By
From the * Department of Immunology, DNAX Research Institute of Molecular and Cellular Biology,
Palo Alto, California 94304; Department of Medicine, University of California, San Francisco,
California 94110; § Schering-Plough Research Institute, Lafayette, New Jersey 07848; and the
Department of Medicine, Allergy Immunology Division, Medical College of Wisconsin and Research
Service, Veterans' Administration Medical Center, Milwaukee, Wisconsin 53295
We have used interleukin-10 (IL-10) gene knockout mice (IL-10/
) to examine the role of
endogenous IL-10 in allergic lung responses to Aspergillus fumigatus Ag. In vitro restimulated
lung cells from sensitized IL-10
/
mice produced exaggerated amounts of IL-4, IL-5, and interferon-
(IFN-
) compared with wild-type (WT) lung cells. In vivo, the significance of IL-10
in regulating responses to repeated A. fumigatus inhalation was strikingly revealed in IL-10
/
outbred mice that had a 50-60% mortality rate, while mortality was rare in similarly treated
WT mice. Furthermore, IL-10
/
outbred mice exhibited exaggerated airway inflammation
and heightened levels of IL-5 and IFN-
in bronchoalveolar lavage (BAL) fluids. In contrast,
the magnitude of the allergic lung response was similar in intranasally (i.n.) sensitized IL-10
/
and wild-type mice from a different strain (C57BL/6). Using a different route of priming (intraperitoneal) followed by one i.n. challenge we found that IL-10
/
C57BL/6 mice had
heightened eosinophilic airway inflammation, BAL-IL-5 levels, and numbers of
T cells in
the lung tissues compared with WT mice. We conclude that IL-10 can suppress inflammatory Th2-like lung responses as well as Th1-like responses given the constraints of genetic background and route of priming.
Aspergillus fumigatus is an opportunistic fungal pathogen
for humans and animals causing lung hypersensitivities
with and without life-threatening growth in the lungs or
sinuses (reviewed in reference 1). In humans, lung hypersensitivity to A. fumigatus can occur in different forms (2).
The two opposite extremes are asthma with increased serum
IgE titers (2) and hypersensitivity pneumonitis with increased serum IgG and low IgE titers (3, 4). Clinically,
asthma presents as recurrent bouts of dyspnoea due to
bronchoconstriction, whereas hypersensitivity pneumonitis is characterized by bouts of dyspnoea accompanied by influenza-like symptoms (e.g., fever, fatigue). Immunologically, asthma has been associated with an exaggerated Th2
response promoting IgE synthesis, eosinophil infiltration,
and activation of mast cells in the lungs (reviewed in reference 5). In contrast, hypersensitivity pneumonitis is characterized by neutrophil influx into the lungs at the acute phase
and T cell and macrophage influx during the chronic phase of
the disease (6). It is thought to be caused by excessive macrophage activation (6) due to an immune complex-mediated Arthus reaction (reviewed in reference 3) together
with a CD4 T cell response probably mediated by Th1 cytokines (7). Most patients who are hypersensitive to A. fumigatus suffer from a disease called allergic bronchopulmonary aspergillosis (ABPA)1. The main features of this disease
are activated Th2 cells (8) and asthma; however, IgG-mediated Arthus reactions (2) and autoimmune reactions (9) can
also contribute to the pathogenesis.
Because IL-10 is constitutively produced by bronchial
epithelial cells (10) and potentially inhibits cytokine production by cultured alveolar macrophages and lung dendritic cells (11), there has been considerable interest in
the role of IL-10 in regulating pulmonary immune responses. IL-10 has been shown to suppress acute inflammation induced by the formation of antigen-antibody complexes in the lungs of mice (localized Arthus reaction) (16).
However, little information is available concerning a role
for IL-10 in regulating Th2-like responses leading to asthmatic lung hypersensitivity reactions. Analysis of bronchoalveolar lavage (BAL) fluids from asthmatic patients have
produced puzzling results as they showed increased IL-10
mRNA expression by BAL cells (17) but diminished IL-10
protein in BAL fluids (18). Based on the results of numerous murine studies, it has been proposed that IL-10 enhances
Th2 responses, albeit indirectly, by inhibiting an accompanying Th1 response (reviewed in reference 19). Although
these studies evaluated antigen-induced responses in organs
other than the lung, the general findings would suggest that
IL-10 may actually contribute to the preferential generation of a Th2 response deemed responsible for allergic pulmonary reactions. On the other hand, a recent study showed
that mice sytemically primed with OVA exhibited diminished lung eosinophilia upon rechallenge with aerosolized
OVA if IL-10 was also administered (20). These latter studies show that IL-10 is at least capable of suppressing eosinophilic inflammation (Th2-like response) under certain in
vivo conditions and thus may have some therapeutic value.
