 binding to L1.2-CCR5^* cellε, whereas PA9-PA12 blocked with similar potencies, and PA8 was unable to block >40% of gpl20/sCD4 binding. Theεe observationε raise questions about the nature of the CCR5 molecules presented on different cellε and about the mechanisms of inhibition of viral fusion and entry. It may be that CCR5 on LI .2 cells, used in the mAb and gpl20-binding assays, iε not in an identical conformation to CCR5 on PBMC, used in the mAb-binding asεay, or to CCR5 on PM1 and U87MG cells used in the fusion and entry assays.

The low staining of PBMC and the partial inhibition of fusion and entry by some of our mAbs indicate that they are only able to bind to a subset of CCR5 molecules expressed on primary lymphocytes, PM1 and U87MG- CD4^*CCR5^* cell lines. Yet, other than PA8 , all mAbs are able to stain >90% L1.2-CCR5^* cells and to completely block binding of the gpl20/sCD4 complex to these cells. At least one difference between L1.2-CCR5^* and the other cells that we have uεed iε the denεity of co-receptor protein on the cell surface. Indeed, we estimate that the L1.2-CCR5^* cells express 10- to 100-fold more cell surface co-receptor than PM1 and U87MG-CD4⁺CCR5^* cellε. But when HeLa cellε are engineered to tranεiently express as much co-receptor as the L1.2-CCR5^* cell line, we are still unable to detect gpl20/sCD4 binding to them (data not shown). Over-expression of CCR5 on L1.2, along with other cell -specific factors therefore, might favor a co-receptor conformation that prominently expoεes the Nt , making it more accesεible to both mAbε and gpl20. Such a conformation might be induced by receptor oligomerization, by diminiεhed or altered associationε with cell surface proteins or by receptor interactions with G proteins (25, 62) . Do multiple conformations of CCR5 co-exist on the cell surface, and are they all permiεεive for viral entry? The patterns of mAb reactivity would εuggeεt εo, εince HIV-1 entry and fusion can occur, albeit at reduced levels, in the presence of mAb concentrations that saturate epitopes required for gpl20 binding to L1.2-CCR5+ cells. We favor the hypothesis that the co-receptor molecules present on L1.2-CCR5^* cellε poεsess one HIV-l entry- competent conformation whereas CCR5 molecules on PBMC, PM1 and CCR5^* U87MG exist in multiple, entry-competent states that display different mAb reactivities. Whereas PA14 and 2D7 may recognize all conformations, other mAbs may not. Why LI .2 cellε are conducive to a particular fusion-competent conformation remains to be determined.

It has recently been demonstrated that the gpl20- binding domain lies in the first twenty residues of the CCR5 Nt domain. MAbs to the gpl20-binding domain on CCR5 potently block this interaction but are not nearly aε efficient at inhibiting HIV-1 fusion and entry into target cells as PA14 and 2D7 , whose epitopes lie outside this region. PA14 recognizes the tip of the Nt and residues in ECL2 , whereas the 2D7 epitope is located exclusively in ECL2. At the mechanism of action of these mAbs can only be speculated. It may be that their binding to the firεt few residues of ECL2 induces conformational changes in the co-receptor that prevent membrane fusion. Alternatively, obstruction of ECL2 epitopes might impede co-receptor oligomerization and the formation of a fusion-competent protein complex. Yet another possibility is that residueε in ECL2 face the inεide of the fuεion pore and binding of the mAbs impedes gp41 from inserting the fusion peptide into the plasma membrane. In contrast, mAbs PA8-PA12 probably inhibit fusion and entry only by directly competing for binding with gpl20/CD4 complexes. We do not know if parameters other than epitope exposure and affinity for CCR5 determine the efficacy of viral entry inhibition by these mAbs. It is unclear why inhibiting steps subsequent to the gpl20/co-receptor interaction would be more efficient than directly blocking that interaction. One way to explain this would be to assume that the off rate of gpl20 binding to CCR5 is much lower than the on rate of mAb binding to CCR5. Thus, every time a mAb detaches itself from a co-receptor molecule, a virion-associated gpl20 molecule replaces it in a quasi- irreversible fashion εince this interaction leads to membrane fusion.

