We previously demonstrated that vaccinia virus (VV)-specific CD4+ cytolytic T cells can persist for >50 years after immunization against smallpox in the absence of re-exposure to VV. Nevertheless, there have been few studies focusing on CD4+ T cell responses to smallpox vaccination. To ensure successful vaccination, a candidate vaccine should contain immunodominant CD4+ T cell epitopes as well as CD8+ T and B cell epitopes. In the present study, we established cytotoxic CD4+ T cell lines from VV-immune donors, which recognize epitopes in VV proteins D1R and A24R in association with HLA-DR1 Ags. Comparisons of sequences between different members of the poxvirus family show that both epitopes are completely conserved among VV, variola viruses, and most mammalian poxviruses, including monkeypox, cowpox, and ectromelia. The CD4+ T cell lines lysed VV-infected, Ag- and peptide-pulsed targets, and the lysis was inhibited by concanamycin A. We also detected these peptide-specific cytolytic and IFN-γ-producing CD4+ T cells in short-term bulk cultures of PBMC from each of the three VV-immune donors tested. These are the first VV-specific CD4+ T cell epitopes identified in humans restricted by one of the most common MHC class II molecules, HLA-DR1, and this information may be useful in analyzing CD4+ T cell responses to pre-existing or new generation VV vaccines against smallpox.

Worldwide immunization has successfully eradicated smallpox infections. Bioterrorism threats have brought a renewed interest in smallpox and its significant potential as a biological weapon. Of concern is the fact that a large majority of the population would be susceptible to smallpox infection, because routine smallpox vaccination was eliminated in the 1970s, when the disease was eradicated worldwide (1). The standard smallpox vaccines were effective, but had rare severe side effects, including myocarditis and encephalitis (2, 3, 4). A new generation of safer smallpox vaccines is being developed, and it is important to test and establish the safety and robustness of immunological responses to these new vaccines.

Both humoral and cellular immunity have been thought to play a role in protection against and recovery from orthopoxvirus infections as evidenced in individuals with either humoral or cellular immune defects who were unable to control vaccinia virus (VV)3 infections (5, 6). A number of studies indicate Ab responses are long-lived and essential for protection against orthopoxviruses (7, 8, 9, 10, 11). Several studies have analyzed the role of different cytokines during infection with VV: some cytokines increased virulence, as with IL-4 (12, 13), whereas others attenuated the infection, as with IFN-γ or IL-2 (14, 15, 16, 17, 18, 19, 20). Both NK cells and γδT cells have been shown to play a role in innate resistance to VV infection (21, 22). VV elicits a robust and long-lasting cellular immune response that includes large numbers of CD4+ and CD8+ T cells (23). CD8+ CTLs are crucial in controlling primary and secondary VV infections in mice and humans (24). VV-specific CD4+ T cells play an important role in expanding CD8+ T cell populations, as evidenced by the failure of control of virus replication in a mouse model with CD4+ T cell-depleted and MHC class II-knockout mice (25). Several laboratories including ours have identified an increasing number of CD8+ CTL epitopes in human (26, 27, 28, 29, 30, 31, 32, 33, 34) and murine systems (35, 36, 37, 38).

We earlier demonstrated that VV-specific CD4+ T cells can persist for up to 50 years after immunization of humans against smallpox in the absence of re-exposure to VV (39), and that several CD4+ CTL clones were able to recognize and kill VV-infected targets (40). There have been a few studies focusing on CD4+ T cell responses to smallpox vaccination (41, 42). Hammarlund et al. (8) measured T cell immunity against VV in 306 vaccinees, up to 75 years after their last vaccination. Within the first 7 years after vaccination, CD4+ and CD8+ T cell responses remained high and then declined slowly over decades. The role of CD4+ T cell in protection in VV-immunized individuals is still poorly characterized. Studies of VV-specific T cell responses in BALB/c mice have shown that VV infection induces a potent primary CD8+ T cell response as well as long-term memory (43). However, β2-microglobulin−/− mice almost completely lacking CD8+ T cells survived high-dose s.c. infection with similar lesion development as control mice (44). In addition, studies in mice show that the absence of either perforin- or Fas-dependent cytotoxicity did not affect clearance of a primary VV infection (45). However, the roles of perforin- and Fas-dependent cytotoxicity have not been defined in human subjects. Xu et al. (25) have shown that, in acute infection, the CD4+ T cell-dependent Ab response is more important for clearing VV using Ab-depleted and gene knockout mice. Recently, Tang et al. (32) identified CD8+ and CD4+ responses to VV envelope proteins A27L, B5R, L1R, and A33R. They studied four VV envelope proteins expressed from mRNA in autologous dendritic cells and reported CD4+ T cell responses. Although they localized three peptide epitopes on the A27L protein of VV using 15-mer peptides, the epitopes were not well characterized in terms of MHC restriction and definition of minimal epitopes.

To analyze human CD4+ T cell responses against VV, it is important to identify CD4+ T cell epitopes, especially the ones restricted by common MHC class II molecules. Because we identified cytotoxic CD4+ T cells specific to VV previously (40), we decided to use cytotoxic CD4+ T cell lines for epitope mapping. We identified two peptide epitopes that are recognized by VV-specific CD4+ T cell lines restricted by HLA-DR1 that were isolated from vaccinated individuals and are encoded by the vaccinia genes A24R and D1R, respectively.

