TNF-related apoptosis-inducing ligand (TRAIL) in HIV-1-infected patients and its in vitro production by antigen-presenting cells

doi:10.1182/blood-2004-08-3058

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Blood, 15 March 2005, Vol. 105, No. 6, pp. 2458-2464.
Prepublished online as a Blood First Edition Paper on December 7, 2004; DOI 10.1182/blood-2004-08-3058.

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IMMUNOBIOLOGY
TNF-related apoptosis-inducing ligand (TRAIL) in HIV-1–infected patients and its in vitro production by antigen-presenting cells
Jean-Philippe Herbeuval, Adriano Boasso, Jean-Charles Grivel, Andrew W. Hardy, Stephanie A. Anderson, Matthew J. Dolan, Claire Chougnet, Jeffrey D. Lifson, and Gene M. Shearer
From the Experimental Immunology Branch, National Cancer Institute (NCI), National Institutes of Health (NIH), Bethesda, MD; Laboratory of Cellular and Molecular Biophysics, National Institute of Child Health and Human Development (NICHD), NIH, Bethesda, MD; Henry M. Jackson Foundation and Infectious Diseases Service, Wilford Hall Medical Center, Lackland Air Force Base, TX; Division of Molecular Immunology, Children's Hospital Research Foundation, Cincinnati, OH; and AIDS Vaccine Program, Science Applications International Corporation (SAIC) Frederick, NCI-Frederick, MD.

   Abstract

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Abstract
Introduction
Patients, materials, and methods
Results
Discussion
References

There is now considerable in vitro evidence that tumor necrosisfactor (TNF)–related apoptosis-inducing ligand (TRAIL)is involved in HIV-1 pathogenesis by inducing CD4⁺ T-cell deathcharacteristic of AIDS. Therefore, we have tested levels ofTRAIL in plasma samples from 107 HIV-1–infected and 53uninfected controls as well as in longitudinal plasma samplesfrom patients who started antiret-roviral therapy (ART). TRAILwas elevated in plasma of HIV-1–infected patients comparedwith uninfected individuals, and patients receiving ART showeddecreased plasma TRAIL levels that correlated with reductionin viral load. In vitro exposure to infectious and noninfectiousHIV-1 induced TRAIL in monocytes and marginally in dendriticcells (DCs) but not in macrophages or T cells. Interestingly,the HIV-1 entry inhibitor, soluble CD4, blocked HIV-1–inducedproduction of TRAIL. Furthermore, production and gene expressionof TRAIL by monocytes were regulated by type I interferon viasignal transducer and activator of transcription-1 (STAT1)/STAT2signaling molecule. Ex vivo HIV-1 infection of human tonsillymphoid tissue also resulted in increased TRAIL production.We demonstrate here that plasma TRAIL is elevated in HIV-1–infectedpatients and is decreased by ART therapy. The high productionof TRAIL by antigen-presenting cells may contribute to the deathof CD4⁺ T cells during progression to AIDS.

   Introduction

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Abstract
Introduction
Patients, materials, and methods
Results
Discussion
References

The depletion of CD4⁺ T cells that results from HIV-1 infectionremains unsolved despite more than 20 years of investigationof AIDS pathogenesis. The direct cytopathic effect resultingfrom HIV-1 infection has been considered to be responsible forCD4⁺ T-cell depletion.¹ However, the low percentage of CD4⁺T cells that are HIV-1 infected prior to and during the earlydecrease in CD4⁺ T-cell numbers cannot account for the severeloss of this cell population.^2,3 This observation led to thesuggestion of infection-induced indirect mechanisms that destroyuninfected T cells by apoptosis, such as activation-inducedcell death.⁴
Tumor necrosis factor (TNF)–related apoptosis-inducingligand (TRAIL), a member of the TNF superfamily,⁵ may be involvedin CD4⁺ T-cell depletion during progression to AIDS.^6,7 TRAILinduced selective apoptosis of uninfected CD4⁺ T cells in ahuman peripheral blood lymphocyte–transplanted nonobesediabetic severe combined immunodeficient (hu-PBL-NOD-SCID) mousemodel,⁸ and TRAIL produced by monocytes exposed to the HIV-1Tat protein killed uninfected CD4⁺ T cells.⁹ Moreover, solubleTRAIL was found in HIV-1–infected patients^10,11 and maybe responsible for the death of neurons in AIDS patients leadingto dementia.¹² TRAIL induces apoptosis in human tumor cell lines¹³and in infected cells¹⁴ but not in normal cells.¹⁵ The 2 biologicallyactive forms of TRAIL, membrane-bound TRAIL (mTRAIL) and solubleTRAIL (sTRAIL), are regulated by type I interferon (interferon-alphaand -beta [IFN- ${alpha}$ and IFN- ${beta}$ ]).^16-18 TRAIL is secreted by leukocytes,including T lymphocytes,¹⁹ natural killer cells,²⁰ dendriticcells,^21,22 and monocytes and macrophages.²³ The lack of involvementof Fas-FasL in HIV-1–induced CD4⁺ T-cell direct killing²⁴implies that other death molecules are involved. Indeed, a recentreport indicates that noninfectious HIV-1 induced T-cell deaththat is not mediated by Fas-FasL and suggested a potential roleof TRAIL.²⁵ However, the role of TRAIL in CD4⁺ T-cell depletionin vivo during progression to AIDS remains to be established.Several reports have shown that macrophages and activated monocytescan play a role in CD4⁺ T-cell depletion that may be due toTRAIL-mediated death.^26-28 HIV-1 infection activates circulatingmonocytes by inducing IFN- ${alpha}$ ²⁹ and secretion of apoptotic cytokinessuch as tumor necrosis factor alpha (TNF- ${alpha}$ ), CD30 ligand (CD30L),and FasL.³⁰ Furthermore, antigen-presenting cells such as monocytesand dendritic cells have been implicated in AIDS pathogenesis,^4,28and macrophages found in brain tissue of AIDS patients wererecently shown to express TRAIL.³¹
Two studies reported sTRAIL in the serum of HIV-1–infectedpatients.^10,11 However, the TRAIL-producing cells were not identified,and no mechanism of TRAIL activation or association with HIV-1disease was provided. Therefore, we compared levels of plasmasTRAIL from HIV-1–infected patients with those of uninfectedcontrol donors and tested whether sTRAIL levels in AIDS patientswere associated with viral load. We recently found that exposureof peripheral blood T cells from HIV-1–uninfected donorsto infectious HIV-1 or to HIV-1 that had been rendered noninfectiousby chemical treatment (aldrithiol-2) (AT-2 HIV-1 particles)resulted in the expression of membrane TRAIL on CD4⁺ but notCD8⁺ T cells (J.P.H. et al, manuscript in preparation). Therefore,we also investigated whether mTRAIL and/or sTRAIL would be producedby monocytes, macrophages, and/or dendritic cells from HIV-1–infectedand uninfected blood donors upon exposure to AT-2 HIV-1 as wellas to infectious HIV-1. We used both HIV-1_MN (CXCR4-tropic)and HIV-1_Ada (CCR5-tropic) to determine if TRAIL productionwas HIV-1 coreceptor dependent. Because type I interferons (IFN- ${alpha}$ and IFN- ${beta}$ ) are required for TRAIL expression and production,we also tested (1) whether inhibition of this pathway wouldinterfere with TRAIL expression and (2) whether agents thatinhibit HIV-1 infection would block HIV-1–induced productionof sTRAIL. Finally, we used the ex vivo tonsil lymphoid tissuehistoculture model to determine whether HIV-1 would induce TRAILproduction in primary human lymphoid tissue.

