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Infection and Immunity, January 2000, p. 352-359, Vol. 68, No. 1
Departamento de Imunologia, Instituto de
Ciências Biomédicas da Universidade de São Paulo,
São Paulo, Brazil
Received 12 April 1999/Returned for modification 7 May
1999/Accepted 7 October 1999
Using a pulmonary model of infection, we demonstrated previously
that A/Sn and B10.A mice are, respectively, resistant and susceptible
to Paracoccidioides brasiliensis infection. Employing the
same experimental model, we examined herein the role of
CD8+ T cells in the course of paracoccidioidomycosis.
Treatment with anti-CD8 monoclonal antibodies caused a selective
depletion of pulmonary and splenic CD8+ T cells in both
mouse strains. The number of pulmonary CD4+ T cells and
immunoglobulin-positive cells was independent of the number of
CD8+ T cells. In susceptible mice, the loss of
CD8+ T cells by in vivo treatment with anti-CD8 monoclonal
antibodies impaired the clearance of yeasts from the lungs and
increased the fungal dissemination to the liver and spleen. The same
treatment in resistant mice increased fungal dissemination to
extrapulmonary tissues but did not alter the pulmonary fungal load.
Furthermore, CD8+ T-cell depletion did not modify
delayed-type hypersensitivity reactions of A/Sn mice but increased
these reactions in B10.A mice. The production of P. brasiliensis-specific antibodies by resistant and susceptible
mice depleted of CD8+ T cells was similar to that of mice
given control antibody. Histopathologically, depletion of
CD8+ T cells did not disorganize the focal granulomatous
lesions developed by both mouse strains. These results indicate that
CD8+ T cells are necessary for optimal clearance of the
fungus from tissues of mice infected with P. brasiliensis
and demonstrate more prominent protective activity by those cells in
the immune responses mounted by susceptible animals.
Paracoccidioidomycosis (PCM), caused
by Paracoccidioides brasiliensis, a thermally dimorphic
fungus, is the major systemic mycosis caused by a frank pathogen in
Latin America (4, 35). The infection is usually acquired by
the respiratory route, probably by inhalation of airborne propagules
(25, 35). Most infected subjects develop an asymptomatic
pulmonary infection, which indicates that they are resistant hosts.
However, some individuals are susceptible to this fungal agent and
develop overt PCM. The disease presents a wide gamut of clinical and
pathological manifestations, ranging from benign and localized forms to
severe disseminated disease (4, 27). In most cases, the
disease involves the lungs primarily and then disseminates to other
organs and systems.
Experimental (14, 36) and clinical (10, 30, 31,
33) investigations have indicated the relevance of humoral and/or cellular immune responses in the pathogenesis and evolution of PCM.
Specific cell-mediated immune responses seem to play an important role
in resistance to P. brasiliensis. Patients with systemic PCM
tend to show depressed cellular immune responses compared to those with
localized disease (31, 33); also, the most severe forms of
infection are associated with high levels of specific antibodies
(reviewed in reference 10).
Using a murine model of intraperitoneally (i.p.) induced PCM, we
observed significant differences in susceptibility among inbred
strains: A/Sn mice were found to be the most resistant, while B10.A
animals were the most susceptible, to P. brasiliensis infection (8, 9, 36). More recently, using the
intratracheal (i.t.) route of infection, we developed a pulmonary PCM
model with the same inbred mouse strains and verified that A/Sn and B10.A mice maintain the same resistance patterns as those observed with
the i.p. route of infection (12). These studies demonstrated that A/Sn mice develop a chronic benign pulmonary-restricted PCM associated with low mortality rates, the presence of positive and
persistent delayed-type hypersensitivity (DTH) reactions, and
production of high levels of specific antibodies in which immunoglobulin G2a (IgG2a) and IgG3 isotypes are higher than those observed in susceptible mice. In contrast, B10.A mice develop a
progressive disseminated disease resulting in high mortality rates,
discrete DTH reactions, and production of an IgG2b isotype at levels
higher than those observed in the resistant strain.
Studies using athymic BALB/c mice (nu/nu) and their
heterozygous counterparts (nu/+), which are phenotypically
normal, revealed that susceptibility to P. brasiliensis
infection is exacerbated in athymic animals (6). This
demonstrates that the integrity of the cellular immune response is
fundamental to the establishment of resistance mechanisms to P. brasiliensis infection. However, the contributions of the
different components of the T-cell response are unclear.