Synergy between combinations of anti-CCR5 mAbs is probably a result of their interactions with distinct epitopes that are involved in inter-dependent, consecutive stepε of HIV-l entry. The degree of εynergy observed between PA12 and 2D7 (CI<0.1 under many circumstances) is extraordinary since CI values <0.2 are rarely observed for combinations of anti-HIV-1 antibodies (33, 35, 61), reverse transcriptase inhibitors (29), or protease inhibitors (44). Because of its potency, the PA12:2D7 combination was examined in multiple assay formats and concentration ratios, for which consistently high ^' levels of synergy were observed. Moderate synergy was observed for PA12 combined with PA14. We also observed moderate synergy between PA12 and CD4-IgG2. The CD4/gpl20 complex is metastable and if it is unable to interact with a coreceptor, decayε into a non-fusogenic state (45-48) . Since PA12 directly blocks the gpl20-binding site on CCR5, its preεence may shift the equilibrium towards inactivation of the gpl20/CD4 complex. This would explain why we obεerve εynergy between CD4-IgG2 and mAb PA12 with reεpect to inhibition of fusion and entry. The lack of synergy between mAb PA14 and CD4-IgG2 suggeεtε that they act on two non-consecutive and independent steps of viral entry. A combination of further studies will be needed to determine the precise mechanisms of synergy of the different compounds with respect to inhibition of viral fusion and entry.

The above reεults are consiεtent with a model wherein HIV-l entry occurε in three diεtinct steps involving receptor binding, co-receptor binding, and co-receptor mediated membrane fusion. Separate co-receptor binding and fusion events are suggeεted by the lack of correlation between the monoclonal antibodies' abilitieε to block gpl20 binding and HIV-l fusion/entry. The chronology of events during fusion is further suggeεted by the patterns of synergies observed. Agents, such as PA12, that potently inhibit the middle step of the process, namely gp 120 binding, act synergistically with inhibitors of prior and subεequent steps .

Example 2

Background: The increasing incidence of multidrug- resistant HIV-1 mandates the search for novel classes of antiretroviral agents. CCR5 is a requisite fusion coreceptor for primary HIV-1 isolates and provides a promising target for antiviral therapy. PRO140 is an anti-CCR5 monoclonal antibody that potently inhibits HIV-1 entry and replication at concentrations that do not affect CCR5 ' s chemokine receptor activity in vi tro . In the present study, we evaluated the therapeutic potential of PRO 140 in vivo using a therapeutic animal model of HIV-1 infection.

Methods : CD-17 SCID mice were reconstituted with normal human PBMC and infected with the R5 isolate HIV-1 JR- CSF. When viral steady state was reached, the animal were treated intraperitoneally with PRO 140 or control antibody and monitored for viral burden using the Roche Amplicor assay. Initial studies examined a single 1 mg dose of PRO140. In multi-dose studies, PRO 140 was administered once every three days for three weeks at doses ranging from 0.1-1.0 mg . In a separate experiment, flow cytometry was used to examine the potential for lymphocyte depletion following PRO 140 injection .

Results : Both single-dose and multi-dose PRO 140 reduced viral loads to undetectable levels in all treated animals, and the viral load reductions ranged to 1.8 log 10. A transitory control of viral replication was observed following single injection of PRO 140 while multiple injections led to a prolonged control with no evidence of viral rebound during therapy. Dose-dependent differences were observed in the kinetics of the PRO 140-mediated reductions in viral load. Flow cytometry analysis showed that treatment with PRO 140 did not lead to lymphocyte depletion, confirming that impact on viral replication in vivo was solely due to CCR5-blockage . Conclusions : PRO 140 is highly effective in controlling established HIV-1 infection in the hu-PBL-SCID mouse model of HIV-1 infection. These findings provide in vivo proof-of-concept for PRO 140 therapy in particular and for CCR5-inhibitors therapy in general.

Exam 1e 3

Methods :

A humanized CCR5 antibody (huPRO 140) was tested for the ability to block RANTES-induced calcium mobilization in L1.2-CCR5 cellε and the ability to block replication of HIV-1 CASE C 1/85 in human PBMC's using ethodε described herein.

Results :

The results as shown in Figure 19 shows that the humanized CCR5 antibody potently blocks HIV-1 but not RANTES .

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Claims

CLAIMSWhat is claimed:

1. An anti-CCR5 antibody which comprises (i) two light chainε, each light chain comprising the expresεion product of a plaεmid deεignated pVK:HuPRO140-VK (ATCC Depoεit Designation PTA- 4097), and (ii) two heavy chains, each heavy chain comprising the expresεion product of either a plaεmid designated pVgl :HuPRO140 HG2-VH (ATCC Depoεit Deεignation PTA-4098) or a plasmid designated pVgl :HuPRO140 (mut B+D+D-VH (ATCC Deposit Designation PTA-4099) , or a fragment of such antibody, which bindε to CCR5 on the surface of a human cell .