   Patients, materials, and methods

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Abstract
Introduction
Patients, materials, and methods
Results
Discussion
References

Patients
Peripheral blood was collected from 107 HIV-1–infectedpatients who were involved in the United States Air Force (USAF)Natural History Study, of the USAF Wilford Hall Medical Center,Lackland Air Force Base (AFB), TX. Peripheral blood was collectedfrom 8 HIV-1–infected patients who were involved in alongitudinal study of antiretroviral therapy (ART) at the Children'sHospital Medical Center, Cincinnati, OH. Approval was obtainedfrom the institutional boards of the National Cancer Institute,the USAF Wilford Medical Center, and the Children's HospitalMedical Center. The voluntary, fully informed consent of thesubjects used in this research was obtained as required by AirForce Regulation (AFR) 169-9 and by Children's Hospital MedicalCenter. Informed consent was provided according to the Declarationof Helsinki. Patients involved in the longitudinal study werefollowed for 40 weeks. Patient I was not on antiretroviral therapyprior starting the study and was then started on tenofovir,D4T, and Kaletra (lopinavir and ritonavir). The patient wentoff ART and did not start another regimen prior to the end ofthe study. Patient II was naive prior to starting the studyand was enrolled into a study that included Trizivir (abacavir,zidovudine, and lamivudine), Combivir (zidovudine and lamivudine),and Sustiva (efavirenz). Therapy continued through week 40.Patient III was naive prior to starting the study and was enrolledin a study that included Trizivir, Combivir, and Sustiva. Thepatient was switched to didanosine (DDI), Combivir, and Sustiva,which continued through week 40. Patient IV was on ART priorstarting the study and was switched to Kaletra and Sustiva atthe start of TRAIL study.
Preparation of AT-2–inactivated virions
HIV-1_MN (X4-tropic) and HIV-1_Ada (R5-tropic) were propagatedas described previously.³² Viral supernatants were inactivatedwith 1 mM AT-2 for 18 hours at 4°C before purification.Microvesicles, used as a control reagent, were isolated fromsupernatants of uninfected cell cultures in a method identicalto that used for virus preparation from infected cells.³³ TheAT-2 HIV-1 glycoproteins remain functional after AT-2 treatmentas previously described.³⁴
Isolation and culture of PBMCs and T cells
Peripheral blood mononuclear cells (PBMCs) were isolated bydensity centrifugation (Ficoll-Hypaque; Pharmacia, Uppsala,Sweden) from peripheral blood from healthy, HIV-1–seronegativedonors by the Department of Blood Transfusion, National Institutesof Health (NIH), Bethesda, MD. Cells were cultured in RPMI medium(Invitrogen, Gaithersburg, MD) with 10% fetal bovine serum (Sigma,St Louis, MO.). CD4⁺ and CD8⁺ cells were purified from PBMCsby positive selection with anti-CD4⁺ or anti-CD8⁺ beads (MiltenyiBiotec, Auburn, CA). Macrophages and dendritic cells were generatedusing monocytes as previously described.³⁵ Cells were incubatedwith AT-2 HIV-1 at a final concentration of 50 ng/mL p24 equivalent.Infectious HIV-1_MN and HIV-1_LAV were used at the same concentration.
Ex vivo human lymphoid tissue preparation and infection
Human tonsils were obtained from patients undergoing routinetonsillectomy within 6 hours from surgery. Tissues were keptin phosphate-buffered saline (PBS) and washed in complete culturemedium composed of RPMI 1640 (Invitrogen) containing 15% heat-inactivatedfetal calf serum (FCS) (Sigma), nonessential amino acids (1mM), sodium pyruvate (1 mM), L-glutamine (292 µg/mL),amphotericin B (2.5 µg/mL; Gibco, Grand Island, NJ), ticarcillindisodium/clavulanate potassium (Timentin; 310 µg/mL; SmithKlineBeckman, Philadelphia, PA), and gentamicin (50 µg/mL;Quality Biologics, Gaithersburg, MD). Tissues were then sectionedinto 2 mm³ blocks and placed on top of medium-hydrated collagensponge gel (Gelfoam; Pharmacia & Upjohn, Kalamazoo, MI)in complete medium at the air-liquid interface in 6-well plates(Costar, Cambridge, MA) with 9 blocks per sponge in each wellin 4 mL medium. Twenty-four hours later, the culture supernatantwas replaced with fresh medium containing 1% penicillin/streptomycin(Gibco), and each tissue block was infected with 1 ng p24_gagof an HIV-1 LAV.04 viral stock (3 µL, 120 median tissueculture infective dose [TCID₅₀]). Culture medium was sampledand changed every 3 days.
Plasma quantification of HIV-1 RNA
Plasma HIV-1 RNA was measured by quantitative reverse transcriptase–polymerasechain reaction (RT-PCR), and all data are expressed in copiesper milliliter (Amplicor Monitor; Roche Diagnostic Systems,Branchburg, NJ; detection limit, 50 copies per milliliter).
Membrane TRAIL detection
