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Infection and Immunity, October 2000, p. 5771-5777, Vol. 68, No. 10
0019-9567/00/$04.00+0
Copyright © 2000, American Society for Microbiology. All rights reserved.
Cellular and Cytokine Correlates of Mucosal
Protection in Murine Model of Oral Candidiasis
Shokrollah
Elahi,1
Gerald
Pang,1
Robert
Clancy,1,* and
Robert B.
Ashman2
Discipline of Immunology and Microbiology,
University of Newcastle, Newcastle, New South Wales,
2300,1 and School of Dentistry,
University of Queensland, Brisbane, Queensland
4072,2 Australia
Received 11 May 2000/Accepted 7 June 2000
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ABSTRACT |
Host protection against Candida albicans infection in a
model of oral candidiasis involving infection-prone [DBA/2
(H-2d)] and less infection-prone [BALB/c
(H-2d)] mouse strains was analyzed in terms of
antibody and cellular responses, and in terms of cytokine patterns from
regional lymph node cells. There was a selective expansion of
/
+ T-cell receptor cells, which correlated with the
patterns of colonization in both mouse strains, with higher numbers of
/ T cells detected in BALB/c mice. Antigen-induced T-cell
proliferation was significantly higher in BALB/c mice than in DBA/2
mice. Higher levels of serum immunoglobulin G (IgG) and salivary IgA
antibodies were detected in BALB/c mice than in DBA/2 mice, but only
after the infection was cleared. The cervical lymph node cells from infected mice were assessed for interleukin-4 (IL-4), IL-12, and gamma
interferon (IFN-) mRNA gene expression by reverse transcription-PCR and protein production in the culture supernatants following
restimulation in vitro. In BALB/c mice, an early increase in levels of
IL-4, IFN-, and IL-12 correlated with rapid elimination of C. albicans. In DBA/2 mice, where resolution of infection was
delayed, IL-4 message expression was delayed and the IL-4 secretion
level was lower. Neutralization of IL-4 by multiple injections of an
anti-IL-4 monoclonal antibody in BALB/c mice resulted in increased
carriage rate and delayed clearance of the yeasts. Collectively, the
data suggest that the T-cell response to C. albicans in the
regional lymph nodes which correlates best with rapid oral clearance of C. albicans is a balanced Th0 cytokine response involving
early secretion of both IFN- and IL-4.
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INTRODUCTION |
Candida albicans is a
yeast-like fungus that colonizes human mucosal surfaces of the mouth,
vagina, and gastrointestinal tract as part of the normal microbial
flora. It is also an opportunistic pathogen that can cause stomatitis
and vaginitis. Under certain conditions it can invade tissues and cause
systemic infection (6, 17, 19, 32, 43). Both clinical and
animal studies indicate that containment within the oral cavity is in
part determined by CD4+ T lymphocytes (7,
12-14), while recurrent vaginal infection is predicated by a
reduction in the circulating Candida-reactive T-cell pool
(8). Invasive infection is uncommon in subjects with T-cell
deficiency but is common in subjects with neutropenia (2) or
neutrophil dysfunction (2), suggesting that different mechanisms operate to contain mucosal spread compared to those responsible for systemic immunity. In murine studies to determine the
exact mechanism of protection using genetically manipulated mice or
contrived experimental conditions, conflicting results have been
obtained as to the cytokine mix most relevant to protection (24,
27, 33-39). Resistance to systemic infection in some murine strains identifies Th1 effector cells producing gamma interferon (IFN-) and interleukin-12 (IL-12) as mediators of protection (9, 37, 41, 42). By contrast, in other studies,
susceptibility to infection has been linked to Th2 cells producing IL-4
and IL-10, which in turn downregulate Th1 effector cells (38,
40). A valuable natural model of oral infection has been the
development of an oral infection in the BALB/c and DBA/2 mouse strains,
which share the same H-2d major
histocompatibility locus complex but which show different rates of
spontaneous clearance from the buccal cavity (12). In this
model the local cellular immune response is characterized by the
recruitment of CD4+, CD8+, and / T cells
within the mucosa (12, 38). The molecular mechanisms
mediating protection, however, remain unclear.
