Prediction of HLA-A*02:01 epitopes and synthetic peptides

The prediction of potential HLA-A*02:01 ligands in the T. cruzi TcCA-2 protein was performed by analyzing the deduced amino acid sequence of the TcCA-2 gene (GenBank, CAI strain, accession number M92049.1 and CL Brenner strain, accession number XM813834) following the criteria described by Rammense et al [38]. For the selected epitopes, two in silico HLA-A*02:01 binding prediction algorithms where used, SYFPEITHI to analyze the affinity (www.syfpeithi.de) and BIMAS to calculate the stability (half-life) of the complex (www-bimas.cit.nih.gov). These epitopes presented the lowest scores using the Immune Epitope Database and Analysis Resource (IEDB), where a low score is associated to a high binding affinity (http://tools.immuneepitope.org/main/html/references.html).

Peptides bearing the described HLA-A*02:01 binding motifs were synthesized by simultaneous multiple-peptide solid-phase methods. The peptides were assembled using the standard t-Boc solid-phase-peptide synthesis (SPPS) strategy on a P-metylbenzhydrilamide (MBHA) resin. Purity was checked by high performance liquid chromatography (HPLC), and the correct composition of the peptide was verified by mass spectrometry [39]. Peptides were dissolved to 1 mM final concentration in water containing 10% DMSO and stored at -20°C.

Cell lines

TAP-deficient T2 cells [40] were used for the HLA-A*02:01 binding assays and the K562-A2 cells [41] for the HLA-A*02:01 restriction assay. The cells were cultured in complete RPMI medium supplemented with 10% of inactivated Fetal Calf Serum (iFCS), 2 mM glutamine, and 100 U/ml penicillin. K562-A2 cells, expressing the HLA-A*02:01 molecule were cultured in the presence of 0.5 μg/ml of G-418, as previously described [41]. The T2 and K562-A2 cells were kindly provided by Dr. Pedro Romero (University of Lausanne) and by Dr Peter Ponsaerts (University of Antwerp, with the permission of Dr. Cedrik Britten from Johanes Gutenberg-University Mainz), respectively.

Study populations

For the screening of the recognition of TcCA-2 epitopes by Chagas disease patients, 10 HLA-A*02:01 adult patients in the asymptomatic phase of the disease (IND) were enrolled. For cytotoxicity, functional activity determinations and phenotypic characterization another group of 19 HLA-A*02:01 adults Chagas disease patients and 9 healthy donors were analyzed. These patients were at the chronic stage of the disease and were considered to be at the asymptomatic phase (IND, n = 8) if there was no evidence of having cardiac or gastrointestinal disorders. Chronic Chagas cardiomyopathy patients (CCC, n = 11) were stratified into G1 to G3 stages following Kuschnir classification according to clinical criteria and radiological, electrocardiographic and echocardiography analyses. The number of patients was the one recommended by the Hospital Ethical Committee. The committee suggested that the amount of patients to be included in the study should be the minimal number that provides a statistically significant result. The patients were enrolled in both studies (functional and phenotypic characterization, IND n = 6 and CCC n = 7) when the available number of purified PBMC (limited by the cellular number isolated from each subject) was enough for both analyses. Another four CCC patients had to be enrolled to perform the phenotypic analysis in order to reach statistical significance.

These patients were Spain-residents coming from endemic areas, diagnosed for Chagas disease following WHO criteria using two conventional serological tests (Chagas ELISA, Ortho Clinical Diagnosis and Inmunofluor Chagas, Biocientífica, Argentina) at Hospital Virgen de la Arrixaca (Murcia-Spain), and that had never received treatment for the disease. HLA-A2-0201 patients selection was made at random among those that were positive after serological tests. These patients were clinically characterized in detail. Thirteen mL of blood samples from each patient were collected in EDTA. Peripheral blood mononuclear cells (PBMC) were purified as previously described in [21], stored in iFCS with 10% DMSO and cryopreserved in liquid nitrogen until use. HLA-A genotyping was carried out using the RELI^TM SSO HLA-A Typing kit (Invitrogen).