Membrane TRAIL expression was determined by incubating cellsfor 20 minutes with phycoerythrin (PE)–conjugated mouseimmunoglobulin G1 (IgG1) anti–human TRAIL monoclonal antibody(clone B-S23; Diaclone, Besançon France) or with controlisotype-matched antibodies (at 5 µg/mL each) in PBS containing2% mouse serum (Sigma). Cells were acquired on FACSCalibur flowcytometer using CellQuest software (Becton Dickinson BioscienceImmunocytometry Systems, San Jose, CA). Samples were gated onviable cells by forward and side light scatter, and at least50 000 live cell events were acquired for each sample.
Soluble TRAIL and type I interferon measurement
Levels of soluble TRAIL were measured in serum of HIV-positiveor HIV-negative individuals or in cell supernatants with thecommercial TRAIL enzyme-linked immunosorbent assay (ELISA) kit(Diaclone), according to the manufacturer's instructions. IFN- ${alpha}$ / ${beta}$ levels were evaluated using ELISA kit (PBL Biomedical Laboratories,Piscataway, NJ).
Blocking assay
To block TRAIL production, monocytes were cultured with AT-2HIV-1MN/Ada in presence of CD4 binding inhibitor soluble CD4(2 µg/mL), the fusion inhibitor T20 (2 µg/mL), theCXCR4 inhibitor AMD-310 (2 µg/mL) (AIDS Research and ReagentsProgram, National Institute of Allergy and Infectious Diseases[NIAID], Bethesda, MD), or in presence of both sheep polyclonalanti–human IFN- ${alpha}$ (2000 IFN- ${alpha}$ neutralizing U/mL) and sheeppolyclonal anti–human IFN- ${beta}$ antibodies (500 IFN- ${beta}$ neutralizingU/mL) (BioSource International, Camarillo, CA). RecombinantIFN- ${alpha}$ and IFN- ${beta}$ (Peprotech, Rocky Hill, NJ) were used at 200 U/mL.
Real-time quantitative RT-PCR
Total RNA was extracted from monocytes with the acid guanidinethiocyanatephenol-chloroform method,³⁶ modified for TRIzol (Invitrogen).One microgram of total RNA was reverse transcribed in a reactioncontaining 1 µM random hexanucleotide primers, 1 µMoligo(dT), and 200 units of Moloney murine leukemia virus reversetransriptase. (Promega, Madison, WI).
Real-time PCR was conducted with the ABI Prism 7900HT (AppliedBiosystems, Foster City, CA). All reactions were performed usinga SYBR green PCR mix (QuantiTect SYBR Green PCR; Qiagen, Valencia,CA). The primer sequences were designed using the Primer ExpressSoftware v2.0 (TRAIL: forward 5-GCTCTGGGCCGCAAAAT-3, reverse5-TGCAAGTTGCTCAGGAATGAA-3; glyceraldehyde-3-phosphate dehydrogenase[GAPDH]: forward 5-CCACCCATGGCAAATTCC-3, reverse 5-TGGGATTTCCATTGATGACAAG-3).All reactions were performed in triplicate (denaturation at95°C for 15 seconds, annealing at 60°C [61°C forTRAIL] for 15 seconds, extension at 72°C for 15 seconds).Data analysis was performed with the SDS2.1 software (AppliedBiosystems). Results are presented as ratios between the targetgene and the GAPDH mRNA.
Western blot
Monocytes were cultured with AT-2 HIV-1_MN, AT-2 HIV-1_Ada, recombinantIFN- ${alpha}$ (10 ng/mL), and IFN- ${beta}$ (10 ng/mL), anti–IFN- ${alpha}$ , and anti–IFN- ${beta}$ (R&D Systems, Minneapolis, MN). After 24 hours, the cellswere pelleted, washed in PBS, and lysed (1% Nonidet P-40 [NP-40],200 mM NaCl, 50 mM Tris [tris(hydroxymethyl)aminomethane] pH7.5, supplemented with protease inhibitor cocktail [Roche]).Total protein was quantified by bicinchoninic acid (BCA) (Pierce,Rockford, IL), and 10 µg protein was mixed 1:1 with SDSProtein Gel Buffer (Quality Biologics, Gaithersburg, MD). Sampleswere run on a 10% or 15% sodium dodecyl sulfate–polyacrylamidegel electrophoresis (SDS-PAGE) gel (Bio-Rad, Hercules, CA).After transfer the blot was blocked in 3% milk/Tris-bufferedsaline Triton (TBST) and then incubated with anti–signaltransducer and activator of transcription-1 (anti-STAT1) oranti-STAT2 (Upstate Biotechnology, Lake Placid, NY) antibodiesfollowed by anti–rabbit horseradish peroxidase (HRP) secondaryantibody (Jackson ImmunoResearch Labs, West Grove, PA). Enhancedchemiluminescence (ECL) was performed, and bands were visualizedon Hyperfilm (Amersham, Piscataway, NJ); ${beta}$ -actin was visualizedas a loading control using a mouse monoclonal antibody (Sigma).
Statistical analysis
All experiments were repeated a minimum of 3 times. All comparisonsof data were made with a 2-sided Student t test (data meet therequirements for a Student t test).
Differences in plasma TRAIL between HIV-1–infected patientsand healthy donors were also analyzed using the F test to comparevariances. All the statistical data were analyzed using Prismsoftware (GraphPad, San Diego, CA). The correlation betweenviral load and TRAIL in the longitudinal study was statisticallyanalyzed as follows. The variations in TRAIL concentration ( ${Delta}$ [TRAIL])and viral load ( ${Delta}$ viral load) between each sampling time for eachpatient were calculated. A linear regression analysis between ${Delta}$ [TRAIL] and log ( ${Delta}$ viral load) was performed using Excel software.