To clarify the mechanisms of protection in this model of oral
candidiasis, we have examined the patterns of cytokine and antibody response in both naive and primed animals. The results support the
proposal that a balanced (Th0) cytokine response is important in
mucosal protection in this model of oral infection.
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MATERIALS AND METHODS |
Mice.
Male BALB/c (H-2d) and DBA/2
(H-2d) mice, 6 to 8 weeks old, were purchased
from the Animal Resource Center, Perth, Western Australia. They were
housed in groups of three to five and provided with food and water ad
libitum. All mice were used after 1 week of acclimatization.
Fungal culture.
C. albicans isolate 3630 was obtained
from the National Reference Laboratory, Royal North Shore Hospital,
Sydney, Australia. The yeast cells were cultured in Sabouraud dextrose
broth (Oxoid, Basingstoke, Hampshire, United Kingdom) for 48 h at
25°C in a shaking water bath. The blastospores were transferred into
fresh medium and cultured at 25°C for a further 18 h. Then the
blastospores were collected by centrifugation, washed twice with
phosphate-buffered saline (PBS), and adjusted to 108
blastospores per ml in PBS until use.
Candida antigen.
Freshly cultured C. albicans
isolate 3630 organisms were resuspended in PBS at 1010
cells/ml and then sonicated in an MSE Soniprep set at an amplitude of
10 for 30 cycles with intermittent cooling and sonication. The sonicate
was centrifuged for 10 min at 2,000 × g, after which the supernatant was collected and dialyzed against PBS. After protein
estimation, the solution was filter sterilized and stored in aliquots
at 
20°C until use.
Oral infection.
Mice were anesthetized by intraperitoneal
injection with 75 µl of ketamine-Xylazil (100 mg/ml and 20 mg/ml,
respectively). They were orally inoculated with the blastospores by the
method described by Chakir et al. (12). Briefly,
108 blastospores/ml in PBS were centrifuged at
14,000 × g for 5 min. The pellet was recovered on a
fine-tip sterile swab (Corsham, MW & E, Wiltshire, United Kingdom)
which was then used for oral inoculation by topical application.
Quantitation of oral infection.
Groups of mice (three to
five per group) were sacrificed at various time points to determine the
number of C. albicans organisms in the oral mucosa. The oral
cavity (i.e., cheek, tongue, and soft palate), was completely swabbed
using a fine-tip cotton swab. After swabbing, the cotton end was cut
off and then placed in an Eppendorf tube containing 1 ml of PBS. The
yeast cells were resuspended by mixing on a vortex mixer before culture
in serial 10-fold dilutions on Sabouraud dextrose agar (Oxoid)
supplemented with chloramphenicol (0.05 g/liter) for 48 h at
37°C. For histological studies, oral tissues were fixed in 10%
formalin and embedded in paraffin. Tissue sections 5 mm thick were cut,
mounted on glass slides, and then stained with hematoxylin and eosin
(H&E) or periodic acid-Schiff (PAS) stain for fungi. The numbers of
blastospores and hyphal forms were enumerated by light microscopy. The
results were expressed as the mean count of five fields at a
magnification of ×40.
Cell separation and flow cytometry.
The cervical lymph nodes
(CLN) were excised from three to five C. albicans-infected
mice for each time point after infection, and single-cell suspensions
were prepared (18). Pooled CLN populations were analyzed in
two-color mode using Lysis 2 software and FACSan cytometry (Becton
Dickinson, Mountain View, Calif.). The monoclonal antibodies (MAbs)
used for staining were fluorescein isothiocyanate (FITC) conjugated
(H129.19 anti-CD4 and H57-597 anti-
/
T-cell receptor [TCR]) or
phycoerythrin (PE) conjugated (H53-6.7 anti-CD8, ID3 anti-CD19, and
GL3 anti-/ TCR). FITC- or PE-conjugated isotype-matched antibodies were used as negative controls. All MAbs were purchased from
PharMingen (San Diego, Calif.). At least 10,000 viable cells from each
preparation were used for analysis.
Lymphoproliferation assay.
Pooled CLN cells in RPMI 1640 medium supplemented with 10% fetal calf serum (FCS) were cultured in
triplicate at 0.2 × 106 cells per well in wells of a
96-well round-bottom microtiter plate (Nunc, Roskilde, Denmark).