Ethical considerations

The protocols were approved by the Ethical Committees at Hospital Clínic, Hospital Virgen de la Arrixaca and Consejo Superior de Investigaciones Científicas (Spain). A signed informed consent was obtained from all individuals prior to their inclusion in the study.

HLA-A*02:01 binding assay

HLA-A*02:01 surface stabilization test was carried out as described in [42]. Briefly, TAP-deficient T2 cells were loaded with different concentrations of each peptide, in duplicate in serum-free RPMI medium, and incubated overnight at room temperature. Afterwards, the cells were stained with a PE-labeled HLA-A2-specific antibody (BB7.2 clone, BD biosciences) and analyzed by flow cytometry. The high-affinity HLA-A*02:01-binding peptide HB-ENV_334–342 (WLSLLVPFV) was included as internal standard [43]. Affinity data were calculated as the percentage of maximum complex stabilization, as described in [44]. The following equation was used: % of maximal stabilization = 100 x [(mean fluorescence with peptide)–(background mean fluorescence)]/[(mean fluorescence with 25 μM HBENV_335-343 peptide)–(background mean fluorescence)]. Background value was obtained with cells incubated in the same conditions without peptide [42].

Granzyme B secretion in peripheral blood mononuclear cells from Chagas disease patients

The frequency of Granzyme B (GzB) producing cells was evaluated by ELISPOT assays using cryopreserved PBMC from Chagas disease patients and healthy donors as control. This protocol was carried out as described in [20]. Briefly, 96-well PVDF membrane-bottom plates (Millipore) were pre-wetted with 35% ethanol and washed five times with PBS. Subsequently, plates were coated with 100 μL of anti-GzB (5 μg/mL) monoclonal antibody (Mabtech) and incubated overnight at 4°C. Plates were washed with PBS and incubated with 200 μL/well of blocking solution (RPMI-1640-10% FCS) at room temperature for 30 minutes. Afterwards, 5 × 10⁴ PBMC/well were added and incubated with 1 μM of each peptide for 30 h at 37°C with 5% CO_2, in triplicates. As a positive control, the PBMC were stimulated with 50 ng/ml phorbol 12-myristate 13-acetate (PMA, Sigma) and 500 ng/ml ionomycin (Sigma), or 10 μg/mL of phytohaemaglutinin (PHA, Sigma). Supernatants were harvested and aliquoted at -80°C for subsequent cytokine secretion profile determination. After five washes, 100 μL/well of a 1 μg/mL solution of biotinylated GzB-specific antibody (Mabtech) was added in 0.5% iFCS in PBS, and the plates were incubated for 2 h at room temperature. Wells were extensively washed with PBS and incubated with 100 μL/well streptavidin-alkaline phosphatase (Sigma) at dilution of 1:6000 for 1 h at room temperature. After washing (5x) with PBS, 50 μL/well of substrate solution (NBT-BCIP substrate, Sigma) were added. The wells were incubated for 20–30 min at room temperature in the dark. The reaction was stopped by rinsing the plates with cold tap water. The spots were visualized in an AXIO PLAN 2 Imagine microscope and quantified using KS ELISPOT software. The results are expressed as the number of peptide-induced spots forming cell (SFC) x10⁶ PBMC after subtracting the spot number of peptide un-stimulated PBMCs (basal response). The results were considered positive when a minimum of 20 SFCx10⁶ PBMCs and of at least over twofold basal spot numbers were detected.

