Increased CD8+-T-Cell Expression and a Type 2 Cytokine Pattern during the Muscular Phase of Trichinella Infection in Humans

Cell-mediated immunity during the muscular phase of Trichinellainfection in humans was studied. Cell proliferation, the phenotypicchanges in the T-cell population, and expression and productionof cytokines were examined by using peripheral blood mononuclearcells (PBMC) collected at different times postinfection from10 individuals who had acquired Trichinella spiralis and fiveindividuals who had acquired Trichinella britovi in two distinctoutbreaks. T. spiralis and T. britovi crude worm extracts inducedproliferation of PBMC from T. spiralis- and T. britovi-infecteddonors. Cytokine gene expression showed a predominant type 2pattern for the entire period of infection studied, althoughgamma interferon (IFN- ${gamma}$ ) was expressed. Interleukin-2 (IL-2),IL-5, IL-10, and IFN- ${gamma}$ production was found in PBMC of all donors.There was a good correspondence between the cytokine expressionand production patterns. Changes in PBMC composition, with atrend toward an increase in CD8⁺ lymphocyte counts, were observed.

INTRODUCTION

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Introduction

The genus Trichinella is a group of nematodes which have a worldwidedistribution and which cause trichinellosis in humans (15).Humans are infected by eating raw or undercooked meat or meatproducts (sausages, salami, etc.) from swine, horses, or gameanimals that are infected with larvae of these worms. In Italy,the main etiological agent of human trichinellosis is Trichinellabritovi; however, some human infections have been attributedto consumption of products from imported animals infected withTrichinella spiralis (17).

From 4 to 5 days after ingestion of infected meat, the larvaedevelop to the adult stage in a row of columnar epithelial cellsin the small intestine. Six days after ingestion, the adultworms begin to reproduce, and the newborn larvae migrate acrossthe lamina propria of the villus into the lymph and bloodstream.However, only the newborn larvae that reach striated musclesdevelop to the infective stage. In laboratory mice, the intestinalphase is longer for T. spiralis than for T. britovi and thefemale fecundity of T. spiralis is at least twice than thatof T. britovi. These differences explain the different clinicalpictures obtained for humans infected with these two species(20). Intestinal symptomatology (diarrhea, abdominal pain, andvomiting) occurs more frequently and lasts longer in human T.spiralis infections than in human T. britovi infections (20).

When a larva penetrates a muscle cell, it causes the cell tobecome what is known as a nurse cell, and it becomes infective15 to 16 days later (i.e., 21 to 22 days after ingestion ofinfected meat) (6).

After ingestion of larvae, a host develops an immunity-mediatedinflammatory response at the intestinal level, and this is followedby rapid expulsion of some of the larvae from the intestine(3). Studies conducted with mouse and rat models have suggestedthat antibodies play the most important role in this response,which depends on type Th2 cytokines derived from CD4⁺ cells,and that mucosal mast cells also play an important role (11).Moreover, it appears that during the host intestinal response,the CD4⁺ cells initially produce type Th1 cytokines and thattype Th2 cytokines are produced only later (10, 12). Alteredbiological parameters (muscular enzymes, eosinophilia, and leukocytosis)and specific immunoglobulin G (IgG) persist longer in peopleinfected with T. spiralis than in people infected with T. britovi(20).

In humans, larvae in the striated muscles can remain infectivefor up to 30 years (8). One of the most distinctive featuresof Trichinella infection is its chronicity, and the resultingpersistent antigenic stimulation could lead to polarizationof T-cell subset populations and modification of immunoregulatorystates, as observed in other parasitic infections (22). However,in humans, our understanding of the immune response is for themost part limited to the antibody response, and nothing is knownabout cell-mediated immunity during the course of the infection.

The objective of the present study was to characterize cell-mediatedimmunity during the muscular phase of Trichinella infectionin humans. To do this, we studied the phenotypic changes inthe T-cell populations of peripheral blood mononuclear cells(PBMC) from people infected with Trichinella and expressionand the production of cytokines in these cell populations. Ourresults showed that CD8⁺ T-cell expression was increased andthe cytokine pattern was predominately type 2.

