Nitric Oxide Inhibits Rhinovirus-Induced Cytokine Production and Viral Replication in a Human Respiratory Epithelial Cell Line

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J Virol, February 1998, p. 934-942, Vol. 72, No. 2
0022-538X/98/$04.00+0
Copyright © 1998, American Society for Microbiology. All rights reserved.

Nitric Oxide Inhibits Rhinovirus-Induced Cytokine Production and Viral Replication in a Human Respiratory Epithelial Cell Line

Scherer P. Sanders,¹^,^* Edward S. Siekierski,² Jacqueline D. Porter,² Stephen M. Richards,² and David Proud²

Division of Pulmonary and Critical Care Medicine¹ and Division of Allergy and Clinical Immunology,² Department of Medicine, The Johns Hopkins Asthma and Allergy Center, Baltimore, Maryland 21224-6801

Received 19 June 1997/Accepted 5 November 1997

	ABSTRACT

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To better understand the early biochemical events that occur in human rhinovirus (HRV) infections, we examined the kineticsand mechanisms of interleukin-8 (IL-8) and IL-6 production frominfected epithelial cells. Several HRV strains caused IL-8 andIL-6 production, but HRV-16 induced maximal IL-8 and IL-6 mRNAexpression and protein production more rapidly than did HRV-14,despite similar rates of replication of the two viral strains.Viral induction of cytokine mRNA does not require new proteinsynthesis, since it was unaffected by cycloheximide treatment.The potent glucocorticoid budesonide did not affect viral replicationor cytokine mRNA induction but modestly inhibited cytokine proteinproduction. Interestingly, the nitric oxide donor 3-(2-hydroxy-2-nitroso-1-propylhydrazino)-1-propanamine(NONOate) inhibited both rhinovirus replication and cytokine productionin a dose-dependent fashion without reducing levels of cytokinemRNA. The NONOate effects were due to release of nitric oxide,because NONOate that had been depleted of its nitric oxide contenthad no effect. Thus, nitric oxide may play an important anti-inflammatoryand antiviral role in colds and nitric oxide donors may representa novel therapeutic approach.

	INTRODUCTION

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Rhinovirus infections are the predominant cause of the common cold (18), the most frequently experienced acute respiratoryillness in humans. Recent evidence also implicates rhinovirusinfections as important precipitating factors for the exacerbationof asthma (21, 22, 37), chronic bronchitis (35), sinusitis(19, 50), and otitis media (3). Despite the high healthcare costs associated with rhinovirus infections, the underlyingprocess by which viral infection leads to symptomatology is poorlyunderstood.

The epithelial cell is the primary site of rhinovirus infection (6, 51). In contrast to other respiratory viruses, suchas influenza, cytotoxic damage of infected epithelial cells doesnot appear to play a role in the pathogenesis of rhinovirus infections,since cytotoxicity is not observed either in infected human epithelialcell cultures (49) or in the nasal mucosa of infected individuals(53, 54). In light of this, emphasis has been focused on theconcept that symptoms may result from the actions of proinflammatorymediators that are generated as a consequence of rhinovirus infection.Support for this hypothesis has come from two lines of evidence:(i) studies of subjects with experimentally induced or naturallyacquired colds have demonstrated increased levels of several mediators,including kinins (36, 41), interleukin-1 (IL-1) (40), andIL-6 (55), in nasal secretions during symptomatic rhinovirusinfections; and (ii) infection of purified human respiratory epithelialcell populations with rhinovirus has been shown to induce productionof proinflammatory cytokines, including IL-8, IL-6, and granulocyte-macrophagecolony-stimulating factor (49, 55), that could contributeto disease pathogenesis. To date, however, the specific biochemicalevents involved in the production of each of these cytokines byrhinoviruses are incompletely understood and the role of specificcytokines, and other mediators, in the pathogenesis of colds remainsto be established.

The present studies were undertaken to further delineate the kinetics and mechanisms of rhinovirus-induced cytokine generationby epithelial cells and to evaluate the effects of potential therapeuticinterventions on these pathways. We have focused on viral productionof IL-8 and IL-6, because these cytokines are produced in relativelylarge amounts upon rhinovirus infection and because they havebiological properties that are of interest with respect to thepathogenesis of colds. IL-8 is a potent chemoattractant for, andactivator of, neutrophils (5) and also has chemotactic activityfor lymphocytes (28), the two predominant cell types in thenasal mucosa during rhinovirus infections (29, 54). IL-6 isnot only capable of stimulating T-cell activation and inducingB-cell differentiation and antibody production (1); it canalso stimulate mucosal immunoglobulin A immune responses (42).Of the potential interventions, we have used two approaches. Basedupon the wide-ranging immunomodulatory and anti-inflammatory effectsof glucocorticoids (44), including their ability to inhibitthe production of several cytokines in a variety of cell types(45), we examined the effects of the potent glucocorticoid budesonideon rhinovirus infection in epithelial cells. As a novel alternativeapproach, we also investigated the ability of a nitric oxide (NO)donor to inhibit viral replication and virally induced cytokineproduction in epithelial cells. Studies have demonstrated thatthe vasodilator NO can exert modulatory effects on inflammation(39), and nitric oxide has been shown to have antiviral effectsin some animal models (7, 12, 20, 24, 32), but thisproperty has not been examined in human respiratory epithelialcells. Our studies show that budesonide modestly inhibits rhinovirus-inducedcytokine generation without affecting viral replication. By contrast,NO markedly inhibits rhinovirus-induced cytokine generation aswell as viral replication and may play a therapeutic role in rhinovirusinfections.