Cytokine-secretion tests

Cytokine secretion (IL-4, IL-10, IL-6, IFN-γ, TNF-α) was determined in the supernatants of PBMC from Chagas disease patients and healthy donors, after in vitro stimulation with 1 μM of each peptide for 30 h at 37°C in RPMI supplemented with 10% iFBS as explained before. The secretion profile was determined by using a bead-based multiplex immunoassay system (Bio-Plex, Bio-Rad), following the manufacturer's instructions. The response was considered positive if an increase in the secretion of cytokines was at least three folds higher than the secretion by un-stimulated cells (basal secretion level) and at least, 4 pg/mL for IL-4, 2 pg/mL for IL-10, 15 pg/mL for IL-6 and 5 pg/mL for IFN-γ and TNF-α. The positive control consisted of 50 ng/mL Phorbol 12 myristate 13-acetate (PMA) and 500 ng/mL ionomycin (Sigma). Cytokine levels were quantified in each sample by using the Bio-Plex Manager software 4.1 (Bio-Rad).

In the HLA-A*02:01 restriction assay, peptide-pulsed K562-A2 cells were used as antigen-presenting cells (APC). Plates were seeded with 20,000 peptide-pulsed K562-A2 [41] or K562 cells as a negative control. After washing of non-bound peptide, APC were incubated with 60,000 effector cells per well and the IFN-γ secretion test was performed as mentioned above.

CD8⁺ T cell peptide-specific phenotypic characterization

TcCA-2-specific CD8⁺ T cells were characterized using a HLA-A*02:01 APC-labeled dextramers loaded with the TcCA-2_442-451 and TcCA-2_607-615 peptides, respectively (Immudex). 1X10⁶ PBMCs from 17 HLA-A*02:01⁺ Chagas disease patients and 6 healthy donors were incubated with 10μL of each dextramer in 40μL of 5% FCS in PBS for10 min at RT in the dark. Afterwards, these cells were incubated 20 min at 4°C with different cocktails of antibodies (BD Pharmigen): CD8-V500, CD8 PerCP-Cy5.5, CD45RA-APC-H7, CCR7-V450, CD27-FITC, CD127-PerCp-Cy5, CD57-FITC and CD44RA-APC. The labeled cells were washed twice with PBS-5% FCS and resuspended in 400 μL of PBS 1X. Data were acquired in a FacsAria III Cell Sorter and analyzed using Flowjo 7.6.5 software (Bio-Rad). At least 100.000 PBMC cells were acquired according to FCS/SSC parameters. The gating strategy is shown in Fig. 1.

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Fig 1. Phenotypic characterization of TcCA-2-specific CD8⁺ T cells.

The dot plots show the lymphocyte gating based on forward-scatter (FSC) and side-scatter (SSC) properties (A), CD8⁺ T cell population (B1-C1) and the percentage of TcCA-2-specific CD8⁺ T cells (B2-C2) from a healthy control subject (B) and from chagasic disease patient (C) respectively. The phenotypic analyses of TcCA-2-specific CD8⁺ T cells, defined by CD45RA, CCR7, CD27, CD127, CD44 and CD57 expression (D-I) allowed to identify naive (CD45RA⁺CD27⁺CCR7⁺) and terminal effector memory (T_EMRA, CD45RA⁺CD27^-CCR7^-) TcCA-2-specific CD8 T cells (E), central memory (T_CM, CD45RA^-CD27⁺CCR7⁺) and effector memory (T_EM, CD45RA^-CD27^-CCR7^-) TcCA-2-specific CD8⁺ T cells (F), early-stage differentiation (T_ED, CD45RA^-CD127⁺) and advanced-stage differentiation (T_TD, CD8⁺CD45RA⁺CD127^-) TcCA-2-specific CD8⁺ T cells (G), senescent memory (CD44⁺CD57⁺) and non-senescent memory (CD44⁺CD57^-) TcCA-2-specific CD8 T cells (H) and CD27 expression in TcCA-2-specific CD8⁺T cells (I). Gates were established based on the control isotypes corresponding to each antibody. Non-stained cells and mononuclear cells incubated with antibodies but not with dextramers were used as reference to define the cut-off for each specific dextramer labeling.

https://doi.org/10.1371/journal.pone.0122115.g001

Statistical analysis

The statistical analysis was performed using Prism V5.0 (GraphPad Software, La Jolla, CA, USA). Nonparametric test were used to test for statistical significance. Comparison between asymptomatic and cardiac Chagas disease patients within the same cell subpopulation was evaluated by the Mann-Whitney U test (pairwise comparisons). In addition, Kruskal—Wallis test with Dunn correction was used to identify groups of cellular subpopulations or more than two groups of subjects (ANOVA for comparisons among ˃ 2 groups). Statistical significance was assigned at a value of p ≤ 0.05.

