Department of Occupational and Environmental Health Sciences, College of Pharmacy and Health Sciences, Wayne State University, Detroit, Michigan 48202
Received March 18, 2002; accepted June 27, 2002
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ABSTRACT |
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Key Words: tumor necrosis factor-; permeability; lung; inflammation; cytokines; rats.
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INTRODUCTION |
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The purpose of our study was to determine the contribution of TNF- in the development of O3-induced lung injury by the administration of anti-TNF-
prior to O3 exposure. Because the focus of this study was on inflammatory mechanisms, genes relevant to inflammation were analyzed using gene array, a pathway-specific gene expression profiling system, to identify the molecular pathways activated in response to O3 exposure. The focused approach in this study allowed us to concentrate on a select group of cytokines, without having to perform microarray analyses commonly used to screen hundreds or thousands of genes. At the same time, this procedure allowed analysis of over 20 genes simultaneously using a single hybridization assay, thus presenting an advantage over the conventional procedures, such as RT-PCR and Northern blot analyses, which detect the expression of one gene in a single assay. Activation of cytokine genes as a function of TNF-
status identified a central role of this cytokine in modulating events critical to inflammation.
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MATERIALS AND METHODS |
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Female White New Zealand rabbits were purchased from Harlan Sprague-Dawley, housed individually in steel wire cages, and quarantined for one week prior to use in the study. The antigen consisted of recombinant rat TNF- (Biosource International, Camarillo, CA) diluted in sterile phosphate-buffered saline (PBS) to a concentration of 20 µg/ml and mixed 1:1 with Freunds Complete Adjuvant to make a total of 2 ml. The rabbits were anesthetized with acepromazine (0.75 mg/kg) and xylazine (5 mg/kg) im and multiple intradermal injections were given using a volume of 100 µl. The remaining antigen solution (0.5 ml) was given ip. Booster injections were given two and four weeks later in the same manner as above using an antigen concentration of 10 µg/ml, then mixing with Freunds Incomplete Adjuvant. Blood was drawn every two weeks and the animals exsanguinated when antibody titers reached a plateau. The antibody was purified by incubating with Protein A and the purified IgG was used in the study.
Experimental design.
The optimal rabbit antirat TNF- IgG dose was derived from pilot studies in which rats received a series of antibody doses prior to O3 exposure. A dose of 20 mg/kg provided maximum protection while minimizing inflammation. For the studies described in this article, rats were given ip injections (20 mg/kg) of either the rabbit antirat TNF-
IgG or preimmune rabbit IgG. Approximately 1 h later, the rats were exposed for 3 h to either filtered air or O3 (1 ppm) using a nose-only exposure system. The rats were returned to their cages and 1012 h later sacrificed. The selection of this time point was based on the results of our previous studies (Bhalla et al., 1999
) showing peak increases in BAL markers of injury and inflammation at 8 to 12 h after the end of O3 exposures comparable to those used in this study. The lungs were lavaged and the BALF analyzed for albumin content. The lavage cells were counted using a coulter counter and identified morphologically. For tissue analyses, lungs were rapidly removed, frozen in liquid nitrogen, and stored at 80°C.
Animal exposure.
Air and O3 exposures were performed using a nose-only exposure system (Fig. 1). The inhalation chambers were purchased from CH Technologies (Westwood, NJ) and the exposure system was assembled in our laboratory. The chambers are designed to permit delivery of atmospheres to individual rats so that air exhaled by one animal is not inhaled by another animal. The chamber atmosphere was maintained at an air temperature of 75.7 ± 0.1°F, an O3 concentration of 1.018 ± 0.003 ppm, and a relative humidity of 45.5 ± 0.5%. The chambers were supplied with dry air that had been passed through activated charcoal, purafil, and a high performance filter before being humidified to the desired level. Ozone was generated by passing medical grade oxygen through an electrical O3 generator (Sander Ozonizer, Osterberg, Germany) and injecting it into the airstream. Ozone concentration was continuously monitored at the rat breathing zone using a calibrated ultraviolet light absortion monitor (Dasibi Environmental Corporation, Glendale, CA). The air temperature and relative humidity were continuously monitored using a hygrometer (EdgeTech, Milford, MA).
