Full text

Turn on search term navigation

About the Authors:

Gonzalo R. Acevedo

Affiliation: Instituto de Investigaciones en Ingeniería Genética y Biología Molecular “Héctor N. Torres” (INGEBI), Consejo Nacional de Investigaciones Científicas y Tecnológicas (CONICET), Buenos Aires, Argentina

Silvia A. Longhi

Affiliation: Instituto de Investigaciones en Ingeniería Genética y Biología Molecular “Héctor N. Torres” (INGEBI), Consejo Nacional de Investigaciones Científicas y Tecnológicas (CONICET), Buenos Aires, Argentina

Alcinette Bunying

Affiliation: Torrey Pines Institute for Molecular Studies (TPIMS), San Diego, California, United States of America

Nazila Sabri

Affiliation: Torrey Pines Institute for Molecular Studies (TPIMS), San Diego, California, United States of America

Augusto Atienza

Affiliation: Hospital General de Agudos J.M. Ramos Mejia, Buenos Aires, Argentina

María P. Zago

Affiliation: Instituto de Patología Experimental (IPE-UNSA), Salta, Argentina

Radleigh Santos

Affiliation: Torrey Pines Institute for Molecular Studies (TPIMS), Port St. Lucie, Florida, United States of America

Valeria A. Judkowski

Contributed equally to this work with: Valeria A. Judkowski, Clemencia Pinilla, Karina A. Gómez

Affiliation: Torrey Pines Institute for Molecular Studies (TPIMS), San Diego, California, United States of America

Clemencia Pinilla

Contributed equally to this work with: Valeria A. Judkowski, Clemencia Pinilla, Karina A. Gómez

Affiliation: Torrey Pines Institute for Molecular Studies (TPIMS), San Diego, California, United States of America

Karina A. Gómez

Contributed equally to this work with: Valeria A. Judkowski, Clemencia Pinilla, Karina A. Gómez

* E-mail: [email protected]

Affiliation: Torrey Pines Institute for Molecular Studies (TPIMS), San Diego, California, United States of America

ORCID http://orcid.org/0000-0001-8115-667X

Introduction

Antigen specific CD4+ and CD8+ T cells are key components of the immune response developed by chronic patients infected with Trypanosoma cruzi, the causative agent of human Chagas disease. Based upon observations in human infection and in experimental models, it is currently accepted that T cells play an important role not only in controlling parasite burden but also modulating disease progression [1–3]. During the chronic phase of the disease, in its asymptomatic or cardiac manifestation forms, CD8+ T cells are believed to be involved in both parasite control and in tissue damage, which contributes to cardiac alterations. This dual action could be attributed to the existence of distinct populations of these cells that shift their functional profile during the course of Chagas disease. In fact, asymptomatic patients have a higher frequency of specific interferon-γ (IFN-γ) producing CD8+ T lymphocytes than people with severe cardiac symptoms [1,4]. Furthermore, as a consequence of decades of low but continuous antigen exposure, in human T. cruzi infection, CD8+ T cells are driven to exhaustion, leading to progressive impairment of their effector function [1,5–7].

On the other hand, CD4+ T cells and monocytes/macrophages participate in the secretion of both inflammatory and anti-inflammatory cytokines, and this release correlates with the clinical outcome of the disease [2,3]. In general, peripheral blood mononuclear cells (PBMC) from cardiac chagasic patients produce more IFN-γ and less IL-10 than do those from asymptomatic patients [8–10]. Accordingly, the majority of recombinant T. cruzi proteins or total lysate induce a Th1 type cytokine profile (IFN-γ, TNF-α) with suppression of Th2 type cytokines (IL-4, IL-10) in cardiac patients [11–18]. However, we recently demonstrated that this is not true for the immune response developed by T. cruzi ribosomal P proteins, since the cytokines released upon their stimulation made it difficult to determine a specific Th cell phenotype [18].

Although significant information has been obtained by studying activation markers and cytokines secreted by CD4+ and CD8+ T cells during T. cruzi infection [3], knowledge about the fine specificity of these cells is restricted to a few parasite epitopes. Most of these are peptides from proteins belonging to the trans-sialidase family, like TS, ASP-1, ASP-2 [19–21]. Some other examples are comprised within the sequences of cruzipain, MASP, KPM-11, Tc24 or hypothetical proteins TcG1, TcG2 and TcG4 [22–27]. The study of T cell repertoire in protozoan parasitic infections is notably dissimilar from those of viruses and bacteria, in that their large genomes and the complexity of their proteomes hamper the finding of relevant epitopes. In the particular case of T. cruzi, its haploid genome encodes more than 12,000 genes [28], providing thousands of potential epitopes that could bind to the class I and class II major histocompatibility complex (MHC) molecules and be presented on the surface of infected host cells or antigen presenting cells.

The study of pathogen specific human T cells is difficult due to their low frequency in PBMC samples, approximately 1 in 105 cells in bulk cell population [29]. The potentially large ratio of non-specific to specific cells, together with the protocol used for T cell expansion could result in the selection of T cell populations different from the ones of interest in terms of specificity, phenotype or function. More importantly, the effects of extended long-term in vitro culture on T cell phenotype and function may therefore hinder the correlation of many T cell clonal attributes with real in vivo characteristics [30].

As part of our ongoing studies to identify parasite epitopes recognized by human T cells in the context of chronic Chagas disease, we decided to optimize the culture conditions of PBMC from asymptomatic and cardiac patients in order to enable a maximum yield of T. cruzi-specific T cells. In the present work, we analyzed the effect of different time lengths of initial T. cruzi lysate stimulation, the number of PHA expansions and the usefulness of Epstein-Barr virus (EBV)-transformed human B lymphocytes (B-LCL) as autologous antigen presenting cells, in a small cohort of chagasic patients and non-infected donors. In addition, we generated clones of memory CD4+ T cells from an asymptomatic patient that recognize the epimastigote and trypomastigote/amastigote forms of the parasite.

Materials and methods

Ethics statement

The research followed the tenets of the Declaration of Helsinki and of the Medical Ethics Committee of the Hospital General de Agudos J.M. Ramos Mejia, which approved the protocols used in this study. All enrolled patients were of age at the time the sample was taken, and they gave written informed consent, according to the Hospital’s Ethics Committee guidelines, before blood collection and after the nature of the study was explained.

Study population

Patient selection was conducted at the Cardiovascular Division of the Hospital General de Agudos J.M. Ramos Mejia, Buenos Aires, Argentina. The study population consisted of 11 patients with positive serology for Chagas disease, determined by two or more tests (indirect immunofluorescence, ELISA, indirect hemagglutination). The patients, in the chronic phase of the infection, underwent a complete clinical and cardiological examination and were classified as asymptomatic (without demonstrable pathology) or cardiac patients. Five non-T. cruzi infected individuals with negative serological tests for Chagas disease were included as the control group.

Parasite lysate

Whole antigenic lysate from T. cruzi epimastigote was prepared from axenic cultures (CL Brenner strain) in LIT medium, as previously described [18]. After lysis, the suspension was filter sterilized through a 0.2 μm pore-size membrane, aliquoted, and stored at -80°C until use. Trypomastigote/amastigote form lysate was similarly prepared and sterilized, from T. cruzi Sylvio infected C2C12 cells (MOI 3:1) supernatants. Lysate composition was typically 52–54% trypomastigotes, 46–48% amastigotes (percentages calculated on absolute parasites numbers).