   Results

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Abstract
Introduction
Patients, materials, and methods
Results
Discussion
References

TRAIL level is elevated in plasma of HIV-1–infected patients
We tested whether the plasma of HIV-1–infected patientscontains higher levels of sTRAIL than plasma from healthy donors.As shown in Figure 1A, mean values of plasma TRAIL were 852± 52 pg/mL for 53 control donors, 1339 ± 79 pg/mLfor 49 HIV-1–infected patients with undetectable viralload (less than 50 HIV-1 RNA copies per milliliter of blood),and 2242 ± 131 pg/mL for 58 HIV-1–infected patientswith detectable load (more than 50 HIV-1 RNA copies per milliliterof blood). These results suggest that in vivo TRAIL productionis significantly increased in HIV-1–infected patientswith high viral loads. However, there appeared to be a saturationof the sTRAIL level in patients (12 of 58) with viral loadsexceeding 40 000 RNA copies per milliliter, because higher viralloads were not associated with further increases in sTRAIL.The data of Figure 1B provide a longitudinal study of 4 HIV-1–infectedpatients who began highly active ART (HAART) therapy and weresubsequently followed for 40 weeks with measurement of plasmaviral load and sTRAIL. Patient I exhibited an initial paralleldrop in viral load and sTRAIL, followed by a concomitant reboundin both of these parameters. This rebound in viral load mayreflect development of HIV-1 drug resistance. Patient II showeda continuous parallel drop in viral load and sTRAIL. PatientIII showed 3 of 4 points in which changes in viral load andsTRAIL levels were similar. Patient IV, who had received ARTprior to enrollment into this study, exhibited a parallel flatand low profile for both viral load and sTRAIL throughout the40 weeks. This patient's initial low viral may have been dueto successful ART prior to enrollment, which continued duringthis ART protocol. Thus, we observed both cross-sectional andlongitudinal association between higher plasma viral loads andelevated sTRAIL levels in 2 different cohorts of HIV-1–infectedpatients and a parallel between HAART-induced reduction in viralload and sTRAIL levels. The correlation between the fluctuationsin viral load and TRAIL in the longitudinal study was statisticallyanalyzed by performing a linear regression between the variationsof TRAIL concentration ( ${Delta}$ [TRAIL]) and viral load ( ${Delta}$ viral load)between each sampling time for each patient. This analysis showeda positive correlation between ${Delta}$ [TRAIL] and log ( ${Delta}$ viral load)in these 4 patients (r = 0.627 and P = .029).

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Figure 1.. Increased plasma levels of TRAIL in HIV-1–infected patients. (A) Plasma samples from 107 HIV-1–infected patients and 53 uninfected controls were tested for their soluble TRAIL content by ELISA. Two groups of HIV-1–infected patients were defined depending on their viral load. The mean values of plasma TRAIL were 852 ± 52 pg/mL for 55 control donors, 1339 ± 79 pg/mL for 49 HIV-1–infected patients with undetectable viral load (less than 50 RNA copies per milliliter of blood), and 2242 ± 131 pg/mL for 58 HIV-1–infected patients with higher viral load (more than 50 RNA copies per milliliter of blood). P indicates P values from unpaired t test. Boxes indicate 25th and 75th percentiles, and error bars indicate 10th and 90th percentiles. (B) Longitudinal study of 4 HIV-1–infected patients who, at time 0, began antiretroviral therapy. Patients were followed for 40 weeks. TRAIL level was measure by ELISA. Data are representative of 4 different groups of the 8 patients tested.

