CD8+-Cell Antiviral Factor Activity Is Not Restricted to Human Immunodeficiency Virus (HIV)-Specific T Cells and Can Block HIV Replication after Initiation of Reverse Transcription

doi:10.1128/JVI.74.10.4456-4464.2000

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Journal of Virology, May 2000, p. 4456-4464, Vol. 74, No. 10
0022-538X/00/$04.00+0
Copyright © 2000, American Society for Microbiology. All rights reserved.

CD8⁺-Cell Antiviral Factor Activity Is Not Restricted to Human Immunodeficiency Virus (HIV)-Specific T Cells and Can Block HIV Replication after Initiation of Reverse Transcription

Sylvie Le Borgne,¹ Michèle Février,¹ Christian Callebaut,¹^, Steven P. Lee,² and Yves Rivière¹^,^*

Département des Rétrovirus, URA CNRS 1930, Institut Pasteur, 75724 Paris Cedex 15, France,¹ and CRC Institute for Cancer Studies, University of Birmingham, Birmingham B15 2TA, United Kingdom²

Received 19 July 1999/Accepted 3 February 2000

	ABSTRACT

Top Abstract Introduction Materials and Methods Results Discussion References

CD8⁺ lymphocytes from human immunodeficiency virus (HIV)-infected patients can suppress in vitro HIV replication in CD4⁺ T cells by a noncytolytic mechanism involving secreted CD8⁺-cell antiviral factor(s) (CAF). Using an HIV Nef-specific cytotoxic-T-lymphocyte(CTL) line and autologous CD4⁺ T cells infected with a nef-deleted HIV-1 virus, we demonstratedthat, after a priming antigenic stimulation, this suppressiondoes not require the presence of the specific antigen during theeffector phase. Furthermore, using an Epstein-Barr virus (EBV)-specificCTL line from an HIV-seronegative donor, we demonstrated thatthe ability to inhibit HIV replication in a noncytolytic manneris not restricted to HIV-specific effector cells; indeed, EBV-specificCTL were as efficient as HIV-specific effectors in suppressingR5 or X4 HIV-1 strain replication in vitro. This HIV-suppressiveactivity mediated by a soluble factor(s) present in the culturesupernatant was detectable for up to 14 days following stimulationof EBV-specific CD8⁺ cells with the cognate epitope peptide. Following acute infectionof CEM cells with an X4 strain of HIV-1, EBV-specific CTL linesupernatant containing HIV-suppressive activity did not blockvirus entry but was shown to interfere with virus replicationafter the first template switching of reverse transcription. Ourresults suggest that the noncytolytic control of HIV replicationby EBV-specific CD8⁺ T lymphocytes corresponded to a CAF-like activity and thus demonstratethat CAF production may not be restricted to CTL induced duringHIV disease. Moreover, CAF acts after reverse transcription atleast for X4 isolate replicationinhibition.

	INTRODUCTION

Top Abstract Introduction Materials and Methods Results Discussion References

Infection with human immunodeficiency virus (HIV) is characterized by an initial acute phase with a high level of plasma viremia.Studies of the immune responses induced in HIV-infected patientssuggest that cytotoxic T lymphocytes (CTL) play an important rolein controlling the virus, since the emergence of antiviral CTLactivity coincides with the clearance of viremia in primary infection(7, 28). Furthermore, a decline in this CTL response coincideswith disease progression in infected individuals (12, 27).Two types of CD8⁺-cell-mediated antiviral functions have been described in HIVinfection: one involves the classical antigen-specific HLA-restrictedcytolysis of infected cells (54), and the other inhibits HIVreplication in the absence of cell killing (33, 55, 59).

This noncytolytic antiviral response was first identified in vitro with lymphocytes from HIV-seropositive patients (57).It is detected by a reduction in HIV p24 production or a decreasein reverse transcriptase (RT) activity in supernatants from coculturesof HIV-infected CD4⁺ cells and activated CD8⁺ T lymphocytes. The effector cells carry the phenotype of activatedCD8⁺ CTL (3, 36, 53), but the antiviral activity does not requireHLA compatibility at the effector phase. This inhibition of HIVreplication is mediated by soluble factor(s) referred to as CD8⁺-cell antiviral factor(s) (CAF) (8, 56); indeed, noncytotoxicHIV-suppressive activity can be mediated by using cell-free supernatantsfrom cultures of activated CD8⁺ T cells (56). However, it has been reported that cell-to-cellcontact (53, 56) and the use of autologous cell cultures (8)can enhance the effect. Furthermore, one CD8⁺ T cell could mediate both CAF secretion and HLA-restricted cytotoxicity,since we have previously demonstrated that a CD8⁺ CTL clone, specific for one HIV-Gag epitope, could also inhibitin vitro HIV replication by soluble-factor secretion (10). HIV-1is not the only virus to be affected by this response since CD8⁺ T cells have also been shown to suppress HIV-2 or simian immunodeficiencyvirus replication; this noncytolytic antiviral activity has alsobeen observed in nonhuman primate species (5, 13, 35, 58).

Recombinant cytokines have been tested independently for their ability to mediate CAF activity, and cytokine-specific monoclonalantibodies have been tested for their ability to block this effect(36, 39) but, to date, the identity of the CAF remains largelyunknown. Recent studies have shown that HIV-suppressive factorsproduced by CD8⁺ T cells include the $beta$ -chemokines macrophage-inflammatory protein-1 $alpha$ (MIP-1 $alpha$ ), MIP-1 $beta$ , and RANTES (14), which block the entry ofR5 HIV strains into CD4⁺ cells by competing for binding to the chemokine receptors CCR5and CCR3 (1, 19, 20). In the same manner, the $alpha$ -chemokinestromal-derivated factor 1 (SDF-1), for which CXCR4 is the receptor,inhibits the entry of T-tropic HIV isolates (44), whereas ithas never been demonstrated to be produced by CD8⁺ lymphocytes (29). Furthermore, the $beta$ -chemokine MDC (45) andinterleukin-16 (IL-16) (2) could be produced by CD8⁺ T cells and suppress HIV replication in vitro. Elsewhere, otherstudies indicate that CAF activity may block viral transcription.Using Jurkat cells transfected with an HIV-1 long-terminal-repeat(LTR)-luciferase construct (38) or an HIV-1 LTR-chloramphenicolacetyltransferase (CAT) construct (17), CD8⁺ T lymphocytes or their supernatants were shown to mediate specificinhibition of the LTR-driven activity, whereas the $beta$ -chemokinescould not suppress HIV RNA transcription (22). Furthermore, $beta$ -chemokines appeared to be distinct from CAF (37).