The present study has focused on the role of endogenous
IL-10 in regulating allergic pulmonary reactions. Previous
studies have shown that sensitization of BALB/c mice with
A. fumigatus Ag normally induces a strong Th2-like response resulting in pulmonary eosinophilia and elevated serum IgE levels (21, 22). We have compared the responses
of IL-10 Animals.
IL-10 A. fumigatus Ag.
The A. fumigatus Ag preparation is a mixture of culture filtrate and mycelial extract prepared free of living
organisms as described (21). This complex preparation has been
particularly useful in detecting serum antibody levels and skin reactivity in human patients (25). Two batches of A. fumigatus Ag
with equivalent activities (lot numbers 5323R1, 5325) were aliquotted at a concentration of 10 mg/ml and stored at Sensitization with A. fumigatus Ag.
Wild-type and IL-10 Airway Inflammation.
Airway inflammation was analyzed using BAL. Lungs were lavaged three times with 1 ml of PBS. Approximately 2.4 ml of fluid was routinely recovered. Total cell
numbers were determined using a hemacytometer. Differential
cell counts were obtained from BAL cells spun onto slides with a
cytocentrifuge and treated with Wright-Giemsa stain (Sigma Chem.
Co., St. Louis, MO). 400 cells were enumerated. Absolute numbers of specific cell types present in BAL fluids were calculated
from the recovered volume, total cell count, and the relative frequency of that particular cell type. BAL supernatants were collected by centrifugation and stored at In Vitro Restimulation of Lung Cells.
Lung tissue, trimmed of
bronchial lymph nodes and trachea, were minced through a sterile no. 100 steel mesh screen (Tylinter, Inc., Mentor, OH) into a
petri dish containing 5 ml of HBSS and antibiotics. The lung cells
were washed once with HBSS and resuspended at 8 × 106 cells/
ml in medium (RPMI-1640 supplemented with 10% FCS, 50 mM
2-ME, 100 U/ml penicillin, and 100 µg/ml streptomycin). 500 µl
to 1 ml of lung cell suspension was pipetted into three sets of 24-well
flat-bottomed plates (Falcon; Becton Dickinson Labware, Lincoln
Park, NJ) containing an equal volume of medium or medium supplemented with A. fumigatus Ag (20 µg/ml). One set of plates had been previously coated with 12 µg/ml hamster anti-mouse
CD3 mAb (clone 32C11). In the case of cultures containing wildtype lung cells, additional wells were supplemented with a neutralizing anti-IL-10 mAb (clone 2A5) at 10 µg/ml. Cultures were
incubated at 37°C in a humidified atmosphere with 5% CO2. Supernatants were harvested 72 h later and stored at Measurement of Cytokine Levels in Culture Supernatants and BAL
Fluids and Determination of Serum Antibody Levels.
Cytokine levels in BAL fluids and cell culture supernatants were determined
by two-site sandwich ELISA assays using the following Ab pairs
provided by Dr. J. Abrams and Dr. R.L. Coffman (DNAX): for
IFN-/
and wild-type (WT) mice after repeated challenges with A. fumigatus Ag to identify altered reactions that
may occur in the absence of IL-10 regulation (i.e., cytokine
production, airway inflammation, airway hyperresponsiveness, and serum antibody titers). Furthermore, different
routes of sensitization and strains of mice were used as these
variables have been shown to influence the type and/or magnitude of an immune response elicited in other experimental systems.