Noninfectious HIV-1 induces TRAIL production by monocytes
To study the effects of noninfectious viruses on TRAIL production,we cultured PBMCs from healthy HIV-1–uninfected donorsand AIDS patients in the presence of microvesicles (negativecontrol), AT-2 HIV-1_MN (CXCR4-tropic), or AT-2 HIV-1_Ada (CCR5-tropic)for 3 to 6 days. Soluble TRAIL levels in the culture supernatantswere determined by ELISA. We did not detect TRAIL productionin untreated cultures or in cultures of PBMCs from healthy donorstreated with microvesicles (n = 10). In contrast, unstimulatedPBMCs from AIDS patients produced 190 ± 10 pg/mL sTRAIL(n = 16). Exposure to AT-2 HIV-1_MN induced sTRAIL productionby PBMCs from control donors (800 ± 160 pg/mL) as wellas from HIV-1–infected patients (760 ± 140 pg/mL).Similarly, exposure to AT-2 HIV-1_Ada induced sTRAIL productionby PBMCs from healthy donors (900 ± 300 pg/mL) and HIV-1–infectedpatients (640 ± 300 pg/mL) (Figure 2A).

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Figure 2.. Effects of AT-2 HIV-1 particles on TRAIL secretion. (A) PBMCs from HIV-1–uninfected or HIV-1–infected individuals were cultured for 3 days in presence or not of AT-2 HIV-1_MN or HIV-1_Ada. Levels of TRAIL were detected using ELISA. (B) CD4⁺, CD8⁺ T cells, DCs, macrophages, and monocytes from infected ( ${square}$ ) or noninfected individuals ( ${bullet}$ ) were cultured 3 days in presence of AT-2 HIV-1_MN. Mean values (± standard errors) are shown for 6 independent experiments for each condition tested. (C) Monocytes from HIV-1–uninfected donors were cultured for 1 day in presence of microvesicles (controls) or AT-2 HIV-1_MN. Cells were analyzed for mTRAIL by fluorescence-activated cell sorting (FACS). Iso indicates isotype control. Data are representative of 6 independent experiments. (D) Monocytes from HIV-1–uninfected individuals were cultured for 1 day in presence of microvesicles or AT-2 HIV-1_MN. TRAIL mRNA level was quantified by real-time PCR. Mean values with standard errors are shown for 4 independent experiments. (E) Monocytes from HIV-1–uninfected donors were cultured in presence of a different concentration of AT-2 HIV-1_MN, and sTRAIL was quantified by ELISA. Mean values with standard errors are shown for 6 independent experiments.