The CD8⁺ antiviral noncytolytic activity has been evidenced with effector cells from HIV-seropositive patients and seems tocorrelate with the clinical status of infected individuals (4,6, 24, 40). However, the ability of CD8⁺ cells from HIV-seronegative donors to inhibit HIV replicationhas been described but is controversial (26, 32, 49). Elsewhere,viral suppression by CD8⁺ lymphocytes from HIV-infected patients appears to be more efficientthan the inhibition observed by effector cells from healthy donors(33). Thus, it is still unclear whether HIV infection of thehost specifically induces in vivo the immune competence to elicitCAF activity or if infection with other viruses could have thesame result as a consequence of activating CD8⁺ Tcells.

In the present study, we have further analyzed this noncytolytic control of HIV replication using both HIV-specific and Epstein-Barrvirus (EBV)-specific CD8⁺ T-cell lines. Our results indicate that antigen-specific T-cellreceptor (TCR) stimulation is not required at the effector phaseof the control and that noncytolytic inhibition of HIV replicationis not restricted to HIV-specific CD8⁺ T cells. Finally, an EBV-specific CD8⁺ T-cell line could control replication of HIV-1 X4 strain by secretionof soluble factor(s) which interacts with the viral cycle, atleast after the first template switching of reversetranscription.

	MATERIALS AND METHODS

Top Abstract Introduction Materials and Methods Results Discussion References

Cell lines. B-lymphoblastoid cell lines (B-LCL) were established by in vitro transformation of peripheral blood B cells with the standardEBV isolate B95.8 (42). CEM cells (clone 13) were kindly providedby L. Montagnier (Institut Pasteur, Paris, France) (31). Allof these cell lines were grown in RPMI 1640 (Whittaker, Gagny,France) supplemented with 2 mM L-glutamine (Gibco BRL, Cergy-Pontoise,France) and 10% heat-inactivated fetal calf serum (FCS; Dutscher,Strasbourg, France) (RPMI-10% FCS). All incubations and cultureprocedures were performed at 37°C in a water-saturated 5% CO₂atmosphere.

Isolation of CD8⁺ T-cell lines. The P1-HIV CTL line was generated as described previously (21) from an HIV-1-seropositive adult who maintained a CTL responseto the HIV-1 p27^Nef protein during a 6-year study period (48). The HLA typing ofthis patient is A2.01, A11, B27, B51, and C1402. The line wasstimulated every 2 to 3 weeks with irradiated (100 Gy) autologousB-LCL and the cognate epitope peptide HIV-1 Nef19 (representingamino acids 73 to 82 from p27^Nef, QVPLRPMTYK, provided by Neosystem, Strasbourg, France, and obtainedthrough the Agence Nationale de Recherche sur le Sida [ANRS]),which has been confirmed as the optimal specific epitope; freshallogeneic irradiated peripheral blood mononuclear cells (PBMC)were also added as feeders. The P1-HIV line was maintained inRPMI 1640 (Whittaker) supplemented with 2 mM L-glutamine, 1 mMnonessential amino acids, 1 mM sodium pyruvate (Gibco BRL), 5%human AB serum (INTS, Bobigny, France), and 50 IU of recombinanthuman IL-2 (rIL2) (RU49637, a generous gift from D. Lando, Roussel-Uclaf,Romainville, France) per ml (cloningmedium).

The 1.6-EBV CTL line was generated from an HIV-seronegative, EBV-seropositive individual as described previously (25). TheHLA haplotype of this person is A2, A29, B8, B40, and Cw3. Thiscell line was restimulated every 2 to 3 weeks in the presenceof fresh allogeneic irradiated PBMC as feeder cells and 0.5 µgof phytohemagglutinin (PHA-p; Difco, Detroit, Mich.) per ml. Inaddition, irradiated autologous B-LCL cells preincubated with1 µg of a peptide representing amino acids 339 to 347 (FLRGRAYGL;Neosystem) per ml from the EBV nuclear antigen-3 (EBNA-3) proteinof the BL74 EBV strain (9) were added at a stimulator/responderratio of 1/10. This peptide represents the minimal target epitoperecognized by the 1.6-EBV line. The cells were cultured in RPMI1640 supplemented with 3% human AB serum (INTS), 10% FCS (Dutscher),2 mM L-glutamine, 1 mM nonessential amino-acids, 1 mM sodium pyruvate(Gibco BRL), 20 IU of rIL2 (RU 49637) per ml, and 15% T-cell growthfactor (Lymphocult T-LF; Biotest, Buc, France) as a source ofcytokines (cloningmix).

Both cell lines were confirmed to be at least 99% CD3⁺ CD8⁺ by cytofluorometric analysis. The T-cell line V $beta$ repertoire wasanalyzed as described previously (46).

Isolation of CD4⁺ T-cell lines. CD4⁺ T-cell lines were derived from the HIV-infected patient P1, from the EBV-seropositive individual 1.6, and from one additionalHIV-seropositive donor (HLA typing: A2, A30, B44, C2, and C5).PBMC from these donors were depleted of CD8⁺ T cells by using magnetic beads coated with anti-CD8 monoclonalantibodies (Immunotech, Marseille, France) according to the manufacturer'sinstructions and then seeded at 10 or 25 cells/well in a 96-wellplate (Costar) with fresh allogeneic irradiated PBMC and 2 µgof PHA (Difco) per ml. Cells were cultured in cloning medium andrestimulated with allogeneic irradiated PBMC and PHA every 3 weeks.The lines were confirmed by cytofluorometric analysis to be atleast 99% CD3⁺ CD4⁺ CD8. Assays for RT activity (50) in the supernatant of uninfectedactivated CD4⁺ T-cell lines derived from HIV-infected patients were consistentlynegative.

Virus stocks. The HIV-1 LAI strain was used as a lymphotropic (X4) virus; the monotropic (R5) molecular clone HIV-1 YU2b (34) and thenef frameshift mutant YU2b $Delta$ nef (43) were kindly provided byO. Schwartz (Institut Pasteur). The frameshift mutation suppressescompletely the expression of the Nef protein by YU2b $Delta$ nef, as evidencedby immunoblotting (43). For production of virus stocks, PBMCfrom healthy donors were prepared by Ficoll-Paque (Pharmacia,Les Ulis, France) density gradient centrifugation, suspended incloning medium, and stimulated for 3 days with 2 µg of PHA (Difco)per ml. PBMC cultures were then infected with the various isolates,and virus production was monitored by measuring RT activity inthe culture supernatant as described previously (50). The coreceptorusage of these virus stocks was checked on HeLa cells bearinghuman CD4 alone, or human CD4 and human CCR5, as described previously(41).