MATERIALS AND METHODS

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Materials and Methods

Panel of donors. We collected blood samples from 10 people who were infectedwith T. spiralis, the most widespread Trichinella species, afterthey had ingested imported horsemeat during a 1998 outbreakin northern Italy (18). The blood samples were collected whenthe infected individuals returned to the hospital for checkups,2, 9, 14, and 36 months after ingestion of the infected meat.All donors had been treated with 50 mg of prednisolone per dayand 1,500 mg of mebendazole per day for 10 days; when the samplesobtained 2 months postinfection (p.i.) were collected, the donorshad completed treatment 3 weeks previously. We also collectedblood samples 1.5, 2.5, and 12 months after ingestion of infectedmeat from five people who were infected with T. britovi afterthey ingested wild boar meat during a 1995 outbreak in centralItaly (17). As described above, the sample collection timescorresponded to checkup times. Two of the donors were treatedwith both prednisolone and mebendazole (80 mg of prednisoloneper day and 1,500 mg of mebendazole per day for 10 days), whereasthe other three donors were treated only with mebendazole. Whenthe blood samples obtained 1.5 months p.i. were collected, thetwo donors treated with both drugs were at the eighth day oftreatment. Samples from three donors who were known to havenever been infected with Trichinella were used as controls inall assays. We obtained written informed consent from the donorsbefore taking blood samples.

PBMC were isolated from samples from T. spiralis-infected donorsand T. britovi-infected donors by centrifugation on densitygradients (Lymphoprep; Nyegaard, Oslo, Norway) and were washedtwice in RPMI medium (GIBCO, Grand Island, N.Y.). The PBMC werethen frozen in fetal calf serum with 10% dimethyl sulfoxide(Sigma Chemical Co.) at -80°C. After rapid thawing at 37°Cin a water bath, the PBMC were washed twice and then dilutedin RPMI medium supplemented with 5% pooled AB serum and antibiotics(100 IU of penicillin [GIBCO] per ml, 0.1 mg of streptomycin[GIBCO] per ml).

Parasites, antigens, and mitogens. T. spiralis larvae (isolate code ISS597) and T. britovi larvae(ISS205) were isolated from meat from the infected horse andthe infected wild boar, respectively. These two isolates weremaintained under laboratory conditions by serial passages inSwiss-CD1 mice. Larvae were collected by enzymatic digestionof the infected meat, and a crude worm extract (CWE) antigenand an excretory-secretory antigen were prepared for both speciesby using previously described procedures (7, 9). The proteinconcentrations of the antigens were estimated by the methodof Bradford (4). Since the two antigens induced the same proliferationin PBMC (data not shown) and the CWE antigen was easier to preparethan the excretory-secretory antigen, we used CWE in all ofthe experiments. For antigen selection, two doses (5.0 and 25µg/ml) of T. spiralis CWE and T. britovi CWE were usedto induce proliferative responses in PBMC from three T. spiralis-infecteddonors and three T. britovi-infected donors (Table 1). A partiallypurified mannoprotein (MP) extract of the cell wall of Candidaalbicans, constituting the major antigenic determinant of thismicroorganism, was used as an antigenic control for proliferation(1). Recombinant interleukin-2 (IL-2) (Amersham International,Buckinghamshire, United Kingdom) and purified phytohemagglutinin(PHA) (Murex Diagnostics, Dartford, United Kingdom) were usedas mitogenic stimulants.

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TABLE 1. Proliferative responses to T. spiralis CWE and to a control stimulant, IL-2, on day 7 of culture of PBMC from T. spiralis-infected individuals obtained at different times p.i.

PBMC proliferation and generation of activated effectors. IL-2 (100 IU/ml) or antigens at optimal concentrations wereadded to PBMC from 10 T. spiralis-infected donors and five T.britovi-infected donors collected at different times p.i. PBMCproliferation was measured in 96-well flat-bottom microwelltrays in triplicate. The trays were incubated in 5% CO₂ at 37°C,and PBMC were harvested on the 3rd, 7th, and 10th days after18 h of incubation in the presence of 0.5 µCi of [³H]thymidine(NEN-Du Pont, Boston, Mass.). The data are expressed below asmeans ± standard deviations. To isolate total RNA, PBMCwere cultured at a concentration of 2 x 10⁶ cells/ml in thepresence of 25 µg of T. spiralis CWE per ml or 25 µgof T. britovi CWE per ml for 48 h under similar conditions.