To determine which cell types in PBMCs produce sTRAIL in responseto AT-2 HIV-1, isolated monocytes as well as CD4⁺ and CD8⁺ Tcells and monocyte-derived macrophages and dendritic cells weretested for TRAIL production after culture with AT-2 HIV-1. Monocytesfrom HIV-1–infected patients but not from healthy donorsproduced sTRAIL (130 ± 40 pg/mL) when cultured withoutAT-2 HIV-1. Monocytes produced high levels of sTRAIL after exposureto AT-2 HIV-1 (MN or Ada) (Figure 2B). No significant differenceswere observed between monocytes from uninfected donors and HIV-1–infectedpatients. Exposure of monocyte-derived dendritic cells fromHIV-1–infected but not from uninfected donors producedsignificant amounts (210 ± 20 pg/mL), although lowerlevels, of sTRAIL than monocytes (1100 ± 210 pg/mL) (Figure 2B).Because membrane and soluble TRAIL are 2 forms of activeTRAIL, the expression of mTRAIL was also studied. We found increasedexpression of mTRAIL in AT-2 HIV-1–exposed monocytes (P< .0001) compared with microvesicle-treated or untreatedmonocytes (controls). After AT-2 HIV-1_MN exposure, 80% ±8% of monocytes expressed mTRAIL with a mean fluorescence intensity(MFI) of 19 ± 3 compared with 7% (MFI, 6 ± 1)in control monocytes (Figure 2C). Similar results were obtainedusing AT-2 HIV-1_Ada (data not shown).
Monocytes from uninfected donors treated with AT-2 HIV-1_MN weretested for TRAIL mRNA expression using real-time quantitativePCR. TRAIL mRNA was barely detectable in untreated or microvesicle-treatedmonocytes, whereas exposure to AT-2 HIV-1_MN induced 20-foldincrease in TRAIL mRNA expression (P = .0045) (Figure 2D). Theseresults indicated that monocytes expressed TRAIL mRNA and producedsTRAIL and mTRAIL upon exposure to AT-2 HIV-1. In contrast,sTRAIL was not produced by CD4⁺ or CD8⁺ T cells or by macrophages.However, CD4⁺ T cells express mTRAIL but not sTRAIL after exposureto AT-2 HIV-1 (J.P.H. et al, manuscript in preparation).
To investigate whether low amounts of virus induce sTRAIL production,we performed a dose response experiment in which monocytes werecultured for 3 days with dilutions of AT-1 HIV-1 spanning 4logs of concentration. Very low concentrations of AT-2 HIV-1_MNinduced measurable production of sTRAIL (Figure 2E). Optimalconcentrations of AT-2 HIV-1 MN for sTRAIL production were inthe 5 to 50 ng/mL (p24^CA equivalents) range, with no furtherincrease in TRAIL at higher virus concentrations. Therefore,AT-2 HIV-1 was used at 50 ng/mL for subsequent experiments.
Noninfectious HIV-1 induces TRAIL production by the type I IFN pathway
To test whether type I IFN was required for TRAIL productionby monocytes isolated from PBMCs of HIV-1–uninfected donors,we attempted to block TRAIL production using anti–IFN- ${alpha}$ and/or anti–IFN- ${beta}$ antibodies. Anti–IFN- ${alpha}$ antibody(Ab) or anti–IFN- ${beta}$ Ab inhibited the sTRAIL production ofAT-2 HIV-1–exposed monocytes by 25% ± 11% and 40%± 3%, respectively. When used together, these antibodiesreduced TRAIL production by 76% ± 4% in monocytes exposedto AT-2 HIV-1_MN (P < .000 01) (Figure 3A). Similar resultswere obtained using HIV-1_Ada. We also tested whether Ab againsttype I interferons would affect AT-2 HIV-1_MN–induced TRAILgene expression. Addition of anti–IFN- ${alpha}$ and - ${beta}$ blockingmonoclonal antibody (mAb) decreased TRAIL mRNA expression by70% ± 30% (P = .046) (Figure 3B). To determine whetherIFN- ${alpha}$ and IFN- ${beta}$ were both involved in TRAIL production, we culturedmonocytes in the presence of recombinant IFN- ${alpha}$ or IFN- ${beta}$ . IFN- ${alpha}$ induced 730 ± 200 pg/mL and IFN- ${beta}$ 1650 ± 300 pg/mLof sTRAIL (Figure 3C). Because AT-2 HIV-1 induction of TRAILis IFN- ${alpha}$ / ${beta}$ dependent, we verified that monocytes from uninfecteddonors cultured with AT-2 HIV-1_MN or AT-2 HIV-1_Ada producedIFN- ${alpha}$ (Figure 3D). Moreover, we demonstrated that AT-2 HIV-1_MNand AT-2 HIV-1_Ada as well as recombinant IFN- ${alpha}$ / ${beta}$ increased monocyteexpression of STAT1 and STAT2 (Figure 3E), the principal signalingmolecules for type I IFN.^37,38 We also observed a decrease ofSTAT1 expression and a strong inhibition of STAT2 expressionwhen monocytes were cultured with HIV-1 and antibodies againsttype I interferons. Taken together, these findings indicatethat AT-2 HIV-1–induced expression and production of TRAILby monocytes is dependent on STAT1/STAT2 type I interferons.

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Figure 3.. Effect of IFN type I antibodies on TRAIL production by monocytes from HIV-1–uninfected donors. (A) Monocytes were cultured 3 days in presence of AT-2 HIV-1_MN alone ( ${bullet}$ ) or with blocking antibodies against IFN- ${alpha}$ (2000 neutralizing U/mL; ), IFN- ${beta}$ (500 neutralizing U/mL; ), or both ( ${square}$ ). The level of sTRAIL was quantified by ELISA. (B) Monocytes were cultured for 1 day in presence of AT-2 HIV-1_MN and with or without blocking antibodies against IFN- ${alpha}$ and IFN- ${beta}$ . The level of TRAIL mRNA was quantified by real-time PCR analysis. (C) Monocytes were cultured for 3 days in presence of recombinant IFN- ${alpha}$ or IFN- ${beta}$ (10 ng/mL). The level of sTRAIL was quantified by ELISA. (D) IFN- ${alpha}$ ( ${square}$ ) and IFN- ${beta}$ production ( ${bullet}$ ) by monocytes cultured for 3 days in presence of microvesicles (control), AT-2 HIV-1_MN, or AT-2 HIV-1_Ada. Mean values with standard errors are shown for 4 independent experiments in panels A-C for each condition tested. (E) STAT1 and STAT2 expression. Monocytes were cultured 24 hours in presence of AT-2 HIV-1_MN, AT-2 HIV-1_Ada, recombinant IFN- ${alpha}$ / ${beta}$ (10 ng/mL), or HIV-1_MN plus anti–IFN- ${alpha}$ / ${beta}$ antibodies. Production of STAT1 and STAT2 was analyzed by Western blot; ${beta}$ -actin was used as a loading control. (F) Blocking assay. Monocytes were cultured for 3 days with AT-2 HIV-1_MN or HIV-1_Ada and in presence of isotype control antibody or the CD4 binding inhibitor soluble CD4 (2 µg/mL). IFN- ${alpha}$ ( ${square}$ ) and TRAIL levels ( ${bullet}$ ) were quantified by ELISA. (G) Monocytes were cultured for 3 days with AT-2 HIV-1_MN and in presence of isotype control antibody; the CD4 binding inhibitor soluble CD4 (2 µg/mL); the CXCR4 inhibitor AMD-3100 (2 µg/mL), or the fusion inhibitor T20 (2 µg/mL). Monocytes cultured without AT-2 HIV-1_MN were used as control. TRAIL level was quantified by ELISA. Mean values with standard errors are shown for 3 independent experiments for each condition tested (panels F-G).