C. albicans antigen was added to each well at a final
concentration of 2.5 µg/ml. The cultures were incubated for 72 h
under an atmosphere of 5% CO2 in a humidified incubator.
Thymidine incorporation was measured by pulsing the cells with 1 µCi
of 3H-labeled thymidine (Amersham, Aylesbury, United
Kingdom) for the final 6 h of incubation before harvesting and
counting. The results were expressed as mean counts per minute ± standard errors of the means (SEM).
Antibody assay.
A microplate enzyme-linked immunosorbent
assay (ELISA) was used to quantitate specific antibody in the saliva
and serum (37, 38). Immunopolysorb microtiter (Nunc) wells
were coated with 50 µl of C. albicans antigen/ml in 0.1 M
sodium borate-buffered saline (pH 8.4). Appropriate serial dilutions of
the serum and saliva samples were added to each well. Bound antibodies
were detected by the addition of biotinylated goat anti-mouse
immunoglobulin G (IgG) or IgA (Sigma-Aldrich) followed by alkaline
phosphatase-conjugated streptavidin (AMRAD, Melbourne, Australia).
After addition of the substrate solution, the optical density of
duplicate samples was read at 450 nm with an ELISA plate reader
(Bio-Rad, Richmond, Va.).
RT-PCR.
RNA extraction and amplification of synthesized cDNA
from lymphoid cells have been described elsewhere (29, 39).
Briefly, 10 µl of total RNA extracted from 4 × 106
CLN cells/ml was added to 20 µl of reverse transcriptase (RT) mix
containing 6 µl of 5× RT reaction buffer (250 mM Tris-HCl, 375 mM
KCl, and 15 mM MgCl2), 3 µl of 100 mM dithiothreitol, 1.5 µl of deoxynucleotides (10 mM), 1 µl of RNase inhibitor (40 U/ml), 0.5 µl of Moloney murine leukemia virus (MMLV) RT (200 U/ml), 3 µl
of oligo(dT)15', 3 µl of acetylated bovine serum albumin (BSA; 1 mg/ml), and 2 µl of diethyl pyrocarbonate (DEPC)-treated water. The cDNA synthesis was carried out at 42°C for 1 h
followed by heating at 72°C for 10 min. PCR amplification was carried
out by adding 5 µl of the first-strand cDNA to the PCR mix containing 1 µM each primer (20 µM), 1 µl of 4 mM deoxynucleoside
triphosphate (dNTP) mix, 5 µl of 10× PCR buffer, 1.2 µl of 1.5 mM
MgCl2, 0.2 µl of Taq DNA polymerase (50 U/ml),
and 31 µl of DEPC-treated water. The mixture was subjected to
amplification using a thermal cycler (Hybaid, Ashford, Middlesex,
United Kingdom) set at 94°C for 1 min (IL-4 and G3DPH) and 30 s
(for IFN-), 60°C for 2 min (IL-4 and G3DPH) and 62°C for 1 min
(IFN-), and 72°C for 3 mins (IL-4 and G3DPH) and 90 s (for
IFN-), with a final elongation step at 72°C for 10 min. PCR
amplification was carried out for 35 to 40 cycles. PCR fragments were
separated by 2% agarose gel electrophoresis, stained with ethidium
bromide, and then viewed under a UV transilluminator. For IL-4, the
sense primer was GAA TGT ACC AGG AGC CAT ATC and the antisense primer
was CTC AGT ACT ACG AGT ATT CCA; for IFN-, the sense primer was TCT
CTC CTG CCT GAA GGA C and the antisense primer was ACA CAG TGA TCC TGT
GGA A. The amplified DNA products for IL-4 and IFN- were 399 and 460 bp, respectively.
Cytokine assay.