RT-PCR. Total cellular RNA was extracted from 2 x 10⁶ cells with a QuickPrepMicro mRNA purification kit (Pharmacia). Reverse transcriptasePCRs (RT-PCR) were performed with 50-µl (total volume)mixtures by using the primer pairs specified by the manufacturer(T-primed First-Strand kit; Pharmacia). cDNAs were amplifiedin the presence of 5' and 3' primers (each at a final concentrationof 0.05 µM), 2.0 mM deoxynucleotides, 1 U of Taq DNA polymerase(Promega, Madison, Wis.), and 1x PCR buffer. Each PCR was performedwith a thermal cycler (Perkin-Elmer, Norwalk, Conn.) by using10 cycles consisting of 30 s of denaturation at 94°C, 30s of annealing at 64°C, and 30 s of extension at 72°Cand then 25 cycles consisting of 30 s of denaturation at 94°C,30 s of annealing at 62°C, and 1 min of extension at 72°C.A housekeeping gene, ß-actin, was amplified in eachexperiment to evaluate the extraction procedure and to estimatethe amount of RNA. The reaction product was visualized by electrophoresisby using 10 µl of the reaction mixture and 2 µlof loading buffer. One microgram of a 100-bp ladder (Pharmacia)was run in parallel as a molecular size marker, providing bandsat 100 to 1,000 bp. Cytokine-specific primer pairs were synthesized(Applied Biosystems, Foster City, Calif.) by using previouslydescribed sequences (2).

Genes for the following cytokines were examined for all 10 T.spiralis-infected donors and for three of the five T. britovi-infecteddonors for all samples except those collected from T. spiralis-infecteddonors 36 months p.i and from T. britovi-infected donors 2.5months p.i.: IL-2, IL-4, IL-5, IL-6, IL-10, and gamma interferon(IFN- ${gamma}$ ). Each cytokine was considered expressed only if the RT-PCRsignal of the T. spiralis- or T. britovi-stimulated sample wasvisibly more intense than the baseline response.

Cytokine production. We determined the concentrations of IL-2, IL-5, IL-10, and IFN- ${gamma}$ in PBMC culture supernatants which were collected after 48 hof incubation by using a commercial enzyme-linked immunosorbentassay, as specified by the manufacturer (R&D Systems Europe).

Flow cytometric analysis. PBMC from three T. spiralis-infected donors and three T. britovi-infecteddonors were cultured for 7 days at a concentration of 1 x 10⁶cells/mlin the presence of 25 µg of T. spiralis CWE per ml, 25µg of T. britovi CWE per ml, or 10 µg of C. albicansantigen per ml. The PBMC were then resuspended in phosphate-bufferedsaline and stained with phycoerythrin (PE)-conjugated or fluoresceinisothiocyanate (FITC)-conjugated monoclonal antibody; to determinevitality, cells were stained with propidium iodine.

Three-color flow cytometric analyses were performed with a FACSCaliburflow cytometer (Becton Dickinson, San Jose, Calif.). Data wereacquired with CELL-Quest software (Becton Dickinson). The instrumentwas set up to measure the fluorescence intensities of forward-anglelight scatter (FSC), side-angle light scatter, FITC (FL1), PE(FL2), and propidium iodine (FL3). The following pairs of monoclonalantibodies were used: CD3 (FITC) and CD4 (PE), CD3(FITC) andCD8 (PE), TCR- ${alpha}$ ß (FITC) and TCR- ${gamma}$ ${delta}$ (PE), and CD45RA (FITC)and CD45RO (PE) (all obtained from Becton Dickinson). The monocyte-specificreagent CD14 (PE) (Becton Dickinson) was used to test for monocytecontamination of lymphocytes. Cells incubated with FITC- andPE-conjugated mouse IgG1/IgG2a served as an isotype control.

Statistical analysis. The results were analyzed by one-way analysis of variance andStudent’s t test. A P value of <0.05 was consideredstatistically significant.