PBMC donors in this study were healthy VV-naive volunteers who received smallpox vaccine, standard Dryvax, by multiple cutaneous punctures made with a bifurcated needle, as recommended by the Centers for Disease Control and Prevention for laboratory personnel working with VV (46). They were enrolled under an approved University of Massachusetts Medical School Institutional Review Board human study protocol. Blood was collected prevaccination or at 2 and 4 wk postvaccination. The postvaccination PBMC demonstrated VV-specific T cell proliferation and CTL activity postvaccination (data not shown). The HLA types of these donors were determined using Biotest HLA-class II SSPtray (Biotest Diagnostics), and HLA DR0101-positive donors’ PBMCs were used in this study.

PBMC were purified by Ficoll-Hypaque density gradient centrifugation. Buffy coats were recovered, and mononuclear cells were resuspended at 5 × 106 to 8 × 106/ml in RPMI 1640-20% FBS-10% DMSO and cryopreserved until needed. B lymphoblastoid cell lines (BLCL) were generated from each donor, as previously described (26), and cultured in RPMI 1640 supplemented with penicillin, streptomycin, l-glutamine, HEPES, and 10% FBS. T2-DR1 is a T × B hybrid cell line T2 transfected with the cDNA for DR1 (DRA*0101/DRB1*0101) and was cultured in RPMI 1640 medium containing 10% FBS (47).

VV New York City Board of Health strain, the same strain used to produce the licensed vaccine, Dryvax, was provided by G. Mazzara and D. Panicali (Applied Biotechnology, Cambridge, MA) and propagated in CV-1 cells (American Type Culture Collection CCL-70). Virus stock was prepared by freezing and thawing infected CV-1 cell lysate. The lysate was then sonicated and cleared by centrifugation at 1000 rpm for 10 min. The supernatant was titrated by plaque assay using CV-1 cells and stored at −80°C until use, as previously described (40, 48). To prepare VV Ag, the same cell lysate was placed in boiling water for 30 min to inactivate the virus after freezing and thawing. Plaque assays were performed to confirm the absence of live VV.

A total of 3 × 106 PBMC was dispensed per well in 24-well plates (Corning Glass) with 2 × 106 (stimulator cells) autologous PBMC infected with VV at a multiplicity of infection (moi) of 1 or pulsed with VV Ag (the same volume of infected cell lysate used for the infection at a moi of 1, but inactivated by boiling for 30 min) in 1 ml of AIM-V medium containing 20% FBS and 25 ng/ml human rIL-7 (PeproTech). After 2 days, human rIL-2 (BD Biosciences) was added to the wells at 50 U/ml final concentration. Cultures were split 1:4 after 5 days and cultured for an additional 5 days. For specific restimulation, 5 × 105 IL-2-expanded T cells were cultured with virus-infected or Ag-pulsed autologous irradiated PBMC. For nonspecific restimulation, allogeneic PBMC irradiated with 30 Gy from a 57Cs source were added along with anti-CD3 Ab (12F6) and rIL-2. Bulk culture 51Cr release assays were performed between days 7 and 14 of culture. CTL responses were determined at each restimulation cycle, using Ag-pulsed or virus-infected radiolabeled autologous BLCL as target cells and effector T cells from the different lines. VV-specific CTL lines were established by limiting-dilution plating, as described previously (40, 49). In vitro stimulated PBMC were plated at 1, 3, 10, or 30 cells/well in 96-well, round-bottom plates in 0.2 ml of AIM/V-10% FBS and stimulated with anti-CD3 Ab (12F6) and γ-irradiated allogeneic PBMC as feeder cells. Medium was replenished every 3 days, and wells were restimulated with 12F6 and γ-irradiated feeder cells every 14 days. Cells from individual wells were tested for recognition of both VV-infected and VV Ag-pulsed targets in Cr release assay, and the remaining cells from positive wells were expanded and restimulated, as described above. T cell line phenotypes were defined by flow analysis (FACScan; BD Biosciences) using mAbs anti-CD4 (clone RPA-T4; BD Pharmingen), anti-CD8 (clone SK1; BD Pharmingen), and anti-CD3 (clone UCHT1; BD Pharmingen).

PBMC (2 × 106 to 5 × 106) were resuspended in 1 ml of AIM/V-20% FBS in each well of a 24-well plate. VV-infected or Ag- or peptide-pulsed autologous PBMC were added as stimulator cells. Human rIL-7 was added, and the culture was incubated at 37°C. Human rIL-2 (BD Pharmingen) (50 U/ml) was added on day 3 in 1 ml of fresh AIM/V-20% FBS, and the medium was replenished every third day thereafter. Bulk culture 51Cr release assays were performed between days 7 and 14 of culture. The cultures were restimulated once with autologous stimulator cells at day 14 and once with allogenic feeder cells at day 28 to reduce nonspecific background lysis and generate enough cells for the assays.