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Analysis of albumin.
The concentration of albumin in the BALF was determined colorometrically using the Sigma Diagnostics Albumin Reagent. Briefly, 100 µl of BALF was pipetted in triplicate into the appropriate wells of a 96 well round-bottomed plate. Standards consisted of dilutions of rat albumin in PBS. This was followed by the addition of 100 µl Sigma Diagnostics Albumin Reagent. The absorbance was immediately measured at 620 nm and the concentration of albumin in the samples was calculated from the standard curve.
Analysis of fibronectin.
The concentration of fibronectin in the BALF was determined by ELISA as described by Gomez-Lechon and Castell (1985). Briefly, high protein-binding multiwell plates were coated overnight with 100-fold dilutions of BALF samples. After washing, the wells were incubated with goat antirat fibronectin as the primary antibody. Secondary antibody consisted of rabbit antigoat IgG conjugated with horseradish peroxidase. Color was developed with o-phenylenediamine HCl and the fibronectin levels determined from the standard curve.
Nonradioactive gene array.
Total tissue RNA was extracted from rat lungs using Qiagen RNeasy Midi Kit (Qiagen Inc., Valencia, CA). RNA integrity was examined by running an RNA gel. Gene array procedure followed a Nonrad-GEArray Kit manual (Superarray Inc., Bethesda, MD). In brief, biotinylated cDNA probe was synthesized by reverse transcription at 42°C by mixing GEA primer mix with dNTP containing biotin-dUTP. Biotinylated cDNA probes were hybridized to gene-specific cDNA fragments spotted on the membranes in hybridization oven overnight at 68°C. GEArray membranes were washed 4 times, blocked with GEA blocking solution, and then incubated with alkaline phosphatase conjugated streptavidin (1:5000). After sequential washes the membranes were incubated with 5 ml CDP-Star chemiluminescent substrate for 2 min and exposed to X-ray film. The exposures were performed for varying lengths of time to determine the abundance of different transcripts. The films were scanned by Personal Densitometer (Molecular Dynamics Inc.) to obtain densitometric volumes.
Statistics.
Results for albumin, fibronectin, and cell count were obtained from 6 rats per exposure/treatment group and expressed as means ± SE. Comparisons between multiple groups were analyzed using Tukeys test with a probability of < 0.05 considered significant.
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RESULTS |
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DISCUSSION |
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The lung epithelium serves as a barrier to prevent entry of serum proteins into the air spaces and inhaled xenobiotics from gaining access to the vascular system. Ozone is known to disturb the tight junctions between cells allowing serum proteins to enter the air spaces (Bhalla, 1999). Albumin being one of the major serum proteins serves as an indicator of epithelial permeability and can be quantitated in the BALF. Collectively, permeability changes arising from O3 exposure may be the result of both direct injury to the cellular tight junctions and indirectly from the release of TNF-
. The administration of anti-TNF-
prior to O3 exposure in our study resulted in a significant reduction in BALF albumin as compared to O3 alone. Similar results have been reported from ischemia/reperfusion injury models (Caty et al., 1990
; Colletti et al., 1990
; Seekamp et al., 1993
) and in gram-negative sepsis (Windsor et al., 1994
). The mechanism by which TNF-
causes permeability changes has received considerable attention. Depletion of granulocytes by cyclophosphamide in guinea pigs has been shown to prevent the TNF-
induced lung injury (Stephens et al., 1988
). In addition, Goldblum and colleagues (1989) have shown that TNF-
is capable of producing in vitro as well as in vivo injury to pulmonary vascular endothelium. Albumin transfer across cultured porcine pulmonary artery endothelial cell monolayers was increased by TNF-
in the absence of granulocytes (Goldblum et al., 1989
).