/
outbred mice, generated on a mixed
C57BL/6 × 129Sv F2 background (23), and outbred WT littermate mice were derived by cesarean section under specific pathogen-free conditions at Simonsen Laboratory (Gilroy, CA) and maintained in micro isolator cages in the animal facility at DNAX
Research Institute (Palo Alto, CA) (24). Inbred C57BL/6 IL-10
/
mice were derived from outbred IL-10
/
mice by 12 backcrosses to C57BL/6 WT mice and interbreeding of heterozygous
offspring. Heterozygous littermates and homozygous WT C57BL/6
mice purchased from The Jackson Laboratory (Bar Harbor, ME)
were used as controls. All of the mice were maintained in the
DNAX animal facility under identical conditions. IL-10
/
, WT,
and sentinel mice were periodically examined by the Research Animal Diagnostic and Investigative Laboratory (University of Missouri, Columbia, MO). Bacterial cultures, parasitological examinations, serologic tests, and special histological stains were negative for known murine viral and bacterial pathogens. 6-9-wk-old
mice were used in the experiments.
70°C for
use in all the experiments described herein. The LPS content of
the Ag extracts was less than 0.2 EU/100 µg of Ag when tested
with the Limulus Amebocyte Lysate test (BioWhittaker, Walkersville, MD).
/
mice were repeatedly primed either i.p. or intranasally (i.n.) followed by a final i.n. challenge (21). In all cases, 100 µg of Ag was
used after dilution in PBS so as to deliver a total volume of 50 or
200 µl for i.n. or i.p. administration, respectively. All mice receiving an i.n. challenge were anaesthetized with isofluorane and
held upright until all of the Ag administered onto their nostrils
with a micropipette tip was inhaled.
70°C until assayed for cytokine levels.
70°C until assayed.
, XMG1.2 and R504 polyclonal rabbit Ab; for IL-4, 11B11 and biotinylated BVD24G2.3; and for IL-5, TRFK5 and biotinylated TRFK4. Before cytokine analysis, BAL supernatants were
concentrated six- to tenfold using Centricon 10 microconcentrators (Amicon, Beverly, MA) with a 10,000 MW cut off. The results were then corrected for the degree of concentration.
Flow Cytometric Analysis of Intracellular Cytokine Production by
Lung Cells.
The assay was performed according to Openshaw et
al. (26) with slight modifications. In brief, cells recovered from
murine lungs as described above were treated with 0.9% ammonium chloride to lyse erythrocytes, washed once with HBSS, resuspended in medium, and cultured at 4 × 106 cells/ml in 6-well
flat-bottomed culture plates in 5-ml volumes. Cells from the
HDK1 Th1 cell line (produces IFN- but not IL-4), or from the
CDC25 Th2 cell line (produces IL-4 but not IFN-
) were included as positive controls. All cell cultures were stimulated with
PMA (50 ng/ml) and ionomycin (500 ng/ml) for 2-2.5 h in the presence of Fas-Ig fusion protein (5 µg/ml) (27) to prevent activation induced cell death. Brefeldin A (10 µg/ml) was then added
to the cultures. After 2 h of incubation, DNAse I (10 µg/ml, Boehringer Mannheim, Mannheim, Germany) was added for a
few min. The cells were removed, washed with PBS, fixed with
formaldehyde (20-25 min), washed with PBS, and then stored in
FACS® buffer (PBS, 1% BSA, 1 mM sodium azide) at 1-2 × 106
cells/ml at 4°C. The staining procedure was carried out at room temperature within 24 h. The presence of intracellular IL-4 and IFN-
was detected with PE-conjugated 11B11 and FITC-conjugated AN18 mAb (provided by Dr. A. O'Garra; DNAX); PE-
and FITC-conjugated rat IgG1 isotype-matched Ab (PharMingen,
San Diego, CA) were used as negative controls. The cells were
treated for 10 min with permeabilization buffer (0.5% saponin
in FACS® buffer) containing 25 µg/ml Fc blocking solution
(PharMingen), spun down, and then incubated with the anti-cytokine or control Ab for 30 min. The cells were washed with permeabilization buffer for two times and with FACS® buffer once
before staining with Tri-ColorTM-conjugated anti-mouse
TCR
mAb (Caltec, San Francisco), or hamster Ig control Ab (Caltec). Samples were examined using a FACScan® flow cytometer (Beckton Dickinson, San Jose, CA). The data were analyzed using
CellQuest software (Becton Dickinson).