PBMC isolation

PBMCs were obtained from whole blood by Ficoll-Hypaque density gradient centrifugation (GE Healthcare Bio-Sciences AB, Uppsala, Sweden) according to manufacturer’s instructions, less than 4 h after collection in EDTA-anticoagulated tubes. Cells were resuspended in T cell medium (RPMI-1640 medium, 100 U/ml penicillin, 100 μg/ml streptomycin, 2 mM L-glutamine and 5% heat-inactivated male AB Rh-positive human serum (HS; Sigma, St Louis, MO, USA)) and directly used in experiment, or in fetal calf serum (FCS; Natocor, Córdoba, Argentina) containing 10% dimethylsulfoxide (DMSO), and cryopreserved in liquid nitrogen.

Generation and antigen priming of Epstein-Barr immortalized B cell lines

Autologous lymphoblastoid B cell lines (B-LCL) were generated for each patient, following an adapted version of a protocol described elsewhere [31]. Briefly, Epstein-Barr virus (EBV) suspension was prepared from B95.8 marmoset lymphoid cells culture supernatant, by centrifugation for 10 min at 300 ×g, 4°C, and filtration through 0.45 μm pore size membrane filter. The resulting virus-containing supernatants were preserved at -80°C until use. For immortalization, 107 PBMC were incubated with 1.25 ml of EBV suspension in a final volume of 5 ml LCL medium (RPMI-1640 supplemented with 100 U/ml penicillin, 100 μg/ml streptomycin, 2 mM L-glutamine and 10% FCS), for 2 h at 37°C. Then, 5 ml of the same medium containing cyclosporine A (Sigma, St Louis, MO, USA) at a final concentration of 1 μg/ml were added, and incubation was continued for 3 weeks. Immortalization success was evaluated during this period by monitoring cultures for cell clumps formation. After this, cells were characterized by flow cytometry, using PE-Cy5-conjugated anti-CD19 and FITC-conjugated anti-CD3 antibodies (BD Biosciences, San Diego, CA, USA.) Immortalized B cell lines (B-LCL) were further expanded in LCL medium without cyclosporine A and cryopreserved in FCS with 10% DMSO, in liquid nitrogen.

For antigen priming, B-LCL were cultured in low serum content LCL medium (RPMI 1640, 2% FCS, 100 U/ml penicillin, 100 μg/ml streptomycin, 2 mM L-glutamine) at a density of 0.5–1.0×106 cells/ml, for 24 h, then washed by centrifugation for 10 min at 400 ×g in 1.5 ml PBS and incubated with 10 μg/ml T. cruzi lysate, either for 3 h or overnight, before irradiation.

PBMC stimulation and culture

For initial antigen stimulation, freshly isolated or cryopreserved PBMC from each subject were seeded in 96-well U-bottom plates and cultured in T cell medium with 2.5 μg/ml T. cruzi lysate (concentration was chosen based on titration experiments [18]). Non-specific stimulation with 5 μg/ml phytohaemagglutinin (PHA, Sigma, St Louis, MO, USA) was used as positive control condition. The presence of clear signs of cellular proliferation (increase in the cell number and clustering) was evaluated as evidence of normal physiological state of the cells at the beginning of the culture process. Similarly, negative control wells were seeded and left unstimulated, exhibiting no signs of cellular proliferation or activation.

Starting at indicated times after antigen stimulation, recombinant human interleukin-2 (IL-2; Peprotech, Mexico DF, Mexico) was added every 3 to 4 days at a final concentration of 50 IU/ml.

Memory CD4+ T cells separation, stimulation and culture

CD4+CD45RO+ T cells were isolated from PBMC using the immunomagnetic negative selection EasySep Human Memory CD4+ T Cell Enrichment Kit and Magnet (StemCell Technologies, Vancouver, Canada), following manufacturer provided indications. Recovery (40.9±14.1%) and purity (93.6±1.2%) of the enriched population was assessed by flow cytometry, staining with PE-Cy7 anti-CD4 (BioLegend, San Diego, CA, USA), FITC anti-CD3, PE-Cy5 anti-CD8, APC anti-CD45RA and PE anti-CD45RO (BD Biosciences, San Diego, CA, USA) antibodies.

For initial stimulation, memory CD4+ T cells were seeded in 96-well plates, in T cell medium, at 5×103 cells/well and incubated with 104 autologous irradiated PBMC and 2.5 μg/ml T. cruzi epimastigote lysate, or at 103 cells/well and incubated with 104 allogeneic irradiated PBMC from 3 non-related, non-infected donors, 1 μg/ml PHA and 50 IU/ml IL-2. This interleukin was also added on every culture since day 3, every 3 to 4 days, at a final concentration of 50 IU/ml. Half the medium (100 μl/well) was refreshed every 10 to 14 days, beginning at day 15.

PHA expansion

For non-antigen specific expansion, cells were stimulated with 1.0 μg/ml PHA and 50 IU/ml IL-2, in the presence of 2.5×104 irradiated (4,000 rads) allogeneic PBMC/well from 3 non-infected, non-related donors. Control cultures were carried out in parallel by seeding 16–48 wells with irradiated allogeneic cells only.

T. cruzi antigen specificity evaluation

Each culture was tested for their response to T. cruzi proteins in the presence of antigen presenting cells (APC). Briefly, a fraction of the cells were transferred to a new 96-well plate and cultured in T cell medium, with 2.5 μg/ml T. cruzi lysate or no antigen. As APC, irradiated autologous PBMC (4,000 rads) or irradiated autologous, antigen-primed B-LCL (10,000 rads) were used.

After 18 h, supernatants were collected for the quantification of IFN-γ and GM-CSF production (OptEIA Human IFN-γ and Human GM-CSF ELISA sets, BD Pharmingen, San Diego, CA, USA). Subtracted medium was replaced with T cell medium and cells were pulsed for 24 h with 0.5 μCi/well [methyl-3H]-thymidine (Perkin Elmer, Waltham, MA, USA). Proliferation was measured as incorporated radioactivity, assessed by liquid scintillation counting.

Limiting dilution assay (LDA)

T cells were plated in 96-well plates, at densities of 10, 3, 1 and 0.3 cells/well, and PHA expansion was carried out, as described above. IL-2 was added every 3 to 4 days at 50 IU/ml. After 2 or 3 subsequent PHA expansions, spaced by 2 to 3 weeks and depending on cell growth, aliquots of these cultures were evaluated for T. cruzi antigens specificity. Based on this, parasite specific cultures which grew to large enough numbers were characterized for TCR-Vβ expression by flow cytometry (see below).

TCR-Vβ flow cytometry staining

TCR-Vβ repertoire was analyzed by flow cytometry, using the IOTest Beta Mark Kit (Beckman-Coulter, USA) to stain 5×105 cells/tube, and following manufacturer’s instructions for the staining protocol. CD3 and CD4 expression was also assessed for the same samples, as described for memory CD4+ T cells.

Results

Impact of different culture conditions on the in vitro expansion and functionality of parasite specific T cells

With the aim of expanding T. cruzi specific T cell populations from Chagas disease patients’ PBMC, different culture conditions were tested (Fig 1A).

[Figure omitted. See PDF.]

Fig 1. Effect of initial stimulation time and PHA expansions on in vitro T cell response against T. cruzi lysate.