The dual-tropic (X4R5) 89.6 strain was obtained through the AIDS Research and Reference Reagent Program, Division of AIDS,National Institute of Allergy and Infectious Diseases, NationalInstitutes of Health (NIH); HIV 89.6 was from Ronald Collman (16)and was propagated in CEMx174cells.

The CEM-adapted HIV-1 LAI strain (31) was amplified on CEM clone 13cells.

Recombinant vaccinia viruses (rVV) expressing individual HIV antigens were as described previously (48).

All virus stocks were stored at $-$ 80°C.

Reverse transcription assays. RT activity was measured as described previously (50). Briefly, using a 96 well-plate, we incubated 50 µl of cell-free supernatantat 37°C for 1 h with 10 µl of a mix containing 0.5% of TritonX-100 (Sigma), 50 mM of dithiothreitol (Sigma), and 0.5 M of KCl(Sigma) and 40 µl of a mix containing 1.25 mM EGTA (Sigma) in0.5 M Tris-HCl solution (pH 7.8), 12.5 mM MgCl₂ (Sigma), 0.125mg of Poly-rA-Oligo d/T (Pharmacia-LKB, Saint-Quentin-en-Yvelines,France) per ml, and 3 µCi of [³H]dTTP (ICN, Orsay, France). The reaction was stopped at 4°C with20 µl of a mix containing 120 mM of Na₄P₂O₇ (Merck, Darmstadt,Germany) in 60% trichloroacetic acid (Prolabo, Paris, France)solution. The supernatants were harvested on a DEAE-treated filter(EGG, Evry, France) and counted on a beta counter. RT activitywas expressed as the counts per minute (cpm) per 50 µl ofsupernatant.

Cytotoxicity assays. CTL activity was measured using a conventional 4-h ⁵¹Cr release assay as described previously (48). Briefly, autologous B-LCLwere infected with rVV 16 h before the assay, labeled for 1 hwith 3.7 MBq of Na₂⁵¹CrO₄ (ICN) per 10⁶ cells, washed three times, and then used as target cells. Forpeptide assays, B-LCL were labeled for 1 h with Na₂⁵¹CrO₄ and washed, and then synthetic peptides were added at 1 µg/ml.These targets were then added to the effector cells at variouseffector-to-target ratios. After incubation, supernatants wereremoved and counted on a beta counter. The percentage of specificrelease was calculated as follows: % release = (experimental release $-$ spontaneous release)/(total release $-$ spontaneous release) ×100. Total release was measured by resuspending target cells inlysis buffer (5% Triton X-100-1% sodium dodecyl sulfate). Spontaneousrelease was obtained from targets incubated with medium aloneand was usually less than 15% of the totalrelease.

Direct coculture of CD8⁺ effectors with HIV-infected CD4⁺ T cells. CD4⁺ T-cell lines stimulated for 5 days with PHA were incubated at 2 × 10⁶ cells/ml with 5 × 10⁴ cpm/10⁶ cells of the HIV viral stock and 5 µg of polybrene per ml for2 h at 37°C. An equal volume of fresh medium was then added, andcells were incubated at 37°C overnight. Infected cells were washed,seeded at 10⁵ cells per well in a 48-well plate (Costar), and mixed with variousconcentrations of CD8⁺ T effector cells at CD8⁺/CD4⁺ ratios ranging from 0/1 to 4/1, in a final volume of 1 ml. UninfectedCD4⁺ and CD8⁺ T lymphocytes alone were used as negative controls, and HIV-infectedCD4⁺ T cells alone were used as a positive control. Half of the culturesupernatant was collected from each well two or three times aweek and stored at $-$ 80°C, and cultures were refed with fresh medium.At the end of the coculture, the RT activity in the supernatantwas measured as described previously (50) and was expressedas cpm per 50 µl of supernatant. The percent inhibition of viralreplication was calculated as follows: [1 $-$ (experimental RT/infectedCD4⁺ cells alone RT)] ×100.

Inhibition of HIV replication by CTL supernatants. (i) Generation of inhibitory supernatants from CTL. Supernatants from cultures of the 1.6-EBV line were tested for their inhibitory activity on HIV replication. After TCR stimulationwith the cognate peptide epitope, cells were maintained at 10⁶ cells/ml in a cloning mix. Supernatants were collected 9 (d9),12 (d12), 14 (d14), or 15 (d15) days after stimulation (i.e.,at least 2 days after the cultures were last fed with fresh medium).Supernatants from autologous PHA-stimulated uninfected CD4⁺ T-cell cultures (maintained at 10⁶ cells/ml) were collected 9 days (d9) after the addition of PHA(i.e., 3 days after the cultures were last fed). Cloning mix orcloning medium alone was used as a negative control. The supernatantswere stored at $-$ 20°C. For these experiments, cell lines were stimulatedwith the same batch of irradiated allogeneic PBMC feedercells.

(ii) HIV infection of CEM cells. Pelleted CEM clone 13 cells were incubated at 37°C for 1 h with the CEM-adapted HIV-1 LAI stock (11) at 150 ng of Gag p24per 10⁶ cells (corresponding to 12 × 10⁴ cpm of RT activity). The cells were infected in 1 ml of culturemedium and then washed. Infected cells were then cultured at 10⁵ cells per well in a 48-well plate for 7 days in the presenceof CD8⁺ T-cell supernatant. CEM cells preincubated with HIV but culturedwithout CD8⁺ supernatant were used as a positive control for HIV infection;uninfected CEM cells cultured alone acted as a negative control.Half of each culture supernatant was collected daily and storedat $-$ 80°C, and the cultures were refed. At the end of the assay,the RT activity in the supernatants was measured as describedpreviously (50).