We tested whether noninfectious HIV-1–induced productionof sTRAIL would be inhibited by (1) soluble CD4, which blocksthe interaction between viral glycoprotein 120 (gp120) and CD4expressed on CD4⁺ cells (monocytes, macrophages, dendritic cells[DCs], or T cells); (2) AMD-3100, which blocks CXCR4 coreceptorbinding; and (3) T20, which prevents fusion of the virus withthe CD4 cell membrane. The results (Figure 3F) demonstrate thatsoluble CD4 inhibited HIV-1_MN and HIV-1_Ada from inducing sTRAILproduction by monocytes. Furthermore, soluble CD4 (sCD4) alsoinhibited IFN- ${alpha}$ production. In contrast, AMD-3100 or T20 didnot statistically block TRAIL production by monocytes culturedwith HIV-1_MN (Figure 3G). These results are consistent witha triggering mechanism that is dependent on very early CD4/gp120binding events but that does not require early post-bindingevents such as coreceptor engagement or membrane fusion.
All of the results presented above were reproduced using theinfectious counterparts of HIV-1_MN and HIV-1_Ada. InfectiousHIV-1_LAV, which is commonly used in tonsil model,³⁹ also inducedTRAIL production in monocytes.
Infection with HIV-1 induces TRAIL production in tonsil tissue culture
To investigate whether TRAIL could be produced in primary lymphoidorgans, we infected human tonsils with infectious HIV-1_Lav,the HIV-1 strain used previously in this model,³⁹ and measuredthe TRAIL production at different times ranging from 1 to 12days. As shown in Figure 4, for each of 3 independent experimentsusing tissues from 3 different individuals, we observed increasedTRAIL secretion after infection with HIV-1_Lav compared withuninfected tonsils. These results suggest that sTRAIL can befound in the primary lymphoid organs of HIV-1–infectedpatients as well as in their blood (Figure 1).

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Figure 4.. Effect of infectious HIV-1 on sTRAIL production in tonsil culture. Ex vivo human lymphoid tissues were cultured for 12 days in absence ( and thin line) or presence of HIV-1_LAV (bold line and ${square}$ ). Soluble TRAIL was measured at days 3, 6, 9, and 12 by ELISA. Culture medium was changed at 3-day intervals. The statistically different (P < .05) samples from control are indicated by an asterisk. Error bars indicate standard deviation derived from 3 different ELISAs for each condition tested.