	MATERIALS AND METHODS

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Materials. The following reagents were purchased from the indicated suppliers: Dulbecco's minimal essential medium, Eagle's minimal essentialmedium (EMEM), Ham's F-12 medium, Hanks balanced salt solution(HBSS), L-glutamine, penicillin-streptomycin-amphotericin B (Fungizone),trace elements, and retinoic acid (Biofluids, Rockville, Md.);hydrocortisone, epithelial cell growth factor, and endothelialcell growth supplement (Collaborative Research, Bedford, Mass.);fetal bovine serum (Gemini Bio Products, Inc., Calabasa, Calif.);transferrin and insulin (GIBCO BRL, Grand Island, N.Y.); 3-(2-hydroxy-2-nitroso-1-propylhydrazino)-1-propanamine(NONOate) (Cayman Chemical Company, Ann Arbor, Mich.); RNAzolB (Tel-Test, Inc., Friendswood, Tex.); agarose (FMC Bioproducts,Rockland, Maine); MOPS (morpholinepropanesulfonic acid) (BoehringerMannheim, Indianapolis, Ind.); and [ $alpha$ -³²P]dCTP (Amersham, Arlington Heights, Ill.). All other chemicalswere purchased from Sigma Chemical Company (St. Louis, Mo.). Budesonidewas generously provided by Per Andersson and Ralph Brattsand (AstraPharmaceuticals, Lund, Sweden).

The following stock buffers were employed: 10× MOPS (0.2 M MOPS, 0.05 M sodium acetate, 0.01 M EDTA), 50× Denhardt's solution(1% Ficoll, 1% polyvinylpyrrolidone, 1% bovine serum albumin),and 20× SSPE (175.3 g of NaCl, 27.6 g of NaH₂PO₄ · H₂O, 7.4 gof EDTA in 1 liter of H₂O [pH 7.4]).

Viruses and cell lines. Human rhinovirus type 14 (HRV-14), HRV-16, HRV-39, and HRV-1A, WI-38 cells, and HeLa cells were purchased from the AmericanType Culture Collection (Rockville, Md.). Additional viral stocksfor HRV-14 and HRV-16 were generated by passage in HeLa or WI-38cells, respectively, as previously described (49). It was notpossible to generate equivalent stocks of these two viral strainswith the same host cell line, since the two strains displayedmarked preferences in terms of their capacities to infect andreplicate in these cell lines. This variable sensitivity of hostcells to different strains of rhinovirus has been documented previously(11). For some experiments, HRV-16 was purified to remove ribosomesand soluble factors of WI-38 origin by centrifugation throughsucrose, according to published methods (16). Inactivation ofHRV-16 was performed by UV exposure for 30 min as previously described(49). For experiments using HRV-39 and -1A, viral stocks wereused directly as obtained from the supplier. The HRV-39 stockhad been prepared in WI-38 cells, while the HRV-1A stock was generatedin HeLa cells. The BEAS-2B cell line (43) was generously providedby Curtis Harris (National Cancer Institute, Bethesda, Md.).

Epithelial cell culture. Primary human tracheal epithelial cells were obtained by protease digestion of human tissue as previously described (10).Both primary cells and BEAS-2B cells were grown in culture mediumconsisting of Ham's F-12 nutrient medium with penicillin (100U/ml), streptomycin (100 U/ml), amphotericin B (250 ng/ml), L-glutamine(2 mM), phosphoethanolamine-ethanolamine (0.5 mM), transferrin(10 µg/ml), endothelial cell growth supplement (3.75 µg/ml), epidermalgrowth factor (12.5 ng/ml), insulin (5 µg/ml), hydrocortisone(10⁷ M), cholera toxin (10 ng/ml), 3,3',5-triiodothyronine (3 × 10⁹ M), retinoic acid (0.1 ng/ml), and trace elements. This mediumis hereafter referred to as F12/10×. The cells were incubatedat 37°C in 95% air and 5% CO₂. For the experiments, cells betweenpassages 35 and 50 were plated on 6-well plates or in 75-cm² flasks (Costar, Cambridge, Mass.) at a density of 2.5 × 10⁴/cm².