Airway Responsiveness. Airway responsiveness to i.v. acetylcholine (ACh) challenge was measured as previously described (28). In brief, mice were anesthetized with Nembutal sodium (Abbott Laboratories, North Chicago, IL) administered i.p. at 0.04 mg/g body weight. The tracheas were surgically exposed, cannulated with a blunt-ended, 20-gauge angiocatheter, and connected to a rodent ventilator (Harvard Apparatus, South Natick, MA). Mice were ventilated with 100% oxygen at a rate of 150 breaths per min and a tidal volume of 9 µl/g. Following paralysis with pancuronium bromide (4 µg/g; Gensia Laboratories, Irvine, CA), i.v. access was established using a 27-gauge needle placed into a tail vein and mice were placed into a rodent plethysmograph capable of determining tidal volume, airflow, dynamic compliance, and transthoracic resistance continuously. Airway responses were expressed as the amount of ACh required to double baseline transthoracic resistance (PC200).
Microscopic Analysis. Lungs from control and sensitized mice were inflated with one ml of 10% (vol/vol) neutral buffered formaldehyde. The inflated lungs were then placed into 10% (vol/ vol) neutral buffered formaldehyde. Tissues were routinely processed, sectioned at 6 µm in a dorsal plane through the center of the lung, and stained with hematoxylin and eosin (Sigma Chem. Co.). Sections were analyzed by two independent examiners who were blinded to treatment information.
Statistical Analysis. Experimental groups were compared to each other or to control groups using the nonparametric, unpaired, two-tailed Mann-Whitney U test. For airway hyperresponsiveness, statistical analysis was performed using analysis of variance (ANOVA) and the Bonferroni T test, on data expressed as the logarithm of PC200. The statistical comparison of mortality seen in different experimental groups was performed using Fisher's Exact Test.
WT and IL-10/
mice on the
C57BL/6 background were repeatedly primed i.p. (four
times) or i.n. (four times) and then given a final i.n. challenge (Fig. 1). Additionally, WT and IL-10
/
mice on a
mixed C57BL/6 × 129Sv background (outbred) were repeatedly exposed to A. fumigatus Ag delivered only by the
i.n. route (Fig. 1) for a limited number of times (2 to 3) due
to the high mortality rate of the IL-10
/
mutants (see below). In all experimental groups, the final i.n. challenge
was followed by a comparative analysis of cytokine production, airway inflammation, antibody responses, airway physiology, and histopathology.
Lung T cells from Sensitized IL-10
Lung cells
from sensitized IL-10/
and WT mice and from unsensitized control mice were restimulated in vitro with immobilized anti-CD3 mAb. Irrespective of the mouse strain or
the route of priming, lung T cells from sensitized IL-10
/
mice consistently produced higher levels of IL-4 and IL-5
than lung T cells from similarly treated WT mice (Fig. 2).
Furthermore, IL-10
/
cells also produced large quantities
of IFN-
, while WT cells produced low to undetectable
levels of IFN-
(Fig. 2). It seems unlikely that the decreased levels of IL-4, IL-5, and IFN-
produced by WT
T cells when compared with IL-10
/
T cells was due to
the suppressive effects of endogenously produced IL-10 in
the WT cultures, as the addition of neutralizing anti-IL-10 mAb did not lead to increased production of these cytokines (Fig. 2).
Given that in vitro restimulation of IL-10/
lung T cells
resulted in the enhanced production of Th2 (IL-4 and IL-5)
as well as Th1 (IFN-
) cytokines, we questioned whether
the absence of IL-10-mediated regulation led to the generation of polarized Th1 and Th2 cells and/or of Th0 cells
capable of producing both types of cytokines. Therefore,
T cells from the lungs of nonsensitized controls and sensitized IL-10
/
and WT mice were analyzed for their intracellular cytokines by flow cytometry (26). T cells from
both WT and IL-10
/
mice displayed a similar pattern of
cytokine-producing cells irrespective of their strain or route
of priming. Representative data (Fig. 3) show that sensitization with A. fumigatus Ag invariably induced the generation of highly polarized IL-4-producing T cells in WT
mice as they represented a very small proportion of the cytokine-producing cells present in the lungs of unsensitized control mice. Because the same results were also obtained with IL-10
/
cells, the generation of polarized Th2
cells was not dependent on the regulatory activities of IL-10.
Our data also show that exposure to A. fumigatus Ag did
not lead to an equivalent increase in Th0 cells or in polarized Th1-like cells in the lungs of either IL-10
/
or WT
mice. These cells were present in approximately the same proportion as they were in samples from unsensitized controls. This latter finding was somewhat surprising in the
case of IL-10
/
mice because the experiments described
above demonstrated that their lung T cells were capable of
producing high levels of IFN-
after restimulation with
anti-CD3 mAb.