PBMC were stimulated and expanded, and aliquots of 1.0–2.0×104 T cells from these cultures were evaluated for T. cruzi antigens specificity, using 2.0–4.0×104 autologous irradiated PBMC as APC. Response was measured as IFN-γ secretion and proliferation. Stimulatory index (SI) was calculated for each culture well as the response against T. cruzi lysate divided by the cells baseline response (media only condition). Cultures considered positive were those with an SI≥2 (dotted line). Scatter plots show individual well SI values. Bars represent the percentage of positive wells among the total wells analyzed for each subject. The numbers of positive vs total studied wells is indicated above the bars. Color codes indicate which group each subject belongs to: chronic Chagas cardiopathy (red, subjects RM11, RM14 and RM25), asymptomatic Chagas disease (blue, subjects RM20 and RM26) or non-infected (green, subjects FI, MF and MM). A. Timeline representation of stimulation and specificity evaluations protocols. Numbers in brackets next to symbols indicate the day (or range of days, when slight variations were required between subjects due to cell growth differences) since protocol start at which each step was performed. Numbers under the ‘initial stimulation’ indicator (grey block) refer to the duration of the stimulus. B. Percentage of positive wells for at least one of the readouts in each subject’s cultures when PBMC were initially stimulated for 6 days with T. cruzi lysate. IL-2 was added every 3–4 days since day 6 post initial stimulation. Specificity evaluation was performed between days 64–71 after initial stimulation, and after 2 PHA expansions. C. Wells response by readout for each subject, in the same experiment as B. D. T. cruzi-specific response in cultures derived from two Chagas disease patients and one non-infected subject. Cells were stimulated with T. cruzi lysate for 1 day, and challenged at day 27 after one PHA expansion (“1st challenge”) or at day 47 after two PHA expansions (“2nd challenge”). IL-2 was added since day 9, and every 3–4 days. E. Paired IFN-γ secretion and proliferation parasite-specific responses for each well, on 1st and 2nd challenges, from the same experiment as D. Values are expressed as SI. Statistical analysis for the percentages of positive wells shown in panels B and C are detailed in S1 Table, and for panel D in S2 Table.

https://doi.org/10.1371/journal.pone.0178380.g001

Overall, the protocol consisted in an initial stimulation with T. cruzi lysate to selectively amplify the cells of interest and subsequent expansions with PHA, IL-2 and irradiated allogeneic feeder cells to increase cell numbers. To assess the success of this procedure, cells were challenged with T. cruzi lysate and the response was evaluated by two different readouts, IFN-γ secretion and proliferation. Based on previous findings [18,32], we tested 6 days as initial stimulation time in cultures from cardiac (RM11 and RM14) and asymptomatic (RM20) patients. Two non-infected individuals (FI and MF) were included as controls. As shown in Fig 1B, cultures from infected patients showed 43.9–53.8% positive wells, clearly suggesting the expansion of parasite specific T cells. Under the same conditions, a substantial number of positive wells were detected in cultures from non-infected individuals, in percentages ranging between 9.5–25.3% of the seeded wells (Fig 1B and 1C). However, the values obtained for the infected subjects were significantly higher (S1 Table).

Given that the response detected in cultures from non-infected subjects could be associated with undesired in vitro activation and amplification of naïve T cells, a following experiment was carried out using a 1-day initial stimulation. This modification led to a reduction in the percentage of positive wells from a non-infected donor’s cells (MM), but affecting the reactivity of cultures from asymptomatic patient RM26 and cardiac patient RM25 as well (Fig 1D). Overall, these results suggest that a shorter initial T. cruzi lysate stimulation period (1 day) leads to a lower in vitro activation of cell populations responsive to parasite antigens, which could involve naïve, in vitro activated T cells, but also memory, specific T cells.

Aiming to address how PHA expansion cycles impacts on T. cruzi specific T cells enrichment and their functional profile and capability, antigen specificity evaluations were performed after 27 days of culture and 1 PHA expansion (“1st challenge”), or after 47 days of culture and 2 PHA expansions (“2nd challenge”, Fig 1D and 1E). In terms of IFN-γ secretion, specific response was observed only for the asymptomatic chronic Chagas patient RM26. For this subject, as shown in Fig 1D, the percentage of positive wells increased after two rounds of PHA expansion, but the overall SI levels were lower, as compared with the values obtained after a single PHA expansion. On the other hand, a smaller percentage of proliferation positive wells, but higher SI values, were observed for both chronic Chagas patients after two PHA expansions. However, for the non-infected subject, positive wells rose from 2.0% after one round, to 10.1% after two rounds of PHA expansion, suggesting that several non-antigen specific stimulations might favor the undesired amplification of T cells that are indeed not related to infection.

Interestingly, many of the wells that responded on the 1st challenge became negative on the 2nd and vice versa, for both proliferation and IFN-γ secretion, as plotted on Fig 1E. No wells switched from IFN-γ positive to proliferation positive, while 5.0% of the RM26 wells switched from proliferation positive to IFN-γ positive. Of these, only 1.0% (on total seeded wells) remained responsive by IFN-γ secretion while gaining proliferative responsiveness (data not shown). Wells from neither the cardiac patient nor the non-infected individual exhibited this behavior.

Overall, these results show that changing the conditions of the initial T. cruzi stimulation and subsequent PHA expansion has an evident impact on the in vitro amplification of T. cruzi specific cells. Furthermore, the data obtained with non-infected individuals indicate that there is a significant and sizeable population of either naïve T cells, or memory T cells with a different specificity, but cross-reactive to T. cruzi antigens, that can be expanded in vitro under these culture conditions.

Autologous immortalized B-cells as antigen presenting cells of T. cruzi lysate to T cell cultures

Due to the limited availability of patients’ PBMC, another important factor to consider when developing T cell lines and clones for using in antigen discovery research is which cells are to be used as antigen presenting cells. In order to assess the capability of autologous Epstein-Barr virus-immortalized B cells (B-LCL) to present T. cruzi antigens in specificity evaluation experiments, T cell culture protocols were carried out (Fig 2A), emulating stimulation and culture conditions from experiments in Fig 1. To load the B-LCL, two different antigen priming conditions were tested (3 h and overnight) by pre-incubating these cells with the lysate at a concentration of 10 μg/ml, prior to the challenge experiment.

[Figure omitted. See PDF.]

Fig 2. Use of autologous Epstein-Barr immortalized B-cells as antigen presenting cells.

PBMC from three cardiac patients, three asymptomatic patients and two non-infected individuals were seeded in two wells of 96-well plates at 2×105 cells/well. Three different protocols (namely A, B and C) were used. IL-2 was added every 3–4 days after the indicated time. At day 27 post-stimulation, cells from each condition were pooled and 2×103 T cells from each of these cultures were challenged with T. cruzi lysate or culture media only, using autologous PBMC (4×103 cells/well), 3 h-antigen primed autologous B-LCL, or overnight-antigen primed autologous B-LCL as APC (4×103 cells/well). A. Timeline representation of protocols A, B and C. Numbers in brackets next to symbols indicate the day since protocol start at which each step was performed. Numbers under the ‘initial stimulation’ indicator (grey blocks) refer to the duration of the stimulus. B. IFN-γ secretion response as measured by ELISA. For each subject, stimulatory index (SI) was calculated as the response against T. cruzi lysate divided by the cells baseline response (media only condition), each dot represents mean SI value of three biological replicates for a single subject. Dashed lines link values belonging to the same subjects. Bars represent mean SI value for each group. Color codes indicate which group each subject belongs to: chronic Chagas cardiopathy (red), asymptomatic Chagas disease (blue) or non-infected (green).

https://doi.org/10.1371/journal.pone.0178380.g002

Although the response was evaluated by IFN-γ secretion and proliferation, only the former type of response was detectable upon challenge. As shown in Fig 2B, although pre-incubation of the B-LCL with T. cruzi lysate induced IFN-γ secretion in T cell cultures from most subjects studied, none of the cultures challenged with lysate primed-B-LCL reached the level of activation induced by irradiated PBMC as APC. However, the overnight priming condition produced SI values that enable a better detection of the response against the parasite lysate in chronic Chagas patient cultures, as compared to the 3 h priming condition. Additionally, the quality of the response was higher in protocols B (1 day of antigen stimulation with IL-2 added since day 9) and C (6 days of antigen stimulation with IL-2 added since day 6) when B-LCL were used as APC. In conclusion, the results presented here demonstrate that overnight primed B-LCL can be used as APC to present T. cruzi antigens to T cells.