2. The anti-CCR5 antibody of claim 1, wherein the heavy chains are expresεed by the plasmid designated pVgl :HuPRO140 HG2-VH (ATCC Deposit Designation PTA- 4098) .

3. The anti-CCR5 antibody of claim 1, wherein the heavy chains are expressed by the plasmid designated pVgl :HuPRO140 (mut B+D+D-VH (ATCC Deposit Designation PTA-4099) .

4. An anti-CCR5 antibody comprising two light chains, each chain comprising consecutive amino acidε, the amino acid sequence of which is set forth in SEQ ID NO: 6, and two heavy chainε, each heavy chain comprising conεecutive amino acids, the amino acid sequence of which is set forth in SEQ ID NO: 9.

5. An anti-CCR5 antibody comprising two light chains, each light chain comprising conεecutive amino acids, the amino acid sequence of which is set forth in SEQ ID NO : 6 , and two heavy chains, each heavy chain comprising consecutive amino acidε, the amino acid εequence of which iε set forth in SEQ ID NO: 12.

6. An isolated nucleic acid encoding a polypeptide comprising consecutive amino acidε, the amino acid sequence of which is set forth in SEQ ID NO : 6.

7. The nucleic acid of claim 6, wherein the consecutive amino acidε are the amino acidε expressed by a plasmid designated pVK:HuPRO140-VK (ATCC Deposit Deεignation PTA-4097) .

8. The nucleic acid of claim 6, wherein the nucleic acid comprises the sequence εet forth in SEQ ID NO: 5.

9. The nucleic acid of any one of claims 6, 7 or 8 , wherein the nucleic acid is RNA, DNA or cDNA.

10.An isolated nucleic acid encoding a polypeptide comprising consecutive amino acids, the amino acid sequence of which is set forth in SEQ ID NO : 9.

11. The nucleic acid of claim 10, wherein the consecutive amino acidε are the amino acidε expreεsed by a plasmid designated pVgl :HuPRO140 HG2-VH (ATCC Deposit Designation PTA-4098) .

12. The nucleic acid of claim 10, wherein the nucleic acid compriseε the εequence εet forth in SEQ ID NO: 8.

13. The nucleic acid of any one of claims 10, 11 or 12 wherein the nucleic acid iε RNA, DNA or cDNA.

14.An isolated nucleic acid encoding a polypeptide comprising consecutive amino acids, the amino acid sequence of which is set forth in SEQ ID NO-.12.

15. The nucleic acid of claim 14, wherein the consecutive amino acids are the amino acids expressed by a plasmid designated pVgl :HuPRO140 (mut B+D+I) -VH (ATCC Deposit Designation PTA- 4099) .

16. The nucleic acid of claim 14, wherein the nucleic acid compriseε the sequence set forth in SEQ ID NO: 11.

17. The nucleic acid of any one of claimε 14, 15 and 16, wherein the nucleic acid iε RNA, DNA or cDNA.

18. A composition comprising at least one of the anti- CCR5 antibody or a fragment thereof, of any one of claims 1-5 and a carrier.

19.A composition comprising the anti-CCR5 antibody or a fragment thereof, of any one of claimε 1-5, having attached thereto a material selected from the group conεiεting of a radioiεotope, a toxin, polyethylene glycol, a cytotoxic agent and a detectable label.

20.A method of inhibiting HIV-1 infection of a CD4+ cell which compriεes contacting the CD4+ cell with an antibody which compriεeε (i) two light chains, each light chain co priεing the expreεsion product of a plasmid designated pVK:HuPRO140-VK (ATCC Deposit Designation PTA-4097) , and (ii) two heavy chains, each heavy chain comprising the expression product of either a plasmid designated pVgl :HuPRO140 HG2-VH (ATCC Deposit Designation PTA-4098) or a plaεmid deεignated pVgl :HuPRO140 (mut B+D+D-VH (ATCC Depoεit Deεignation PTA- 4099) , or a fragment of εuch antibody which binds to CCR5 on the εurface of the CD4+ cell, in an amount and under conditions such that fusion of HIV-1 or an HIV-1 infected cell to the CD4+ cell is inhibited, thereby inhibiting HIV-1 infection of the CD4+ cell .

