Involvement of Thromboxane A2 and Histamine in Experimental Allergic Rhinitis of Guinea Pigs

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Vol. 280, Issue 3, 1471-1479, 1997

Involvement of Thromboxane A₂ and Histamine in Experimental Allergic Rhinitis of Guinea Pigs

M. Yamasaki, T. Matsumoto, S. Fukuda, T. Nakayama, H. Nagaya and Y. Ashida

Pharmaceutical Research Laboratories I, Pharmaceutical Research Division, Takeda Chemical Industries, Ltd., Osaka, Japan

	Abstract

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To identify the chemical mediators involved in the pathogenesis of allergic rhinitis, we studied the effects of the thromboxane(TX) A₂ receptor antagonist seratrodast, the peptide leukotrienereceptor antagonist pranlukast and the antihistamine azelastineusing a guinea pig model of allergic rhinitis. In guinea pigsactively sensitized by aerosol inhalation of antigen, antigenchallenge into the nasal cavity increased both the nasal vascularpermeability and the intranasal pressure; it also induced swellingof the nasal mucosa, which was evaluated by magnetic resonanceimaging. Both seratrodast and azelastine significantly inhibitedthese antigen-induced responses when the drugs were administeredp.o. 1 hr before antigen challenge. Also, the TX synthetase inhibitorozagrel reduced the antigen-induced increase in nasal vascularpermeability. On the other hand, pranlukast had little effecton the antigen-induced increases in nasal vascular permeabilityand intranasal pressure. Perfusions and inhalations of U-46619,a stable TXA₂ mimetic, or of histamine into the nasal cavity causedconcentration-dependent increases in nasal vascular permeabilityand intranasal pressure in normal guinea pigs. Leukotriene C₄also induced these responses, but the maximal responses to leukotrieneC₄ were less than the maximal responses to U-46619 or histamine.On the other hand, these responses were not induced by prostaglandinD₂ or prostaglandin F₂. Moreover, the U-46619- and histamine-inducedincreases in vascular permeability and intranasal pressure weresignificantly inhibited by seratrodast and azelastine, respectively.In addition, levels of TXB₂, a stable breakdown product of TXA₂,and histamine in nasal lavage fluid increased after antigen challengein actively sensitized guinea pigs. These results suggest thatTXA₂ and histamine play important roles in the pathogenesis ofexperimental allergic rhinitis in guinea pigs.

	Introduction

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Nasal blockage is one of the typical symptoms of allergic rhinitis. It is caused by edema and congestion induced by chemicalmediators that are released by several inflammatory cell typesafter antigen challenge and are capable of increasing vascularpermeability and dilating the capacitance vessels of the nasalmucosa (Holmberg et al., 1989; Norman, 1985; Raphael et al., 1991;Sherwood et al., 1993). Histamine provocation into the nasal cavityincreases the vascular permeability of the nasal mucosa (Svenssonet al., 1992) and increases nasal airway resistance (Austin andForeman, 1994). In addition, high levels of histamine have beenidentified in nasal secretions of patients with allergic rhinitisafter antigen challenge (Naclerio et al., 1983). These resultssuggest that histamine is a chemical mediator responsible forthe induction and pathogenesis of nasal blockage. However, otherchemical mediators may be implicated in the pathogenesis of nasalblockage, because antihistamine drugs have little effect on nasalblockage in allergic rhinitis (Horak et al., 1993 and 1994).

Recently, in addition to histamine, arachidonic acid metabolites including TXA₂ and peptide leukotrienes, which have variousbiological activities, were detected in nasal lavage fluid frompatients with allergic rhinitis after antigen provocation (Creticoset al., 1984; Brown et al., 1987). TXA₂ and peptide leukotrieneshave been considered to be important mediators in allergic diseasesbecause of their potential ability to contract airway smooth muscle(Dahlén et al., 1980; Svensson et al., 1977) and to increasevascular permeability (Hay et al., 1995; Lötvall et al., 1992).On the other hand, the roles of TXA₂ and peptide leukotrienesin allergic rhinitis are not yet clear.

In this study, to determine whether histamine and arachidonic acid metabolites contribute to the pathogenesis of allergicrhinitis, we investigated 1) changes in the vascular permeabilityof the nasal mucosa and intranasal pressure, by intranasal challengewith histamine or arachidonic acid metabolites in normal guineapigs and 2) the effects of azelastine, an antihistamine drug,seratrodast, a TXA₂ receptor antagonist, and pranlukast, a peptideleukotriene receptor antagonist, on a) antigen-induced increasesin vascular permeability and intranasal pressure and b) an antigen-induceddecrease in the area of the airway lumen in actively sensitizedguinea pigs. In addition, we measured the levels of histamineand TXB₂ in nasal lavage fluid after antigen challenge.