RESULTS

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Results

PBMC proliferation. Both T. spiralis CWE and T. britovi CWE induced blastogenesisin PBMC (data not shown). T. spiralis CWE induced stronger proliferationof PBMC than T. britovi CWE, independent of the infecting Trichinellaspecies, and the greatest responses occurred at a concentrationof 25 µg/ml. Thus, T. spiralis CWE was selected for thesubsequent experiments. The PBMC from noninfected donors didnot show any proliferative response to Trichinella antigens(data not shown).

To determine the kinetics of proliferation, PBMC from one T.spiralis-infected donor were cultured for 10 days with T. spiralisCWE (25 µg/ml) or PHA (1.5 µg/ml). The T. spiralisCWE-induced proliferation peaked on day 7 of culture, whereasthe PHA-induced proliferation showed typical mitogenic kinetics,peaking on day 3 (data not shown).

The PBMC from the 10 donors infected with T. spiralis (collected2, 9, 14, and 36 months p.i.) proliferated when they were stimulatedwith T. spiralis CWE, and the greatest response occurred 9 monthsp.i. (Table 1). The PBMC from the five T. britovi-infected donors(collected 1.5, 2.5, and 12 months p.i.) showed three differentpatterns of proliferative response (Table 2). For three of thesedonors (Table 2, donors 1 to 3), none of whom had undergonecorticosteroid therapy, PBMC collected 1.5 and 2.5 months p.i.showed a high level of proliferation when they were stimulatedwith T. spiralis CWE and with IL-2, whereas PBMC collected 12months p.i. showed a lower level of proliferation. For donor4, PBMC collected 1.5 months p.i. did not respond to eitherT. spiralis CWE or IL-2, whereas PBMC collected 2.5 months p.i.showed a high level of proliferation with both, which decreasedlater (Table 2). For donor 5, PBMC collected 1.5 months p.i.did not respond to either T. spiralis CWE or IL-2. For the PBMCcollected 2.5 months p.i., the level of proliferation was lowwith T. spiralis CWE and high with IL-2; for the PBMC collected12 months p.i., no proliferation was observed with T. spiralisCWE, whereas proliferation was observed with IL-2, as expected(Table 2).

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TABLE 2. Proliferative responses to T. spiralis CWE and to a control stimulant, IL-2, on day 7 of culture by PBMC from five T. britovi-infected individuals obtained at different times p.i.

Cytokine gene expression in T. spiralis CWE-stimulated PBMC from T. spiralis- and T. britovi-infected donors. Expression of cytokine genes in T. spiralis CWE-stimulated PBMCfrom T. spiralis-infected donors produced three different patterns(Fig. 1). When samples collected 2 months p.i. were used, PBMCfrom five donors showed expression of IL-2, IL-5, and IL-6 (Fig.1A); PBMC from three donors showed expression of IL-2, IL-4,IL-5, and IL-6 (Fig. 1B); and PBMC from two donors showed expressionof IL-2, IL-6, and IFN- ${gamma}$ (Fig. 1C). When samples collected 9months p.i. were used, PBMC from all donors showed expressionof IL-2 and IL-5 (Fig. 1); signals were also observed for IL-6(Fig. 1A), for IL-4 (Fig. 1B), or for IL-6, IL-10, and IFN- ${gamma}$ (Fig. 1C). When samples collected 14 months p.i. were used,PBMC from all donors showed expression of IL-2 (Fig. 1); signalswere also observed for IFN- ${gamma}$ (Fig. 1A), for IL-4, IL-5, and IL-10(Fig. 1B), or for IL-5, IL-6, IL-10, and IFN- ${gamma}$ (Fig. 1C).

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FIG. 1. RT-PCR analysis of cytokine gene expression in stimulated and nonstimulated PBMC cultures with representative patterns (A, B, and C) for 10 T. spiralis-infected donors at 2, 9, and 14 months p.i. (m.p.i.) for ß-actin, IL-2, IL-4, IL-5, IL-6, IL-10, and IFN- ${gamma}$ after 48 h of culture. Lanes 1, nonstimulated PBMC; lanes 2, PBMC stimulated with T. spiralis CWE. The lanes indicated by the arrows contained molecular weight markers.