Various studies have shown that the role of CD8+ T cells in
the immune response may be protective (15, 19, 32),
suppressive (34), or just innocuous (1),
depending both on the infecting organism and on the genetic
characteristics of the host. To our knowledge, the role of
CD8+ T cells in resistance against P. brasiliensis pulmonary infection has never been investigated.
Thus, we have undertaken a series of studies of CD8+
T-cell-depleted A/Sn and B10.A mice, investigating their responses to
i.t. infection. In particular, we have characterized the T- and B-cell
subpopulations in the spleen and lung of infected and CD8+
T-cell-depleted animals and investigated the progression of pulmonary and extrapulmonary infections, the specific DTH reactions, the specific
humoral responses, and the histopathology of pulmonary lesions at weeks
4 and 8 postinfection. The data obtained demonstrate that, irrespective
of the mouse strain, CD8+ T cells are involved in clearance
of fungal cells and in control of dissemination to extrapulmonary
tissues. These cells also seem to play a role in suppressing DTH
reactions in susceptible mice but show a negligible effect on the
pattern of pulmonary lesions, as well as the production of specific
antibody, by both resistant and susceptible mice.
Animals.
Unless otherwise stated, groups of 8 to 10 male
mice (8 to 11 weeks old) from the susceptible (B10.A) and resistant
(A/Sn) strains were used for each period of infection. All animals were bred at the University of São Paulo animal facilities and
provided with acidified water and sterilized food and bedding.
Fungus.
P. brasiliensis Pb18, a highly virulent
isolate (21), was used throughout this investigation. To
ensure the maintenance of its virulence, the isolate was used after
three animal passages (22). Pb18 yeast cells were then
maintained by weekly subcultivation in semisolid Fava Netto's culture
medium (16) at 35°C and used on day 7 after culture. The
yeast cells were washed in phosphate-buffered saline (PBS) (pH 7.2) and
adjusted to 20 × 106 cells/ml based on hemacytometer
counts. Viability was determined with Janus green B vital dye
(3) (Merck, Darmstadt, Germany) and was always higher than
80%.
P. brasiliensis infection.
Mice were
anesthetized and submitted to i.t. P. brasiliensis
infection, as previously described (12). Briefly, after i.p. anesthesia the animals were infected with 106 P. brasiliensis Pb18 yeast cells, contained in 50 µl of PBS, by
surgical i.t. inoculation that allowed dispensing of the fungal cells
directly into the lungs. The skin was then sutured and the mice were
allowed to recover under a heat lamp.
In vivo depletion of CD8+ T cells.
H-35
hybridoma cells secreting rat IgG1 anti-Lyt-2 monoclonal antibody (MAb)
(murine CD8) were used in this study. These cells were grown as ascites
in pristane (Sigma Chemical Co., St. Louis, Mo.)-primed, sublethally
irradiated (550 rads) BALB/c mice. The H-35 antibodies were purified
from ascites as described elsewhere (26) and assessed for
purity by sodium dodecyl sulfate-polyacrylamide gel electrophoresis.
Groups of B10.A and A/Sn mice were given 150 µg of H-35 MAb or normal
rat IgG (controls) by the i.p. route at 1 day before infection with
P. brasiliensis cells (day Cell preparation.
Spleen and lung lymphocyte cell
suspensions were prepared as previously described (19).
Spleen cells were removed and homogenized in RPMI to obtain a single
cell suspension. Erythrocytes were lysed before washing of cells for
staining. Lung-infiltrating lymphocytes were obtained from individual
mice after bronchoalveolar lavage by repeated injections of 1 ml of
sterile PBS (final volume, 3 ml). Lungs were then removed, minced, and
digested for 60 min in digestion buffer (RPMI, 10% fetal calf serum,
antibiotics, and 1 mg of collagenase per ml [Boehringer Mannheim
Biochemicals, Indianapolis, Ind.]). The cell suspension and undigested
fragments were further dissociated by using thick-walled glass tubes
fitted with Teflon pestles, washed, and pelleted, and erythrocytes were lysed. The lymphocytes were then isolated by standard Percoll (Pharmacia Biotech AB, Uppsala, Sweden) gradient centrifugation. Cells
were recovered and counted, and viability was determined with trypan
blue vital stain.
Cytofluorometry.