(iii) Assays for inhibition of HIV replication. Target cells (PHA-activated CD4⁺ T lymphocytes or CEM cells) were acutely infected with HIV-1 as described above, in the presenceor absence of CTL supernatants (see Results), and were platedat 10⁵ cells per well (in 1 ml) in a 48-well plate. CTL supernatantswere tested at a dilution of 1/2 and maintained at this concentrationthroughout the course of the assay. Supernatant fluid (0.5 ml)was removed for RT activity testing (50) every day for CEM cellsand twice a week for CD4⁺ lymphocytes and then replaced with fresh medium containing 50%CTL supernatant fluid. Infected T cells alone were used as a positivecontrol for HIV infection. PHA-stimulated CD4⁺ T-cell supernatants or cloning medium alone acted as negativecontrols for CAF activity. The percent inhibition of viral replicationwas calculated as follows: [1 $-$ (experimental RT/infected CD4⁺ cells alone RT)] ×100.

PCR analysis. DNA was extracted from CEM cells 24 h after HIV-1 LAI infection using the QIAamp blood kit (Qiagen, Hilden, Germany) as describedby the manufacturer and then tested for proviral DNA using a PCR-basedassay. PCR was performed with 770 ng of DNA matrix. Amplification(25 cycles) of viral DNA was carried out using primers correspondingto U3+ (5'-CACACAAGGCTACTTCCCTGA-3') and U5 $-$ (5'-GATCTCTAGTTACCAGAGTCAC-3')domains in the HIV-1 LTR to generate a 540-bp fragment as describedpreviously (15). The plasmid pBru2 (47) containing the completegenome of HIV-1 was used to estimate the linearity of the HIVDNA amplification. As a control, part of the $beta$ -globin gene wasamplified independently (30 cycles) using the primer $beta$ -globin+from the region from 1614 to 1633 (exon) (5'-CCTTTGTTCCCTAAGTCCAA-3'),and the primer $beta$ -globin $-$ from the region from 1851 to 1832 (intron)(5'-CCTCACCTTCTTTCATGGAG-3') to generate a 238-bp fragment asdescribed previously (15). PCR products were resolved in 2%agarose gels and quantified using NIH 1.61 software (Wayne Rasband,NIH, Bethesda, Md.).

	RESULTS

Top Abstract Introduction Materials and Methods Results Discussion References

Characterization of the CD8⁺ CTL lines. As tools to study CD8⁺-cell-mediated HIV-suppressive activity, we characterized two CD8⁺ CTL lines: P1-HIV obtained from an HIV-1-infected patient and1.6-EBV isolated from an EBV-seropositive, HIV-1-seronegativeindividual. P1-HIV is an HIV-1 Nef-specific line, which lysedautologous B-LCL infected with rVV encoding the entire Nef protein,and B-LCL coated with peptide Nef19 (amino acids [aa] 73 to 82)from p27^Nef (Fig. 1A). The irrelevant peptide Nef2 (aa 86 to 100 from p27^Nef) did not elicit any cytotoxic response. The Nef-specific CTLresponse was restricted by HLA-A11 (data not shown). Flow cytometricanalysis demonstrated that the P1-HIV line was at least 99% CD3⁺ CD4 CD8⁺ TCR $alpha$ $beta$ ⁺ $gamma$ $delta$ . This line, as demonstrated by using antibodies specific forTCR V $beta$ chains, was composed of 80% V $beta$ 8⁺ cells, while the remaining 20% of cells were not recognized byany of the available antibodies specific for 14 different TCRV $beta$ chains (data not shown). The V $beta$ 8⁺ cell population was clonal, as confirmed in a runoff method (46)(data not shown), and mediated the Nef-specific cytotoxic activity,as demonstrated by depletion experiments (data not shown).

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FIG. 1. Cytotoxic activity of CD8⁺ T-cell lines. CTL assays were conventional 4-h ⁵¹Cr release assays. (A) P1-HIV line was tested against autologous B-LCL alone as a negative control (

), B-LCL previously infected with a rVV expressing the entire nef gene (*), B-LCL preincubated with the specific peptide Nef19 (aa 73 to 82 of p27^Nef;

), or B-LCL preincubated with an irrelevant peptide (Nef2, aa 86 to 100 of p27^Nef, $triangle$ ). (B) 1.6-EBV line was assayed against autologous B-LCL alone as a negative control (

), B-LCL previously incubated with the specific peptide (aa 339 to 347 of EBNA-3 from BL74 virus;

), or B-LCL previously incubated with an irrelevant peptide (HIV 25-5; aa 168 to 184 of HIV p25^Gag; $triangle$ ). Results represent the mean of triplicate cultures and are expressed as the percent specific lysis plus the standard deviation.

The 1.6-EBV line recognized the minimal epitope peptide FLRGRAYGL (aa 339 to 347) from the EBNA-3 protein of the EBV strainBL74 (Fig. 1B). The variant epitope sequence from the EBV strainB95.8 (FLRGRAYGI) was not recognized (9). Thus, the autologousB-LCL was not lysed in this assay, nor was it lysed if it wasprecoated with an irrelevant peptide 25-5 from HIV-1 p25^Gag (aa 168 to 184) (Fig. 1B). This CTL response was restricted byHLA-B8 (51). By flow cytometric analysis the 1.6-EBV line wasfound to be at least 98% CD3⁺ CD8⁺ CD16 CD38⁺ HLA-DR⁺. Using a runoff method (46), we observed that the CTL linewas composed of two clones, one expressing V $beta$ 6B and one expressingV $beta$ 3 (data notshown).

The P1-HIV line is a potent inhibitor of HIV-1 replication even in the absence of the cognate epitope. We investigated the HIV-suppressive capacity of the P1-HIV line on autologous acutely infected CD4⁺ T cells. The CD4⁺ lymphocytes were infected with the R5 HIV-1 YU2b isolate andcocultured with the P1-HIV line at multiple CD8⁺/CD4⁺ ratios. Even at a ratio of 1/1, the P1-HIV line could completelysuppress viral replication in target cells (Fig. 2A). In thisexperiment it is likely that the Nef-specific P1-HIV line wasat least partly inhibiting virus replication through the classicalHLA-restricted antigen-specific cytolytic mechanism. In orderto assess HIV inhibition capacity of the line in the absence ofthis cytotoxicity, the P1-HIV line was cocultured with the sameautologous CD4⁺ cell line infected with a mutant YU2b virus deleted for the nefgene (YU2b $Delta$ nef). These targets could not express the cognate epitopeNef aa 73 to 82 on their surface since Nef expression is completelysuppressed in the molecular clone YU2b $Delta$ nef (43). In this cocultureexperiment, replication of YU2b $Delta$ nef was inhibited by 80% at aCD8⁺/CD4⁺ ratio of 1/1. Since the only HIV-specific cytotoxic activitymediated by P1-HIV was directed against Nef, this suggests thatthis HIV suppression was induced by a noncytotoxic activity. Theviral replication inhibition was not due to the elimination ofinfected cells because CD4⁺ cells were present in the coculture with the CD8⁺ T cells at the peak of HIV replication, as confirmed by flowcytometry analysis (data not shown). In the absence of cytotoxicactivity, this suppressive effect was less efficient than withthe wild-type virus but acted in a dose-dependent manner (Fig.2B). This anti-HIV response seemed to be inherent to the cellline since it was efficient even without TCR recognition of thespecific HLA-peptide complex during the effector phase. Thus,P1-HIV line was able to control HIV replication in autologousCD4⁺ lymphocytes by a mechanism distinct to cytotoxicity. This antiviralactivity dependent on the initial CD8⁺/CD4⁺ ratio could correspond to CAF activity as described initially(33). We next investigated the possibility that a non-HIV-specificCTL line could express the same anti-HIV activity.