Selection of HLA-A*02:01-binding peptides within T. cruzi TcCA-2 protein

In order to identify peptides containing potential HLA-A*02:01-binding sites, the deduced amino acid sequence of T. cruzi TcCA-2 was screened following the criteria described by Rammense et al [38] and using two computer algorithms. The SYFPEITHI and (IEDB) algorithms were employed to analyze binding affinity of the peptides to MHCI HLA-A*02:01 and the BIMAS to analyze the stability of the preformed complex. Eight peptides presented mid-to-high affinity score for HLA-A*02:01 (Table 1) and were consequently synthesized. All these peptides presented a low percentile rank score using the Immune Epitope Database and Analysis Resource (IEDB), which is associated to a high binding affinity (Table 1).

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Table 1. Sequences of the TcCA-2-derived HLA-A*02:01 binding peptides.

https://doi.org/10.1371/journal.pone.0122115.t001

The percentage of maximal binding stabilization of these eight TcCA-2 peptides was evaluated using TAP-deficient T2 cells and different concentrations of each peptide. The experimental results were referred with the fluorescence index values obtained with the HB-ENV_335–343 peptide as it has been previously shown that this peptide has a high binding affinity to HLA-A*02:01 MHC I [43]. The maximal binding affinity is shown for each peptide in Table 1.

Detection of CD8⁺ T lymphocytes specific for HLA-A*02:01⁺

In order to analyze whether the Chagas disease patients CD8⁺ T cells recognize the TcCA-2-derived peptides in the context of the HLA-A*02:01⁺ molecule, peptide-pulsed K562-A2 cells were used as APC in a multiplex immunoassay for detection of IFNγ secretion (Table 2). PBMC from HLA-A*02:01⁺ asymptomatic Chagas disease patients (IND) recognized four TcCA-2 epitopes (TcCA-2_657-666, TcCA-2_442-451, TcCA-2_607-615 and TcCA-2_273-281) while being presented on K562-A2 but not on K562 cells, which do not express Class I molecules. Two out of 9 patients responded to the TcCA-2_657-666 peptide, 2 out of 10 to the TcCA-2_442-451 peptide, 3 out of 9 to the TcCA-2_607-615 peptide and 1 out of 10 to TcCA-2_273-281.

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Table 2. Recognition of TcCA-2 epitopes by HLA-A*02:01 Chagas disease patients.

https://doi.org/10.1371/journal.pone.0122115.t002

The cytotoxic activity of the CD8⁺ T cells specific for these four TcCA-2-derived epitopes was evaluated by secretion of GzB through ELISPOT assays. Thus, PBMC from 15 HLA-A*02:01 chagasic patients (8 IND and 7 CCC) and 9 healthy donors were incubated with the peptides under study. A positive GzB response was detected in 3 patients (2 IND and 1 CCC) out of 10 in response to incubation with the TcCA-2_657-666 peptide, 5 patients (3 IND and 2 CCC) out of 14 in response to the TcCA-2_442-451 peptide, 3 patients (3 CCC) out of 14 in response to the TcCA-2_607-615 peptide and 2 patients (2 IND) out of 11 in response to the TcCA-2_273-281 peptide (Table 3). Cytotoxic activities were not detected in any healthy donor.