Viral infection of BEAS-2B cells. Monolayers of BEAS-2B cells (70 to 80% confluent) were washed three times with HBSS. HRV-14, -16, -39, or -1A was added tothe cells at a concentration of 10⁴ 50% tissue culture infective dose (TCID₅₀) units/ml of HBSS.This equates to an infectious dose of 0.01 TCID₅₀ units/BEAS-2Bcell, although it is unclear what this represents in terms ofmultiplicity of infection (infectious units per cell) for BEAS-2Bcells, since the capacity of rhinovirus to infect different hostcells is quite variable (see above). The cells were incubatedwith the virus at 34°C for 1 h and washed three times with F12/10×,and then fresh F12/10× medium was added to the cells. Supernatantswere removed from the cells at various times after infection andstored at $-$ 80°C for later analysis of cytokine protein productionand viral content. In some experiments, total cellular RNA wasextracted from the cells at various times after infection andstored at $-$ 80°C for later analysis.

Titration of viruses. Supernatants from infected cultures of BEAS-2B cells were collected at various times postinfection and assessed for viralcontent by cytotoxicity assays. For detection of HRV-14, confluentmonolayers of HeLa cells in 96-well plates were exposed to serialdilutions of the supernatants as described previously (49).In a similar assay, HRV-16 was detected by incubating confluentmonolayers of WI-38 cells in 96-well plates with serial dilutionsof the virus-containing supernatants in EMEM with 10% fetal bovineserum. The plates were incubated at 34°C for 5 days. The mediumwas removed, and the cells were washed with HBSS and then fixedwith methanol for 1 min. The methanol was removed, and the cellswere incubated with 0.1% crystal violet in distilled water for20 min. The plates were washed, and the absorbance at 570 nm wasdetermined with a plate reader. The dilution of supernatant requiredto infect 50% of the monolayers was determined and expressed aslog TCID₅₀ units.

Quantification of IL-8 and IL-6. Levels of cytokines in cell supernatants were determined by specific enzyme-linked immunosorbent assays (ELISAs). Measurementsof IL-8 were performed by a previously described ELISA sensitiveto 30 pg of cytokine/ml (49), while levels of IL-6 were assayedwith a commercial kit sensitive to 15 pg of IL-6/ml (BiosourceInternational, Camarillo, Calif.). Neither the culture mediumnor vehicles for drugs used in our experiments caused any nonspecificinterference effects in either assay.

Probes for Northern blotting. A full-length cDNA for IL-8 was obtained by reverse transcription-PCR with RNA extracted from the human BEAS-2B cell line.The full-length cDNA was cloned into a pCR II vector (InvitrogenCorp., San Diego, Calif.) between two EcoRI sites and grown incompetent Escherichia coli XL1-Blue cells (Stratagene, La Jolla,Calif.). The sequence of the cDNA probe used for Northern analysiswas identical to the published sequence of IL-8 (31, 34),as determined by dideoxy sequencing. A full-length cDNA for IL-6was kindly provided by Steven Gillis (Immunex, Seattle, Wash.).The full-length cDNA for glyceraldehyde-3-phosphate dehydrogenase(GAPDH) was purchased from Clontech (Palo Alto, Calif.). Probesfor IL-8, IL-6, and GAPDH were labeled to a high specific activityby the random-primer method (15) with [ $alpha$ ³²P]dCTP and a random-primer DNA labeling kit (Boehringer Mannheim).Unincorporated nucleotides were separated with Nuctrap push columns(Stratagene).

RNA extraction and Northern analysis. Total cellular RNA was extracted from BEAS-2B cells with RNAzol B (1 ml/10 cm²) in a modification of the method of Chomczynski and Sacchi (9).Briefly, cell monolayers were lysed with RNAzol B and transferredto a 13-ml polypropylene tube to which chloroform (0.1 ml/1 mlRNAzol) was added. After being chilled on ice for 5 min, the sampleswere centrifuged at 7,900 × g for 30 min at 4°C. The aqueous phasewas precipitated with an equal volume of ice-cold 95% ethanolat $-$ 20°C overnight. After a second centrifugation, the RNA pelletwas washed twice in 75% ethanol, dried, and dissolved in 50 µlof 0.2% diethylpyrocarbonate-treated water. The integrity of eachRNA was assessed by electrophoresis of an aliquot (0.5 µg) ona 1% agarose gel with 0.5 µg of ethidium bromide/ml of buffer.RNA was stored at $-$ 80°C.

For Northern analysis, equal amounts (15 to 20 µg) of RNA from each experimental condition were electrophoresed on a 1% agarose-2.2M formaldehyde gel in a MOPS buffer system. The RNA was transferredto a nylon membrane (GeneScreen Plus; New England Nuclear ResearchProducts, Wilmington, Del.). The membranes were cross-linked byexposure to UV light and then prehybridized in 10 ml of buffercontaining 4.5 ml of formamide, 2.5 ml of 10× Denhardt's solution,2 ml of 20× SSPE, 1 ml of 20% sodium dodecyl sulfate (SDS), and100 µg of denatured salmon sperm DNA/ml in a hybridization ovenfor 2 h at 42°C. Immediately following the prehybridization, theappropriate $alpha$ -³²P-labeled cDNA probe was added to the prehybridization solution,and the mixture was rotated for an additional 18 h at 42°C. Theblots were washed to a final stringency of 0.2× SSC (1× SSC is0.15 M NaCl plus 0.015 M sodium citrate)-0.2% SDS at 60°C andexposed to film (Biomax MS; Kodak, New Haven, Conn.) with twoLightening Plus screens at $-$ 70°C. Films were routinely developedfor various times to ensure that band intensities assessed bydensitometry were within the linear range for the film. Densitometrywas performed with a scanning densitometer (UVP [San Gabriel,Calif.] gel documentation system), and densitometric analysiswas performed with National Institutes of Health Image software.