The absolute numbers of IL-4-producing and/or IFN-producing cells recovered from the lungs of sensitized
C57BL/6 mice are presented in Fig. 4. We detected higher
numbers of cytokine-producing T cells in the lungs of
IL-10
/
mice primed i.p. when compared with similarly
treated WT mice. This particular comparison suggested that
increased T cell numbers in the lungs of IL-10
/
mice
may account for the higher levels of IL-4, IL-5, and IFN-
detected in their lung cultures when restimulated in vitro
with anti-CD3 mAb (see Fig. 2). However, the number of
cytokine-producing T cells recovered from IL-10
/
mice
primed i.n. were roughly equivalent to the number recovered from WT mice primed i.n. (Fig. 4), although mutant
cells consistently produced more IL-4, IL-5, and IFN-
after anti-CD3-stimulation (see Fig. 2). Therefore, it appeared that sensitization with A. fumigatus Ag in the absence of IL-10 regulation, generated cytokine producing T
cells in larger numbers and/or T cells that had acquired the
inherent potential to produce larger quantities of cytokines.
Attempts to use A. fumigatus Ag to restimulate in vitro cytokine production by lung cells from primed WT or IL-10/
mice proved uninformative. A. fumigatus Ag-induced IL-5
production was low, IL-4 production was barely at the detection limit, and IFN-
production was undetectable (data
not shown). Therefore, we focused on experiments designed to measure A. fumigatus Ag-induced cytokine production in vivo and to correlate these findings with numbers and types of inflammatory cells infiltrating the airways.
Morbidity was evident after the second i.n. exposure to A. fumigatus Ag. Compared with unsensitized controls, sensitized IL-10/
and WT mice lost weight. However, weight
loss was more pronounced in IL-10
/
mice (87.4 ± 6.3%
of the initial wt; n = 19) than in WT mice (93.2 ± 3.0%,
n = 17) (P = 0.0014). Furthermore, IL-10
/
mice became dehydrated and hypothermic. Approximately 2/3 of the
IL-10
/
mice died within 2-3 d after the third sensitization, whereas mortality was rare in similarly treated WT mice
(Fig. 5). Because of the high mortality rate of sensitized
IL-10
/
mice, in vivo cytokine production and airway inflammation was assessed after the second sensitization. The
BAL fluids from IL-10
/
and WT mice contained equivalent levels of IL-4 (Fig. 6). However, the same fluids from
IL-10
/
mice contained much higher levels of IL-5 and
IFN-
(Fig. 6). The cellular composition of BAL fluids recovered from IL-10
/
and WT mice was also different as
increased numbers of neutrophils were present in BAL fluids of IL-10
/
mice (Fig. 6). In the BAL fluids of IL-10
/
mice, neutrophils (59 ± 8%) predominated, while eosinophils (11 ± 5%) were less frequent. In contrast, neutrophils
(19 ± 3%), and eosinophils (25 ± 10%) were present in approximately equal ratios in the BAL fluids of WT mice.
These results fit well with the fact that IL-10
/
mice appeared to suffer from an uncontrolled acute inflammatory response as evidenced by their high morbidity and mortality rates with increasing exposure to A. fumigatus. Although
eosinophils in the BAL samples from both groups were already increased well above the levels exhibited by unsensitized controls, the numbers detected in the IL-10
/
samples were not as high as those in the WT samples. This finding was surprising given that IL-5 production was higher in
IL-10
/
than in WT mice. One possible explanation for
this outcome is that the lung eosinophilia in IL-10
/
mice
was suppressed because of their simultaneous production of
IFN-
, which is known to inhibit the influx of eosinophils during an inflammatory response (29).
IL-10
When C57BL/6
IL-10/
and WT mice repeatedly inhaled A. fumigatus Ag
(five times), significant levels of IL-5 and low levels of IL-4
were detected in their BAL fluids as compared with unsensitized controls (Fig. 7). However, there were no differences between sensitized IL-10
/
and WT mice as equivalent amounts of IL-4 and IL-5 were detected and IFN-
levels were negligible. Moreover, the total number of cells
present in their BAL fluids were similar, including eosinophils (Fig. 7). In both groups, eosinophils (63 ± 11%) predominated and neutrophils (0.3 ± 0.4%) were rare. Furthermore, when we examined crude lung cell suspensions,
IL-10
/
and WT mice had similar numbers of
T cells
capable of making IL-4, or IFN-
(see Fig. 4) and of
T
cells that made neither cytokine (data not shown).