The efficiency of in vivo CD8+
T-cell depletion and the effect of i.t. infection on the profile of
lymphocyte subpopulations were determined at 4 weeks postinfection by
flow cytofluorometric analysis. Cells were obtained from the spleen and
lung of mice inoculated with the MAb or normal rat IgG and i.t.
infected with 106 P. brasiliensis yeast cells.
Normal, saline-injected as well as only infected animals were used as
controls. Cell suspensions of each animal were washed, adjusted to
5 × 106 viable cells/ml, and stained with
phycoerythrin-conjugated anti-CD4, anti-CD8, or rat anti-mouse Ig MAb
(Pharmingen, San Diego, Calif.). The stained cells were analyzed
immediately by FACScan equipment using PC-Lysys software (Becton
Dickinson, San Jose, Calif.) and gating on lymphocytes as judged from
forward and side light scatter. Ten thousand lymphocytes were counted,
and the data are expressed as the number of viable CD8+ T
cells, CD4+ T cells, and Ig+ cells. The
efficiency of the CD8+ T-cell depletion was assessed by
calculating the decrease of this subpopulation relative to infected,
normal IgG-treated animals.
Assay for organ CFU.
The numbers of viable microorganisms in
the lungs, liver, and spleen from CD8+ T-cell-depleted and
nondepleted mice were determined by counting the numbers of CFU. Eight
to 10 animals from each mouse strain were sacrificed at 4 and 8 weeks
postinfection, and enumerations of viable organisms in the three organs
were done by counting the numbers of CFU, as previously described
(37). Briefly, aliquots (100 µl) of the cellular
suspensions of each organ were plated on brain heart infusion agar
(Difco) supplemented with 4% (vol/vol) horse serum (Instituto
Butantan, São Paulo, Brazil) and 5% Pb192 culture filtrate, the
latter constituting a source of growth-promoting factor. Plates were
incubated at 35°C, and colonies were counted daily until no increase
in counts was observed. The numbers (log10) of viable
P. brasiliensis colonies per gram of tissue are expressed as
means ± standard errors.
DTH assay.
DTH reactions were always evaluated just before
sacrifice of the animals used in the CFU assays by the footpad test,
under previously determined conditions (17). Briefly, mice
were inoculated with 25 µl of Fava Netto's antigen (16)
and footpad thickness was measured with a caliper (Mitutoyo
Corporation, Tokyo, Japan) immediately before and 24 h after
antigen inoculation. The increase in thickness was calculated and
expressed in millimeters. Noninfected mice submitted to the footpad
test were used as controls.
Specific antibody levels.
Specific antibody levels (total
Ig, IgM, IgG1, IgG2a, IgG3, and IgG2b) were measured by a previously
described enzyme-linked immunosorbent assay (ELISA) (12)
employing a cell-free antigen (11) prepared from a pool of
different P. brasiliensis isolates (Pb339, Pb265, and Pb18).
The average of the optical densities obtained with sera from control
mice (PBS inoculated), diluted 1:20, was considered the cutoff for each
respective isotype. Optical densities for each dilution of experimental
serum were compared to control values. The titer for each sample was
expressed as the reciprocal of the highest dilution which presented
absorbance higher than the cutoff.
Histopathologic analysis.
Groups of five normal rat
IgG-treated and CD8+ T-cell-depleted P. brasiliensis-infected A/Sn and B10.A mice were killed at week 4 after infection. Lungs were collected, fixed in 10% formalin, and
embedded in paraffin. Five-micrometer sections were stained by the
hematoxylin-eosin method. Pathologic changes were analyzed based on the
number, size, morphology, and cell composition of granulomatous
lesions, number of fungi, and intensity of inflammatory infiltrates.
Statistical analysis.
The results obtained in the groups of
each mouse strain were analyzed by nonparametric two-way analysis of
variance (Kruskal-Wallis method) followed by multiple comparisons
according to Dunn's procedure (41). A P value of
<0.05 was considered significant.
Phenotypic characterization of cells in the spleen and lungs of
mice.