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Table 3. Cytokine-secretion and Granzyme B response to TcCA-2 epitopes by PBMCs from HLA-A*02:01 Chagas disease patients and healthy donors.

https://doi.org/10.1371/journal.pone.0122115.t003

Functional analysis of the epitope-specific CD8⁺ T cells was carried out by the determination of the secretion profile of IFN-γ, TNF-α, IL-4, IL10 and IL-6 cytokines. The results, presented in Table 3, show that CD8⁺ T cells from 2 out of 14 patients recognized peptides TcCA-2_442-451 by secreting IFN-γ, TNF-α and IL-6 and 2 out of 14 by secreting TNF-α and IL-6. The TcCA-2_607-615 peptide was recognized by 2 out of the 14 patients cells, by secreting IFN-γ, TNF-α and IL-6, 1 out 14 by secreting TNF-α and IL-6 and 1 out 14 by secreting IL6. CD8⁺ T cells from 2 out of 11 patients responded to stimulation with peptide TcCA-2_273-281 by secreting IL-6. Any production of cytokines was detected after stimulation with the TcCA-2_657-666 peptide. There was no secretion of IL-4 and IL-10 in PBMC after stimulation with any one of the four TcCA-2 peptides (data not shown). IFN-γ, TNF-α and IL6 cytokines secretion levels were higher in patients at the asymptomatic phase of the disease than in Chagas patients with associated cardiomyopathy.

Phenotypic characterization of T CD8⁺ lymphocytes specific for TcCA-2 derived peptides

After having shown the lymphocyte activation capacity of TcCA-2-derived epitopes (TcCA-2_657-666, TcCA-2_442-451, TcCA-2_607-615, and TcCA-2_273-281) we decided to phenotypically characterize, the specific CD8⁺ T lymphocytes that recognized the two peptides that exhibited the greatest recognition by specific CD8⁺ T cells (TcCA-2_442-451 and TcCA-2_607-615) (scheme in Material and Methods Section, Fig. 1). With that aim, mononuclear cells from Chagas patients in different phase of the disease (IND, n = 6 and CCC, n = 11) as well as from healthy donors (HD, n = 6) were incubated with HLA-A*02:01 APC-labeled dextramers loaded with the TcCA-2_442-451 and-TcCA-2_607-615 peptides. As shown in Fig. 2A, the percentage of total CD8⁺ T lymphocyte in the PBMC gate was significantly higher in asymptomatic Chagas disease patients (IND) than in healthy donors (p≤0.05). In addition, we observed that IND and CCC Chagas disease patients had a higher percentage of TcCA-2_442-451 and TcCA-2_607-615 specific CD8⁺ T cells than healthy individuals (p≤0.05 and p≤0.01) (Fig. 2B).

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Fig 2. TcCA-2_442-451 and TcCA-2_607-615 CD8⁺ specific T cells.

(A), percentage of CD8⁺ T cells in the PBMC region (see Fig. 1C1). (B), peptide-specific cells of total CD8⁺ T cells. Cell subpopulations were determined by flow cytometry in 6 healthy donors (HD), 6 patients in the asymptomatic phase (IND) and 11 patients in the cardiac phase (CCC). Median values are represented by horizontal lines. Error bars represent standard deviation intervals. Statistical analyses were carried out using Kruskal—Wallis test with Dunn correction (*). Statistically significant differences are indicated ⁽*⁾ p≤0.05, ⁽**⁾ p≤0.01, ⁽***⁾ p≤ 0.001.