HLA-DR1 (DRB*0101)-binding epitopes were predicted using genomic sequences of the VV strain modified vaccinia Ankara (MVA; U94848) (50). MVA was chosen as a prototype for epitope prediction because it is a potential smallpox vaccine for the future, and most open reading frames in MVA strain are conserved in WR, Copenhagen, and the Dryvax strains. All 193 MVA open reading frames were subjected to the scan using a prediction algorithm (L. Stern, J. Calvo-Calle, I. Strug, M. Nastke, S. Baker, and L. Stern, unpublished data). Briefly, matrices of predicted peptides were derived using two different algorithms (P9 and SYFPEITHI). P9 modified from a published algorithm (51) predicts HLA-DR1 peptide binding based on inhibition-binding asaays of a set of minimal peptides (available at http://rcdev.umassmed.edu/nwpredict.php), and SYFPEITHI predicts HLA-DR1-restricted epitopes based on analysis of naturally processed endogeneous peptides (52) (available at www.syfpeithi.de). The top 45 predicted binding peptides were selected for synthesis as 21-mer peptides, of which 36 peptides were successfully synthesized by Genemed Synthesis and purified to >70% purity. Each peptide has an HLA-DR1-binding motif (9 aa) flanked by 6 aa on each side. Peptide pools containing 4 μg/ml each of six peptides were used to screen the T cell lines. The 21-mer peptides from positive pools were then tested individually with the CTL lines in ELISPOT assays at 4 μg/ml to identify specific epitopes. Sequential deletions of specific reactive peptides were generated to determine minimal epitopes. These peptides were synthesized at the Peptide Core Facility at the University of Massachusetts Medical School or were purchased from Anaspec, and peptide identity was verified by mass spectrometry or amino acid analysis.

A competition assay was used to determine binding affinities of peptides to the HLA-DR1 molecule. Peptide-free HLA-DR1 produced in Escherichia coli (25 nM) was mixed together with biotinylated Ha(306–318) peptide probe (Habio, 25 nM) and varying concentrations of unlabeled competitor peptide (10−12–10−5 M). The mixtures were incubated for 3 days at 37°C in 100 mM sodium phosphate buffer (pH 5.5), containing protease inhibitors and 0.5 mg/ml octylglucoside, followed by detection of bound biotinylated peptide using an immunoassay that used anti-DR1 capture Ab LB3.1 and alkaline phosphatase-labeled streptavidin. IC50 values were obtained by fitting a binding curve to the plots of absorbance vs concentration of competitor peptide.

Virus-infected targets.

Autologous BLCL, T2, or T2-DR1 cells were infected with VV at a moi of 10 for 60 min at 37°C. The cells were then diluted in 1 ml of RPMI 1640-10% FBS for an additional 16 h. Target cells were then radiolabeled or used directly.

Ag-pulsed targets.

Autologous BLCL, T2, or T2-DR1 cells were incubated with VV Ag preparation (the same volume of infected cell lysate used for the infection at a moi of 10, but inactivated by boiling for 30 min) for 60 min at 37°C. The cells were then diluted in 1 ml of RPMI 1640-10% FBS for an additional 16 h. Target cells were then radiolabeled or used directly.

Peptide-pulsed targets.

BLCL, T2, or T2-DR1 cells were 51Cr labeled or used unlabeled in the assays. Cells were incubated with 25 μg of peptide/ml in 96-well round-bottom plates at 1 × 103 to 2 × 103/well for 30 min at 37°C before addition of effector cells. The peptides remained in the wells for the duration of the assay.

T cell lines or bulk culture effector cells were added to 2 × 10351Cr-labeled target cells at various E:T ratios. For inhibition of the perforin pathway, effector T cells were preincubated with concanamycin A (Sigma-Aldrich) at various concentrations (100, 50, 20, and 10 nM) (53) for 2 h at 37°C, washed, and added to labeled targets on 96-well plates at a ratio of 30:1 (54, 55, 56). Similarly, to inhibit the Fas-Fas ligand (FasL) pathway of cytotoxicity, effortors were treated with anti-FasL Ab (clone 100419; R&D Systems) at 50, 10, and 5 μg/ml (57) for 1 h at 37°C, washed, and added to labeled targets at a ratio of 30:1. Plates were incubated for 4 h at 37°C, supernatants were harvested (Molecular Devices), and specific lysis was calculated as follows: ((experimental release − spontaneous release)/(maximum release − spontaneous release)) × 100. All assays were performed in triplicate. All experiments were performed at least twice. Negative controls included unpulsed target cells as APC. Spontaneous lysis was <30% in all assays.

ELISPOT assays were performed, as described previously (58, 59, 60). Briefly, 96-well filtration plates (MSIPS4W; Millipore) were coated with 15 μg of mouse anti-human IFN-γ mAb (clone D1K; Mabtech) per ml at 4°C overnight. Plates were blocked with RPMI 1640-10% FBS for at least 2 h. A total of 2.5 × 103 APC and 2 × 103 T cells was added in RPMI 1640-10% FBS. Peptides were added at 2.5 μg/ml, PHA at 10 μg/ml, VV at a moi of 10 or VV Ag (the same volume of infected cell lysate used for the infection at a moi of 10, but inactivated by boiling for 30 min), and plates were incubated for 18–20 h at 37°C. The cells were removed by washing, and biotinylated mouse anti-human IFN-γ mAb (clone 7-B6-1; Mabtech) was then added and left for 2 h at room temperature, followed by a 1/400 dilution of streptavidin HRP for 30 min. Substrate (Novared; Vector Laboratories) was added and left for 10 min at room temperature. The frequency of IFN-γ-producing T cells was calculated as number of spots/total number of cells/well. Experiments were performed in triplicate.