C57BL/6 IL-10
A striking difference in the response of
C57BL/6 IL-10/
as compared with WT mice was observed when A. fumigatus Ag-priming was given i.p. (four
times) followed by a single i.n. challenge. IL-5 levels in BAL
fluids of IL-10
/
mice were significantly increased. Both
groups produced significant but similar levels of IL-4, and
IFN-
was extremely low or undetectable (Fig. 8). This cytokine profile was consistent with the significantly increased
numbers of eosinophils in the BAL fluids of IL-10
/
mice
compared with similarly treated WT mice (Fig. 8). Similar ratios of cell types with predominance of eosinophils (82.6 ± 5.9%) were present in BAL fluids from WT and IL-10
/
mice primed i.p., suggesting qualitatively similar but quantitatively increased airway inflammation in IL-10
/
mice.
Furthermore, numbers of
T cells capable of producing IL-4 and/or IFN-
(see Fig. 4) as well as numbers of
T
cells that made neither of these two cytokines (data not
shown) were significantly increased in lung tissues of IL-10
/
mice over levels seen in similarly treated WT mice.
Serum Antibody Titers and Airway Hyperresponsiveness Elicited by A. fumigatus Ag Are Not Altered in IL-10
Because of the sensitization-induced mortality in IL-10/
outbred mice, serum antibody titers and airway responsiveness were evaluated in C57BL/6 mice only. Both IL-10
/
and WT mice exhibited increased total serum IgE and
IgG1 titers compared with unsensitized controls (Table 1).
Independent of the route of sensitization, IgE and IgG1 serum titers in IL-10
/
mice were not statistically different
from those of WT mice. Neither IL-10
/
nor WT mice
showed increased IgG2a titers as compared with unsensitized controls (data not shown). The antibody response
(IgE and IgG1) was always higher in mice primed by the
i.n. route as opposed to the i.p. route.
|
Sensitization via either route elicited marked airway hyperresponsiveness (decreases in PC200) in both IL-10/
and WT mice as compared with unsensitized controls (Table 1). However, PC200 values were less variable in mice
primed by the i.n. route rather than by the i.p. route (Table
1). PC200 values measured in i.n. or i.p. primed IL-10
/
mice and similarly treated WT mice were statistically indistinguishable (Table 1).
Lungs from unsensitized mice (Fig. 9 A) served as controls.
Microscopic changes in all groups of sensitized mice (Fig.
9, B-F), were qualitatively similar, but differed in severity.
Changes tended to be multifocal in less severely affected
mice, but coalesced and became more diffuse in severely
affected animals. Lung changes were generally characterized by inflammatory cell infiltrates adjacent to airways
(Fig. 9, open arrows) and blood vessels (closed arrows), and by
filling of alveoli with inflammatory cells and by thickening
of alveolar septa (arrowheads). The epithelium lining airways
in affected regions of lung was often hyperplastic and contained numerous goblet cells. Inflammatory infiltrates adjacent to airways and blood vessels consisted primarily of
eosinophils, accompanied by smaller numbers of lymphocytes, macrophages, plasma cells, and neutrophils. Inflammatory cells within alveoli consisted of macrophages, lymphocytes, eosinophils, neutrophils, and multinucleated giant
cells. Alveolar septa in affected areas of lung were often thickened by similar inflammatory cells, with the exception
of multinucleated giant cells, which were only seen within
alveoli.
Comparisons among the sensitized groups showed that
alveolar lesions that developed in WT mice were least severe in C57BL/6 mice (Fig. 9, B and C) and most severe in
outbred mice (Fig. 9 D). When comparisons were made
between IL-10/
mice and their WT counterparts,
C57BL/6 IL-10
/
and WT mice sensitized i.n. developed
minimal to mild multifocal lesions that were very similar
(refer to representative section shown in Fig. 9 B). No differences could be detected between these groups morphologically. In contrast, C57BL/6 IL-10
/
mice primed i.p.
and challenged i.n. had more severe lesions than similarly
treated C57BL/6 WT mice (Fig 9, C and E), especially with respect to the inflammatory infiltrates around airways and blood vessels. In addition, changes in the C57BL/6 IL-10
/
mice were often more diffuse than in the similarly treated
C57BL/6 WT mice. Both WT and IL-10
/
outbred mice
sensitized i.n. developed the most severe alveolar changes
of all the experimental groups, and the changes in the IL-10
/
mice were more severe and diffuse than those seen in the
WT outbred mice (Fig. 9, D and F).