Generation of T. cruzi specific memory CD4+ T cell lines from an asymptomatic patient

Given the results presented above, we hypothesized that using enriched memory T cells, instead of bulk PBMC, would favor the amplification of T cells that emerged in vivo, in response to infection. Seeking to contribute to the scarce existing knowledge on the specificity of memory CD4+ T cells in Chagas disease, we decided to focus our efforts on this population. For this, CD3+CD4+CD45RO+ cells from an asymptomatic chronic Chagas patient (RM30) and a non-infected individual (MM) were magnetically sorted from PBMC samples, and initially cultured with two different stimuli: T. cruzi lysate with irradiated autologous PBMC as APC (antigen specific, selective expansion) or PHA, IL-2 and irradiated allogeneic PBMC as feeder cells (non-antigen specific, non-selective expansion). An overview of the protocols used is represented in Fig 3A. The stimulation of cells from both subjects with PHA resulted in a clear growth of all the seeded wells (Fig 3B). In contrast, the percentages of wells that grew in response to T. cruzi lysate was lower and significantly different between subjects (58.3% for RM30 vs 12.4% for MM, Fisher’s exact test, p<0.001, Fig 3C).

[Figure omitted. See PDF.]

Fig 3. Effect of stimulus used for initial expansion of antigen specific memory CD4+ T cells and their in vitro response against T. cruzi antigens.

Sorted memory CD4+ T cells from an asymptomatic Chagas patient (RM30) and a non-infected subject (MM) were stimulated with PHA (B, D) or parasite lysate (C, E) as detailed under Materials and Methods. Five thousand cells from each culture well were challenged between days 27–32 (depending on cell growth) with parasite lysate or culture media only and the antigen-specific response was measured as IFN-γ secretion and proliferation. Ten thousand autologous overnight-primed B-LCL per well were used as APC. SI was calculated for each well as the response against T. cruzi lysate divided by the cells baseline response (media only condition). Statistical analysis of the percentage of positive wells is shown in S3 Table. A. Timeline representation of stimulation and challenge protocols. Numbers in brackets next to symbols indicate the day (or range of days) since protocol start at which each step was performed. B, C. Pie chart representations of the wells that showed cell growth after initial stimulation, and different degrees of antigen specific response against T. cruzi lysate. D, E. SI values (scatter plots) and percentage of positive wells (bars) for each readout. Cultures considered positive were those with an SI≥2 (dotted line). Positive and total studied wells are indicated in numbers above the bars.

https://doi.org/10.1371/journal.pone.0178380.g003

After the initial expansion, specificity was assessed for these cultures using overnight antigen primed autologous B-LCL as APC. Most of RM30 wells initially stimulated with parasite lysate responded against T. cruzi antigens (73.2% for IFN-γ secretion, 17.9% for proliferation, Fig 3C and 3E) in contrast to the remarkably lower number found in wells initially expanded with PHA (25.0% for IFN-γ, 4.2% for proliferation, Fig 3B and 3D). On the other hand, 21.0% of the lysate expanded wells (only 1.53% out of the total seeded wells) from the non-infected subject responded by IFN-γ secretion, and none responded by proliferation (Fig 3B and 3D). Fisher’s exact test was applied to analyze the difference in frequencies of wells responding, by at least one of the readouts, between the infected and the non-infected donors, and a statistical significance was observed under both initial stimulation conditions, T. cruzi lysate (p = 0.0003) and PHA (p = 0.02). Furthermore, the IFN-γ secretion levels measured in cultures initially expanded with T. cruzi lysate were significantly higher for the chronic Chagas patient as compared to those from the non-infected individual’s cultures (p<0.01, Mann-Whitney test).

Several T cell lines were generated from cultures detected as parasite-specific, and they were further expanded and re-tested for specificity, as previously described. As shown in Fig 4, lines originated from cultures initially stimulated with T. cruzi maintained their responsiveness against parasite lysate by IFN-γ secretion, while those expanded from cells stimulated with PHA did not. Moreover, response by proliferation was no longer observed at this point, even from T cell lines RM30.I and RM30.II, which had been positive for this readout on previous specificity evaluations. In order to avoid limiting the evaluation of specificity only to the quantification of IFN-γ, a multiplex cytokine detection assay (MesoScale Discovery, San Diego, CA) was performed on selected supernatants from experiment shown in Fig 3. A panel of 8 inflammatory and regulatory cytokines (IL-2, IL-4, IL-10, IL-13, IL-17a, TNF-α, GM-CSF, IFN-γ) was evaluated. Results from these experiments pinpointed IFN-γ and GM-CSF as the most reliable readouts for T. cruzi CD4+ T cell specificity (data not shown).

[Figure omitted. See PDF.]

Fig 4. Antigen specific response in selected cultures from subject RM30.

Cell lines were established from T. cruzi specific cultures, based on results from experiment depicted on Fig 3. Cells were submitted to 2 PHA expansion cycles prior to specificity evaluation. Five thousand cells from each culture well were challenged with T. cruzi lysate, using 104 autologous overnight-primed B-LCL per well as APC. SI was calculated for each well as the response against T. cruzi lysate divided by the cells baseline response (media only condition), cultures considered positive were those with an SI≥2 (dotted line). Bars show the mean values and standard deviation for three replicates of each measure.

https://doi.org/10.1371/journal.pone.0178380.g004

In summary, these results confirm the advantages of an initial stimulation with the parasite lysate on memory CD4+ T cells obtained from chronic Chagas patients, both in terms of expansion capability and selectivity.

Generation of T. cruzi specific memory CD4+ T cell clones

In order to isolate an antigen-specific clonal population from the T cell lines generated as described above, we used line RM30.II from the previous section to set up a limiting dilution assay (LDA) using 4 different cell density conditions (10, 3, 1 and 0.3 cells/well), in 10 U-bottom 96-well plates for each condition. Of note, RM30.II was selected for this process based on its growth rate, besides the observed specific response. Cells were expanded with PHA 7 times (except for the 10 cells/well condition, which were expanded 5 times), and specificity evaluations were performed, measuring IFN-γ and GM-CSF secretion, as detailed on S1 Fig. Using growth rate and specificity as criteria, several T. cruzi-specific cultures were selected. On day 99 after the LDA start, all of these cultures showed a clear parasite-specific response (Fig 5A).

[Figure omitted. See PDF.]