CLN cells in RPMI 1640 medium supplemented
with 10% FCS were cultured at 4 × 106 cells per well
in the presence of 2.5 µg of C. albicans antigen/ml in a
24-well plate for 3 days (as described above). The culture supernatants
were collected and then assayed for IL-4, IL-12, and IFN- by ELISA
using matched-antibody pairs and recombinant cytokines as standards
(PharMingen). Briefly, Immuno-polysorb microtiter plates (Nunc) were
coated with a capture rat monoclonal anti-IL-4 (IgG1), anti-IL-12
(IgG2a), or anti-IFN- (IgG1) antibody at 1 µg/ml in sodium
bicarbonate buffer (pH 9.6) overnight at 4°C. The wells were washed
and then blocked with 1% BSA before the culture supernatants and the
appropriate standard were added to each well. Biotinylated rat
monoclonal anti-IL-4, anti-IL-12, or anti-IFN- antibody at 2 µg/ml
was added as the second antibody. Detection was done with streptavidin
peroxidase (AMRAD) and TMB (Sigma-Aldrich). The sensitivity of the
cytokine ELISAs was 31 pg/ml. The results were expressed as net
Candida-induced counts from which the background was subtracted.
Infection and treatment with anti-IL-4 MAb.
Mice were
injected intraperitoneally (i.p.) with 30 µg of rat anti-recombinant
IL-4 (rIL-4) (29) (clone 11B11; PharMingen) or with the
purified rat IgG1 matched isotype in 200 µl of PBS per mouse at days
1, 3, and 5 after oral infection with 108 yeast cells. The
number of yeasts in the oral cavity was determined as described above.
Statistical analysis.
The data were compared using the
nonparameteric Mann-Whitney U test. P values of < 0.05 were considered significant. All calculations were performed using a
statistical software program (StatView; Abacus Concepts, Berkeley,
Calif.).
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RESULTS |
Kinetics of oral infection by C. albicans in BALB/c and
DBA/2 mice.
The oral mucosae of BALB/c and DBA/2 mice were
infected with 108 C. albicans blastospores on
day 0, after which time the level of colonization was examined over 28 days. As shown in Fig. 1A, the levels of
colonization 6 h after infection were similar in BALB/c and DBA/2
mice. However, resistance to infection in BALB/c mice was evident at
day 2 after an initial reduction in colonization at day 1 after
inoculation, compared with a 1-log-unit increase in the number of
yeasts in DBA/2 mice (P < 0.05). While there was a
decrease in colonization in BALB/c and DBA/2 mice on day 4, a
2-log-unit increase in the number of yeasts occurred on day 6 in DBA/2
mice (P < 0.001), compared with BALB/c mice. By day 8, the BALB/c mice had no yeasts in the oral cavity, whereas in DBA/2 mice
the number of yeasts was above 3 log units, which gradually declined to
background level by day 15. Cultures of fecal pellets from mice after
inoculation of C. albicans showed no growth or <3 CFU per
fecal pellet, thus excluding the possibility that the repeat cycle of
infection in DBA/2 mice was due to coprophagia in the mice.
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FIG. 1.
Patterns of colonization with C. albicans in
BALB/c and DBA/2 mice. (A) Mice were infected by swabbing the oral
mucosa with C. albicans (108 CFU/mL). At various
times indicated, the level of colonization was assessed by swabbing the
oral cavity. Data shown are means ± standard errors for three to
five mice. *, P < 0.05; **, P < 0.01; ***, P < 0.0001 (for values from BALB/c
versus DBA/2 mice). (B) The numbers of blastospore and hyphae in oral
tissues were counted by light microscopy (magnification, ×40) after
staining with H&E and PAS stains. Data are means ± standard
errors for three to five mice.
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To determine whether the pattern of infection was characterized by
different morphological forms of
C. albicans, the
proportions
of blastospores and hyphal forms in oral tissues were
enumerated.
Figure
1B represents the ratios of blastospores to hyphal
forms
of
Candida in tissue sections of the oral mucosa in
BALB/c and
DBA/2 mice. After inoculation, the ratios of blastospores to
hyphal
forms were about similar in DBA/2 and BALB/c mice. By day 2, the
ratio was lower in DBA/2 than in BALB/c mice. On day 4, about
equal
ratios of blastospores to hyphae were detected in the two
mice strains.
In BALB/c mice, the ratios of blastospores to hyphae
continued to rise
over time; when 100% of yeasts present in the
oral mucosa were
blastospores on day 6 before they were cleared
by day 8. In marked
contrast, a low blastospore-to-hypha ratio
was detected in DBA/2 mice
on day 6; then it rose by day 10 before
the yeasts, consisting
predominantly of blastospores, were cleared
on day
15.
Cellular response in the CLN.