Effect of cycloheximide on HRV-16-induced IL-8 and IL-6 mRNA expression. BEAS-2B cells were treated with cycloheximide (10 µg/ml) or the medium control for 1 h before viral infection. The drug wasalso present during and after infection with HRV-16. At 1 h postinfection,RNA was harvested for Northern analysis. This concentration ofcycloheximide was used because it has previously been shown toinhibit tumor necrosis factor alpha (TNF- $alpha$ )- and gamma interferon-inducedexpression of RANTES mRNA in this cell line (48).

Effect of budesonide on cytokine production and viral replication. Budesonide was prepared as a 10² M stock solution in dimethyl sulfoxide. Since the BEAS-2B cells are usually maintained ingrowth medium containing low levels of hydrocortisone, the cellsfor these experiments were placed in medium without hydrocortisonefor 24 h prior to treatment with the glucocorticoid. The cellswere then treated with 10⁷ M budesonide or appropriately diluted vehicle control for 24h prior to viral infection. Budesonide was again included in themedium after viral infection. The concentration of budesonideused was selected because it has previously been shown to maximallyinhibit TNF- $alpha$ -induced RANTES production from BEAS-2B cells (48).Supernatants from cells with and without budesonide were removedat various times after viral infection and stored at $-$ 70°C fordetermination of IL-8 and IL-6 protein and viral content. In someexperiments, Northern analysis was used to compare RNA extractedfrom the budesonide-treated cells 1 h after infection with thatextracted from control infected cells.

Effect of NONOate on cytokine production and viral replication. NONOate was prepared in alkaline solution (0.01 M NaOH) as a 100 mM stock solution, which was kept at 4°C until use. New stocksolutions of NONOate were prepared for each experiment and usedwithin 1 h of preparation. The defined half-life of NO releasefrom NONOate is 76 min at pH 7.4 and 22°C (Cayman Chemical Co.).Under alkaline conditions, the NONOate does not release nitricoxide. Aliquots of the alkaline stock solution were added directlyto the BEAS-2B culture medium (pH 7.4) in a final concentrationrange of 100 to 1,000 µM. For most experiments, the NONOate waspresent both during and following the virus exposure. In someexperiments, the NONOate was added only during or only after exposureto virus. Supernatants from BEAS-2B cells incubated with or withoutNONOate were removed at various times after viral infection andstored at $-$ 70°C for later determination of IL-8 and IL-6 proteinand viral content. In some cases, RNAs extracted at various timesafter infection from the NONOate-treated cells and from controlinfected cells were compared by Northern analysis. To controlfor nonspecific effects of the NONOate compound, experiments wereperformed in which cells were treated with an inactive solutionof NONOate. Inactivation was accomplished by placing a 1,000 µMsolution of NONOate in medium at pH 7.4 at room temperature for24 h to allow the NONOate to release all of the available NO priorto adding it to the cell cultures.

Statistical analysis. Data are expressed as the mean ± standard error of the mean (SEM). Comparisons of the kinetics of RNA expression, proteinsecretion, and viral titers were performed by a one-way analysisof variance (ANOVA). The effects of cycloheximide and glucocorticoidon RNA expression and protein secretion were compared by Student'st test for paired samples. Comparisons of the effects of NONOateon cytokine production, viral titers, and RNA expression weremade by two-way ANOVA with one repeated measure, except for theexperiments comparing active and inactive NONOate, which wereanalyzed by a one-way ANOVA. When significant variance ratioswere obtained, pairwise comparisons of the means were performedwith the least significant difference multiple-range test (47).Differences were considered significant for values of P of <0.05.

	RESULTS

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Effects of cell passage. Preliminary studies indicated that there was a marked effect of repeated cell passage on cytokine production from BEAS-2Bcells. Although the data obtained were always qualitatively identicalfor each passage, there was a progressive effect of cell passageon absolute levels of cytokines produced. For example, in fourexperiments performed with identical protocols with consecutivecell passages, production of IL-8 decreased from 7,690 to 3,090pg/ml. For this reason, each type of experiment described belowwas always carried out in matched experiments with the same cellpassages.

Comparison of effects of several rhinovirus strains on cytokine production from BEAS-2B cells. The effects on cytokine production of equal infective doses of four different strains of rhinovirus were compared in culturesof BEAS-2B cells. Three of the strains used, types 14, 16, and39, are members of the major group of rhinoviruses, which useintercellular adhesion molecule-1 (ICAM-1) as their receptor,while type 1A is a member of the ICAM-1-independent minor group.All of the strains induced IL-8 and IL-6 production measured at24 h following infection (Fig. 1). With all viral strains, generatedlevels of IL-8 were approximately 10-fold higher than those ofIL-6.