Fig 5. Antigen specific response in cultures resulting from limiting dilution assay (LDA) of culture RM30.II.

A. Twenty-five thousand cells from each culture well were challenged with T. cruzi lysate, using 5×104 autologous overnight-primed B-LCL per well as APC. Specificity against T. cruzi antigens was assessed for several potentially monoclonal lines by IFN-γ and GM-CSF secretion. N/A: Non applicable. B. Specific response was tested using lysates from different stages in the parasite’s life cycle (epimastigote and trypomastigote/amastigote) for T cell lines RM30.II.84 and .85.

https://doi.org/10.1371/journal.pone.0178380.g005

In addition, T cell lines RM30.II.84 and .85 were tested for specificity against epimastigote and trypomastigote/amastigote lysate. As shown in Fig 5B, line RM30.II.84 responded specifically to both parasite forms. Seeking to assess whether this line was monoclonal, we performed a TCR-Vβ repertoire characterization by flow cytometry. Results showed these cells exclusively express a TCR from the Vβ 5.2 family, demonstrating RM30.II.84 is a clonal T cell line (Table 1).

[Figure omitted. See PDF.]

Table 1. Detected frequencies of TCR-Vβ families expressed on T cells from lines RM30.II and RM30.II.84.

https://doi.org/10.1371/journal.pone.0178380.t001

Discussion

It is known that the in vitro expansion of lymphocytes collected from peripheral blood mononuclear cells (PBMC) could modify the ex vivo phenotype and function of CD4+ and CD8+ T cells, which in part, could be reflected in the loss of antigen specific memory subsets, changes in specificity and the acquisition of late effector or exhausted phenotypes over time [33–36].

Here, we generated enriched T. cruzi specific T cell lines after an initial PBMC stimulation with parasite lysate. The frequency of T. cruzi responsive cell cultures was greater in asymptomatic and cardiac patients than in non-infected individuals, and it increased in a stimulation time dependent manner. Noticeably, when statistical analysis was applied population-wise to each subject’s cultures, only T cells from Chagas disease patients showed a significantly higher response against T. cruzi lysate, as compared to the baseline response. Conversely, non-infected individuals exhibited either no response, or response inhibition induced by the parasitic antigens (S2 and S3 Figs). However, when bulk PBMC were used to generate the libraries, some of the T cell cultures expanded from non-infected donors’ samples were responsive to T. cruzi. This response, provoked by whole parasite lysate, could be the result of: 1) lectins or superantigens, which could induce a polyclonal, non-specific activation; 2) an antigen-specific primary response from naïve T cells, or 3) memory T cells being specific for host or other pathogens epitopes, and cross-reactive to T. cruzi antigens. In this regard, Piuvezam et al (1993) demonstrated that short term T cell lines generated against T. cruzi from healthy donors PBMC were predominantly memory cells and proliferative response was MHC dependent, suggesting that parasite lysate contains epitopes that cross-react with other antigens of environmental origin, and ruling out a potential involvement of lectins or superantigens as non-specific mitogens [37]. Seeking to minimize the potential contribution of naïve T. cruzi reactive T cells expansion, we undertook our subsequent experiments with enriched memory T cells instead of whole PBMC. Our observation of a certain degree of reactivity in memory CD4+ T cells from a non-infected subject favors the hypothesis of cross-reactivity, meaning these cells have most probably been selected in vivo at the setup of an adaptive response to non-T. cruzi related agents, and cross-react against T. cruzi epitopes. It is also likely that they would be activated early in the context of a first exposure of this subject to the parasite, which makes their specificity an interesting subject for further studies. Nevertheless, under our experimental conditions, the frequency and reactivity of such parasite-responsive cultures were remarkably lower than in those derived from a Chagas disease patient, reinforcing the reliability of our approach.

Another important conclusion drawn from our results lies on the fact that, for memory CD4+ T cell cultures, initially stimulated with T. cruzi lysate, the proportion of wells exhibiting cellular growth was dramatically higher in the chagasic patient RM30 as compared to the non-infected individual MM. On the contrary, when PHA was the initial stimulus, cell growth was observed across all the culture wells, from both subjects. Furthermore, initial stimulation of the Chagas disease patient’s cells with parasite lysate rendered not only a greater proportion of parasite-reactive wells, but also higher specific response values. On that regard, Geiger et al. (2009) demonstrated that within the memory compartment, polyclonal PHA stimulation of CD4+ T cells allows the expansion of T cells specific for recall antigens from tetanus, CMV and M. tuberculosis, at high frequencies [38]. However, even though we were able to reproduce this phenomenon with cells from Chagas disease patients, our results highlight the role of a single initial in vitro stimulation with parasite proteins to increase the frequency at which specific cultures were detected, enabling the subsequent expansion and characterization of pathogen-specific T cells. Several other reported protocols using a specific antigen or its peptides as initial stimulus support our finding [39, 40].

To yield an appropriate quantity of specific T cells, another important step is the expansion of the cultures. Our results showed that, when starting with bulk PBMC, two rounds of non-specific re-stimulation with PHA could increase the number of naïve/cross-reactive T cells not related to infection, as shown by the proliferation response rendered by T cells derived from non-infected individuals. In addition, each round affected the specificity of the cell populations. This dynamic change in antigen specificity could also be associated with a direct effect of the mitogen over the functional characteristics of T cells [41], or be the consequence of the enrichment of certain T cells in the well, leading to gain or loss in frequency of parasite specific T cells. The same phenomenon was observed in T cell lines RM30.IV and .V, which came from a chronic asymptomatic Chagas patient enriched memory CD4+ T cells with a non-specific initial stimulus. However, the specificity of lines RM30.I, .II and .III, which were generated by antigen-specific stimulation of the same T cell subset seems to be long-term stable, regardless of the number of subsequent PHA expansions.

An interesting finding of the present study lies in the use of T. cruzi primed B-LCL to function as antigen-presenting cells (APCs) for the assessment of T cell responses. Although autologous PBMC or dendritic cells are a better source of the so called “professional” APC, their usage relies on repeated blood donations [42]. In contrast, although B-LCL have less capacity to present soluble antigens compared to monocytes or dendritic cells, they are a sustainable and scalable source of APC. In fact, immortalized B-LCL have been broadly used with success in different protocols that require in vitro antigen presentation to T cells. However, no data were available about their use as APC for the presentation of T. cruzi proteins. Here, our results showed that both PBMC and overnight parasite lysate-pulsed B-LCL induced similar IFN-γ secretion profiles in T cells from asymptomatic and cardiac patients.

After LDA, T cell lines generated from memory CD4+ T cells from a chagasic patient and maintained under the described culture conditions, retained their specific response capability towards T. cruzi lysate for more than 98 days. Moreover, T cell line RM30.II.84 responded against epimastigote and trypomastigote/amastigote lysate with similar strength, indicating that these cells recognize a common epitope expressed in both non-infective and infective parasite forms. Finally, TCR-Vβ analysis demonstrated a prevalence of TCR-Vβ 2, 5.1 and 5.2 families in memory CD4+ T cell line RM30.II while its derived clone RM30.II.84 expresses TCR-Vβ 5.2.