The mean number of cells
recovered from the CLN increased from 9.8 × 106 to
22 × 106 cells per mouse, and from 9.5 × 106 to 18 × 106 cells per mouse 4 days
after infection with C. albicans in BALB/c and DBA/2 mice,
respectively (Table 1). A drop in cell
counts on day 6 followed the clearance of C. albicans in
both BALB/c and DBA/2 mice, but in DBA/2 mice it was followed by a rise
in cell counts after reinfection before decline on day 15. While the
relative proportions of CD19+ B cells and the various
T-cell subsets remained constant, there was a significant increase in
the percentage of / T cells above the background level during the
course of infection. In BALB/c mice, the number of / T cells
increased five- to sixfold on day 6 and then declined thereafter when
the infection was cleared. In contrast, in DBA/2 mice, the increase in
the numbers of / T cells was cyclical, with maximum levels
occurring on days 8 and 10 before falling to background levels on day
15, when the infection was cleared.
In vitro stimulation of CLN cells.
The effect of C. albicans colonization on T-cell proliferation was determined in
culture of CLN cells stimulated with C. albicans antigens.
As shown in Fig. 2, there was a
significantly higher antigen-stimulated T-cell proliferative response,
which peaked at day 4 (P < 0.05) and day 10 (P < 0.05), in DBA/2 mice than in unstimulated
controls. In contrast, a lower (but significant) increase in the
proliferative response in BALB/c mice occurred at day 4 (P < 0.05) and was maintained thereafter at a similar level after a
peak response at day 6 (P < 0.01). The proliferative response in DBA/2 mice, however, continued to decline to control levels
by day 28.
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FIG. 2.
Lymphocyte proliferation. CLN cells were stimulated or
not with C. albicans antigen for 3 days, after which time
thymidine incorporation was assessed. The results shown are mean counts
per minute ± standard errors for three mice. *,
P < 0.05; **, P < 0.01 (compared
with values from unstimulated cells).
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Serum and local IgG and IgA antibody responses.
As shown in
Fig. 3, an increase in serum IgG antibody
levels was detected in both BALB/c and DBA/2 mice 10 days after
infection, with maximum levels detected on day 15. The levels of IgG
antibody were significantly higher in BALB/c mice compared to DBA/2
mice at days 10 and 15 (P < 0.05) and at day 28 (P < 0.01). Similarly, significantly higher levels of
IgA antibody were detected in the saliva of BALB/c mice compared to
DBA/2 mice at all time points from day 8, with maximum levels at day 15 (P < 0.05), before dropping at day 28 (P < 0.05).
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FIG. 3.
Serum IgG and salivary IgA antibody levels. IgG and IgA
antibody levels were measured in serum and saliva from infected mice by
ELISA. Time zero represents uninfected mice. The results shown are
means ± SEM for three mice. *, P < 0.05;
**, P < 0.01 (for values from BALB/c or DBA/2
mice).
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Effect of infection on IL-4 and IFN- mRNA gene expression.
The effect of colonization on mRNA expression of IL-4 and IFN- in
CLN cells was examined by RT-PCR. As shown in Fig.
4, IL-4 gene expression was detected on
day 2 in BALB/c mice, whereas it was not expressed until day 6 in DBA/2
mice. While IL-4 gene expression disappeared by day 10 in BALB/c mice,
it continued in DBA/2 mice at day 15. In contrast, IFN- mRNA gene
expression was first detected at 6 h after infection and then
gradually declined in BALB/c mice, whereas it continued strongly in
DBA/2 mice over the 28 days.
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FIG. 4.
IL-4 and IFN- mRNA gene expression in CLN cells.
Total RNAs were extracted from CLN cells of mice infected with C. albicans and analyzed by RT-PCR using cytokine-specific primers.
Equivalent loading of each sample was determined by the G3DPH
message.