	Materials and Methods

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Drugs and chemicals. Seratrodast and LTC₄ were synthesized by Takeda Chemical Industries, Ltd. (Osaka, Japan). Ozagrel hydrochloride and pranlukasthydrate were extracted from tablets of VEGA (Ono PharmaceuticalCo., Ltd., Osaka, Japan) and capsules of ONON (Ono PharmaceuticalCo., Ltd., Osaka, Japan), respectively. Azelastine hydrochloridewas extracted from tablets of AZEPTIN (Eisai Co., Ltd., Tokyo,Japan). Indomethacin and OA (Grade III) were purchased from SigmaChemical Co. (St. Louis, MO). U-46619 was from Cayman ChemicalCo. (Ann Arbor, MI). Histamine dihydrochloride, PGD₂, PGF₂,methanol, ethanol and EDTA were obtained from Wako Pure ChemicalIndustries, Ltd. (Osaka, Japan). Pontamine sky blue was from TokyoKasei, Ltd. (Tokyo, Japan), pentobarbital sodium was from AbbottLaboratories (North Chicago, IL), a surgical bonding agent (Aronalpha A) was from Sankyo, Ltd. (Tokyo, Japan) and sterile 0.9%sodium chloride solution was from Otsuka Pharmaceutical Ltd. (Tokyo,Japan). OA and histamine were dissolved in saline. U-46619, PGD₂and PGF₂ were dissolved in ethanol, and LTC₄ in methanol.Each solution was diluted with saline before use. The concentrationsof methanol and ethanol were less than 0.3 and 3% (v/v), respectively.Seratrodast, ozagrel, pranlukast and azelastine were suspendedin a 5% (w/v) gum arabic solution and were administered p.o. 1hr before the challenge in a volume of 2 ml/kg b.wt.

Animals and sensitization procedure. Male Hartley guinea pigs, weighing 300 to 350 g (Seiwa Experimental Animals Ltd., Fukuoka, Japan), were sensitized by exposureto an OA aerosol (1% w/v in saline) for 10 min on two occasions,separated by 7 days. The animals were positioned in a box (28× 28 × 20 cm) made of polyacrylamide while they inhaled the aerosol,which was generated by an ultrasonic nebulizer (TUR-3200, Nihon-Koden,Tokyo, Japan). Seven days after the second sensitization period,the animals were used for the antigen challenge. In experimentsin which we studied the effect of histamine and arachidonic acidmetabolites on nasal vascular permeability and intranasal pressureof nonsensitized (normal) guinea pigs, male Hartley guinea pigsweighing 450 to 550 g (Japan SLC Ltd., Hamamatsu, Japan) wereused.

Measurement of the change in vascular permeability. To evaluate the change in vascular permeability in the nasal mucosa, we administered dye i.v. and measured the amount exudedinto the nasal cavity. Guinea pigs were anesthetized with pentobarbitalsodium (30 mg/kg i.p.) and were placed in a supine position ona thermal pad (Deltaphase Isothermal Pad; Braintree Scientific,Inc., Braintree, MA). The trachea was surgically exposed and cannulatedso that the animal could breathe spontaneously through the trachealcannula. A polyethylene cannula (Hibiki, Tokyo, Japan) was insertedinto the nasopharynx from the side of the larynx, and the otherend of the cannula was connected to an artificial infusion pump(STC-523; Terumo, Tokyo, Japan). The oral cavity was filled withglycerin-soaked absorbent cotton and was closed with Aron alphaA to interrupt perfusate flow across the cavity. Solutions wereperfused into the nasal cavity at the rate of 0.25 ml/min. Salinewas perfused for 10 min to wash the nasal cavity. Then 5% (w/v)pontamine sky blue (1 ml/kg i.v.) was administered through thejugular vein cannula. Saline perfusion was continued for 10 min,and perfusate dropping from the nostrils was collected (Period1). Vehicle, arachidonic acid metabolites, histamine or OA insolution was then perfused through the nasal cavity for 10 min,and the perfusate was collected (Period 2). Saline was subsequentlyperfused for 40 min, and the perfusate was collected for fourintervals of 10 min (Periods 3, 4, 5 and 6). The perfusate sampleswere centrifuged at 1700 × g for 10 min, and the absorptions at610 nm of the supernatants were measured with a spectrophotometer(TR-1000T; Corona Electric Co., Ltd., Ibaragi, Japan). The amountof pontamine sky blue dye extravasated into the perfusate wasquantified by interpolation on a standard curve of dye concentrationsranging from 0 to 25 µg/ml and was expressed as micrograms ofdye per milliliter of perfusate. Our evaluation of the effectsof the drugs on the induced increase in vascular permeabilitywas based on the change in the amount of dye exuded during Period3 from that exuded during Period 1.