To evaluate the efficiency of anti-CD8 MAb in vivo
administration as well as its specificity, the phenotypes of
lymphocytes obtained from the lungs and spleen of infected and control
mice were determined by flow cytometric analysis. Four groups
(n = 4 to 6) of A/Sn and B10.A mice were used:
saline-injected normal mice, P. brasiliensis-infected mice,
and infected mice treated with either normal rat IgG or
anti-CD8+ T cell MAb. At week 4 of the experiment, splenic
lymphocytes were analyzed to monitor T-cell depletion and revealed a
significant decrease of CD8+ T lymphocytes in the
anti-CD8-treated group (71.5%, P = 0.004 [for A/Sn
mice]; 67.1%, P = 0.005 [for B10.A mice]). This
fact is reflected in the increased CD4/CD8 ratios detected in the
MAb-treated groups (Fig. 1). Flow
cytometric analysis of lymphocytes found in the lungs of B10.A mice by
week 4 of infection (Table 1)
demonstrated an increased number of CD4+ T cells,
CD8+ T cells, and Ig+ cells in the P. brasiliensis-infected and normal IgG-treated groups. The
equivalent groups of A/Sn mice presented increased numbers of
CD4+ T cells and Ig+ cells but not of
CD8+ T lymphocytes. These data indicate that both
CD4+ and CD8+ T cells are involved in the
pulmonary immune response developed by susceptible animals, while in
the resistant strain the CD4+ T cells constitute the major
subpopulation involved in the local inflammatory response. Thus, a
twofold increase in the CD4/CD8 ratio was detected in A/Sn mice but not
in B10.A animals. Treatment with anti-CD8 MAb led to a specific
decrease in the CD8+ T-cell subset in both mouse strains
(62.8%, P = 0.05 [for A/Sn mice]; 77.7%,
P = 0.035 [or B10.A mice]) when compared with the normal IgG-treated group. An important observation was that
Ig+ and CD4+ T-cell influx still occurred in
mice depleted of CD8+ cells. Analysis of bronchoalveolar
lavage cells gave results similar to those obtained with
lung-infiltrating lymphocytes (data not shown).
0019-9567/0/$04.00+0
Copyright © 2000, American Society for Microbiology. All rights reserved.
Depletion of CD8+ T Cells In Vivo Impairs Host
Defense of Mice Resistant and Susceptible to Pulmonary
Paracoccidioidomycosis
ABSTRACT
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Abstract
Introduction
Materials and Methods
Results
Discussion
References
INTRODUCTION
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Abstract
Introduction
Materials and Methods
Results
Discussion
References
MATERIALS AND METHODS
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Abstract
Introduction
Materials and Methods
Results
Discussion
References
1) and 100 µg of H-35 MAb or
rat IgG weekly for 8 weeks thereafter. Infected, noninfected, and
nondepleted mice were all used as controls.
RESULTS
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Abstract
Introduction
Materials and Methods
Results
Discussion
References
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FIG. 1.
Quantitation of splenic lymphocytes and CD4/CD8 ratios
in infected and CD8+ T-cell-depleted mice. Groups
(n = 4 to 6) of A/Sn and B10.A mice are as follows:
saline-injected normal mice (Saline), P. brasiliensis-infected mice (Pb), infected mice treated with normal
rat IgG (Pb + Normal IgG), and infected mice treated with
anti-CD8+ T-cell MAb (Pb + 
-CD8). Spleens were
harvested at week 4 of the experiment. Data represent the numbers of
positively fluorescent cells expressing forward- and side-scatter
characteristics of lymphocytes.
TABLE 1.
Flow cytometric analysis of CD4+,
CD8+, and Ig+ lung-infiltrating lymphocytes
from P. brasiliensis-infected mice treated with
anti-CD8+ T-cell MAb
Effect of in vivo depletion of CD8+ T cells on severity of infection. The evolution of disease in IgG-treated and CD8-depleted A/Sn and B10.A mice was monitored by CFU counts in the lungs, spleen, and liver at 4 and 8 weeks after infection (Fig. 2). Depletion of CD8+ T cells of resistant animals did not alter the infection pattern at the 4th week postinfection. The fungal load in the lungs (4.1472 ± 0.2740 log10 CFU/g of tissue) was similar to that found in the nondepleted A/Sn mice (4.1184 ± 0.2557 log10 CFU/g of tissue), and no fungal dissemination to other organs could be observed in either depleted or nondepleted mice. However, at the 8th week after infection, CD8+ T-cell-depleted A/Sn mice displayed fungal dissemination to the liver (0.9938 ± 0.2770 log10 CFU/g of tissue) and spleen (1.6480 ± 0.7098 log10 CFU/g of tissue) that could not be seen in nondepleted A/Sn mice. Although depletion of CD8+ T cells induced a disseminated pattern of disease, the pulmonary fungal load (5.7208 ± 0.0855 log10 CFU/g of tissue) was similar to that found in nondepleted animals (5.4815 ± 0.0627 log10 CFU/g of tissue).