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FIG. 2. P1-HIV line suppression of viral replication in autologous CD4⁺ T cells. (A) CD4⁺ T lymphocytes were acutely infected with the HIV-1 R5 strain YU2b. (B) CD4⁺ T cells were infected with the nef frameshift mutant YU2b $Delta$ nef. Infected cells were either cultured alone (

) or cocultured with antigen-stimulated P1-HIV line at CD8⁺/CD4⁺ ratios of 4/1 ( $black-lozenge$ ) or 1/1 ( $open circle$ ). Results are expressed as the RT activity (cpm)/50 µl of culture supernatant.

The 1.6-EBV line inhibited HIV replication as efficiently as the P1-HIV line. We cocultivated the CD8⁺ 1.6-EBV line with autologous CD4⁺ T lymphocytes acutely infected with HIV-1 YU2b at various CD8⁺/CD4⁺ ratios. At the peak of viral replication, the 1.6-EBV line couldinhibit at least 98% of HIV replication even at the lowest effectorcell concentration (Fig. 3A). In YU2b-infected allogeneic CD4⁺ lymphocytes, the 1.6-EBV line suppressed viral replication byat least 93% (Fig. 3B). Thus, although the 1.6-EBV line is notcapable of mediating HIV-specific cytotoxicity, it controlledHIV replication in vitro as efficiently as the P1-HIV line bya noncytotoxic mechanism. The ability of the 1.6-EBV line to suppressHIV replication in allogeneic CD4⁺ cells, as well as in autologous target cells, suggested thatthis effect was neither HLA class I nor class II restricted. Inboth cases, the presence of CD4⁺ T cells at the end of cocultures with CD8⁺ T lymphocytes was confirmed by flow cytometry analysis (datanot shown). When cocultivated with allogeneic CD4⁺ lymphocytes infected with the X4 strain HIV-1 LAI, the 1.6-EBVline suppressed virus replication by 85% (Fig. 3C). Although thislevel of suppression was slightly lower than that seen with theR5 HIV-1 YU2b virus isolate, this difference was not consideredsignificant. Therefore, the EBV-specific CTL line could suppressin a non-HLA-restricted manner replication of R5 and X4 HIV strainsin acutely infected CD4⁺ lymphocytes. The ability to control HIV replication in vitrodid not depend on recognition of HIV specificity.

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FIG. 3. 1.6-EBV line control of HIV-1 replication in autologous or heterologous CD4⁺ lymphocytes. Autologous CD4⁺ T cells were infected with the molecular clone YU2b (A); heterologous CD4⁺ T lymphocytes were infected with YU2b (B) or LAI virus (C). Infected cells were cultured alone (

) or with antigen-stimulated 1.6-EBV line at CD8⁺/CD4⁺ ratios of 0.5/1 ( $open circle$ ) or 1.5/1 ( $black-lozenge$ ) (A and B) or 0.5/1 ( $open circle$ ) and 1/1 ( $black-lozenge$ ) (C). Results are expressed as the RT activity (cpm)/50 µl of culture supernatant. The results shown are from a representative experiment.

Inhibition of HIV replication by the 1.6-EBV line is mediated by a soluble factor(s). We next investigated the nature of the noncytotoxic anti-HIV suppressive activity of the anti-EBV CTL line. The 1.6-EBV linewas stimulated with the cognate epitope peptide, and culture supernatantswere collected at various time points. Autologous CD4⁺ lymphocytes were infected with three different HIV-1 strainsovernight, washed, and then cultured in medium containing 50%cell-free supernatant from the 1.6-EBV line. The percent inhibitionof RT activity was calculated at the peak of viral replicationin each culture. Figure 4A shows that a supernatant taken 9 daysafter specific stimulation of the 1.6-EBV line completely suppressedreplication of the R5 strain HIV-1 YU2b (98% inhibition of RTactivity) and the X4R5 virus 89.6 (97% inhibition) and almostcompletely controlled replication of the X4 HIV-1 LAI isolate(85% inhibition) in autologous CD4⁺ T cells. Supernatants taken 12 and 14 days after specific stimulationhad little effect on HIV-1 YU2b and 89.6 (<30% inhibition) butwere still capable of inhibiting HIV-1 LAI replication (93 and82% inhibition, respectively) (Fig. 4A). These results indicatethat the efficiency of this HIV-suppressive activity dependedupon the virus isolate and may be related to viral tropism, butthese findings need to be confirmed with primary isolates. Chemokinesproduced by CD8⁺ T cells have been demonstrated to inhibit HIV replication. Byenzyme-linked immunosorbent assay (ELISA) a significant levelof $beta$ -chemokines in HIV-suppressive supernatants was detected (Fig.4A). The lower $beta$ -chemokine titers in d12 and d14 supernatantscould explain their reduced efficiency to control YU2b and 89.6replication. But these factors could account in part only forthe antiviral effect on R5 (YU2b) and X4R5 (89.6) isolates (22,37). No SDF-1 mRNA was detected by RT-PCR in the activated 1.6-EBVline (data not shown). Ruling out a possible role of this $alpha$ -chemokinein the inhibition of X4 strain replication, we conclude that 1.6-EBVline could control HIV replication in vitro by secretion of solublemediators. $beta$ -chemokines could participate in this activity forR5 or X4R5 virus, but other unidentified factors need to be implicatedin the X4 strain suppression. The noncytolytic control of HIV-1LAI replication by 1.6-EBV cells or supernatants appeared to befunctionally similar to CAF activity.