Even though the generality of our findings is limited due to the small number of subjects (patients and non-infected donors) included throughout the study, it is possible to ascertain a suitable protocol for the generation of specific oligo- and monoclonal T cell lines from patients with Chagas disease. Although our first efforts were focused on the generation of memory CD4+ T cell clones from an asymptomatic subject, we expect that this method will be useful for the expansion of T. cruzi specific T cells from cardiac patients. However, it could represent a greater challenge, due to the higher frequency of CD4+ T cells with senescent and exhausted phenotype in the peripheral blood of these patients as compared to asymptomatic ones [43]. We speculate that it will not be possible to obtain as many detectable specific T cell lines per patient as we have for asymptomatic patients assayed so far, or that it will be more difficult to amplify them to numbers large enough. Hoping to shed some light in this issue, we are currently looking into the ex vivo expression profiles of several inhibitory receptors which have been associated to T cell exhaustion [44], and how they vary during in vitro culture and expansion.

In conclusion, our data demonstrate that: 1) starting the expansion from enriched memory T cells instead of PBMC allow the increase of the stimulation time, enabling the selection of a larger number of parasite specific T cell cultures; 2) an antigen specific initial stimulation is beneficial for the ex vivo selective expansion of pathogen related memory CD4+ T cell populations, as compared with a non-antigen specific, although stronger, stimulation (as PHA); 3) the use of different readouts, in this particular case IFN-γ and GM-CSF secretion, is important in order to detect the largest number of antigen-specific positive wells and 4) B-LCL primed with T. cruzi lysate by an overnight incubation are capable to perform antigen presentation and stimulate parasite specific T cells. This work constitutes the first step in our ongoing T cell driven approach to the identification of human immunogenic T. cruzi epitopes, a matter of key relevance for the understanding of the immune response in Chagas disease.

Supporting information

[Figure omitted. See PDF.]

S1 Fig. Schematic representation of the LDA protocol.

T cells were plated in 96-well plates, at densities of 10, 3, 1 and 0.3 cells/well (rows), and submitted to PHA expansion. Numbers indicate the amount of wells that were expanded each time (columns), after the previous round of selection, according to the criteria indicated by arrows.

https://doi.org/10.1371/journal.pone.0178380.s001

(EPS)

S2 Fig. IFN-γ secretion raw values for specificity experiments on T cells derived from PBMC.

For each challenge experiment on Fig 1, paired results for each culture were statistically analyzed using Wilcoxon’s signed rank test. (*/#: p<0.05; **/##: p<0.01; ***/###: p<0.001; ****/####: p<0.0001). Asterisks show statistical significance in cases were the T. cruzi lysate challenged response was significantly higher than the one from the culture medium only condition (W>0). Similarly, number signs show significance in the cases in which the baseline response was significantly higher than the one from the lysate challenged aliquots (W<0). Color codes indicate which group each subject belongs to: chronic Chagas cardiopathy (red), asymptomatic Chagas disease (blue) or non-infected (green). NA: No antigen condition; Tc: T. cruzi lysate. A. Results from experiment explained in Fig 1B and 1C. B. Results from experiment explained in Fig 1D.

https://doi.org/10.1371/journal.pone.0178380.s002

(PDF)

S3 Fig. Proliferation raw values for specificity experiments on T cells derived from PBMC.

For each challenge experiment on Fig 1, paired results for each culture were statistically analyzed using Wilcoxon’s signed rank test. (*/#: p<0.05; **/##: p<0.01; ***/###: p<0.001; ****/####: p<0.0001) Asterisks show statistical significance in cases were the T. cruzi lysate challenged response was significantly higher than the one from the culture medium only condition (W>0). Similarly, number signs show significance in the cases in which the baseline response was significantly higher than the one from the lysate challenged aliquots (W<0). Color codes indicate which group each subject belongs to: chronic Chagas cardiopathy (red), asymptomatic Chagas disease (blue) or non-infected (green). NA: No antigen condition; Tc: T. cruzi lysate. A. Results from experiment explained in Fig 1B and 1C. B. Results from experiment explained in Fig 1D.

https://doi.org/10.1371/journal.pone.0178380.s003

(PDF)

S1 Table. Statistical analysis for the effect of 6 days stimulation with parasite lysate on PBMC.

The numbers correspond to Fisher's exact tests p values with Bonferroni-Holm correction for multiple comparisons applied to the analysis of the percentage of positive wells. Data from two non-infected subjects (FI and MF) was pooled for comparison with each infected subject, see Fig 1B and 1C. p<0.05 was considered statistically significant.

https://doi.org/10.1371/journal.pone.0178380.s004

(DOCX)

S2 Table. Statistical analysis for the effect of PHA expansions on T. cruzi specific T cell response.

The numbers correspond to p values of Fisher's exact tests with Bonferroni-Holm correction applied to the percentage of positive wells from each patient in comparison with non-infected subject, named MM, see Fig 1D and 1E. p<0.05 was considered significantly.

https://doi.org/10.1371/journal.pone.0178380.s005

(DOCX)

S3 Table. Statistical analysis for the effect of initial stimulus on memory CD4+ T cells.

The numbers correspond to p values of Fisher's exact tests with Bonferroni-Holm correction applied to the percentage of positive wells from the patient in comparison with non-infected subject, named MM, see Fig 3. p<0.05 was considered significantly.

https://doi.org/10.1371/journal.pone.0178380.s006

(DOCX)

Acknowledgments

We thank all the patients and non-infected individuals who participated in this study. We are also very grateful to the staff of the Hospital General de Agudos J.M. Ramos Mejia and Violeta Chiauzzi for technical assistance.

Author Contributions

1. Conceptualization: GRA SAL VAJ CP KAG.

2. Formal analysis: GRA RS.

3. Funding acquisition: CP KAG.

4. Investigation: GRA SAL AB NS KAG.

5. Methodology: GRA SAL VAJ CP KAG.

6. Project administration: CP KAG.

7. Resources: AA MPZ CP KAG.

8. Supervision: VAJ CP KAG.

9. Visualization: GRA.

10. Writing – original draft: GRA KAG.

11. Writing – review & editing: GRA SAL VAJ CP KAG.

Citation: Acevedo GR, Longhi SA, Bunying A, Sabri N, Atienza A, Zago MP, et al. (2017) Methodological approach to the ex vivo expansion and detection of T. cruzi-specific T cells from chronic Chagas disease patients. PLoS ONE 12(5): e0178380. https://doi.org/10.1371/journal.pone.0178380

References

1. Padilla AM, Bustamante JM, Tarleton RL. CD8+ T cells in Trypanosoma cruzi infection. Curr Opin Immunol. 2009;21:385–390. pmid:19646853

2. Fiuza JA, Fujiwara RT, Gomes JA, Rocha MO, Chaves AT, de Araújo FF, Fares RC, Teixeira-Carvalho A, Martins-Filho OA, Cançado GG, Correa-Oliveira R. Profile of central and effector memory T cells in the progression of chronic human chagas disease. PloS Negl Trop Dis. 2009;3:e512. pmid:19742301

3. Scharfstein J, Gomes JA, Correa-Oliveira R. Back to the future in Chagas disease: from animal models to patient cohort studies, progress in immunopathogenesis research. Mem Inst Oswaldo Cruz. 2009;104:187–198. pmid:19753474

4. Machado FS, Dutra WO, Esper L, Gollob KJ, Teixeira MM, Factor SM, Weiss LM, Nagajyothi F, Tanowitz HB, Garg NJ. Current understanding of immunity to Trypanosoma cruzi infection and pathogenesis of Chagas disease. Semin Immunopathol 2012;34:753–770. pmid:23076807