Expression of cytokine genes in T. spiralis CWE-stimulated PBMCfrom T. britovi-infected donors was studied for the donors whoconsistently showed proliferation (Table 2, donors 1 to 3).At 1.5 months p.i., PBMC from all three of these donors showedexpression of IL-5, IL-10, and IFN- ${gamma}$ (Fig. 2A). PBMC from onedonor also showed expression of IL-2, IL-4, and IL-6 (data notshown). At 12 months p.i., PBMC from all three donors showedexpression of IL-2 and IL-5 (Fig. 2B, C, and D); PBMC from onedonor also showed expression of IL-10 and IFN- ${gamma}$ (Fig. 2B); andPBMC from another donor also showed expression of IL-4, IL-6,IL-10, and IFN- ${gamma}$ (Fig. 2D).

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FIG. 2. RT-PCR analysis of cytokine gene expression in cultures of stimulated and nonstimulated PBMC from three T. britovi-infected donors at 1.5 months p.i. (A) and 12 months p.i. (B, C, and D) for ß-actin, IL-2, IL-4, IL-5, IL-6, IL-10, and IFN- ${gamma}$ after 48 h of culture. Lanes 1, nonstimulated PBMC; lanes 2, PBMC stimulated with T. spiralis CWE. The lanes indicated by the arrows contained molecular weight markers.

Cytokine production. Production of IL-2, IL-5, IL-10, and IFN- ${gamma}$ was determined insupernatants of T. spiralis CWE-stimulated PBMC from T. spiralis-and T. britovi-infected donors after 48 h of culture (Table3). In the three T. spiralis-infected donors, the IL-2 productionat 2 months p.i. was similar to the IL-2 production at 9 monthsp.i. and to the IL-2 production in noninfected controls. At14 months p.i., IL-2 production had slightly increased. IL-5production was greatest at 2 months p.i. IL-10 production remainedconstant over time. IFN- ${gamma}$ production was greatest at 9 monthsp.i. In the three T. britovi-infected donors, IL-2, IL-5, IL-10,and IFN- ${gamma}$ production was also detected at 1.5 months p.i. (Table3).

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TABLE 3. IL-2, IL-5, IL-10, and IFN- ${gamma}$ production in supernatants of PBMC, stimulated or not stimulated with T. spiralis CWE, from three T. spiralis-infected individuals, three T. britovi-infected individuals, and three individuals without a Trichinella infection^a

Flow cytometric analysis. Dead cells were excluded by labeling the cells with propidiumiodine. A cytometric analysis performed with T. spiralis CWE-stimulatedPBMC produced similar results for all infected donors (i.e.,irrespective of the etiological agent) and for all PBMC samples(i.e., irrespective of the time of blood collection). Figure3 shows the results for 36 months p.i. for one T. spiralis-infecteddonor, as an example. The T. spiralis CWE stimulation inducedlight scatter changes in the lymphocyte population, which allowedit to be gated into two subpopulations (Fig. 3B). One subpopulation,with high forward and side scatter (H-FSC), represented 60%of the total lymphocyte population, and the other subpopulation,with low forward and side scatter (L-FSC), represented 40% ofthe total lymphocyte population. In the nonstimulated PBMC,the percentage of L-FSC cells was 82%, whereas the percentageof H-FSC cells was 18% (Fig. 3A); similar results were obtainedwhen MP was used as the antigen (Fig. 3C).

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FIG. 3. Dot plots of cytometric analysis (SSC and FSC) of nonstimulated (A), T. spiralis CWE-stimulated (B), and C. albicans MP-stimulated (C) PBMC collected 36 months p.i. from one T. spiralis-infected donor, showing the L-FSC and H-FSC regions. (A) L-FSC accounted for 82% and H-FSC accounted for 18% of the total cell population. (B) L-FSC accounted for 40% and H-FCS accounted for 60% of the total cell population. (C) L-FSC accounted for 80% and H-FSC accounted for 20% of the total cell population.

A phenotypic analysis was carried out with the H-FSC and L-FSCsubpopulations of T. spiralis CWE-stimulated PBMC, MP-stimulatedPBMC, and nonstimulated PBMC from three T. spiralis-infecteddonors and three T. britovi-infected donors. In the L-FSC subpopulation,no phenotypic variation was observed over time, nor were anyvariations observed among the six donors or for the specificantigens (data not shown).