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FIG. 4. Effect of 1.6-EBV line supernatants on HIV-1 replication in CD4⁺ T cells. (A) Autologous CD4⁺ T lymphocytes were infected with HIV-1 strains YU2b, LAI, or 89.6 and were cultured with or without antigen-stimulated 1.6-EBV line supernatant collected at days 9 (d9,

), 12 (d12,

), and 14 (d14,

) after specific activation. ELISA titers of $beta$ -chemokines in 1.6-EBV line supernatants were evaluated according to the manufacturer's instructions (R&D). (B) The CEM cell line was infected with HIV-1 LAI CEM-adapted strain, cultivated with or without antigen-stimulated 1.6-EBV line supernatants collected at days 9 (d9,

), 12 (d12,

), and 15 (d15,

) after specific activation. The final concentration of supernatants was 1/2 in both experiments. The peaks of RT activity in cultures of PHA-stimulated CD4⁺ lymphocytes alone (A) were 26,100 cpm/50 µl for YU2b-infected targets, 33,000 cpm/50 µl for LAI-infected lymphocytes, and 76,200 cpm/50 µl for 89.6-infected CD4⁺ T cells; in infected CEM cells alone (B) the peak RT activity was 17,100 cpm/50 µl. The amount of antiviral activity exhibited (percent inhibition of HIV replication) was calculated by comparing the RT activity levels with those in infected CD4⁺ cultures alone.

Inhibition of HIV replication by the 1.6-EBV line occurs after viral reverse transcription. To further characterize the mechanism of HIV-suppressive activity mediated by the 1.6-EBV line, CEM cells were infected withan HIV-1 LAI CEM-adapted strain as a model system. This experimentalmodel allows the generation of a synchronous infection in CEMcells, i.e., all cells were infected by the input virus, and at2 to 3 days postinfection more than 90% of the cells producedHIV proteins (31). In addition, the inhibition of T-tropic virusinfection does not depend upon antiviral effects of $beta$ -chemokines.The infected CEM cells were grown for 1 week in medium containing50% supernatant from the antigen-stimulated 1.6-EBV line and wereassessed for viral replication by measuring the RT activity inthe culture medium (Fig. 4B). Supernatant collected from 1.6-EBVline 9 days after antigenic stimulation (d9) suppressed HIV-1LAI replication by 71%, but supernatants harvested at later timepoints (d12 and d15) were only very weakly effective (Fig. 4B).Since these supernatants were derived from the same culture of1.6-EBV line as those used in the previous experiment (Fig. 4A),these results indicated that 1.6-EBV line inhibition of HIV-1LAI replication was less efficient in CEM cells than in PHA-stimulatedCD4⁺ lymphocytes (Fig. 4A). It could be due to the faster viral replicationin infected CEM cells or to the nature of the target cells. SinceCEM cells divide and grow more quickly than PHA-stimulated lymphocytes,the suppressive activity could interfere differently with HIVreplication in these two celltypes.

To determine which stage in the HIV life cycle is sensitive to anti-HIV activity, supernatant from antigen-stimulated 1.6-EBVline was added at different times during the culture of acutelyinfected CEM cells. Following HIV infection and washing of CEMcells, addition of T-cell supernatants resulted in 67% inhibitionof virus replication (Table 1) compared to virus-infected CEMcells cultured without supernatant. This level of suppressioncompared favorably with that observed in the previous experiment(Fig. 4B). However, if supernatant was added only during the virus-to-cellcontact period and was then completely removed, there was no inhibitionof virus replication, suggesting that anti-HIV factors in thesupernatant had little or no effect on virus entry. Furthermore,if the T-cell supernatant was not subsequently removed, HIV replicationwas inhibited to the same extent regardless of whether T-cellsupernatant was added before or after virus infection of CEM cells(Table 1). In this model of synchronous infection of CEM cellszidovudine (AZT) had, on the one hand, no effect on HIV replicationwhen added more than 24 h after infection. AZT inhibits specificallyviral reverse transcription (31): 24 h after synchronous infectionall of the viral genomes had been reverse transcribed. On theother hand, supernatant from the antigen-stimulated 1.6-EBV linewas still able to suppress viral replication in CEM cells evenwhen added 2 days after infection (data not shown). These observationssuggested that the inhibition of viral replication observed withsoluble factors produced by the 1.6-EBV CTL line was not due toa decrease in viral entry but rather acted after HIV reverse transcription.

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TABLE 1. Inhibition of viral replication of HIV-1 LAI strain in CEM cells by a TCR-stimulated 1.6-EBV line supernatant added during or after cell-to-virus contact^a

To confirm these conclusions, CEM cells were infected with HIV-1 LAI and grown in the presence of culture supernatant taken9 days after antigenic stimulation of the 1.6-EBV line. After24 h DNA was extracted from the infected cells and full-lengthHIV-1 LTR was detected by PCR. Since the PCR was performed usingprimers located in the U3 and the U5 regions of the HIV LTR, itonly allowed detection of newly reverse transcribed viral DNAobtained after the first template switching (52). As shown inFig. 5, the 1.6-EBV line supernatant had no effect in this system(lane 10) compared with HIV-1 LAI-infected CEM cells culturedin medium alone (lane 7) or in medium supplemented with supernatantfrom a PHA-activated CD4⁺ T-lymphocyte culture (lane 9). In contrast, AZT treatment ofCEM cells before and during virus infection greatly reduced theamount of newly reverse-transcribed viral DNA that could be detected(lane 8). In this experiment, the infected CEM cells were alsomonitored 4 days after infection (which corresponded to the peakof HIV replication) for RT activity. As shown in Fig. 5, althoughsupernatant from the 1.6-EBV line did not reduce the level ofnewly reverse-transcribed viral DNA detected by PCR, it did inhibitRT activity by 60% (lane 10) when compared to CEM cells infectedwith virus in the presence of control culture medium (lane 7)or in the presence of a nonsuppressive PHA-activated CD4⁺ T-lymphocyte culture supernatant (lane 9). AZT treatment of CEMcells during virus infection almost completely blocked RT activity(lane 8). Altogether, these data suggest that noncytolytic suppressionof HIV-1 LAI replication in CEM cells by the 1.6-EBV line didnot act at the level of virus entry, but rather occurred followingthe first template switching of viral reverse transcription.