5. Alvarez MG, Postan M, Weatherly DB, Albareda MC, Sidney J, Sette A, Olivera C, Armenti AH, Tarleton RL, Laucella SA. HLA Class I-T cell epitopes from trans-sialidase proteins reveal functionally distinct subsets of CD8+ T cells in chronic Chagas disease. PLoS Negl Trop Dis. 2008;2:e288. pmid:18846233

6. Albareda MC, Laucella SA, Alvarez MG, Armenti AH, Bertochi G, Tarleton RL, Postan M. Trypanosoma cruzi modulates the profile of memory CD8+ T cells in chronic Chagas' disease patients. Int Immunol. 2006;18:465–471. pmid:16431876

7. Tzelepis F, de Alencar BC, Penido ML, Claser C, Machado AV, Bruna-Romero O, Gazzinelli RT, Rodrigues MM. Infection with Trypanosoma cruzi restricts the repertoire of parasite-specific CD8+ T cells leading to immunodominance. J Immunol. 2008;180:1737–1748. pmid:18209071

8. Souza PE, Rocha MO, Rocha-Vieira E, Menezes CA, Chaves AC, Gollob KJ, et al. Monocytes from patients with indeterminate and cardiac forms of Chagas’ disease display distinct phenotypic and functional characteristics associated with morbidity. Infect Immun. 2004;72:5283–5291. pmid:15322024

9. Cuellar A, Santander SP, del Thomas MC, Guzman F, Gomez A, López MC, Puerta CJ. Monocyte-derived dendritic cells from chagasic patients vs healthy donors secrete differential levels of IL-10 and IL-12 when stimulated with a protein fragment of Trypanosoma cruzi heat-shock protein-70. Immunol Cell Biol. 2008;86:255–260. pmid:18180802

10. Dutra WO, Gollob KJ, Pinto-Dias JC, Gazzinelli G, Correa-Oliveira R, Coffman RL, et al. Cytokine mRNA profile of peripheral blood mononuclear cells isolated from individuals with Trypanosoma cruzi chronic infection. Scand J Immunol. 1997;45:74–80. pmid:9010503

11. Abel LC, Rizzo LV, Ianni B, Albuquerque F, Bacal F, Carrara D, et al. Chronic Chagas' disease cardiomyopathy patients display an increased IFN-gamma response to Trypanosoma cruzi infection. J Autoimmun. 2001;17:99–107. pmid:11488642

12. Ribeirao M, Pereira-Chioccola VL, Nia L, Augusto Fragata FA, Schenkman S, Rodrigues MM. Chagasic patients develop a type 1 immune response to Trypanosoma cruzi trans-sialidase. Parasite Immunol. 2000;22:49–55. pmid:10607290

13. Michailowsky V, Luhrs K, Rocha MOC, Fouts D, Gazzinelli RT, Manning JE. Humoral and cellular immune responses to Trypanosoma cruzi-derived paraflagellar rod proteins in patients with Chagas’ disease. Infect Immun, 2003; 71:3165–3171. pmid:12761095

14. Lorena VM, Verçosa AF, Machado RC, Moitinho-Silva L, Cavalcanti MG, Silva ED, et al. Cellular Immune Response From Chagasic Patients to CRA or FRA Recombinant Antigens of Trypanosoma cruzi. J Clin Lab Anal. 2008;22:91–98. pmid:18348314

15. de Melo AS, de Lorena VM, de Moura Braz SC, Docena C, de Miranda Gomes Y. IL-10 and IFN-γ gene expression in chronic Chagas disease patients after in vitro stimulation with recombinant antigens of Trypanosoma cruzi. Cytokine. 2012;58:207–212. pmid:22325340

16. Morán-Utrera Y, López-Monteon A, Rosales-Encina JL, Mendez-Bolaina E, Ramos-Ligonio A. Trypanosoma cruzi SSP4 Amastigote Protein Induces Expression of Immunoregulatory and Immunosuppressive Molecules in Peripheral Blood Mononuclear Cells. J Trop Med. 2012;2012:829139. pmid:23209478

17. Arnholdt AC, Piuvezam MR, Russo DM, Lima AP, Pedrosa RC, Reed SG, Scharfstein J. Analysis and partial epitope mapping of human T cell responses to Trypanosoma cruzi cysteinyl proteinase. J Immunol. 1993; 51:3171–3179.

18. Longhi SA, Atienza A, Perez Prados G, Buying A, Balouz V, Buscaglia CA, et al. Cytokine production but lack of proliferation in peripheral blood mononuclear cells from chronic Chagas' disease cardiomyopathy patients in response to T. cruzi ribosomal P proteins. PLoS Negl Trop Dis. 2014;8: e2906. pmid:24901991

19. Eickhoff CS, Van Aartsen D, Terry FE, Meymandi SK, Traina MM, Hernandez S, et al. An immunoinformatic approach for identification of Trypanosoma cruzi HLA-A2-restricted CD8(+) T cell epitopes. Hum Vaccin Immunother. 2015;11: 322–2328.

20. Garg N, Tarleton RL. Genetic immunization elicits antigen-specific protective immune responses and decreases disease severity in Trypanosoma cruzi infection.Infect Immun. 2002;70:5547–5555. pmid:12228281

21. Rampazo EV, Amorim KN, Yamamoto MM, Panatieri RH, Rodrigues MM, Boscardin SB. Antigen targeting to dendritic cells allows the identification of a CD4 T-cell epitope within an immunodominant Trypanosoma cruzi antigen. PLoS One. 2015;10:e0117778.Martinez-Campos V, Martinez-Vega P, Ramirez-Sierra MJ, Rosado-Vallado pmid:25679777

22. Cerny N, Sánchez Alberti A, Bivona AE, De Marzi MC, Frank FM, Cazorla SI, et al. Coadministration of cruzipain and GM-CSF DNAs, a new immunotherapeutic vaccine against Trypanosoma cruzi infection. Hum Vaccin Immunother. 2016; 2:438–450.

23. Gupta S, Garg NJ. A Two-Component DNA-Prime/Protein-Boost Vaccination Strategy for Eliciting Long-Term, Protective T Cell Immunity against Trypanosoma cruzi. PLoS Pathog. 2015;11:e1004828. pmid:25951312

24. M , Seid CA, Hudspeth EM, et al. Expression, purification, immunogenicity, and protective efficacy of a recombinant Tc24 antigen as a vaccine against Trypanosoma cruzi infection in mice. Vaccine. 2015;33:4505–4512. pmid:26192358

25. Serna C, Lara JA, Rodrigues SP, Marques AF, Almeida IC, Maldonado RA. A synthetic peptide from Trypanosoma cruzi mucin-like associated surface protein as candidate for a vaccine against Chagas disease. Vaccine. 2014;32:3525–3532. pmid:24793944

26. Lasso P, Cárdenas C, Guzmán F, Rosas F, Thomas MC, López MC, et al. Effect of secondary anchor amino acid substitutions on the immunogenic properties of an HLA-A*0201-restricted T cell epitope derived from the Trypanosoma cruzi KMP-11 protein. Peptides. 2016;78:68–76. pmid:26854383

27. Quijano-Hernandez I, Dumonteil E. Advances and challenges towards a vaccine against Chagas disease. Hum Vaccin. 2011;7:1184–1191. pmid:22048121