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FIG. 1. Cytokine production from BEAS-2B cells 24 h after infection with each of several strains of HRV. Data represent the mean plus SEM from three experiments. (A) Production of IL-8; (B) production of IL-6.

Kinetics of cytokine mRNA expression and protein secretion. Figure 2 demonstrates that mRNAs for IL-8 and IL-6 were significantly elevated within 1 h post-HRV-14 infection. Maximal expressionoccurred by 3 h postinfection, but mRNA levels were still higherthan those in noninfected controls at 24 h postinfection. Inductionof mRNA was followed by significant elevations in IL-8 and IL-6proteins in the supernatants. Increased cytokine production occurredby 3 h postinfection and reached maximal concentrations by 24h. Interestingly, the time course of IL-8 and IL-6 productionafter HRV-16 infection was more rapid than that observed for HRV-14(Fig. 3). Maximal mRNA expression occurred within 1 h postinfection,and maximal protein production occurred within 7 h. Consistentwith the data shown in Fig. 1, the magnitude of cytokine generationwas about fourfold greater following HRV-16 infection than theresponse following HRV-14 infection (Fig. 3 versus 2). BecauseHRV-16 produced a more rapid and robust production of cytokines,and because it is the strain that will be used for later in vivostudies, subsequent experiments on the mechanism of virus-inducedcytokine generation were performed with HRV-16. To confirm thespecificity of HRV-16 effects, three matched experiments wereperformed comparing IL-8 generation by active and UV-inactivatedviral preparations. Active virus generated 3,307 ± 1,156 pg ofIL-8/ml, while UV-inactivated virus produced only 520 ± 90 pg/ml(control, noninfected cells produced 345 ± 110 pg/ml). Specificitywas further confirmed by demonstrating that similar amounts ofIL-8 were generated, in matched experiments, when cells were infectedwith our standard viral preparation or with an equal infectivedose of the same stock of HRV-16 purified by sucrose density centrifugation(2,080 ± 340 and 1,750 ± 500 pg/ml, respectively; n = 3). Thetime course of viral induction of IL-8 and IL-6 was also identicalfor the standard and purified preparations of HRV-16 (data notshown).

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FIG. 2. Time course of induction of steady-state mRNA levels and proteins for IL-8 (left) and IL-6 (right) from HRV-14-infected BEAS-2B cells. The upper panels show Northern blots for each cytokine and for the housekeeping gene product, GAPDH. The center panels show densitometric ratios, while the lower panels show protein levels produced at each of the indicated time points. Data are from a representative experiment (n = 3).

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FIG. 3. Time course of induction of steady-state mRNA levels and protein for IL-8 (left) and IL-6 (right) from HRV-16-infected BEAS-2B cells. The upper panels show representative Northern blots for each cytokine and for the housekeeping gene product, GAPDH. The center panels show the means plus SEM of densitometric ratios for four experiments. The lower panels show the means plus SEM of amounts of protein produced for four experiments at each time point. Asterisks indicate significant increases in each parameter relative to the zero time control (P < 0.05 in each case).

Viral titers post-HRV-16 infection. Supernatants were collected at various times postinfection and assessed for viral titers in the WI-38 cell cytotoxicity assayfor HRV-16. Virus was detected in the culture medium beginningapproximately 7 h following infection and progressively increasedbetween 7 and 24 h after infection (Table 1). Supernatants collectedduring a second 24-h period after infection contained levels ofvirus similar to those seen after 24 h (Table 2). This patternof viral titers is virtually identical to that previously observedwith HRV-14 (49).

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TABLE 1. Viral content of supernatants from BEAS-2B cells at different times after infection with HRV-16

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TABLE 2. Effect of NONOate on viral titers decreases with time

Effects of cycloheximide on IL-8 and IL-6 mRNA expression. Levels of mRNA for IL-8 and IL-6 from HRV-16-infected cells treated with cycloheximide (10 µg/ml) were not different fromthose of control infected cells (Fig. 4). Comparisons were madeat 1 h after viral infection, the time of peak mRNA expressionin the kinetics studies described above.

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FIG. 4. Cycloheximide does not alter steady-state mRNA levels for IL-8 (left) and IL-6 (right) measured 1 h after infection with HRV-16. The upper panels show representative Northern blots, while the lower panels show the means plus SEM of densitometric ratios for four experiments.

Effect of glucocorticoid pretreatment on cytokine production and viral titers. Cells were treated with 10⁷ M budesonide or vehicle control for 24 h prior to viral infection. Comparisons of RNA expressionand protein production were made at the times of maximal responseas determined in the kinetics experiments described above: 1 hfor mRNA and 7 h for cytokine protein production. IL-8 and IL-6mRNA expression in HRV-16-infected BEAS-2B cells was not significantlyaltered by budesonide (Fig. 5). In every experiment, however,the production of IL-8 and IL-6 proteins from budesonide-treatedBEAS-2B cells was lower than from control infected cells (P <0.05 for paired comparison of normalized data). Viral titers (2.2± 0.6 log TCID₅₀ units) were not altered by budesonide exposure.