Ozone exposure also resulted in a significant increase in PMNs recovered in the BALF. In contrast, the administration of TNF- antibody resulted in a significant reduction in PMNs. This is consistent with the findings of Windsor and colleagues (1994) that anti-TNF-
administered to swine made septic with Pseudomonas aeruginosa reduced the sequestration of PMNs into the lung. While the pathophysiological significance of the neutrophilia induced by O3 exposure is a matter of some debate, PMNs are capable of releasing a variety of cytokines, proteases, and reactive oxygen species that could be injurious to the epithelial cells. We have previously shown that by depleting leukocytes with cyclophosphamide, the BALF albumin levels following O3 exposure could be significantly reduced as compared to controls (Bhalla et al., 1992
). In our present study the neutralization of TNF-
in vivo failed to completely abolish the influx of PMNs into the air spaces. This observation suggests that other chemotactic factors are involved in the recruitment of PMNs following O3 exposure. While O3 exposure resulted in a significant increase in PMNs, the overall BALF cell counts were similar between the groups. Since PMNs constitute only a small fraction of the total inflammatory cell population in the lung, a change in the number of PMNs does not significantly impact the total cell number. Furthermore, a decrease in macrophage number after O3 exposure has been reported. This is attributed to the effect O3 has on macrophage adherence (Bhalla, 1996
). Greater adhesion of macrophages following O3 exposure would promote their retention in the lung and reduced recovery by BAL.
Fibronectins are multifunctional proteins that provide a site for cell attachment, thereby promoting cell adhesion, cell migration, and wound repair (Hynes, 1990; Yamada, 1987
). Enhanced fibronectin expression has been observed in a variety of lung disorders and after O3 exposure of animals (Gupta et al., 1998
; Limper and Roman, 1992
). A significant increase in fibronectin levels in the BALF of O3 exposed animals over that in air-exposed controls in this study is consistent with the earlier reports. Although the role of fibronectin in injury and inflammation is supported by its ability to promote tissue repair and cell recruitment (Denholm et al., 1989
; Everitt et al., 1996
; Rennard et al., 1981
), in our study the treatment with anti-TNF-
had no effect on the BALF fibronectin levels despite a reduction in injury and inflammation. This suggests that fibronectin upregulation as a result of O3 exposure is independent of the effects of TNF-
release under these experimental conditions.
Besides increased permeability and recruitment of inflammatory cells, pulmonary responses to environmental and other insults are characterized by the activation of recruited cells for the release of inflammatory cytokines. While the increase in number of PMNs provides a morphological indication of inflammation, the release of cellular mediators reflects their state of activation. The mediator release in response to O3 has been studied both in tissue culture and in in vivo settings. These studies have shown increased in situ levels of TNF- and IL-1
in rats infected with Listeria monocytogenes and exposed to O3 (Cohen et al., 2001
), an increased release of TNF-
and IL-1ß by macrophages isolated from rats exposed to O3 (Ishii et al., 1997
), and increased release of IL-1
, IL-6, IL-8, and TNF-
following exposure of nasal mucosa to O3 in an organ culture system (Schierhorn et al., 1999
). IL-1, secreted by macrophages, is also increased in infectious diseases and inflammatory processes (Le and Vilcek, 1987
). Therefore, we regard an upregulation of IL-1 gene following O3 exposure of rats as an observation consistent with its role as an inflammatory stimulus. Since IL-1 release may be regulated by TNF-
, it is not surprising that the induction of IL-1 gene by O3 was blocked in animals treated with anti-TNF-
antibody prior to O3 exposure. As a simple explanation, it can be assumed that the treatment with anti-TNF-
antibody caused an attenuation of inflammation through an IL-1 sensitive pathway. However, this interpretation fails to emphasize the notion that inflammatory response is the result of a complex set of events involving multiple cytokines and other cellular components and molecules. In addition to changes in IL-1 gene, our gene array approach revealed an upregulation of proinflammatory IL-6 and anti-inflammatory IL-10 following O3 exposure. The expression of these cytokines was blocked by anti-TNF-
treatment. IL-6, a chemotactic cytokine, is implicated in the recruitment and activation of PMNs. Its role in O3 induced lung inflammation is supported by studies demonstrating increased release of this cytokine in animals (Mango et al., 1998
; McKinney et al., 1998
) and humans (Torres et al., 1997
) following exposure. In humans, IL-6 release immediately postexposure correlated with the PMN peak at 18 h after exposure of adult smokers and nonsmokers to O3. In the current study, IL-6 expression supports the role of this cytokine in O3 induced changes in the lung.