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FIG. 5. Estimation of HIV proviral DNA in CEM cells infected with the HIV-1 LAI CEM-adapted virus. At 24 h after infection, DNA was extracted from uninfected CEM (lane 6), infected CEM alone (lane 7), infected CEM cultivated with 5 µM AZT (lane 8), with supernatant from a 9-day-old culture of PHA-activated CD4⁺ cells from the EBV-positive donor (lane 9), with supernatant from a 9-day-old culture of antigen-stimulated 1.6-EBV line (lane 10), and with 1.6-EBV line cloning mix (lane 11). The quality of DNA extracts was monitored with a $beta$ -globin-specific PCR. A fourfold range of dilutions of the pBru2 plasmid, encoding the full-length HIV-1 Bru genome, from 1 × 10⁵ to 6.4 × 10⁶ copies per sample (lanes 2 to 5) was used as a calibration curve. Lane 1 corresponds to the negative control containing no DNA. The products obtained after the first template switching of the reverse transcription were amplified by a PCR-specific for the complete HIV-1 LTR. PCR products were quantified by using NIH 1.61 software, and their intensities were expressed as arbitrary units (A.U.) on a histogram. For CEM cells (lanes 6 to 11), the RT activity in supernatant fluids was expressed as the cpm/50 µl at the peak of viral replication (day 4, ---*---).

	DISCUSSION

Top Abstract Introduction Materials and Methods Results Discussion References

In the present study, we have analyzed the potent antiviral effects of two virus-specific CTL lines on HIV replication. Wehave shown that both a CD8⁺ cytotoxic cell line specific for HIV-1 Nef and an EBV-specificCTL line could suppress in vitro HIV-1 replication by a noncytolyticmechanism in acutely infected CD4⁺ cells. We focused the study on the anti-HIV noncytotoxic activityof the EBV-specific CTL line and demonstrated that this activitywas mediated by soluble factor(s). Using synchronous infectionof CEM cells we demonstrated that this inhibition acted afterviral reverse transcription regarding X4 strain replication. Allof the characteristics of this HIV replication control by the1.6-EBV line are in agreement with the functional definition ofCAF activity described previously (33). Therefore, we concludethat CAF-like activity is not restricted to HIV-specific CD8⁺ Tcells.

The HIV-1 Nef-specific CTL line, P1-HIV, exerted in vitro a potent antiviral effect on HIV replication in autologous CD4⁺ T cells infected with the R5 strain YU2b (Fig. 2A), in part dueto major histocompatibility complex (MHC) class I-restricted cytolysisof infected cells. However, P1-HIV could mediate also a noncytolyticHIV-1 suppression, as demonstrated by using the same autologousCD4⁺ cell line infected with the R5 strain YU2b $Delta$ nef (Fig. 2B) devoidof the nef gene (43). Compared to wild-type virus inhibition,the control of deleted virus replication was less effective inthe absence of conventional cytotoxicity. This system allows usto dissociate HIV-specific cytotoxicity from noncytolytic HIVsuppression. Yang et al. (60) attempted to estimate the relativeimportance of CAF activity in the global HIV suppression by usingHLA-mismatched target cells. CAF activity was shown to be lessefficient in an HLA-mismatched setting (8), and therefore thisapproach may underestimate the importance of CAF-mediated control.In our study, we have been able to assess the relative contributionof both anti-HIV cytotoxic and noncytolytic mechanisms withinan HLA-matched system using the same target CD4⁺population.

Surprisingly, we observed that the 1.6-EBV CTL line, obtained from an HIV-seronegative individual and specific for EBV, couldalso suppress in vitro replication of both R5 and X4 HIV-1 isolatesin acutely infected CD4⁺ T cells. This CD8⁺ T-cell line controlled R5 virus replication as efficiently asthe HIV-1-specific CTL line P1-HIV (Fig. 2 and 3). This anti-HIVfunction is distinct from cytolysis of infected cells given thatthe conventional cytotoxic activity expressed by the 1.6-EBV lineis specific for a defined epitope of EBV and that this HIV inhibitionappeared to be not restricted by MHC class I (Fig. 3). Since thisHIV-suppressive effect could be mimicked using cell-free supernatants,it could be considered as a CAF-like activity at a functionallevel. Altogether, we conclude that CAF production is not restrictedto HIV-specific CD8⁺ effector cells. Further studies of additional CTL lines withother recognition specificities, however, are required to extendthisobservation.

Our data provide an example of HIV suppression by CD8⁺ lymphocytes from an uninfected individual, devoid of HIV specificity.Previous attempts to identify CAF activity in HIV-seronegativedonors have yielded conflicting results (26, 32, 49). Accordingto these observations the proportion of HIV-suppressive CD8⁺ clones in an HIV-seronegative donor may be relatively low. Inour experimental model, 5 of 6 CD8⁺ PHA-stimulated lines from two HIV-seronegative individuals werenot able to inhibit HIV (YU2b and LAI) replication in vitro, whereas5 of 13 CD8⁺ PHA-stimulated lines from one HIV-1 infected patient could controlHIV (YU2b and LAI) replication (data not shown). Furthermore,the HIV-suppressive activity of CD8⁺ T cells needed to be primed by cellular activation, althoughthe presence of the cognate epitope was not required during theeffector phase of the inhibition. Indeed, in HIV-infected patientsthe anti-HIV activity was associated with an increase in activatedCD8⁺ T cells (23, 30). Furthermore the efficiency of CAF activityincreased following strong stimulation of the effector CD8⁺ cells (with CD28) (3), and cells mediating this activity presentedan activated cell phenotype (36). Since an EBV-specific CTLline could control HIV replication, the immune ability to produceCAF activity is not exclusively induced by HIV infection. We proposethat CAF secretion is a consequence of an activation state ofthe immune system and of the CD8⁺ effector cells in particular that is induced by the HIV infectionbut which could eventually occur during other types of activationof the immunesystem.