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FIG. 5. Effects of budesonide (10⁷ M) on steady-state mRNA levels and proteins for IL-8 (left) and IL-6 (right) from HRV-16-infected BEAS-2B cells. The upper panels show representative Northern blots with mRNA extracted 1 h after infection. The center panels show the means plus SEM of densitometric ratios from three experiments. The lower panels show the means plus SEM of amounts of protein produced 7 h after infection in three experiments.

Effect of a nitric oxide donor on cytokine production and viral titers. Supernatants were collected at 4 and 24 h post-HRV-16 infection from BEAS-2B cells incubated in the absence or presence ofNONOate and were assayed for viral content and levels of cytokines.NONOate significantly inhibited IL-8 and IL-6 production in adose-dependent manner (Fig. 6). IL-6 production was significantlyinhibited by doses of NONOate as low as 100 µM. The levels ofcytokine generated were inhibited more at 4 than at 24 h, presumablydue to the waning levels of NO at 24 h. Viral titers were alsosignificantly inhibited by NONOate (Fig. 7). Viral content inthe supernatant collected at 24 h was almost completely eliminatedby 1,000 µM NONOate. Supernatants from a second 24-h collection,however, contained similar amounts of virus whether the cellshad been treated with NONOate or not (Table 2). In parallel studies,the effects of NONOate on epithelial cell viability and cell numberswere assessed. There was no significant effect of NONOate on cellviability at any dose or time. There was a small, but significant,decrease in cell numbers with 1,000 µM NONOate at 24 h only ([1.7± 0.4] × 10⁶ cells/well without NONOate versus [1.2 ± 0.4] × 10⁶ cells/well with NONOate [n = 3, P < 0.05]). No such effects wereobserved at lower NONOate doses. The effects of NONOate were alsoconfirmed with purified HRV-16 (data not shown).

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FIG. 6. Dose-dependent inhibition of cytokine production from HRV-16-infected BEAS-2B cells by NONOate. The upper panel shows the means plus SEM from four experiments for IL-8 production at 4 and 24 h after HRV-16 infection, while the lower panel shows data for IL-6 production. The asterisks indicate significant inhibition compared to levels produced at the same time after infection in the absence of NONOate (P < 0.05 in each case).

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FIG. 7. Dose-dependent inhibition by NONOate of HRV-16 titers in BEAS-2B supernatants recovered 24 h after viral exposure. Data represent the means plus SEM of values from four experiments. The asterisks indicate significant inhibition compared to levels produced in the absence of NONOate (P < 0.05 in each case).

The inhibitory effects of NONOate were not limited to HRV-16 infection. Cytokines produced from BEAS-2B cells infected withanother major-group strain, HRV-14, or a minor-group strain, HRV-1A,were also significantly inhibited by NONOate. In the presenceof 500 µM NONOate, virus-induced IL-8 production in BEAS-2B cellswas inhibited by about 60% at 4 h (350 ± 51 to 117 ± 59 pg/mlfor HRV-14 and 1,857 ± 58 to 670 ± 64 pg/ml for HRV-1A [n = 3,P < 0.01]). In addition, NONOate inhibited viral titers in supernatantscollected from BEAS-2B cells 24 h post-HRV-14 infection (datanot shown). The capacity of NONOate to inhibit rhinovirus-inducedcytokine production was also observed in primary human cells.In one experiment, 1,000 µM NONOate reduced virally induced levelsof IL-8, measured 4 h after infection, from 1,400 to 366 pg/ml,while in a second experiment, IL-8 was reduced from levels of3,420 pg/ml in virally infected cells to 1,980 and 1,030 pg/mlin cells treated with 500 and 1,000 µM NONOate, respectively.

To further examine NONOate effects, additional experiments were conducted in which NONOate was added only during or afterviral infection. Figure 8 demonstrates that NONOate present onlyduring virus exposure, or only following virus infection, inhibitedIL-8 and IL-6 production by 50 to 60%. Complete inhibition ofprotein production was observed if NONOate was present both duringand after viral exposure.

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FIG. 8. Comparison of the effects of inactive NONOate and of active NONOate added at different times during the infection procedure on HRV-16-induced cytokine production from BEAS-2B cells. NONOate was used at a final concentration of 1,000 µM, and protein levels were measured 4 h after infection. (A) Means plus SEM of values for IL-8 production from three experiments; (B) data for IL-6. Asterisks indicate significant inhibition compared to levels produced by virus alone (P < 0.05 in each case).

To determine if the observed inhibition was specifically due to nitric oxide, experiments were conducted with active NONOateand with NONOate that had released all the available NO. Figure8 shows that the inactive compound did not inhibit IL-8 production.