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Effect of CD8+ T-cell depletion on pulmonary lesions. The increased fungal load and extrapulmonary dissemination observed in CD8+ T-cell-depleted mice suggested that this T-cell subpopulation could interfere, at least in susceptible mice, in the morphology of pulmonary lesions. Thus, we analyzed lung sections from IgG-treated and anti-CD8 MAb-treated A/Sn and B10.A mice at week 4 postinfection. All studied mice presented circumscribed granulomatous lesions scattered in the lungs, localized preferentially around the bronchi, bronchioles, and blood vessels. In both groups of A/Sn mice (anti-CD8 MAb or rat IgG treated), the patterns of the lesions were similar, with few granulomas and preservation of the pulmonary parenchyma (Fig. 3A and C). The cellular compositions of the lesions were also qualitatively the same, with multinucleated giant cells often containing P. brasiliensis yeasts and the presence of a peripheral sheet of lymphocytes and plasmocytes, although in the CD8-depleted group the multinucleated giant cells were more frequent and larger than those observed in the IgG-treated group (Fig. 3B and D). In B10.A mice, the depletion of CD8+ T cells also did not change the pattern of granulomas but increased the intensity of the inflammatory reaction (Fig. 3E and G). Actually, B10.A mice depleted of CD8+ T cells showed more severe pulmonary involvement than all the other studied groups, as verified by the increased size of granulomas and their fungal load. The lesions observed in B10.A mice were formed by foci of macrophages and polymorphonuclear leukocytes around Pb18 yeasts; in the CD8-depleted group the polymorphonuclear cell infiltrate was more prominent than in the control group (Fig. 3F and H). In this mouse strain, the presence of multinucleated giant cells was less intense than that observed in A/Sn mice.
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Effect of in vivo depletion of CD8+ T cells on DTH response. To assess the influence of CD8+ T cells on the DTH response during pulmonary PCM, CD8+ T-cell-depleted A/Sn and B10.A animals were evaluated at weeks 4 and 8 after infection. The reactions of these animals were compared to three nondepleted control groups: normal (noninfected) mice, infected mice, and mice infected and treated with normal rat IgG. As shown in Fig. 4, infected A/Sn and B10.A mice, regardless of the treatment, always presented significant DTH responses compared to normal mice at the two assayed points postinfection. Depletion of CD8+ T cells in A/Sn mice induced a slightly lower DTH reaction compared to their infected, nondepleted counterparts, at both the 4th and 8th week postinfection. Susceptible mice displayed the opposite behavior: depletion of CD8+ T cells induced DTH responses at week 4 and 8 postinfection that were significantly more intense than those found in nontreated or normal rat IgG-treated, infected controls.
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Effects of in vivo depletion of CD8+ T cells on specific humoral immune responses. Cytokines produced by CD4+ and CD8+ T cells play an important role in regulation of the humoral immune response and isotype switching (23, 38, 39). Moreover, previous studies from our group have demonstrated that the humoral immune response against most P. brasiliensis components is T-cell dependent (7). Thus, we studied the influence of the integrity of the CD8+ T-cell subset on specific antibody production during pulmonary infection of mice treated with control IgG or H-35 MAb. At 4 and 8 weeks postinfection, sera were collected and assayed for their contents of specific total Ig, IgM, IgG1, IgG2a, IgG2b, and IgG3. Control animals treated with normal rat IgG commonly presented higher levels of specific anti-P. brasiliensis antibodies than did nontreated controls, although the difference was usually not significant (Fig. 5). At week 4 of infection, no significant differences were found between normal IgG-treated and CD8-depleted groups (data not shown). When treatment was given for 8 weeks, antibody titers were usually higher than those verified at week 4 postinfection. A decrease in total Ig and IgG1 levels was observed in A/Sn MAb-treated mice compared to their normal rat IgG-treated counterparts. On the other hand, prolonged CD8+ T-cell depletion in B10.A mice did not induce significant differences in isotype titers relative to normal IgG-treated animals.