The $beta$ -chemokines RANTES, MIP-1 $alpha$ , and MIP-1 $beta$ have been shown to inhibit R5 isolate infection by blocking virus entry (1,19). The two factors MDC (45) and IL-16 (2) have also beendemonstrated to suppress HIV replication. By ELISA we detectedsignificant amounts of $beta$ -chemokines in HIV-suppressive supernatantswhich could account in part for the control of R5 and X4R5 virusreplication by the 1.6-EBV line (Fig. 4A) (37). However, tocharacterize the mechanism of CAF-like activity mediated by thiscell line, we studied the synchronous infection of CEM cells withthe X4 strain HIV-1 LAI. In this experimental model, no knownchemokines produced by CD8⁺ T cells could be implicated in potent control of viral replication.Supernatants from the 1.6-EBV line were then demonstrated notto affect viral entry on CEM cells (Table 1). Furthermore, weobserved that the number of LTR copies detected in infected CEMcells was not affected by the presence of fluids containing CAF-likeactivity (Fig. 5). Thus, this CAF-like activity may not interferewith HIV replication until the first template switching of reversetranscription. These results are in agreement with previous studiesdemonstrating that CAF mediates specific inhibition of LTR-drivenactivity (17, 38). Copeland et al. also showed that this inhibitionmay be mediated via the NF- $kappa$ B or the NFAT-1 element (18). Therefore,our data combined with these previous observations indicate thatCAF is active at a post-reverse transcriptional level, and especiallyat the transcriptionlevel.

In summary, we have demonstrated that an EBV-specific CTL clone could express a CAF-like activity. In the case of X4 strains,this HIV suppression is distinct from a blocking on viral entryand acts after the first template switching of the reverse transcription.Thus, CAF-mediated inhibition of HIV replication is not restrictedto HIV-specific CD8⁺ cells. In HIV disease, production of antiviral soluble factorsby CD8⁺ T cells could be of importance in the in vivo control of virallatency. Our data imply that CD8⁺ T lymphocytes, regardless of their recognition specificity, maycontribute to this effect by an in vivo bystander CAF secretionafter TCRstimulation.

	ACKNOWLEDGMENTS

We thank Mandaleshwar K. Singh for critical review of the manuscript and Geneviève Janvier for excellent technical assistance.We also thank Alan B. Rickinson for his interest in thiswork.

This work was supported by grants from the Agence Nationale de Recherche sur le SIDA, the Pediatric AIDS Foundation, and theInstitut Pasteur. Sylvie Le Borgne is a fellow of the "FondationRoux." Yves Rivière is an Elisabeth Glaserscientist.

	FOOTNOTES

^* Corresponding author. Mailing address: Laboratoire d'Immunopathologie Virale, URA CNRS 1930, Département des Rétrovirus,Institut Pasteur, 28, rue du Docteur Roux, 75724 Paris Cedex 15,France. Phone: 33-1-45-68-87-78. Fax: 33-1-40-61-32-98. E-mail:riviere{at}pasteur.fr.

Present address: Gladstone Institute of Virology and Immunology, University of California at San Francisco, San Francisco,CA 94141-9100.

REFERENCES

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
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53. Tsubota, H., C. I. Lord, D. I. Watkins, C. Morimoto, and N. L. Letvin. 1989. A cytotoxic T lymphocyte inhibits acquired immunodeficiency syndrome virus replication in peripheral blood lymphocytes. J. Exp. Med. 169:1421-1434[Abstract/Free Full Text].

54. Walker, B. D., and F. Plata. 1990. Cytotoxic T lymphocytes against HIV. AIDS 4:177-184[Medline].

55. Walker, C. M., A. L. Erickson, F. C. Hsueh, and J. A. Levy. 1991. Inhibition of human immunodeficiency virus replication in acutely infected CD4⁺ cells by CD8⁺ cells involves a noncytotoxic mechanism. J. Virol. 65:5921-5927[Abstract/Free Full Text].

56. Walker, C. M., and J. A. Levy. 1989. A diffusible lymphokine produced by CD8⁺ T lymphocytes suppresses HIV replication. Immunology 66:628-630[Medline].

57. Walker, C. M., D. J. Moody, D. P. Stites, and J. A. Levy. 1986. CD8⁺ lymphocytes can control HIV infection in vitro by suppressing virus replication. Science 234:1563-1566[Abstract/Free Full Text].

58. Walker, C. M., G. A. Thomson-Honnebier, F. C. Hsueh, A. L. Erickson, L. Z. Pan, and J. A. Levy. 1991. CD8⁺ T cells from HIV-1-infected individuals inhibit acute infection by human and primate immunodeficiency viruses. Cell. Immunol. 137:420-428[CrossRef][Medline].

59. Wiviott, L. D., C. M. Walker, and J. A. Levy. 1990. CD8⁺ lymphocytes suppress HIV production by autologous CD4⁺ cells without eliminating the infected cells from culture. Cell. Immunol. 128:628-634[CrossRef][Medline].

60. Yang, O. O., S. A. Kalams, M. Rosenzweig, A. Trocha, N. Jones, M. Koziel, B. D. Walker, and R. P. Johnson. 1996. Efficient lysis of human immunodeficiency virus type 1-infected cells by cytotoxic T lymphocytes. J. Virol. 70:5799-5806[Abstract].

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54.	Walker, B. D., and F. Plata. 1990. Cytotoxic T lymphocytes against HIV. AIDS 4:177-184[Medline].
55.	Walker, C. M., A. L. Erickson, F. C. Hsueh, and J. A. Levy. 1991. Inhibition of human immunodeficiency virus replication in acutely infected CD4⁺ cells by CD8⁺ cells involves a noncytotoxic mechanism. J. Virol. 65:5921-5927[Abstract/Free Full Text].
56.	Walker, C. M., and J. A. Levy. 1989. A diffusible lymphokine produced by CD8⁺ T lymphocytes suppresses HIV replication. Immunology 66:628-630[Medline].
57.	Walker, C. M., D. J. Moody, D. P. Stites, and J. A. Levy. 1986. CD8⁺ lymphocytes can control HIV infection in vitro by suppressing virus replication. Science 234:1563-1566[Abstract/Free Full Text].
58.	Walker, C. M., G. A. Thomson-Honnebier, F. C. Hsueh, A. L. Erickson, L. Z. Pan, and J. A. Levy. 1991. CD8⁺ T cells from HIV-1-infected individuals inhibit acute infection by human and primate immunodeficiency viruses. Cell. Immunol. 137:420-428[CrossRef][Medline].
59.	Wiviott, L. D., C. M. Walker, and J. A. Levy. 1990. CD8⁺ lymphocytes suppress HIV production by autologous CD4⁺ cells without eliminating the infected cells from culture. Cell. Immunol. 128:628-634[CrossRef][Medline].
60.	Yang, O. O., S. A. Kalams, M. Rosenzweig, A. Trocha, N. Jones, M. Koziel, B. D. Walker, and R. P. Johnson. 1996. Efficient lysis of human immunodeficiency virus type 1-infected cells by cytotoxic T lymphocytes. J. Virol. 70:5799-5806[Abstract].