Bulk culture cells at day 28 (donors A, B, and C) or day 14 (donors D and E) of in vitro culture were resuspended at 106/ml in RPMI 1640 medium supplemented with 10% FBS. For in vitro stimulation, peptides were used at 2.5 μg/ml final concentration. For each sample, a negative control containing only medium and a positive control (PHA; final concentration 10 μg/ml) was used to ensure that cells were responsive. The cultures were incubated for 1 h at 37°C in a 5% CO2 incubator, followed by an additional 5 h in the presence of GolgiPlug (BD Biosciences). Stimulated cells were washed, fixed/permeabilized (Cytofix/Cytoperm; BD Biosciences), and stained for surface markers and IFN-γ. Cells were then washed and resuspended in Permwash buffer for flow cytometric analysis. Responses are reported after background correction, using the unstained and single-stained controls to define nonspecific responses. FITC, PECy7, PerCPCy5.5, PE, Pacific blue, and allophycocyanin were used as the fluorophores for these experiments. Multiparameter flow cytometric analyses were performed using a FACSCalibur or ARIA flow cytometer. The list-mode data files were analyzed using FlowJo (version 6.3; Tree Star). Graphs were plotted as biexponential transformed dot plots of CD19, CD3+CD8, T cells in the live cell population of each bulk culture tested.

Bulk culture lines were generated by incubating PBMC (drawn at 28 or 45 days after vaccination) from four VV-immune donors with either VV-infected or VV Ag-pulsed autologous stimulator cells. The bulk cultured cells were tested for CTL activity after 7 days of culture and specifically lysed autologous BLCL target cells that were either infected with VV or pulsed with VV Ag. The lines were subjected to limiting dilution, and a total of 14 cell lines was found to possess substantial VV-specific CTL activity. The cell lines were then stained with Abs to CD3, CD8, and CD4, and the 12 cell lines that were >98% CD4+ T cells were further studied.

The CD4+ CTL lines were tested for their ability to secrete IFN-γ when incubated with T2-DR1 cells (T2 cells expressing only HLA DR1) that were pulsed with each of 6 peptide pools comprising a total of 36 peptides in a screening ELISPOT assay. These peptides were selected based on an HLA-DR1-binding and epitope prediction algorithm (L. Stern, J. Calvo-Calle, I. Strug, M. Nastke, S. Baker, and L. Stern, unpublished data). Two cell lines showed positive reactivity to different peptide pools. T cell lines 1F2 from donor B and 3F3 from donor C recognized cells pulsed with peptides MVA 344 and MVA 302, respectively. The cell lines were tested for their ability to lyse peptide-pulsed APC in addition to VV-infected and VV Ag-pulsed targets and, as shown in Fig. 1, A and B, they lysed targets pulsed with the respective peptide in a specific manner. The ELISPOT assay was repeated with autologous BLCL as APC-testing peptides at different concentrations, and we found that both cell lines generated IFN-γ responses to the respective epitopes in a peptide dose-dependent manner (Fig. 2,B). The cell lines lysed T2-DR1 cells presenting cognate peptides, but not untransfected T2 cells in a CTL assay, indicating that they are HLA-DR1-restricted CD4+ CTLs (Fig. 2 A). We also confirmed that these cytotoxic CD4+ T cell lines recognized cells pulsed with cognate peptides, VV-infected and VV Ag-pulsed APC (T2-DR1 cells), and secrete IFN-γ in an ICS assay (data not shown). MVA 344 is encoded by the VV gene, A24R (DNA-dependent RNA polymerase subunit rpo132) gene, and MVA 302 is encoded by the VV gene, D1R (mRNA capping enzyme large subunit).

FIGURE 1.

Cytotoxic CD4+ T cell lines kill VV-infected, VV Ag-pulsed, and peptide-pulsed autologous BLCL targets in a 51Cr release assay. The 1F2 (A) or 3F3 (B) cells were cocultured with 51Cr-labeled autologous BLCL targets, which were untreated, infected with VV at a moi of 1, pulsed with VV Ag (the same volume of infected cell lysate used for the infection at a moi of 1, but inactivated by boiling for 30 min), or pulsed with 2.5 μg/ml specific peptide in a U-bottom plate in triplicates. Cells were incubated at the indicated E:T cell ratio for 4 h, after which the percent lysis of target cells was calculated. The mean 51Cr release of the CTL lines ± SD is shown.

FIGURE 1.