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DISCUSSION |
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Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
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Data determined by CFU counts in the lungs, liver, and spleen of i.t. infected mice clearly demonstrated that, during experimental P. brasiliensis infection, depletion of CD8+ T cells induces a more severe and/or disseminated disease in both resistant and susceptible mice. Depletion of CD8+ T cells of A/Sn mice during 4 weeks did not alter the degree of infection, thus suggesting that CD8+ T cells may not play an important role at the initial phases of the disease of resistant animals. However, CD8+ T cells appear to be involved in later control of pulmonary infection, hampering the escape of fungal cells to other organs, since prolonged depletion (8 weeks) resulted in extrapulmonary fungal dissemination, although the pulmonary infection remained unaffected. In susceptible mice, however, CD8+ T cells seem to have a protective role already at the beginning of the infection, since at the 4th week postinfection CD8+ T-cell-depleted mice presented an exacerbated pulmonary infection and precocious fungal dissemination to the liver and spleen; this profile was maintained after prolonged times of depletion.
The decrement in splenic and pulmonary CD8+ T cells in resistant and susceptible mice given anti-CD8+ T-cell MAb ranged from 62.8 to 77.7%. Despite the incomplete elimination of CD8+ T cells in P. brasiliensis-infected mice, at week 4 the number of pulmonary yeast cells increased more than 10,000-fold in susceptible mice, demonstrating that CD8+ T cells play at an early time an important role in the clearance of P. brasiliensis. A similar degree of CD8+ T-cell depletion, however, did not affect the fungal burden in the lungs of resistant animals, showing a more prominent participation of this T-cell subpopulation in the susceptible strain.
An important observation was that the inflammatory influx into the lungs of susceptible mice was composed of CD4+ and CD8+ T cells, whereas in resistant mice only the former subpopulation appears in slightly increased numbers. This picture agrees with CFU data at week 4 of infection when depletion of CD8+ T cells affected fungal pulmonary loads only of susceptible mice. Altogether these data appear to indicate that the pulmonary protective immune responses mounted by B10.A mice involve the contribution of CD4+ and CD8+ T cells, whereas in A/Sn mice the CD4+ T-cell subset is mainly involved.
Imbalances in T-cell subsets have also been described for human PCM. In T-cell subpopulations in the peripheral blood of patients with acute or chronic forms of PCM, a significant fall in the CD4/CD8 T-cell ratio was detected (2, 30). Some authors observed decreased numbers of CD4+ and CD8+ T cells (30), whereas others reported a decrease only in the CD4+ subset (2). The mucous and skin granulomatous lesions of PCM patients presented an elevated CD4/CD8 T-cell ratio due to high numbers of infiltrating CD4+ T cells; this ratio in the blood, however, was very low (29). These findings showed that the phenotype of cells found in the blood does not reflect the subsets infiltrating the lesions.
In an analysis of the histopathological data obtained at 4 weeks
postinfection, two intensities of lesions were detected: more
pronounced in B10.A mice depleted of CD8+ T cells and less
pronounced in the three other groups studied. Thus, the increase in the
severity of the lesions and in the number of yeasts present in the
lungs of depleted animals confirm the protective role of
CD8+ T cells in the susceptible strain. This picture was
not found in resistant A/Sn mice, in which the absence of
CD8+ T cells did not affect the number and intensity of
pulmonary inflammatory lesions. Even in susceptible mice, absence of
CD8+ T cells did not cause remarkable alterations in the
patterns of pulmonary lesions, such as those caused by the depletion of gamma interferon (IFN-
), which resulted in complete disorganization of the pulmonary structure (13). The data presented herein
are in accordance with those reported by Deepe (15), who
studied the role of CD8+ T cells in murine histoplasmosis;
no differences in the histopathological patterns of splenic and hepatic
lesions were detected between depleted and control mice. As already
shown, multinucleated giant cells were found more consistently in
resistant than in susceptible mice. Analogously to what was reported by
Hill in experimental cryptococcosis (18), most of these
cells contained ingested fungi, suggesting a protective role of giant
cells in experimental PCM.