   Discussion

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Abstract
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Patients, materials, and methods
Results
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In the present study, we observed elevated sTRAIL levels inthe plasma of HIV-1–infected patients compared with healthycontrol donors. After in vitro exposure to either infectiousor noninfectious HIV-1, we found that both sTRAIL and mTRAILwere produced by monocytes. Monocyte-derived dendritic cellsfrom HIV-1–infected patients also produced low levelsof sTRAIL. In contrast, sTRAIL was not produced by macrophagesor by CD4⁺ or CD8⁺ T cells upon exposure to HIV-1. TRAIL productionwas associated with increased transcription of the TRAIL genein monocytes exposed to HIV-1 particles and was mediated bythe type I IFN pathway. Induction of sTRAIL by HIV-1 is likelyto be dependent on CD4-gp120 interaction because it was blockedby soluble CD4. Finally, the ex vivo tonsil model demonstratesthat TRAIL can be produced in primary lymphoid tissue afterHIV-1 infection.
Soluble TRAIL was reported in HIV-1–infected patients,¹⁰and in vitro studies linked TRAIL to the depletion of T cellsfrom HIV-1–infected patients.^6,8,9 However, the identificationof TRAIL-producing cells in vivo, the association of viral loadwith the level of sTRAIL produced, and the mechanism responsiblefor TRAIL-mediated T-cell death remain to be established. Thepresent study demonstrates that sTRAIL can be detected in theplasma of HIV-1–infected patients. Furthermore, the amountof sTRAIL is higher in patients with elevated viral load thanin patients with low or undetectable viral loads. However, plasmafrom all HIV-1 patients tested showed higher TRAIL content thanplasma from healthy donors. Our 40-week longitudinal study ofpatients on HAART showed striking parallel changes between viralload and TRAIL levels. Thus, when HAART decreased viral load,we observed a concomitant decrease in plasma TRAIL, which maybe one of the reasons for the efficacy of antiviral therapy.
More than 95% of HIV-1 virions detected in HIV-1–infectedpatients' plasma do not possess culturable infectivity,⁴⁰ whichraises the possibility that noninfectious virus particles contributeto HIV-1 pathogenesis. We demonstrate here that the major cellularsource of TRAIL is monocytes, which produce TRAIL in responseto both infectious and chemically inactivated X4 (MN) and R5(Ada) HIV-1. Interestingly, PBMCs and DCs from HIV-1–infecteddonors produced sTRAIL without further stimulation, suggestingthat previous contact with HIV-1 was sufficient to induce sTRAILsecretion. However, after 3 days of culture, sTRAIL productiondisappeared if the patients' PBMCs were not stimulated by HIV-1particles (data not shown), suggesting that continuous cell-virusinteraction is required to maintain sTRAIL production.
Our results do not conflict with the effect of Tat on TRAILproduction by monocytes or macrophages.⁹ We confirmed that Tatinduced TRAIL production; however, the range of concentrationat which Tat was efficient was narrower (data not shown) thanthe range at which HIV-1 was inducing TRAIL. We think that bothTat and HIV-1 particles likely induce TRAIL production in HIV-1–infectedpatients and these 2 nonmutually exclusive but rather concomitantmechanisms contribute together to the high level of TRAIL measuredin the serum of HIV-1–infected patients.
Type I interferons are produced as a result of viral infectionand can exert antiviral effects.⁴¹ Type I interferons activatethe signaling molecules STAT1 and STAT2, which bind to the interferon-stimulatedresponse element (ISRE), which activates IFN-inducible genes¹⁶such as TRAIL.^42,43 Here we demonstrate that in monocytes, typeI interferons, STAT1 and STAT2 expressions are induced by exposureto HIV-1 virions. Recombinant IFN- ${alpha}$ or IFN- ${beta}$ induced STAT1 andSTAT2 and sTRAIL production, while antibodies against theseinterferons greatly reduced STAT2 expression and both TRAILgene transcription and production in monocytes exposed to AT-2HIV-1. We showed that sCD4 blocked the effects of HIV-1_MN andHIV-1_Ada on TRAIL and IFN- ${alpha}$ production by monocytes. This blockadestrongly suggests that the interaction between viral gp120 andthe CD4 molecule is required for HIV-1 induction of type I interferonsand sTRAIL production. Conversely, our findings that AMD-310and T20 did not significantly inhibit sTRAIL production suggestthat coreceptor binding and viral fusion with the target cellmembrane are not required for HIV-1 activation of sTRAIL productionby monocytes. Thus, only the earliest interaction between HIV-1and CD4 on monocytes is essential for initiation of TRAIL production.
We also tested whether HIV-1 induced TRAIL production in anex vivo human tonsil model that resembles human lymphoid organswhere critical events of HIV disease occur. Increased TRAILsecretion was seen in tonsil organ cultures from 3 differentdonors after HIV-1 infection. TRAIL production was maintainedover an extended time, because we still observed higher TRAILproduction in infected than in uninfected tonsil cultures after10 days. Detection of TRAIL in these HIV-1–infected culturesis consistent with increased apoptosis of CD4⁺ T cells afterHIV-1 infection of tonsil cultures.² Because CD4⁺ T cells expressmTRAIL but do not produce sTRAIL upon exposure to HIV-1,¹⁸ thesTRAIL that we detected in plasma of HIV-1–infected patientsis unlikely to have been secreted by CD4⁺ T cells and may havebeen produced by monocytes and/or dendritic cells after exposureto HIV-1. Furthermore, because B cells, present in large numberin tonsil, did not produce TRAIL (data not shown), it is possiblethat dendritic cells in the tonsil were the source of sTRAILin our HIV-1–infected tonsil cultures, a possibility thatwe are now investigating.
The findings of the present study, in combination with our observationthat the membrane DR5 death receptors required for inductionof cell death via TRAIL are expressed on CD4⁺ but not CD8⁺ Tcells from HIV-1–infected patients (J.P.H. et al, manuscriptin preparation), suggest a plausible mechanism for preferentialloss of CD4⁺ T cells in HIV-1 infection. In this model, sTRAILand/or mTRAIL produced by monocytes contribute to TRAIL-mediateddeath of CD4⁺ T cells in HIV-1–infected patients by directlyinteracting with the DR5 death receptor expressed on CD4⁺ Tcells.
Establishment of the in vivo relevance of our in vitro findingsto the loss of CD4⁺ T cells in HIV-1–infected patientsmay point toward novel therapeutic approaches for maintainingimmune cell numbers and function. In particular, we found thatsCD4 was the most efficient inhibitor of TRAIL production, suggestingthat this reagent might provide effective therapy that wouldinhibit the interaction of either infectious or noninfectiousHIV-1 with the CD4 molecule that results in TRAIL productionby CD4-expressing cells.

   Acknowledgements

We thank Dr Leonid Margolis, Laboratory of Cellular and MolecularBiophysics, NICHD, NIH, Bethesda, MD, for reviewing the manuscript;Julian Bess, AIDS Vaccine Program, NCI-Frederick, MD, for preparingAT-2 HIV-1; and Dr David Venzon, Biostatistics and Data ManagementSection, National Cancer Institute, NIH, Bethesda, MD, for statisticalanalysis and helpful suggestions concerning the longitudinalstudy.
The views expressed herein are those of the authors and do notreflect the official policy of the Department of Defense orother departments of the US Government.

   Footnotes

Submitted August 6, 2004; accepted November 9, 2004.
Prepublished online as Blood First Edition Paper, December 7,2004; DOI 10.1182/blood-2004-08-3058.

Supported by the Intramural Program of the Centers for CancerResearch, NCI, NIH, and by the NIH Intramural AIDS TargetedAntiviral Program. This project has been funded in part withfederal funds from the National Cancer Institute, National Institutesof Health, under contract no. N01-CO-12400 (Article H.36 ofthe Prime Contract). The content of this publication does notnecessarily reflect the views or policies of the Departmentof Health and Human Services, nor does mention of trade names,commercial products, or organizations imply endorsement by theUnited States government.

An Inside Blood analysis of this article appears in the frontof this issue.

The publication costs of this article were defrayed in partby page charge payment. Therefore, and solely to indicate thisfact, this article is hereby marked "advertisement" in accordancewith 18 U.S.C. section 1734.

Reprints: Gene M. Shearer, NCI, NIH, 9000 Rockville Pike, Bethesda, MD; e-mail: gene_shearer{at}nih.gov.

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	Copyright © 2005 by American Society of Hematology Online ISSN: 1528-0020