https://doi.org/10.1371/journal.pone.0122115.g002

Labeling, using antibodies against CD45RA, CD27 and CCR7 molecules, allowed us to phenotypically characterize TcCA-2_442-451 and TcCA-2_607-615-specific CD8⁺ T cells from patients at different phases of the disease (IND and CCC). Thus, as shown in Fig. 3A₁ we observed that the TcCA-2_442-451-specific CD8⁺ T cells from IND patients have a higher percentage of cells expressing the T_NAIVE phenotype (CD45RA⁺CD27⁺CCR7⁺) than the cells from CCC patients (p≤0.01). However, the percentage of terminal effector memory CD8⁺ T cells (T_EMRA cells, CD45RA⁺CD27^-CCR7^-) was significantly lower in IND patients than in CCC (p≤0.05) (Fig. 3A₁). Moreover, the TcCA-2_442-451-specific CD8⁺ T cells from CCC patients have a higher percentage of T_EMRA cells than that having a phenotype T_NAIVE (p≤0.05). Regarding the TcCA-2_607-615-specific CD8⁺ T cells, the percentage of cells expressing CD45RA⁺CD27⁺CCR7⁺ (T_NAIVE) was also significantly higher in IND versus CCC patients (p≤0.01) (Fig. 3B₁). The percentage of T_EM is higher in CCC patients than that in IND patients (p≤0.05). Moreover, the percentage of T_EM versus of T_CM cells is also higher in CCC patients than that in IND patients (p≤0.05). In fact, the TcCA-2_607-615-specific CD8⁺ T cells from CCC patients had mainly an effector phenotype showing a predominant profile of T_EM cells versus of T_CM cells (p≤0.05) (Fig. 3B₁). By combining the CD45RA and CD127 surface markers it was observed (Fig. 3A₂ and 3B₂) that both IND and CCC patients have a higher percentage of TcCA-2_442-451 and TcCA-2_607-615—specific CD8⁺ T cells at an advanced-stage differentiation (T_TD, CD45RA⁺CD127^-) phenotype than at an early-stage differentiation (T_ED, CD45RA^-CD127⁺) phenotype (p≤0.01).

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Fig 3. Immunophenotyping of memory and differentiation status of the specific CD8⁺ T cells in patients with Chagas disease.

(A) TcCA-2_442-451 peptide. (B) TcCA-2_607-615 peptide. PBMCs from 6 asymptomatic form patients (IND) and 11 patients with the cardiac form (CCC) were stained for CD45RA, CD27 and CCR7 and analyzed by flow cytometry. According to the combination of antibodies used the CD8 peptide-specific cells were divided in: T_NAIVE (CD8⁺CD45RA⁺CD27⁺CCR7⁺), T_EMRA (CD8⁺CD45RA⁺CD27^-CCR7^-), T_CM (CD8⁺CD45RA^-CD27⁺CCR7⁺), T_EM (CD8⁺CD45RA^-CD27^-CCR7^-), T_ED (CD8⁺CD45RA^-CD127⁺), T_TD (CD8⁺CD45RA⁺CD127^-). Median values are represented by horizontal lines. Error bars represent standard deviation intervals. Statistical analyses were carried out using Mann-Whitney U test (#) and Kruskal—Wallis test with Dunn correction (*). Statistically significant differences are indicated ^(#) or ⁽*⁾ p≤0.05, ^{(# #)} or ⁽**⁾ p≤0.01, ^{(# # #)} or ⁽***⁾ p≤ 0.001.

https://doi.org/10.1371/journal.pone.0122115.g003

Since the CD57 expression is associated with replicative senescence we evaluated the CD57 expression in CD44⁺ cells (marker of antigen-experience T cells) of both TcCA-2_442-451 and TcCA-2_607-615-specific T CD8⁺ cells. The results shown in Fig. 4A and 4B indicate that in IND patients the predominant phenotype is of non-senescent memory cells (CD44⁺CD57^-, p≤0.001) and that the percentage of circulating senescent memory cells (CD44⁺CD57⁺) specific for both epitopes is significantly higher in CCC patients than that in IND patients (p≤0.01).

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Fig 4. Expression of the senescence marker CD57 in antigen-experienced specific CD8⁺ T cells.

(A) TcCA-2_442-451-specific T cells. (B) TcCA-2_607-61-specific T cells. Cells from 6 patients in asymptomatic phase (IND) and 11 patients with the cardiac form (CCC) were analyzed. Median values are represented by horizontal lines. Error bars represent standard deviation intervals. Statistical analyses were carried out using Mann-Whitney U test (#) and Kruskal—Wallis test with Dunn correction (*). Statistically significant differences are indicated ^(#) or ⁽*⁾ p≤0.05, ^{(# #)} or ⁽**⁾ p≤0.01, ^{(# # #)} or ⁽***⁾ p≤ 0.001.

https://doi.org/10.1371/journal.pone.0122115.g004