In humans (reviewed in reference 4), as well as in
our isogenic murine model of PCM (reviewed in reference
8), positive DTH reactions correlate with less
severe disease. Regarding the involvement of CD8+ T cells
in the specific DTH reaction, it became clear from our studies that in
vivo depletion of CD8+ T cells does not alter significantly
the DTH responses of resistant animals but significantly increases
these reactions in susceptible mice. These results suggest that
CD8+ T-cell subsets could be suppressing, at least
partially, the DTH reactions in susceptible animals and confirm the
studies by Jimenez-Finkel and Murphy (20), demonstrating
that intravenous treatment of mice with P. brasiliensis
antigens induces production of suppressor T cells that impair specific
DTH responses. Thus, unexpectedly, in B10.A mice, protective immunity
and DTH responses are dissociated traits. Our results suggest that
CD8+ T cells could be involved in both protection against
P. brasiliensis (perhaps by mean of their cytotoxic activity
or ability to secrete IFN-) and negative regulation of DTH
responses. This dual role exerted by CD8+ T cells in
susceptible mice deserves further investigation using purified T-cell
subsets. In murine leishmaniasis, using susceptible BALB/c mice Liew et
al. (24) have also observed a dissociation between
protective immunity and DTH responses. They reported that previous
subcutaneous immunization with irradiated promastigotes of
Leishmania major induced an increased DTH reactivity in
parallel with more severe disease. The influence of CD8+ T
cells on DTH reactions was also observed in studies with other fungal
diseases. Depletion of CD8+ T cells during experimental
cryptococcosis is associated with suppression of specific DTH responses
(28), whereas depletion of these cells does not alter the
onset or maintenance of DTH reactions in histoplasmosis
(15).
High levels of circulating antibodies are directly related to the severity of PCM, although their pathophysiologic significance is still unknown (4, 10). When antibody production was analyzed herein, it was observed that treatment with normal IgG stimulated production of higher antibody levels independently of the mouse strain. A recent publication (40) reported that high concentrations of normal Ig induce the activation of CD4+ T cells and B cells. This fact could explain, at least partially, the increments in antibody levels observed in this study. When IgG-treated controls were compared to CD8-depleted mice, no significant differences in antibody levels were detected except for the decreased levels of total Ig and IgG1 in strain A/Sn at week 8 of infection, indicating that CD8+ T cells are not primarily involved in control of antibody production. In a previous work using athymic and euthymic BALB/c mice (7), it was verified that the majority of P. brasiliensis antigens are T-cell-dependent components since only T-cell-sufficient mice were able to produce anti-P. brasiliensis antibodies. The results obtained herein confirm the CD4+ T-cell subset as the major regulator of antibody production, since depletion of CD8+ T cells only peripherally affected antibody production. Indeed, in vivo CD4+ T-cell depletion experiments practically abrogate antibody production by resistant and susceptible mice after P. brasiliensis infection (L. E. Cano and V. L. G. Calich, unpublished data).
It is well known that exogenous foreign protein antigens are presented to CD4+ T cells by class II major histocompatibility complex (MHC) molecules, whereas CD8+ T lymphocytes recognize endogenous peptides bound to class I MHC molecules. Despite the preferential endosomal behavior of P. brasiliensis yeast cells (5), the experiments described herein indicate that fungal antigens probably can be presented by MHC class I molecules. Moreover, our results suggest that, early in disease, antigen processing by antigen-presenting cells of susceptible animals may be different from that of resistant mice. Although many aspects of CD8+ T-cell recruitment, activation, and interaction with other cells remain to be better elucidated, our results clearly show, for the first time, that CD8+ T cells are protective in experimental PCM and that the genetic pattern of the host is a determinant in the intensity of CD8+ T-cell activation.
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ACKNOWLEDGMENTS |
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We are grateful to R. G. Landgraf and B. P. Albe for technical assistance. We are also grateful to G. B. Huffnagle for expert orientation in obtaining lung-infiltrating lymphocytes.
C. Arruda was a recipient of a fellowship from Fundação de Amparo à Pesquisa do Estado de São Paulo (FAPESP), and L. E. Cano was supported by a Ph.D. fellowship (92/0962-9) from FAPESP. This work was supported by grants from FAPESP and CNPq.
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FOOTNOTES |
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* Corresponding author. Mailing address: Depto. de Imunologia, Instituto de Ciências Biomédicas, Universidade de São Paulo, Av. Prof. Lineu Prestes 1730, Cep 05508-900, São Paulo SP, Brazil. Phone: 55-11-818 7397. Fax: 55-11-818 7224. E-mail: vlcalich{at}icb.usp.br.
Present address: Laboratório de Micologia Experimental,
Corporación para Investigaciones Biológicas (CIB),
Medellín, Colombia.
Editor: S. H. E. Kaufmann
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REFERENCES |
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Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
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