Cytotoxic CD4+ T cell lines kill VV-infected, VV Ag-pulsed, and peptide-pulsed autologous BLCL targets in a 51Cr release assay. The 1F2 (A) or 3F3 (B) cells were cocultured with 51Cr-labeled autologous BLCL targets, which were untreated, infected with VV at a moi of 1, pulsed with VV Ag (the same volume of infected cell lysate used for the infection at a moi of 1, but inactivated by boiling for 30 min), or pulsed with 2.5 μg/ml specific peptide in a U-bottom plate in triplicates. Cells were incubated at the indicated E:T cell ratio for 4 h, after which the percent lysis of target cells was calculated. The mean 51Cr release of the CTL lines ± SD is shown.

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FIGURE 2.

A, 1F2 and 3F3 are HLA-DR1-restricted CD4+ CTL lines. The 1F2 and 3F3 cells were incubated with T2 or T2-DR1 cells pulsed with peptides or infected with VV (as positive control) at different E:T ratios for a standard 4-h Cr release assay. The graphs are representative of the values of specific lysis at an E:T ratio of 30:1, Bars, Mean of triplicate samples ± SD. B, Dose-dependent reactivity of the MVA peptides with the cell lines in ELISPOT assay. The 1F2 or 3F3 cells were cocultured with autologous BLCL on ELISPOT plates with different dilutions of cognate peptide or VV, VV Ag, or PHA (as positive controls) for 16 h. Graph shows the number of IFN-γ-secreting cells. Bars, Mean of triplicate wells ± SD.

FIGURE 2.

A, 1F2 and 3F3 are HLA-DR1-restricted CD4+ CTL lines. The 1F2 and 3F3 cells were incubated with T2 or T2-DR1 cells pulsed with peptides or infected with VV (as positive control) at different E:T ratios for a standard 4-h Cr release assay. The graphs are representative of the values of specific lysis at an E:T ratio of 30:1, Bars, Mean of triplicate samples ± SD. B, Dose-dependent reactivity of the MVA peptides with the cell lines in ELISPOT assay. The 1F2 or 3F3 cells were cocultured with autologous BLCL on ELISPOT plates with different dilutions of cognate peptide or VV, VV Ag, or PHA (as positive controls) for 16 h. Graph shows the number of IFN-γ-secreting cells. Bars, Mean of triplicate wells ± SD.

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We tested the ability of these CD4+ T cell lines to lyse specific targets after pretreatment with inhibitors of the Fas-FasL and the perforin pathways. The 1F2 and 3F3 effector T cell lines were preincubated with anti-Fas Ab or concanamycin A, an inhibitor of the perforin-mediated pathway. Although inhibition of the Fas pathway had no effect on their killing, pretreatment with concanamycin A significantly decreased CTL activity in a dose-dependent manner, indicating that both CTL lines lyse epitope-specific cells via a perforin-mediated pathway (Fig. 3). The cell lines were stained with anti-perforin Ab for intracellular perforin. However, we did not see any detectable differences between anti-perforin Ab (perforin-FITC kit, clone δG9; BD Biosciences) and the isotype-matched control Ab (data not shown).

FIGURE 3.

Concanamycin A, but not neutralizing anti-FasL Ab, blocks epitope-specific cytotoxicity of 1F2 and 3F3. Autologous BLCL from each donor were VV infected or VV Ag pulsed for 16 h or peptide pulsed for 30 min, then used as targets for 1F2 or 3F3. Cytotoxicity was determined using a 51Cr release assay in the presence or the absence of anti-Fas Ab (50, 10, and 5 μg/ml)- or concanamycin A (100, 50, 20, and 10 nM)-treated CD4+ T cell lines. Assays were performed in triplicate.

FIGURE 3.

Concanamycin A, but not neutralizing anti-FasL Ab, blocks epitope-specific cytotoxicity of 1F2 and 3F3. Autologous BLCL from each donor were VV infected or VV Ag pulsed for 16 h or peptide pulsed for 30 min, then used as targets for 1F2 or 3F3. Cytotoxicity was determined using a 51Cr release assay in the presence or the absence of anti-Fas Ab (50, 10, and 5 μg/ml)- or concanamycin A (100, 50, 20, and 10 nM)-treated CD4+ T cell lines. Assays were performed in triplicate.

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To define the minimal epitope recognized by the 1F2 and 3F3 cell lines, we made a series of truncations of the 21-mer MVA 344 and MVA 302 peptides. A 14-mer peptide, 177WPKFRVVKPNSFTF190, appeared to be the minimal epitope recognized by 1F2, because only 1F2 cells stimulated with T2-DR1 cells pulsed with MVA 344.03 and MVA 344.11 peptides and not MVA 344.04, MVA 344.06, and MVA 344.12 peptides secreted IFN-γ (Fig. 4,A). We also performed ELISPOT assays to determine the minimal epitope for the 3F3 cell line using truncations of the original 21-mer MVA 302 peptide. The data (Fig. 4 B) indicate that both 10-mer peptides, MVA 302.02, 406VFRYMSSEPI415, and MVA 302.03, 407FRYMSSEPII416, were minimal epitopes for the 3F3 cell line. Comparisons of sequences between different members of the poxvirus family show that both epitopes are completely conserved among VV (WR, GenBank accession number NC 006998; Copenhagen, M35027; MVA, U94848; Dryvax, DQ377945, AY313847, and AY313848), variola viruses (India 1967, NC 001611; Bangladesh-1975, L22579; Garcia-1966, Y16780), and most mammalian poxviruses, including monkeypox (Zaire-96-I-16, NC_003310), cowpox (GRI-90, X94355), and ectromelia (Moscow, NC_004105).