28. El-Sayed NM, Myler PJ, Bartholomeu DC, Nilsson D, Aggarwal G, Tran AN, et al. The genome sequence of Trypanosoma cruzi, etiologic agent of Chagas disease. Science. 2005;309:409–415. pmid:16020725

29. Hondowicz BD, Schwedhelm KV, Kas A, Tasch MA, Rawlings C, Ramchurren N, et al. Discovery of T Cell Antigens by High-Throughput Screening of Synthetic Minigene Libraries. PLoS One. 2012;7:e29949. pmid:22253836

30. Mazzatti DJ, White A, Forsey RJ, Powell JR, Pawelec G. Gene expression changes in long-term culture of T-cell clones: genomic effects of chronic antigenic stress in aging and immunosenescence. Aging Cell. 2007;6:155–163. pmid:17286612

31. Tosato G, Cohen JI. 2007. Generation of Epstein-Barr Virus (EBV)-immortalized B cell lines. Curr Protoc Immunol. Chapter 7:Unit 7.22. pmid:18432996

32. Gomes JA, Bahia-Oliveira LM, Rocha MO, Martins-Filho OA, Gazzinelli G, Correa-Oliveira R. Evidence that Development of Severe Cardiomyopathy in Human Chagas’ Disease Is Due to a Th1-Specific Immune Response. Inf Immun. 2003;71:1185–1193.

33. Geginat J, Sallusto F, Lanzavecchia A. Cytokine-driven proliferation and differentiation of human naive, central memory, and effector memory CD4(+) T cells. J Exp Med. 2001;194:1711–1719.

34. Kim M, Moon HB, Kim K, Lee KY. Antigen dose governs the shaping of CTL repertoires in vitro and in vivo. Int Immunol. 2006;18:435–444. pmid:16431877

35. Leggatt GR, Narayan S, Fernando GJ, Frazer IH. Changes to peptide structure, not concentration, contribute to expansion of the lowest avidity cytotoxic T lymphocytes. J Leukoc Biol. 2004;76:787–795. pmid:15240746

36. Tumeh PC, Koya RC, Chodon T, Graham NA, Graeber TG, Comin-Anduix B, et al. The impact of ex vivo clinical grade activation protocols on human T cell phenotype and function for the generation of genetically modified cells for adoptive cell transfer therapy. J Immunother. 2010;33:759–768. pmid:20842061

37. Piuvezam MR, Russo DM, Burns JM Jr, Skeiky YA, Grabstein KH, Reed SG. Characterization of responses of normal human T cells to Trypanosoma cruzi antigens. J Immunol. 1993;150:916–924. pmid:8423347

38. Geiger R, Duhen T, Lanzavecchia A, Sallusto F. Human naive and memory CD4+ T cell repertoires specific for naturally processed antigens analyzed using libraries of amplified T cells. J Exp Med. 2009;206:1525–1534 pmid:19564353

39. Lewinsohn DM, Briden AL, Reed SG, Grabstein KH, Alderson MR. Mycobacterium tuberculosis-reactive CD8+ T lymphocytes: the relative contribution of classical versus nonclassical HLA restriction. J Immunol. 2000;165:925–930. pmid:10878367

40. Lewinsohn DA, Winata E, Swarbrick GM, Tanner KE, Cook MS, Null MD, et al. Immunodominant tuberculosis CD8 antigens preferentially restricted by HLA-B. PLoS Pathog. 2007;3:1240–1249. pmid:17892322

41. Duarte RF, Chen FE, Lowdell MW, Potter MN, Lamana ML, Prentice HG, et al. Functional impairment of human T-lymphocytes following PHA-induced expansion and retroviral transduction: implications for gene therapy. Gene Ther. 2002;9:1359–1368. pmid:12365001

42. Sun Q, Burton RL, Dai LJ, Britt WJ, Lucas KG. B lymphoblastoid cell lines as efficient APC to elicit CD8+ T cell responses against a cytomegalovirus antigen. J Immunol. 2000;165:4105–4111. pmid:11034422

43. Albareda MC, Olivera GC, Laucella SA, Alvarez MG, Fernandez ER, Lococo B, et al. Chronic human infection with Trypanosoma cruzi drives CD4+ T cells to immune senescence. J Immunol. 2009;183:4103–4108. pmid:19692645

44. Anderson AC, Joller N, Kuchroo VK. Lag-3, Tim-3, and TIGIT: Co-inhibitory Receptors with Specialized Functions in Immune Regulation. Immunity. 2016;44:989–1004. pmid:27192565

Word count: 8549

Show less

© 2017 Acevedo et al. This is an open access article distributed under the terms of the Creative Commons Attribution License: http://creativecommons.org/licenses/by/4.0/ (the “License”), which permits unrestricted use, distribution, and reproduction in any medium, provided the original author and source are credited. Notwithstanding the ProQuest Terms and Conditions, you may use this content in accordance with the terms of the License.

Abstract

The discovery of T cell epitopes is essential not only for gaining knowledge about host response to infectious disease but also for the development of immune-intervention strategies. In Chagas disease, given the size and complexity of the Trypanosoma cruzi proteome and its interaction with the host’s immune system, the fine specificity of T cells has not been extensively studied yet, and this is particularly true for the CD4+ T cell compartment. The aim of the present work was to optimize a protocol for the generation of parasite-specific memory T cell lines, representative of their in vivo precursor populations and capable of responding to parasite antigens after long-term culture. Accordingly, peripheral blood mononuclear cells (PBMC) from both chronic asymptomatic and cardiac patients, and from non-infected individuals, underwent different in vitro culture and stimulation conditions. Subsequently, cells were tested for their capacity to respond against T. cruzi lysate by measuring [3H]-thymidine incorporation and interferon-γ and GM-CSF secretion. Results allowed us to adjust initial T. cruzi lysate incubation time as well as the number of expansions with phytohemagglutinin (PHA) and irradiated allogeneic PBMC prior to specificity evaluation. Moreover, our data demonstrated that parasite specific T cells displayed a clear and strong activation by using T. cruzi lysate pulsed, Epstein-Barr virus (EBV)-transformed human B lymphocytes (B-LCL), as autologous antigen presenting cells. Under these culture conditions, we generated a clone from an asymptomatic patient’s memory CD4+ T cells which responded against epimastigote and trypomastigote protein lysate. Our results describe a culture method for isolating T. cruzi specific T cell clones from patients with Chagas disease, which enable the acquisition of information on functionality and specificity of individual T cells.

Details

Title
Methodological approach to the ex vivo expansion and detection of T. cruzi-specific T cells from chronic Chagas disease patients
Author
Acevedo, Gonzalo R; Longhi, Silvia A; Bunying, Alcinette; Sabri, Nazila; Atienza, Augusto; Zago, María P; Santos, Radleigh; Judkowski, Valeria A; Pinilla, Clemencia; Gómez, Karina A
First page
e0178380
Section
Research Article
Publication year
2017
Publication date
May 2017
Publisher
Public Library of Science
e-ISSN
19326203
Source type
Scholarly Journal
Language of publication
English
DOI
https://doi.org/10.1371/journal.pone.0178380
ProQuest document ID
1902656967
Copyright
© 2017 Acevedo et al. This is an open access article distributed under the terms of the Creative Commons Attribution License: http://creativecommons.org/licenses/by/4.0/ (the “License”), which permits unrestricted use, distribution, and reproduction in any medium, provided the original author and source are credited. Notwithstanding the ProQuest Terms and Conditions, you may use this content in accordance with the terms of the License.