21. The method of claim 20, wherein the CD4+ cell expreεεeε CCR5.

22.A method of treating a εubject afflicted with HIV- 1 which compriεeε adminiεtering to the εubject an effective HIV-1 treating doεage amount of an anti- CCR5 antibody comprising (i) two light chains, each light chain comprising the expresεion product of a plasmid designated pVK:HuPRO140-VK (ATCC Depoεit Deεignation PTA-4097), and (ii) two heavy chainε, each heavy chain compriεing the expresεion product of either a plaεmid deεignated pVgl :HuPRO140 HG2-VH (ATCC Deposit Designation PTA-4098) or a plasmid designated pVgl :HuPR0140 (mut B+D+D-VH (ATCC Deposit Designation PTA- 4099) , or a fragment of such antibody, which binds to CCR5 on the surface of a human cell, under conditions effective to treat said HIV-l-afflicted subject .

23.A method of preventing a subject from contracting an HIV-1 infection which compriseε administering to the εubject an effective HIV-1 infection- preventing doεage amount of an anti-CCR5 antibody compriεing (i) two light chains, each light chain comprising the expression product of a plasmid designated pVK:HuPRO140-VK (ATCC Deposit Designation PTA-4097), and (ii) two heavy chains, each heavy chain comprising the expreεsion product of either a plasmid designated pVgl: HuPRO 140 HG2- VH (ATCC Deposit Designation PTA-4098) or a plasmid deεignated pVgl :HuPRO140 (mut B+D+D-VH (ATCC Depoεit Deεignation PTA-4099) , or a fragment of such antibody, which binds to CCR5 on the εurface of a human cell, under conditionε effective to prevent εaid HIV-1 infection in said εubject .

24. The method of claim 22 or 23, wherein the anti- CCR5 antibody iε adminiεtered to the εubject by a method selected from the group consisting of intravenous, intramuscular and subcutaneous means.

25. The method of claim 22 or 23, wherein the anti- CCR5 antibody iε adminiεtered continuously to said subject .

26. The method of claim 22 or 23 wherein the anti-CCR5 antibody is administered at predetermined periodic intervals to said subject.

27. The method of claim 22 or 23, which further comprises labeling the anti-CCR5 antibody with a detectable marker.

28. The method of claim 27, wherein the detectable marker is a radioactive or a fluorescent marker.

29. The method of claim 22 or 23, wherein the dosage of said anti-CCR5 antibody rangeε from about 0.1 to about 100,000 μg/kg body weight of εaid subject .

30. The method of claim 29, wherein the dosage of said anti-CCR5 antibody doeε not inhibit an endogenous chemokine activity on CCR5 in εaid εubject.

31.An anti-CCR5 antibody conjugate comprising an anti-CCR5 antibody which compriεes (i) two light chains, each light chain compriεing the expression product of a plasmid designated pVK:HuPR0140-VK

(ATCC Depoεit Designation PTA-4097) , and (ii) two heavy chains, each heavy chain comprising the expresεion product of either a plaεmid designated pVgl :HuPR0140 HG2-VH (ATCC Depoεit Designation PTA-4098) or a plasmid designated pVgl : HuPRO140

(mut B+D+D-VH (ATCC Deposit Deεignation PTA- 4099) , or a fragment of such antibody which binds to CCR5 on the surface of a human cell, conjugated to at least one polymer.

32. The anti-CCR5 antibody conjugate of claim 31, wherein the polymer is εelected from the group conεiεting of hydrophilic polyvinyl polymers, polyalkylene ethers, polyoxyalkylenes , polymethacrylateε, carbomers, branched polysaccharideε , unbranched polysaccharides, polymers of sugar alcohols, heparin and heparon.

33. The anti-CCR5 antibody conjugate of claim 32, wherein the polyalkylene ether is polyethylene glycol (PEG) or a derivative thereof.

34. The anti-CCR5 antibody conjugate of claim 33, wherein at least one PEG has an average molecular weight of at least 20 kD.

35. The anti-CCR5 antibody conjugate of claim 31, wherein the apparent size of the conjugate is at least about 500 kD.

36.The anti-CCR5 antibody conjugate of claim 31, wherein the conjugate has at least one of an increase in serum half-life, an increase in mean residence time in the circulation and a decrease in serum clearance rate, compared to a nonconjugated anti-CCR5 antibody or fragment thereof .