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IL-4, IL-12, and IFN- production by CLN cells stimulated with
C. albicans antigen.
To determine the pattern and the
kinetics of cytokine production following infection, CLN cells were
stimulated with C. albicans antigen for 72 h, after
which time the levels of IL-4 and IFN- in the culture supernatants
were measured. As shown in Fig. 5, significantly higher levels of IL-4 were produced at day 2, with maximum levels occurring at days 4 and 6, in BALB/c mice than in DBA/2
mice at those times (P < 0.01 and (P < 0.05). In contrast, increases in IFN- levels were observed in
both BALB/c and DBA/2 mice, but with significantly higher levels
produced in DBA/2 mice at 6 h and at day 2 after infection than
were seen in BALB/c mice at those times (P < 0.05 and
(P < 0.01). By days 4 and 6, IFN- production was at
its highest level in BALB/c mice compared to DBA/2 mice, where IFN-
production was at background levels by day 6 (P < 0.01). While the production of IFN- declined, except for a
small increase at day 15, in BALB/c mice, a marked increase in
production was detected in DBA/2 mice at days 8 (P < 0.05) and 10 (P < 0.01). By day 28, the levels of
IFN- returned to background in both mouse strains.
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FIG. 5.
IL-4, IL-12, and IFN- production by CLN cells
stimulated in vitro. CLN cells from infected mice were stimulated with
C. albicans antigen for 3 days, after which time the culture
supernatants were assayed for cytokines by ELISA. Time zero represents
uninfected mice. The results shown are means ± SEM for three to
five mice. *, P < 0.05; **, P < 0.01 (values from BALB/c versus DBA/2 mice).
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To determine whether the different levels of IL-4 and IFN-
production are related to IL-12 production, CLN cells were isolated
at
various times from BALB/c and DBA/2 mice that were infected
and then
stimulated with
C. albicans antigen for 3 days, after
which
IL-12 was measured in the culture supernatant. As shown
in Fig.
5,
significantly higher production of IL-12 was detected
as early as 2 days after infection in DBA/2 mice (
P < 0.05). In
BALB/c mice, an increase in IL-12 production was detected at day
6 and
day 8 (
P < 0.05). Following a further increase in
DBA/2
mice, IL-12 was maintained at similar levels for 28 days in both
mice
strains.
Effect of multiple injections of anti-IL-4 MAb on susceptibility to
Candida infection in BALB/c mice.
To determine whether
the higher production of IL-4 in BALB/c mice was associated with rapid
clearance of the yeasts, the effect of anti-IL-4 administration was
assessed. Figure 6 demonstrates that
BALB/c mice infected with the yeasts followed by administration of 30 µg of anti-IL-4 on days 1, 3, and 5 after oral infection had a higher
carriage rate, with a delayed clearance of the yeasts, compared with
untreated controls. However, there was no detectable difference in the
amounts of IFN- in CLN cell culture supernatants between anti-IL-4
MAb-treated and control C. albicans-infected mice (data not
shown).
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FIG. 6.
Effect of treatment with an anti-IL-4 MAb on resistance
to acute infection with C. albicans. BALB/c mice were
injected i.p. with 30 µg of rat anti-IL-4 or with purified rat IgG1
matched isotype on days 1, 3, and 5 after challenge with yeast cells.
On various days, the number of yeasts in the oral cavity was determined
and the results were expressed as mean CFU ± SEM for three to
five mice. *, P < 0.05.
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Anti-IL-4 MAb-treated
C. albicans-infected mice had no
detectable IL-4 in CLN cell culture supernatants in the first 8 days;
thereafter, small amounts of IL-4 could be detected (data not
shown).
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DISCUSSION |
The results of this study demonstrate that host resistance to
C. albicans infection in the oral mucosa in a murine model
is linked to a particular pattern of cytokine response and an
accumulation of / T cells in the regional lymph nodes. The
differences between the colonization patterns of C. albicans
in "infection-resistant" BALB/c mice and "infection-prone"