FIGURE 4.

The 1F2 (A) or 3F3 (B) cells were used in an ELISPOT assay for mapping of the minimal epitopes with T2-DR1 cells as APC on ELISPOT plates with different peptide deletions of each cognate peptide or PHA (as positive control) for 16 h. Graph shows the number of IFN-γ-secreting cells. Bars, Mean of triplicate wells ± SD. The sequences of the peptides are given below.

FIGURE 4.

The 1F2 (A) or 3F3 (B) cells were used in an ELISPOT assay for mapping of the minimal epitopes with T2-DR1 cells as APC on ELISPOT plates with different peptide deletions of each cognate peptide or PHA (as positive control) for 16 h. Graph shows the number of IFN-γ-secreting cells. Bars, Mean of triplicate wells ± SD. The sequences of the peptides are given below.

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We generated bulk cultures from PBMC derived from three different vaccine recipients, including the donors from whom the cell lines were originally generated. Two different bulk cultures were set up from each donor PBMC and stimulated with VV-infected autologous PBMC and VV Ag-pulsed PBMC. Bulk culture cells from all three donors were tested in a CTL assay at day 28 to determine whether there were any T cells specific to these two epitopes (Fig. 5). In donor A, we found significant lysis (>20%) of MVA 302-pulsed target cells by both the live VV- and VV Ag-stimulated bulk culture, and the lysis of MVA 344 peptide-pulsed targets was 5–8%. With donor B, there was significant killing ranging between specific lysis of 20–40% by the VV Ag-stimulated bulk culture. The specific target cell lysis by VV-stimulated cultures was lower (3–10%). In the third donor, C, we detected higher CTL lysis to both epitopes in VV-stimulated bulk culture (10–25%), and killing by the VV Ag-stimulated bulk culture cells of this donor was low. To determine whether the peptide-specific responses observed were indeed a product of vaccinia immunization, PBMCs obtained from five individuals, including donors A, B, and C, before vaccination were tested for the presence of precursors. Bulk cultures were set up using similar methods, and the cells were tested for VV-, VV Ag-, and cognate peptide-specific CTL lysis. None of the short-term bulk culture lines from the day 0 PBMC had any detectable levels of VV-, VV Ag-, or peptide-specific CTL activity.

FIGURE 5.

VV epitope-specific cytotoxicity was analyzed in short-term bulk cultures. Donor PBMCs were obtained at day 28 (donors A and C) or day 45 (donor B) postvaccination, and short-term bulk lines were generated with VV-infected or VV Ag-pulsed autologous stimulator cells, as described in Materials and Methods. After two rounds of in vitro amplification (28 days of culture), the cultures were analyzed for the ability to lyse autologous BLCL expressing the peptide shown in the figure. Cytotoxicity was plotted, and killing of irrelevant peptide-pulsed targets did not exceed 10%. Spontaneous lysis was <30% in all assays. Data are the mean of triplicate wells of each bulk culture.

FIGURE 5.

VV epitope-specific cytotoxicity was analyzed in short-term bulk cultures. Donor PBMCs were obtained at day 28 (donors A and C) or day 45 (donor B) postvaccination, and short-term bulk lines were generated with VV-infected or VV Ag-pulsed autologous stimulator cells, as described in Materials and Methods. After two rounds of in vitro amplification (28 days of culture), the cultures were analyzed for the ability to lyse autologous BLCL expressing the peptide shown in the figure. Cytotoxicity was plotted, and killing of irrelevant peptide-pulsed targets did not exceed 10%. Spontaneous lysis was <30% in all assays. Data are the mean of triplicate wells of each bulk culture.

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An ICS assay was also performed to determine whether the bulk cultures contain CD3+CD4+ T cell precursors that secrete IFN-γ in response to specific epitope peptides. We tested bulk cultures set up from day 0 (prevaccination bleeds) PBMC for VV-, VV Ag-, or peptide-specific IFN-γ responses, but did not see any discernable precursor frequencies in any of the five donors. Among five vaccinia-immune donors, the postvaccination bulk lines stimulated with live VV (Fig. 6, A and C) or VV Ag (Fig. 6, B and D) from donors C and D had detectable IFN-γ-secreting CD4+ cells in response to VV, VV Ag, and peptides MVA 302 and MVA 344 (Fig. 6), whereas the bulk cultures from the three donors, A and B, after two rounds of in vitro restimulation, and donor E, after one round of in vitro restimulation, showed no responses to these two peptides (data not shown).

FIGURE 6.

ICS assay was performed to determine whether the short-term bulk cultures that generated with VV-infected (rows A and C) or VV Ag-pulsed (rows B and D) autologous stimulator cells contain CD3+CD4+ T cell precursors that secrete IFN-γ in response to VV, VV Ag, and the specific epitope peptides. These FACS plots show the frequency of CD4+ T cells from donor C (rows A and B) and donor E (rows C and D) responding to autologous BLCL cells pulsed with specific peptides for 6 h or untreated; stained for CD3, CD19, CD4, CD8, and IFN-γ; and assessed by flow cytometry. Cells were gated on lymphgate, CD19, CD3+CD8 populations and subsequently analyzed for CD4+ IFN-γ+ cells. Biexponential graphs were plotted to accurately depict all the cells in a gated population.