37.A method of inhibiting infection of a CCR5+ cell by HIV-l, which method compriseε adminiεtering to a subject at risk of HIV-1 infection the conjugate of claim 31 in an amount and under conditions effective to inhibit infection of CCR5+ cellε of said subject by HIV-1.

38. method of treating an HIV-l infection in a^' subject, which method comprises adminiεtering to an HIV-l-infected subject the conjugate of claim 31 in an amount and under conditions effective to treat the εubject' ε HIV-1 infection.

39. The method of claim 38, wherein the amount of the conjugate is effective in reducing a viral load in the subject.

40. The method of claim 38, wherein the amount of the conjugate is effective in increasing a CD4+ cell count in the subject.

41. The method of claim 38, which further comprises administering to said subject at least one conventional anti-viral agent.

42. The method of claim 37 or 38, wherein the conjugate is administered to the subject by a method selected from the group consiεting of intravenouε, intramuscular and subcutaneous means.

43. The method of claim 37 or 38, wherein the conjugate is administered continuously to said εubject .

44. he method of claim 37 or 38, wherein the conjugate iε administered at predetermined periodic intervals to said subject.

45. The method of claim 37 or 38, which further compriseε labeling the conjugate with a detectable marker .

46. The method of claim 45, wherein the detectable marker iε a radioactive or a fluorescent marker.

47.A transformed host cell comprising at least two vectors, at least one vector comprising a nucleic acid sequence encoding heavy chains of an anti- CCR5 antibody, and at least one vector comprising a nucleic acid sequence encoding light chains of the anti-CCR5 antibody, wherein the anti-CCR5 antibody compriseε two heavy chains having the amino acid sequence set forth in SEQ ID NO: 9, and two light chains having the amino acid sequence εet forth in SEQ ID NO: 6.

48.A transformed host cell comprising at least two vectors, at least one vector comprising a nucleic acid sequence encoding heavy chains of an anti- CCR5 antibody, and at least one vector comprising a nucleic acid sequence encoding light chains of the anti-CCR5 antibody, wherein the anti-CCR5 antibody comprises two heavy chains having the amino acid εequence set forth in SEQ ID NO: 12, and two light chains having the amino acid sequence set forth in SEQ ID NO: 6.

49. The transformed host cell of claim 47 or 48, wherein the cell is a mammalian cell.

50. The transformed host cell of claim 49 wherein the cell is a COS cell, a CHO cell or a myeloma cell.

51. The transformed host cell of claim 47 or 48, wherein the cell secreteε the anti-CCR5 antibody.

52. The transformed host cell of claim 47, wherein the vector encoding heavy chainε iε deεignated pVgl:HuPRO140 HG2-VH (ATCC Deposit Deεignation PTA-4098) .

53. The transformed host cell of claim 48, wherein the vector encoding heavy chainε is designated pVgl:HuPRO140 (mut B+D+D-VH (ATCC Depoεit Deεignation PTA-4099) .

54. The transformed host cell of claim 47 or 48, wherein the vector encoding light chains is designated pVK:HuPRO140-VK (ATCC Deposit Designation PTA-4097) .

55. The transformed host cell of claim 47, wherein the vector encoding heavy chainε is designated pVgl:HuPRO140 HG2-VH (ATCC Deposit Designation PTA- 4098) and the vector encoding light chains iε deεignated pVK:HuPRO140-VK (ATCC Deposit Designation PTA-4097) .

56. The transformed host cell of claim 48, wherein the vector encoding the heavy chains is designated pVgl:HuPRO140 (mut ' B+D+D-VH (ATCC Deposit Deεignation PTA-4099) and the vector encoding light chains iε designated pVK-HuPRO140-VK (ATCC Deposit Designation PTA-4097) .

57. The transformed host cell of claim 47, wherein the nucleic acid sequence encoding heavy chains has the nucleic acid sequence set forth in SEQ. ID NO: 8.

58. The transformed host cell of claim 48, wherein the nucleic acid εequence encoding heavy chainε haε the nucleic acid εequence set forth in SEQ ID

NO: 11.

59. The transformed host cell of claim 47 or 48 wherein the nucleic acid sequence encoding light chainε haε the nucleic acid εequence εet forth in SEQ ID NO: 5.