DBA/2 mice following infection correlated with both T-cell
proliferation and the secretion pattern of the cytokines IL-4, IL-12,
and IFN-. Colonization patterns for both blastospore and hyphal
forms of C. albicans were cyclical, with higher levels of
colonization in DBA/2 mice. The more "infection-resistant" BALB/c
strain showed a single peak, with lower levels of colonization and more
rapid clearance of C. albicans from the oral cavity. There
was a selective expansion of / T cells in the regional lymph
node, which correlated in time with the clearance of infection in both
mouse strains. Sustained antigen-specific T-cell proliferation was
produced only in the infection-resistant BALB/c mouse strain. Higher
levels of serum IgG and salivary IgA antibodies followed resolution of
infection in BALB/c mice, but levels of these antibodies were lower in
DBA/2 mice. In DBA/2 mice, a cyclic colonization pattern with high
numbers of fungi, and relatively delayed clearance of infection,
correlated with high levels of IFN- and IL-12 soon after infection
and a delayed and blunted IL-4 response. In contrast, the
infection-resistant BALB/c strain showed a lower and more transient
colonization with C. albicans, which correlated with early
production of both IL-4 and IFN-. Neutralization of IL-4 in these
mice with an anti-IL-4 MAb (11B11) directly demonstrated that IL-4
contributed to protection. Collectively, these results indicate that
the induction of a balanced Th1 and Th2 helper cell response
characterized by the production of both IFN- and IL-4, and the
proliferation of / T cells, contributes to host resistance to
C. albicans infection in oral candidiasis.
The mechanisms of host protection against C. albicans
infection have been extensively studied in murine models of candidiasis in terms of the impact of T-cell cytokines operating through various effector mechanisms of immunity (10, 11, 29, 31). In
invasive candidiasis, neutrophils and macrophages are involved in host defense (2, 3, 22). A link between resistance and
susceptibility, and T-cell cytokine profiles, has been demonstrated in
these models in terms of mortality or survival (reviewed in reference
2). For instance, IFN- is rapidly produced
following infection in both resistant and susceptible mice (27,
41). Neutralizing IFN- increased the susceptibility of
resistant mice to infection (37), an outcome also achieved
by overproduction of IFN- mediated by IL-12 (27). In a
study of IFN--deficient mice, IFN--induced activation of
macrophages was essential for survival (24). Yet other
studies have shown that IFN- is not essential for host defense
against systemic candidiasis (34). It is important in such
studies to distinguish among mechanisms that limit mucosal colonization, those that prevent systemic invasion, and those essential
for survival. Studies involving manipulation of single components of
the host response, while valuable, must be interpreted with caution.
The present study examined mechanisms of host resistance and
susceptibility in a natural model of self-limited oral mucosal candidiasis. Different patterns of colonization and IFN- and IL-4
production were compared in an "infection-resistant" strain (BALB/c) and an "infection-prone" strain (DBA/2). While IFN- transcripts were detected early (at 6 h) in both BALB/c and DBA/2 mice following initial infection with C. albicans, the
production of IFN- did not on its own prevent more-protracted
colonization in DBA/2 mice. Whether deficiency of the fifth component
of complement in DBA/2 contributes to the protracted colonization in
oral candidiasis is unclear. However, several studies with congenic
mice, including those bred from different genetic backgrounds of the
DBA/2 strain, have reported that C5 deficiency is not an essential
factor contributing to the pathogenesis of invasive candidiasis
(1, 2, 28).
The present study showed that high levels of IL-12 and IFN-,
together with a delayed message expression and lower production of
IL-4, correlated with higher levels of colonization and delayed clearance of C. albicans in DBA/2 mice. This is consistent
with the observation which showed that C. albicans infection
of the gastric mucosa in susceptible DBA/2 mice correlates with
decreased expression of IL-4 in Peyer's patches (10). By
contrast, the lower levels of IL-12 and IFN-, together with earlier
and higher production of IL-4, correlated with a lower colonization and
more-rapid clearance of C. albicans in BALB/c mice,
suggesting that the degree, the kinetics, and the mix of cytokines may
be critical factors in determining the level of protection after
challenge. Both Th1 and Th2 cytokines, albeit in different amounts with
different kinetics of production, were present in DBA/2 and BALB/c mice recovering from oral candidiasis, as was seen in gastric candidiasis (10). Thus, resistance to primary infection with C. albicans in the oral mucosa is associated with Th1 and Th2
responses. Support for a role for IL-4 in clearance was directly
demonstrated by the increased carriage rate and delayed clearance of
C. albicans from the oral mucosae of BALB/c mice following
treatment with anti-IL-4 antibody.