Kinetics and mechanisms of the NONOate inhibition of IL-6 and IL-8 production. To examine the time course of NONOate inhibition, BEAS-2B cells were studied in the presence (500 µM) and absence of NONOateat various times after HRV-16 infection. The inhibitory effectof NONOate was most pronounced at the earliest time points, witha 60 to 70% reduction in protein levels at 1 h, 50% at 3 h, and30 to 40% at 7 h (Fig. 9). These results probably reflect thedeclining concentration of nitric oxide in the medium as the NONOatedegraded. Interestingly, the NONOate did not alter levels of cytokinemRNA expression. As shown in Fig. 9, mRNA levels for BEAS-2B cellsinfected with HRV-16 in the presence or absence of NONOate werenot significantly different. There was a tendency for the 3- and7-h IL-8 mRNA levels to be higher in the NONOate-treated cells.In additional control studies, NONOate alone had no effect onmRNA expression for IL-8 or IL-6, nor did inactive NONOate altervirally induced expression of mRNA for IL-8 or IL-6 in BEAS-2Bcells (data not shown).

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FIG. 9. Effects of NONOate (500 µM) on steady-state mRNA levels and proteins for IL-8 (left) and IL-6 (right) at different times after infection with HRV-16. The upper panels show representative Northern blots for each cytokine and for the housekeeping gene product, GAPDH. The center panels show the means plus SEM of densitometric ratios for three experiments. The lower panels show the means plus SEM of amounts of protein produced for three experiments at each time point. The asterisks indicate significant inhibition by NONOate compared to levels produced by virus alone (P < 0.05 in each case).

	DISCUSSION

Top Abstract Introduction Materials & Methods Results Discussion References

We have previously demonstrated that HRV-14 induces the production of IL-8 and IL-6 from BEAS-2B cells (49), and we nowshow that other major-group strains (HRV-16 and HRV-39) and HRV-1Aof the minor group all share this ability, suggesting that theinduction of proinflammatory cytokines may occur with many, ifnot all, rhinoviruses. We have already shown that cytokine productionby HRV-14 can be blocked both by antibodies to ICAM-1 and by UVinactivation of the virus (49). Our present studies showed notonly that the effects of HRV-16 can be abrogated by UV inactivationbut also that a purified preparation of HRV-16 induced cytokineproduction. Taken together, these data indicate that cytokineinduction is specifically due to virus and not to some contaminantof the viral stock solutions. Moreover, the common nature of thisresponse implies that the induction of epithelial cell cytokineproduction may play an important role in the pathogenesis of upperrespiratory viral infections in humans, a concept that is supportedfurther by the fact that other viruses, such as influenza andrespiratory syncytial virus, also induce epithelial cytokine productionbefore they cause overt cytotoxicity (2, 8, 33, 38).

The significance of the differences in levels of cytokine production by each strain is difficult to interpret because thetiters of viral strains were determined in several different celllines and may not be exactly comparable. It is clear, however,that the kinetics of cytokine mRNA expression and protein secretionvaried between strains of rhinovirus. Infection with HRV-14 ledto a time-dependent accumulation of mRNA for IL-8 and IL-6, withobserved levels being maximal at 3 h postinfection and remainingelevated at 24 h after infection. Consistent with our earlierreport (49), production of protein for each cytokine increasedup to 24 h postinfection but production during a second 24-h periodwas not different from that of control noninfected cells (datanot shown). This time course of protein production was similarto that observed with this viral strain in A549 type II epithelialcells (55), although the time course for mRNA accumulation differssomewhat, presumably reflecting differences of the two cell populations.Interestingly, the time courses of mRNA expression and cytokineproduction were more rapid, and the magnitude of the responsewas greater, for cells infected with HRV-16 than for those infectedwith HRV-14. Not only were maximal mRNA and protein levels achievedmore quickly, but they were more transient in nature, being essentiallycomplete within 7 h. As for HRV-14, cytokine production duringa second 24-h period after infection with HRV-16 was not differentfrom that for control noninfected cells (not shown). The reasonsfor the difference in initial rates of IL-8 and IL-6 productionby HRV-14 and HRV-16 are unknown but could be related to a differencein recognition, uptake, or uncoating of the two viral strainsin BEAS-2B cells. Despite the different rates of cytokine production,no differences in the rates of viral replication were observedbetween the two strains. In each case, virus was detected in thesupernatants of BEAS-2B cells by 7 h after infection and reachedmaximal levels by 24 h. A second 24-h collection produced titerssimilar to those of the first 24-h sample, suggesting that viralproliferation and release into the culture medium were occurringat a constant rate. The transient induction of IL-8 and IL-6 byboth viral strains in the setting of continued viral replicationsuggests that an early event in the viral infection, and not viralreplication itself, stimulates the production of proinflammatorycytokines. This rapid production of cytokines raises the speculationthat this relatively early event in the pathogenesis of coldsmay be important to initiate rapid inflammatory cell infiltration.

To further elucidate the biochemical mechanisms of virus-induced cytokine generation, we examined the effects of selecteddrugs on virus-induced expression of mRNA and protein for cytokines.The protein synthesis inhibitor, cycloheximide, did not alterlevels of mRNA for IL-8 or IL-6, suggesting that de novo synthesisof proteins was not required for rhinovirus-induced mRNA expression.This is consistent with the recent observations for A549 cells,indicating that induction of IL-6 by HRV-14 occurs via a nuclearfactor $kappa$ B-dependent pathway that is unaffected by cycloheximide(55).