In the H-FSC subpopulation from T. spiralis-infected donors,the percentages of CD3⁺ and CD4⁺ cells and of cells bearing ${alpha}$ ß T-cell receptor (TCR) decreased from 2 to 9 monthsp.i.; thereafter, no variation was observed. The percentageof CD8⁺ cells increased slightly from 2 to 9 months p.i. anddid not change thereafter. The percentages of CD45RO⁺ and CD45RA⁺cells and of cells bearing ${gamma}$ ${delta}$ TCR (data not shown) remained almostconstant from 2 to 36 months p.i. (Fig. 4).

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FIG. 4. Kinetics and percentages of H-FSC PBMC stimulated with T. spiralis CWE expressing CD3⁺, CD4⁺, CD8⁺, TCR ${alpha}$ ß, CD45RA⁺, and CD45RO⁺ markers from three T. spiralis-infected donors. m.p.i., months postinfection.

In the H-FSC subpopulations from T. britovi-infected donors,at 12 months p.i. the T. spiralis CWE-stimulated PBMC consistedof 27% ± 7% CD4⁺ CD3⁺ cells and 62% ± 9% CD8⁺CD3⁺ cells with 11% ± 6% CD45RA⁺, 76% ± 13% CD45RO⁺,and 56% ± 9% ${alpha}$ ß TCR (Fig. 5). At the same time,the nonstimulated PBMC consisted of 30% ± 8% CD4⁺ CD3⁺cells and 40% ± 13% CD8⁺ CD3⁺ cells with 23% ±6% CD45RA⁺, 56% ± 12% CD45RO⁺, and 59% ± 9% ${alpha}$ ßTCR (Fig. 5). When interpreting the difference in the percentagesof CD8⁺ CD3⁺ cells in the stimulated and nonstimulated PBMC(62% ± 9% and 40% ± 13%, respectively), we hadto take into account the finding that in the nonstimulated PBMCthe H-FSC subpopulation represented only 18% of the total (Fig.3A), whereas in the T. spiralis CWE-stimulated PBMC the H-FSCsubpopulation represented 60% (Fig. 3B).

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FIG. 5. Phenotypic analysis of the high-scatter population of PBMC from one representative T. britovi-infected donor that were not stimulated (dotted bars) or were stimulated with T. spiralis CWE (open bars) or with C. albicans MP (striped bars). Asterisks indicate significant differences (P $<=$ 0.05).

DISCUSSION

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Discussion

Our results show that T. spiralis CWE can induce proliferationfor at least 36 months in PBMC from T. spiralis-infected individualsand for at least 12 months in PBMC from T. britovi-infectedindividuals. A trend toward an increase in CD8⁺ CD3⁺ lymphocytesand a type 2 pattern of cytokines were also observed duringthe muscular phase of Trichinella infection. Muscle biopsy samplescollected 36 months p.i. from T. spiralis-infected donors werestill positive for the presence of viable and mouse-infectingmuscle larvae (data not shown) in spite of the mebendazole treatment(19).

Although both T. spiralis CWE and T. britovi CWE were able toinduce proliferation of PBMC from Trichinella-infected donors,acting as T-cell recall antigens (data not shown), the proliferationinduced by T. spiralis CWE was stronger than that induced byT. britovi CWE, independent of the etiological agent of infection.It is known that in T. spiralis-infected mice, T. spiralis CWEinduces shock and death more often than T. britovi CWE (5).Furthermore, in humans, T. spiralis induces a stronger humoralimmune response than T. britovi (20). Our results also suggestthat the immunogenicity of T. spiralis CWE and the immunogenicityof T. spiralis larvae are greater than the immunogenicity ofT. britovi CWE and the immunogenicity of T. britovi larvae,respectively, as observed in other studies (5).

In the T. spiralis-infected donors, blastogenesis peaked at9 months p.i. (Table 1), whereas in the T. britovi-infecteddonors it peaked at 1.5 months p.i. (Table 2). In the two T.britovi-infected donors who were treated with prednisolone,at 1.5 months p.i. there was a lack of PBMC proliferation withboth T. spiralis CWE and IL-2; proliferation with both was restoredat 2.5 months p.i. in one donor (Table 2, donor 4) and was onlypartially restored (IL-2) at 12 months p.i. in the other donor(donor 5). For donor 5, the low level of proliferation at 2.5months p.i. and the lack of proliferation at 12 months p.i.with T. spiralis CWE could have been due to successful mebendazoletreatment in a person who had acquired a low-level infection.