We have examined the response to inhaled A. fumigatus
Ag in mice deficient in IL-10 production. Previous studies
have demonstrated that A. fumigatus Ag elicit a dominant
Th2-like response in the lungs of WT mice (21, 22). There
were two main hypotheses regarding the outcome of our
experiments. Sensitization of IL-10/
mice would lead to
an increased macrophage and Th1 response (reviewed in
reference 19) or to increased Th1 and Th2 responses as observed in human studies (reviewed in references 32, 33).
Our results showed clearly that the presence of IL-10 is not
necessary for the development of polarized IL-4-producing
Th2 cells as this population was consistently generated regardless of the route of sensitization or the mouse strain
used. Furthermore, compared with WT mice, lung T cells
from sensitized IL-10
/
mice consistently secreted more
Th2 (IL-4 and IL-5) and Th1 (IFN-
) cytokines when restimulated in vitro. Therefore, our findings are more in
agreement with those of human studies, suggesting that IL-10
negatively regulates both Th1 and Th2 responses to Ag
most probably by inhibiting antigen-presenting cells (11, 12, 32).
Although our in vitro studies have shown that sensitizing
IL-10/
mice with A. fumigatus Ag led to the generation
of T cells capable of producing high levels of Th1 and Th2
cytokines, it was not clear how this potential would be
manifested in vivo where other regulatory factors could
come into play. Would increased Th1 and Th2 cytokine
production lead to more inflammation in the lungs? Alternatively, would IFN-
production antagonize potentially
increased IL-4 and IL-5 levels and protect mice from increased
eosinophilic inflammation of the lungs, IgE production,
and airway hyperresponsiveness (29)? We found that each
of the three different experimental protocols used provided
us with a different answer that appeared to be profoundly influenced by the genetic strain and the route of Ag-exposure.
The disease in outbred IL-10/
mice sensitized i.n. appears to represent a mixture between ABPA and Aspergillus-induced hypersensitivity pneumonitis. Although the increased BAL-neutrophilia, BAL-IFN-
levels, morbidity,
and alveolar lesions in the sensitized IL-10
/
outbred
mice could be interpreted as typical for hypersensitivity pneumonitis, the large numbers of eosinophils in the BAL
fluid of these mice and increased BAL-IL-5 levels do not fit
with the classification of hypersensitivity pneumonitis (2,
3). Although lung lesions in sensitized IL-10
/
outbred
mice were more extensive than those elicited in WT mice, they were of similar quality. Therefore, we suspect that
mortality in IL-10
/
mice induced by repeated inhalation
of A. fumigatus Ag was caused by the uncontrolled production of proinflammatory cytokines (e.g., IL-5, IFN-
),
which led to an acute shock-like state. This outcome was
also seen in IL-10
/
mice challenged with LPS (24) or infected with Toxoplasma gondii (37).
In striking contrast with the outbred strain, C57BL/6
mice sensitized i.n. with A. fumigatus Ag developed mild
lung lesions. These changes, together with the pronounced
airway hyperresponsiveness and high IgE serum titers, are
typical for murine experimental asthma (28, 38). Surprisingly, airway inflammation (BAL eosinophilia) that developed in the IL-10/
mice was indistinguishable from that
of WT mice. Moreover, the BAL fluids of the IL-10
/
and WT mice contained equivalent amounts of IL-4 and IL-5
and no IFN-
. Therefore, it appears that IL-10
/
mice developed a dominant Th2 lung response of the same magnitude as that of WT mice. Despite the fact that IL-10
/
mice, repeatedly exposed to A. fumigatus Ag through inhalation, developed T cells with the capacity to secrete large
amounts of Th1 and Th2 cytokines when polyclonally activated in vitro, their in vivo response appeared to be just as
tightly regulated as that of WT mice.
Thus far, our data have illustrated the profound part that
genetic factors can play in lung disease induced by A. fumigatus Ag. Even though the same Ag preparation was administered i.n. to both outbred and C57BL/6 mice, the
outbred mice developed a complex disease resembling a
mixture of asthma and hypersensitivity pneumonitis, whereas
C57BL/6 mice developed primarily an asthma-like disease.