The mechanism of IL-4-enhanced resistance to C. albicans
infection in the oral mucosa is unclear. In primary systemic
candidiasis, IL-4 may limit C. albicans infection through
promoting effector mediators of immunity, including the differentiation
of effector Th1 cells (29, 30). In particular, IL-4 promotes
the development of a protective Th1 response in systemic and gastric
candidiasis (10, 30). Other studies have shown that mice
deficient in IL-4 were more susceptible to acute systemic infection
than normal controls (30, 45), though no difference in
susceptibility to orogastric candidiasis after challenge was noted
(45). These paradoxical findings may be explained by
different experimental models, different mouse strains, and different
routes of challenge and doses of C. albicans to induce
systemic or mucosal candidiasis. For example, intragastric challenge
with C. albicans induced a more severe gastric candidiasis
in BALB/c mice than in DBA/2 mice, whereas the reverse was true for
systemic candidiasis (10). In the present model, acute oral
candidiasis was induced by topical application of C. albicans, as opposed to an intragastric bolus of C. albicans to induce gastric candidiasis (30, 45).
Furthermore, topical application of C. albicans to the oral
mucosa restricts the supply of antigen to the gut-associated lymphoid
tissue (GALT) compartment, limiting modification of the course of
infection via activation of the common mucosal immune system
(14). Little or no fungus was recovered from fecal pellets.
In the present study both BALB/c and DBA/2 mice cleared infection
before the onset of antibody production, indicating that production of
serum IgG and secretory IgA antibodies did not play a significant role
in mucosal clearance, in agreement with findings in murine gastric
candidiasis (10). In the latter model, enhanced production
of secretory IgA antibody did not accelerate the resolution of
infection (10). Despite an increase in cell counts in the CLN after infection, the relative proportions of CD4+,
CD8+, and / T cells and B cells remained constant,
suggesting cell recruitment rather than antigen-induced proliferation
of cells. However, there was a selective expansion of / T cells,
which correlated with the elimination of C. albicans. While
the numbers were low, the increase was significant, considering the
paucity of / T cells in peripheral lymphoid tissues
(21). Increased numbers of / T cells have been
reported after bacterial, viral, and parasitic infections, suggesting a
role for / T cells in the first line of host defense (25,
26). It has previously been reported that / T cells enhance
resistance to mucosal candidiasis (16, 23), and increased
numbers of / T cells in the oral mucosa correlated with the
pattern of colonization in BALB/c and DBA/2 mice infected with C. albicans (12). It is not clear, however, whether
/ T cells are a source of IL-4. Although it has been reported
that / T cell clones and cell lines are capable of secreting IL-4
(4, 46, 47), we could not demonstrate significant amounts of
IL-4 in / T cells in these mice (data not shown). It has recently
been reported that / T cells can enhance nitric oxide (NO)
production by macrophages in mice injected i.p. with C. albicans (23), further linking / T cells with potential mechanisms of resistance. Furthermore, NO can enhance IL-4
expression in T cells (15), further influencing the balance of cytokine secretion. Thus, mucosal containment of C. albicans may depend on the interaction between macrophages and T
cells through the release of NO and IL-4, mediators which have been reported to enhance the killing of yeast cells by both neutrophils (5) and macrophages (20, 35) bearing IL-4 surface
receptors. / T cells can secrete IFN- and IL-4, which both
activate macrophages to act directly on C. albicans
(35, 44). Preliminary studies with the current model show
high levels of NO in saliva to support this hypothesis (unpublished results).
In summary, analysis of regional lymph node cell populations provides
data consistent with current ideas about cytokine function in
experimental models of infection. The findings presented in this study
of a model of oral candidiasis indicate that the production of IL-4 and
IFN- is critical to the resolution of mucosal infection in the
intact animal. The early appearance of IL-4 production suggests the
importance of this cytokine in enhancing immunity against C. albicans infection in the oral mucosa, a correlation directly
supported by data obtained following treatment with anti-IL-4 antibody.
The concurrent presence of high levels of IL-12 and IFN- supports
the concept of a balanced Th1 and Th2 response as being an efficient
host defense mechanism in clearing oral mucosal infection.
| |
FOOTNOTES |
*
Corresponding author. Mailing address: Discipline of
Immunology and Microbiology, Faculty of Medicine and Health Sciences, David Maddison Clinical Science Building, Royal Newcastle Hospital, Newcastle, NSW 2300, Australia. Phone: 61 2 49 236 135. Fax: 61 2 49 236 998. E-mail: rclancy{at}mail.newcastle.edu.au.
Editor:
J. D. Clements
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Abstract
Introduction