FIGURE 6.

ICS assay was performed to determine whether the short-term bulk cultures that generated with VV-infected (rows A and C) or VV Ag-pulsed (rows B and D) autologous stimulator cells contain CD3+CD4+ T cell precursors that secrete IFN-γ in response to VV, VV Ag, and the specific epitope peptides. These FACS plots show the frequency of CD4+ T cells from donor C (rows A and B) and donor E (rows C and D) responding to autologous BLCL cells pulsed with specific peptides for 6 h or untreated; stained for CD3, CD19, CD4, CD8, and IFN-γ; and assessed by flow cytometry. Cells were gated on lymphgate, CD19, CD3+CD8 populations and subsequently analyzed for CD4+ IFN-γ+ cells. Biexponential graphs were plotted to accurately depict all the cells in a gated population.

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We identified two HLA-DR1-restricted epitopes by screening cytotoxic CD4+ T cell lines against computer-predicted peptides encoded by the VV genes A24R and D1R, and both epitopes are completely conserved among vaccinia, variola, and monkeypox viruses. To our knowledge these are the first VV-specific cytotoxic CD4+ T cell epitopes restricted by HLA-DR1, one of the common MHC class II alleles. In a recent report, CD4+ T cell responses were demonstrated against four envelope proteins on VV, A27L, B5R, L1R, and A33R (32). The study analyzed three class II-restricted epitopes on A27L defined using overlapping 15-mer peptides, but did not define MHC restrictions of the epitopes, nor are the minimal epitopes outlined. We adopted a different criterion for our screening assays by selecting our peptides based on a HLA-DR1-binding score and not any particular proteins. The prediction algorithm used in this study (L. Stern, J. Calvo-Calle, I. Strug, M. Nastke, S. Baker, and L. Stern, unpublished results) is a combination of two previously approaches, as follows: one is modified from a published algorithm developed by Hammer et al. (51), which predicts HLA-DR1 peptide binding based on inhibition-binding assays of a set of minimal peptides, and one developed by Rammensee et al. (52), which predicts HLA-DR1-restricted Ag processing and presentation based on analysis of naturally processed endogenous peptides. Peptides from MVA open reading frames scoring highly in both algorithms were selected for further analysis. HLA-DR1 was selected for this analysis because it is one of the well-studied human MHC class II alleles. In Caucasoid lineage, average frequency of HLA-DR1 was 9.42% (range of frequency is from 4.50 to 26.00%); in Blacks, 5.46% (0.00–9.20%); and in Orientals, 2.98% (0.00–16.10) (61). Imanishi et al. (62) reported similar frequencies. Considering the promiscuity of HLA-DR-restricted CD4+ T cell epitopes (63, 64, 65) and the presence of DR1 supermotif (66, 67), these epitope peptides may also be presented by HLA-DR molecules other than DR1.

We synthesized 36 21-mer peptides based on the predicted HLA-DR1-binding motifs. Each peptide has a 9-aa-long HLA-DR1-binding motif flanked by 6 aa at each side, which were added in case flanking amino acid sequences would influence the binding to HLA or interaction with TCR. The predicted binding scores for the two peptides identified in our screen are 3.3 (P9 score) and 32 (SYFPEITHI) for MVA 302, and 2.1 (P9) and 32 (SYFPEITHI) for MVA 344, respectively. They are in between the highest (3.8 (P9) or 38 (SYFPEITHI)) and the lowest (1.9 (P9) or 29 (SYFPEITHI)) predicted binders among the 45 predicted epitopes (the range of possible scores for the P9 algorithm is −16 to 23, with positive scores indicating predicted binding, and for the SYFPEITHI algorithm is 0–42, with scores >28 indicating predicted presentation). Measured IC50 values for the MVA 302 and MVA 244 peptides are 37 and 33 nM, respectively, as compared with 12 nM for the tight binding influenza hemagglutinin-derived peptide (68).

The minimal epitope for MVA 344 is a 14 mer and MVA 302 is a 10 mer (Fig. 4). Our results corroborate findings by other studies that the optimal epitope peptides for CD4+ T cells are sometimes longer than the binding motifs and a given T cell can tolerate peptides of variable length and sequence (61).

Several human virus infections, such as HSV, varicella-zoster virus, EBV, CMV, hepatitis B virus, Dengue virus, poliovirus, and HIV, induce CD4+ CTL responses, which may contribute to clearance of virus, as well as producing cytokines (69, 70, 71, 72, 73, 74, 75, 76, 77). In most reports, CD4+ CTL activity has been defined using T cell clones that lyse Ag-expressing cells (78). Direct ex vivo CD4+ CTLs have been described using T cells from patients for HIV (79). Mouse CD4+ T cells specific for lymphocytic choriomeningitis virus were shown to be cytotoxic in vivo (80). Recent reports highlight the evidence for roles played by the effector CD4+ T cells in virus clearance in influenza in mice (81) and by a distinct subset of a mature CD4+ subpopulation in CMV infections in humans (82). It will be interesting to find the role(s) that VV-specific cytotoxic CD4+ T cells play in VV infection.