This adds to the body of evidence that genetic factors may
modify lung responses to A. fumigatus Ag. A previous study has shown that inhalation of A. fumigatus Ag by mice from
two different mouse strains produced lung lesions of different severity (39). Genetic susceptibility factors in the case
of human ABPA have been suggested by the familial occurrence of the disease (40, 41) and by an increased frequency of mutations in the cystic fibrosis transmembrane
conductance regulator gene in ABPA patients (42). In addition, our studies showed that the inability to produce IL-10
leads to marked dysregulation and heightened disease on
the outbred but not the C57BL/6 background. A logical conclusion would be that C57BL/6 mice have the inherent
ability to compensate for the absence of IL-10 by using
other negative regulatory mechanisms that could be provided by alveolar macrophages (43) or by TGF- (44).
The specific mechanism evoked in C57BL/6 mice to
compensate for the absence of IL-10 regulation is unknown.
However, it is insufficient to prevent exaggerated eosinophilia and IL-5 production in the airways and heightened
infiltration of the lungs with T cells, when the route of
priming with A.fumigatus Ag is i.p. rather than i.n. This
priming protocol appeared to elicit strong Th2 responses in
both IL-10
/
and WT mice as inflammatory lung lesions
were of intermediate severity typical of experimental ABPA
(21) and BAL-IL-4 levels were high, whereas IFN-
was
undetectable. In this particular model of ABPA, the absence of IL-10 results in dysregulated IL-5 production, a
factor that appears to play a pivotal role in generating allergic eosinophilic lung inflammation (38). In support of the
view that IL-10 can suppress IL-5-dependent eosinophilic
inflammation, IL-10 administered at the time of the Ag recall has been shown to diminish numbers of eosinophils in
the peritoneal cavity of primed BALB/c mice (45).
It has been reported previously that antibody responses
in IL-10/
mice are not different from WT mice following Ag stimulation (23). Our results confirm this observation as serum IgE and IgG1 titers elicited in C57BL/6
IL-10
/
and WT mice were roughly equivalent. Our results show additionally that endogenous IL-10 neither promotes nor reduces airway hyperresponsiveness. Sensitization elicited similar airway hyperresponsiveness in WT and
IL-10
/
mice. The equivalent antibody and airway responses
in WT and IL-10
/
mice might reflect equivalent in vivo
IL-4 production, or elicitation of compensatory mechanisms
in IL-10
/
mice. Throughout our experiments, BAL-IL-4
levels were similar in sensitized IL-10
/
and WT mice,
supporting the former hypothesis.
In conclusion, our in vitro studies show that endogenous IL-10 limits the potential to make large Th2 and Th1 responses elicited by A. fumigatus Ag in the lungs. In vivo, endogenous IL-10 suppresses lung cytokine secretion and airway inflammation induced by inhaled A. fumigatus Ag. Therefore, IL-10 may be effective in ameliorating inflammation in human allergic lung diseases. However, the success of IL-10 therapy for allergic lung diseases may depend on as yet undefined genetic factors and the route of exposure.
Address correspondence to Gabriele Grünig, D.V.M., Ph.D., DNAX Research Institute of Molecular and Cellular Biology, 901 California Avenue, Palo Alto, CA 94304.
Received for publication 16 December 1996 and in revised form 15 January 1997.
DNAX Research Institute of Molecular and Cellular Biology is supported by Schering-Plough Corporation. This work was partially supported by a US Veterans Affairs Medical research grant (V.P. Kurup) and by grant HL 03344 from the National Institutes of Health (D.B. Corry).The authors thank Drs. R. Kühn, W. Müller, and K. Rajewsky (Institute for Genetics, University of Cologne, Cologne, Germany) for providing outbred IL-10/
mice. We gratefully acknowledge the generous
contributions of antibodies by Drs. R.L. Coffman, A. O'Garra, and J. Abrams (DNAX), and of Fas-Ig fusion
protein by Dr. Miyuki Azuma (Department of Immunology, Jutendo University, School of Medicine, Tokyo, Japan), Dr. N.A. Hosken, and S. Zurawski (DNAX). We also thank the staff of the Histology Laboratory at the Schering-Plough Research Institute.
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