The pattern of cytokine gene expression varied among donors.Independent of the time after infection, most of the T. spiralisCWE-stimulated PBMC from T. spiralis-infected donors showedexpression of IL-5 and IL-6, and some of these PBMC also showedexpression of IL-4, IL-10, and IFN- ${gamma}$ (Fig. 1). Expression ofIL-2 was not considered because it also occurred in nonstimulatedPBMC. The results suggest that type 2 cytokines were predominantin the first 9 months p.i., and although 14 months p.i. a type2 pattern was still predominant, the presence of IFN- ${gamma}$ expressionsuggested an intermediate type 0 pattern, even if a non-T-cellorigin of IFN- ${gamma}$ could be postulated. T. spiralis CWE-stimulatedPMBC from T. britovi-infected donors showed a pattern similarto that of T. spiralis-infected donors but with earlier expressionof IL-10 and IFN- ${gamma}$ (Fig. 2).

Production of cytokines by the T. spiralis CWE-stimulated PBMCfrom the T. spiralis-infected donors showed different trends;IL-2 production increased slightly over time, IL-10 productionwas constant, IL-5 production reached the highest level 2 monthsp.i., and IFN- ${gamma}$ production increased up to 9 months p.i. anddecreased thereafter. There was a good correspondence betweenthe cytokine expression and production patterns and the antibodyresponse because infected individuals still had high antibodylevels (i.e., IgG titers of $>=$ 1/1,600) at 36 months p.i. (datanot shown). The finding that the T. spiralis CWE-stimulatedPBMC from the T. britovi-infected donors exhibited lower IL-5and IFN- ${gamma}$ cytokine production than the T. spiralis CWE-stimulatedPBMC from the T. spiralis-infected donors is further evidencethat T. spiralis larvae in humans and antigen in vitro bothhave greater immunogenicity than T. britovi larvae and antigen(5, 20). A good correspondence between expression and productionof cytokines by PBMC from all infected individuals was observed,supporting the conclusion that the cytokine response is predominantlya type 2 response during the first 9 months p.i.

The phenotypic analysis of the H-FSC subpopulation showed thatthere was a trend toward a decrease in CD4⁺ cells and a trendtoward an increase in CD8⁺ cells in all Trichinella-infectedindividuals. Phenotypic changes over time were observed in T.spiralis CWE-stimulated PBMC from both T. spiralis- and T. britovi-infecteddonors compared with nonactivated PBMC and MP-activated PBMC.

The increase in the number of CD8⁺ cells and the decrease inthe number of CD4⁺ cells were accompanied by a reduction inthe number of naïve cells and an increase in the numberof memory cells. Changes in PBMC composition, with an increasein the number of CD8⁺ cells and a decrease in the number ofCD4⁺ cells, have been observed in individuals with general immuneactivation caused by persistent helminthic infection (13, 16).

Although PBMC cultures provide no information concerning thenature of the cells that express and produce cytokines, it hasbeen shown that not only CD4⁺ cells but also CD8⁺ cells canbe placed in different subsets on the basis of their cytokineproduction profiles (14, 21). In conclusion, our study of cellularimmunity during the muscular phase of Trichinella infectionin humans showed that CD8⁺ cells were involved and that thecytokine pattern was predominantly a type 2 pattern.

ACKNOWLEDGMENTS

We are grateful to F. Bruschi for his insightful criticism andhelpful suggestions. We are also grateful to M. J. Gomez Miguelfor providing the C. albicans MP.

This work was supported by a research project on emerging andreemerging infectious diseases (Istituto Superiore di Sanitàno. 502/12, Ministry of Health of Italy).

FOOTNOTES

* Corresponding author. Mailing address: Laboratory of Parasitology, Istituto Superiore di Sanità, viale Regina Elena 299, 00161 Rome, Italy. Phone: 39 06 4990 2304. Fax: 39 06 4938 7065. E-mail: pozio{at}iss.it.

Editor: T. R. Kozel

REFERENCES

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