Both proteins encoding the epitopes described in this study are enzymes involved in mRNA synthesis. A24R is a DNA-dependent RNA polymerase subunit rpo132, and D1R is an mRNA capping enzyme large subunit (D1R). We have observed specific cell lysis of up to 80% of target cells infected with VV, pulsed with VV Ag or peptides by the VV-specific cytotoxic CD4+ T cell lines, 1F2 and 3F3, in vitro cytotoxicity assays suggesting potent cytotoxicity of these cells in vivo (Fig. 1). We characterized the cytolytic mechanism used by the VV-specific cytotoxic CD4+ T cell lines. We found the lysis by these cell lines was inhibited by concanamycin A, an inhibitor of perforin, not by anti-Fas Ab (Fig. 3), although we were not able to detect intracellular perforin in the cell lines; therefore, there is a possibility that concanamycin A may inhibit a pathway other than perforin, which might be involved in cytotoxicity by CD4+ T cells.

Bulk culture cell lines generated from PBMC from three VV-immune donors demonstrated MVA 302- and MVA 344-specific CD4+ CTLs (Fig. 5). Interestingly, VV Ag- and live VV-stimulated bulk cultures performed differently in these donors. In donor C, the bulk culture stimulated with VV Ag had higher cytotoxicity than the bulk culture stimulated with live VV. In donor B, the bulk culture stimulated with live VV had a higher level of cytotoxicity. In donor A, the VV Ag- and live VV-stimulated bulk cultures induced similar levels of cytotoxicity against VV in in vitro CTL assays.

As shown in Fig. 6, among five vaccinia-immune donors, the postvaccination bulk lines stimulated with live VV or VV Ag from two donors had detectable IFN-γ-secreting CD4+ cells in response to VV, VV Ag, and peptides MVA 302 and MVA 344. In both donors’ bulk lines, the sum of the epitope-specific T cell frequencies was higher than the T cell frequencies for whole live virus or viral Ag. We and others reported that total numbers of IFN-γ-secreting cells responding to individual peptides (in these cases the peptides were 9-mer or 10-mer CD8+ T cell epitopes) were higher than the number of IFN-γ-secreting cells responding to whole VV in some human donors’ PBMC (26, 29, 83).

CD4+ T cells can survey for presentation of extracellular proteins by MHC class II molecules. At the same time, class II proteins can present peptides that are derived from endogenous or intracellular proteins. In fact, most peptides that are extracted from class II molecules are derived from endogenous membrane proteins that traffic into exocytic and endocytic pathways (84, 85). Several studies have described class II presentation of endogenous viral Ags (86). Measles virus proteins are presented by TAP-dependent or -independent pathways, although the cytoplasmic matrix protein required high and sustained levels of expression compared with class I presentation (87, 88). Certain epitopes derived from influenza virus membrane proteins were presented in a proteasome- and TAP-dependent class II pathway, whereas other epitopes were presented only as exogenous Ags (89, 90). There may be donor to donor differences in determining which pathway is dominant in presenting VV epitopes to CD4+ T cells.

In this study, we were unable to directly detect MVA 302- and MVA 344-specific CD4+ T cells using IFN-γ ELISPOT assays without in vitro restimulation (data not shown). Because the PBMC samples analyzed in the IFN-γ ELISPOT assays were from either 28 days (donor A and C) or 45 days (donor B, D, and E) after immunization, we probably did not catch the early highest peak of the responses. A relatively low frequency of CD4+ T cells specific for virus is also not unexpected (91, 92, 93). The two HLA-DR1-restricted epitopes described in this work may be useful to monitor and analyze CD4+ T cell responses to the licensed smallpox vaccine or new poxvirus vaccines. To ensure successful vaccination, a candidate vaccine should contain immunodominant CD4+ T cell epitopes as well as CD8+ T and B cell epitopes.

We thank Dr. Alan Rothman for valuable suggestions and critical reading of our manuscript, Dr. Jeff Kennedy for providing some of the human PBMC samples, Pamela Pazoles and Patrick Mulcahy for the assistance with HLA typing, and Marcia Woda for the assistance with the FACS data analysis. Drs. Walter E. Demkowicz, Jr., and Iwona Strug are acknowledged for assistance with peptide selection and characterization. We acknowledge Acambis for providing some PBMC samples from vaccine recipients, and Dr. Thomas Monath for supporting our efforts to define human T cell epitopes in VV.

The authors have no financial conflict of interest.

The costs of publication of this article were defrayed in part by the payment of page charges. This article must therefore be hereby marked advertisement in accordance with 18 U.S.C. Section 1734 solely to indicate this fact.

1

This work was supported by the National Institute of Allergy and Infectious Diseases/National Institutes of Health Grants U19 AI-057319.

3

Abbreviations used in this paper: VV, vaccinia virus; BLCL, B lymphoblastoid cell line; FasL, Fas ligand; ICS, intracellular cytokine staining; moi, multiplicity of infection; MVA, modified vaccinia Ankara.

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