Glucocorticosteroids have been shown to inhibit the production of several cytokines in patients with allergic inflammatorydiseases (46, 52) as well as in cell culture systems (45,48). We evaluated, for the first time, the effects of a potentglucocorticoid on viral replication and on induced IL-8 and IL-6mRNA expression and protein production in rhinovirus-infectedepithelial cells. Budesonide had no effect on mRNA expressionfor either cytokine but caused a modest inhibition of secretedprotein levels. This reduction in protein secretion in the absenceof changes in mRNA levels could reflect an ability of glucocorticoidsto alter posttranscriptional events involved in cytokine proteinproduction or secretion. It has previously been reported thatglucocorticoids at best modestly inhibit IL-8 mRNA and proteinproduction from cultured epithelial cells exposed to cytokines(27, 30), but dexamethasone has been reported to inhibit TNF- $alpha$ -inducedIL-6 mRNA and protein production from BEAS-2B cells (30). Thelack of effect of budesonide on viral titers and the modest inhibitionof IL-8 and IL-6 secretion are consistent, however, with in vivostudies of experimental rhinovirus infections, in which glucocorticoidshad little or no effect on viral shedding and symptoms (14,17).

It is now clear that NO can perform a broad range of actions, serving as a vasodilator, neurotransmitter, antimicrobial, andimmune regulator (39). In recent years, NO has also been shownto have antiviral properties in murine cell lines and in an invivo mouse model. Replication of several viruses, including vacciniavirus (20), herpes simplex virus type 1 (12, 24), vesicularstomatitis virus (7), coxsackievirus (32), and poliovirus(26), was inhibited by induction of NO synthase, the enzymethat generates NO, or by the addition of the NO donor S-nitroso-1-acetylpenicillamine. Given that levels of NO are increased in exhaledair from human subjects with upper respiratory viral infections(25), we investigated whether NO could inhibit rhinovirus replicationand extended these studies to evaluate the effects of NO on rhinovirus-inducedproduction of IL-6 and IL-8. Although normal human respiratoryepithelial cells have been shown to express both the constitutiveand inducible forms of NO synthase (4), the expression of theseenzymes is markedly reduced in the BEAS-2B cell line (data notshown). For this reason, and to ensure a controlled level of NOexposure, we used NONOate, a donor that releases NO with a definedhalf-life. Our data show, for the first time, that NO can inhibitboth rhinovirus replication and rhinovirus-induced productionof IL-8 and IL-6 in human respiratory epithelial cells. Theseeffects were dose dependent and occurred in the absence of anyeffects on epithelial cell viability. Inhibition of cytokine productionwas more pronounced at 4 than at 24 h postinfection, while viralshedding from epithelial cells also recovered to normal levelsduring a second 24-h collection period. These data are consistentwith the ability of NONOate to cause inhibition only when it isable to release significant amounts of NO, and they indicate thatboth viral replication and cytokine production resume as the compounddegrades. Further support for the key role of NO release is providedby our data showing that inactivated NONOate had no effect onviral titers or cytokine production.

The ability of NONOate to cause partial inhibition of cytokine production even when present only after the viral infectionperiod suggests that NONOate is not inhibiting by directly killingthe virus or by preventing the virus from entering the BEAS-2Bcells. This is also supported by the ability of viral titers torecover after NONOate degradation. Rather, it seems likely thatNO is inhibiting one or more early events in the viral infectionprocess. The failure of NONOate to inhibit cytokine mRNA expressionat any time point examined suggests that NO may be functioningby a posttranscriptional mechanism, but further studies are necessaryto confirm this. Precedent exists, however, for the capacity ofNO to inhibit protein synthesis in other cell types (13, 23).

In summary, we have demonstrated that multiple strains of rhinoviruses induce production of proinflammatory cytokines fromhuman respiratory epithelial cells but that there are variationsin the levels and kinetics of cytokine production by differentstrains. Although glucocorticoids modestly inhibit cytokine secretioninduced by rhinovirus infection, they do not alter cytokine mRNAexpression or viral replication. In contrast, NO markedly inhibitsrhinovirus replication and virally induced cytokine expressionwithout affecting mRNA levels for these cytokines. Although furtherstudies are necessary to elucidate the mechanisms by which NOinhibits viral replication and cytokine production, our data indicatethat topical application of NO donors may provide a novel therapeuticapproach for the treatment of rhinovirus-induced colds and theircomplications.

	ACKNOWLEDGMENTS

This work was supported by National Institutes of Health grant AI37163 and by a grant from the Center for Indoor Air Research.

	FOOTNOTES

^* Corresponding author. Mailing address: Johns Hopkins Asthma and Allergy Center, 5501 Hopkins Bayview Circle, Baltimore, MD21224-6801. Phone: (410) 550-2514. Fax: (410) 550-2612. E-mail:ssanders{at}welchlink.welch.jhu.edu.

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Top
Abstract
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Materials & Methods
Results
Discussion
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