60. A vector compriεing a nucleic acid sequence encoding a heavy chain of an anti-CCR5 antibody, wherein the heavy chain compriεes the amino acid εequence εet forth in SEQ ID NO: 9.

61. The vector of claim 60, wherein the vector is deεignated pVgl :HuPRO140 HG2-VH (ATCC Deposit Deεignation No. PTA-4098) .

62.A vector compriεing a nucleic acid εequence encoding a heavy chain of an anti-CCR5 antibody, wherein the heavy chain comprises the amino acid sequence set forth in SEQ ID NO: 12.

63. The vector of claim 62, wherein the vector is designated pVgl :HuPRO140 (mut B+D+D-VH (ATCC Deposit Designation No. PTA-4099) .

64.A vector comprising a nucleic acid εequence encoding a light chain of an anti-CCR5 antibody, wherein the light chain compriεeε the amino acid εequence εet forth in SEQ ID NO: 6.

65. The vector of claim 64, wherein the vector iε designated pVK:HuPRO140-VK (ATCC Deposit Deεignation No. PTA-4097) .

66.A process for producing an anti-CCR5 antibody which compriseε culturing a hoεt cell containing therein (i) a plasmid designated pVK:HuPRO140-VK

(ATCC Deposit Deεignation PTA-4097) , and (ii) either a plasmid deεignated pVgl :HuPRO140 HG2-VH

(ATCC Depoεit Deεignation PTA-4098) or a plasmid designated pVgl:PRO140 (mut B+D+D-VH (ATCC Depoεit Deεignation PTA-4099) under conditionε permitting the production of an antibody compriεing two light chains encoded by the plasmid deεignated pVK:HuPRO140 HG2-VH (ATCC Deposit Deεignation PTA-4097) and two heavy chainε encoded either by the plaεmid designated pVgl :HuPRO140 HG2-VH (ATCC Deposit Designation PTA-4098) or by the plaεmid designated pVgl: HuPRO 140 (mut B+D+D- VH (ATCC Deposit Designation PTA-4099) , so as to thereby produce an anti-CCR5 antibody.

67.A process for producing an anti-CCR5 antibody which comprises:

a) transforming a host cell with (i) a plasmid designated pVK:HuPRO140-VK (ATCC Deposit Designation PTA-4097), and (ii) either a plasmid designated pVgl :HuPR0140 HG2-VH (ATCC Deposit Designation PTA-4098) or a plasmid designated pVgl :HuPRO140 (mut B+D+D-VH (ATCC Deposit Designation PTA-4099) ; and b) culturing the transformed host cell under conditions permitting production of an antibody comprising two light chains encoded by the plasmid designated pVK:HuPRO140-VK (ATCC Deposit Designation PTA-4097) and two heavy chainε encoded either by the plaεmid deεignated pVgl :HuPRO140 HG2-VH (ATCC Deposit Deεignation PTA-4098) or by the plasmid deεignated pVgl :HuPRO140 (mut B+D+D-VH (ATCC Depoεit Designation PTA-4099) , so aε to thereby produce an anti-CCR5 antibody.

68. The method of claim 66 or 67, which further compriεes recovering the anti-CCR5 antibody so produced in isolated form.

69. The method of claim 66 or 67, wherein the host cell is a mammalian cell.

70. The method of claim 69, wherein the mammalian host cell is a COS cell, a CHO cell or a myeloma cell.

71. The method of claim 66 or 67, wherein the heavy chainε of the anti-CCR5 antibody are encoded by the plasmid designated pVgl :HuPRO140 HG2-VH (ATCC Deposit Designation PTA-4098) .

72. The method of claim 66 or 67, wherein the heavy chains of the anti-CCR5 antibody are encoded by the plasmid designated pVgl :HuPRO140 (mut B+D+I) (ATCC Deposit Designation PTA-4099) .

73.A kit for use in a process of producing an anti- CCR5 antibody comprising: a) a vector comprising a nucleic acid sequence encoding a light chain of an anti-CCR5 antibody, wherein the light chain comprises the amino acid sequence set forth in SEQ ID NO: 6; and b) a vector comprising a nucleic acid sequence encoding a heavy chain of an anti-CCR5 antibody, wherein the heavy chain comprises the amino acid sequence set forth in SEQ ID NO: 9, or a vector comprising a nucleic acid sequence encoding a heavy chain of an anti-CCR5 antibody, wherein the heavy chain comprises the amino acid sequence set forth in SEQ ID NO: 12.