Despite a growing interest in the role of cytokines in the induction of lung inflammation, not much is known about the effects of O3 on the production and release of IL-10. In a human study IL-10 was detected in the BAL from 6 out of 23 subjects exposed repeatedly to 200 ppb O3 (Jorres et al., 2000). In our rats exposed to a much higher O3 concentration, IL-10 gene was clearly upregulated. The expression of IL-10 is contrary to the expected downregulation of this cytokine by proinflammatory stimuli, such as O3 and TNF-
. A likely explanation for this observation is the production of proinflammatory TNF-
and IL-1
by the PMNs recruited in the lung following O3 exposure, and an effort on the part of macrophages to downregulate these cytokines and maintain a balance through an increased production of anti-inflammatory IL-10. This explanation is supported by other injury models, where increases in IL-10 levels were observed after inflammatory insults. Steinhauser and colleagues (1999) have reported an increase in IL-10 production following P. aeruginosa challenge in septic mice. This increase was associated with an influx of PMNs and an increase in myeloperoxidase activity in the lung. The suggestion that IL-10 is a modulator of lethal excessive production of inflammatory cytokines (Steinhauser et al., 1999
), and the observation that the neutralization of IL-10 caused an excessive expression of proinflammatory cytokines and death (Howard et al., 1993
; Standiford et al., 1995
) further support its role in limiting inflammation. We, therefore, propose that the induction of this anti-inflammatory cytokine serves to regulate inflammation as a part of recovery process following initial injury.
Although the results of this study show that the treatment of animals with anti-TNF antibody caused a reduction in O3-induced PMNs, albumin, TNF-, IL-1
, IL-6, and IL-10, the levels were still higher than the baseline values. While these results offer an insight into the inflammatory mechanisms and provide support to the role of TNF-
as an important regulatory cytokine, they recognize a complex mechanism involving multiple cytokines. It is possible that the administration of serum along with anti-TNF-
antibody caused some inflammation and partially compromised the attenuating effects of the antibody. It is also likely that cytokines and chemokines other than those examined in this study contribute to lung inflammation. Additionally, chemokines that are not chemotactic for PMNs may be modified to recruit PMNs. For instance, C-C chemokines, such as MCP-1 and RANTES, are primarily regarded as chemoattractants for monocytes and lymphocytes, while C-X-C chemokines, such as MIP-2 and IL-8, are chemoattractants for neutrophils (Baggiolini et al., 1994
; Bonecchi et al., 1999
; Premack and Schall, 1996
). Although the induction of neutrophilic inflammation in the lung is not associated with a change in MCP-1 and RANTES levels (Johnston et al., 1998
), PMNs activated by proinflammatory cytokines under certain conditions undergo a change in their receptor expression and become responsive to CC chemokines (Cheng et al., 2001
). These studies raise the possibility that stimuli such as O3 could cause a change in receptor expression and induce responsiveness to CC chemokines. Although this possibility remains to be tested, it provides an alternative mechanism for lung inflammation and an explanation for partial reversal of O3 effects by anti-TNF-
antibody.
In summary, we have shown that the administration of anti-TNF- prior to O3 exposure can significantly reduce the inflammation and epithelial injury as evidenced by the reduction in PMNs and BALF albumin levels. However, the neutralization of TNF-
did not completely abolish the O3-induced effects, adding further support to the idea that the pathophysiology seen following O3 exposure is a result of a variety of complex cellular and molecular interactions. Some of these interactions are evident in the cytokine genes expressed in response to O3 exposure and anti-TNF-
treatment. Both TNF-
and IL-1 are multifactorial cytokines and may act in concert. Because IL-1 may be a stimulus for the production of IL-6 (Sugawara et al., 2001
), the upregulation of IL-6 gene is a likely consequence of IL-1 activation by O3. This sequence may also provide an explanation to the role of anti-TNF-
in reducing O3-induced inflammation. Accordingly, a modulatory role of anti-TNF-
may be exerted through an attenuation of IL-1, which in turn leads to the downregulation of IL-6 and decreased inflammation.
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ACKNOWLEDGMENTS |
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NOTES |
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2 Present address: 2612 Fifth Street, Bldg. 433, Wright-Patterson Air Force Base, OH 45433.
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