Measurement of intranasal pressure. The intranasal pressure was continuously measured by the method described by Mizuno et al. (1991), with slight modifications.Guinea pigs were anesthetized with pentobarbital sodium (30 mg/kgi.p.) and were placed in a supine position. Animals breathed spontaneouslythrough a cannula inserted into the trachea. A polyethylene cannulawas inserted into the nasopharynx from the side of the larynx,and the other end of the cannula was connected to an artificialrespirator (model 683; Harvard Bioscience, South Natick, MA) setat a flow volume of 4 ml and a frequency of 70 strokes/min. Thetwo duct pores, which are situated in the upper oral cavity walland lead to the nasal cavity, were closed with Aron alpha A. Intranasalpressure was measured by a transducer (model DP-45-22; ValidyneCorp., Northridge, CA) connected to a lateral port at the proximalend of the endonasopharynx cannula. Vehicle, arachidonic acidmetabolites, histamine or OA aerosols, generated by an ultrasonicnebulizer (model 5000D; DeVilbiss, Somerset, PA) placed betweenthe nasopharynx and the artificial respirator, were inhaled for3 min into the nasal cavity. The increase in intranasal pressurewas expressed as the pressure minus the prechallenge base-linepressure. The effects of histamine and arachidonic acid metaboliteson intranasal pressure were determined by calculating the AUCfor the increase in intranasal pressure from 0 to 15 min afterinhalation ended. Evaluation of the effects of the drugs on theinduced increase in intranasal pressure was also based on theAUC for the increase in intranasal pressure.

Imaging of nasopharynx using MRI. MRI has been used to identify pathological changes in nasal tissue (Ryan et al., 1991; Sherwood et al., 1993), because itis a very useful technique for imaging soft tissues, especiallytissues with high water contents. Therefore, we used MRI to evaluatethe edema of the nasopharyngeal airway after antigen challenge.Actively sensitized guinea pigs were anesthetized with ketamine(50 mg/kg i.m.; Sankyo Co., Ltd.) and xylazine (5 mg/kg i.m.;Bayer). As described above, cannulas were inserted into the tracheaand nasopharynx, and then the guinea pigs were challenged by infusionof 0.3% OA solution for 10 min into the nasal cavity. After antigenchallenge, their nasal cavities were washed by flushing with 3ml of saline and then with 10 ml of air 10 times. Transverse imagesof the nasopharyngeal airway were obtained using an MRI systemduring the 5 to 25-min period after antigen challenge.

Imaging of the nasopharynx was performed with a nuclear magnetic resonance spectrometer (CSI-II OMEGA system; Brucer, Germany)operating at 4.7 Tesla magnet/33 cm according to the method describedby Sherwood et al. (1993)

, with slight modifications. A multislicelongitudinal relaxation time (T₁)-weighted spin-echo imaging sequencewas used to acquire proton density images. The recycle time (T_R)and echo time (T_E) were 800 and 25 msec, respectively. T₁-weightedsagittal images were first obtained to determine the region inwhich transverse slices would be taken. Contiguous T₁-weightedtransverse slices 4 mm thick were then obtained. The cross-sectionalarea of the nasopharyngeal airway lumen in the transverse viewswas measured using an image analysis system (IBAS2000; Zeiss,Germany). The cross-sectional area of the nasopharyngeal airwaywas expressed as the total value of three contiguous slices.

Measurement of TXB₂ and histamine in nasal lavage fluid. As described above, actively sensitized guinea pigs were challenged by perfusing the nasal cavity with 0.3% OA solution for10 min. Then the nasal cavity was perfused with saline, and perfusatedropping from the nostrils was collected for 10-min periods intoice-cooled polyethylene tubes containing 0.1 ml of 250 µM indomethacinand 2% (w/v) EDTA. Perfusate samples were centrifuged at 1700× g for 10 min at 4°C. The supernatant was stored at $-$ 80°C untilassay. The levels of TXB₂ and histamine were measured using anenzymeimmunoassay kit (Amersham International plc., Buckinghamshire,U.K.) and a radioimmunoassay kit (Immunotech S.A., Marseille,France), respectively.

Statistical analysis. All values are presented as the mean ± S.E.. Statistical comparisons were performed with a one-way analysis of variance andDunnett's test or bilateral unpaired Student's t tests, when appropriate.Differences were considered significant when P < .05. All statisticalcalculations were made using a SAS (Statistical Analysis System).

	Results

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Changes in vascular permeability of the nasal mucosa. Perfusion of U-46619 (0.1 ~ 100 µg/ml) through the nasal cavity caused a concentration-dependent increase in dye exudation.This response peaked during Period 3 at 100 µg/ml U-46619, duringPeriod 4 at 1 and 10 µg/ml U-46619 and during Period 5 at 0.1µg/ml U-46619 (fig. 1A). In the groups perfused with 10 and 100µg/ml U-46619, the concentrations of dye in the Period 3 perfusatewere 4.8 ± 0.8 (P < .05) and 8.5 ± 1.4 µg/ml (P < .01), respectively,and were significantly higher than in the vehicle (2% ethanol)-perfusedgroup (0.9 ± 0.2 µg/ml). Perfusion of histamine (3 ~ 100 µg/ml)also caused a concentration-dependent increase in exudation ofdye into the nasal cavity, peaking during Period 3 (fig. 1B).The concentrations of dye in the Period 3 perfusate in the groupsperfused with 30 and 100 µg/ml histamine were 9.8 ± 1.8 (P < .05)and 12.8 ± 4.2 µg/ml (P < .01), respectively, and were significantlyhigher than in the saline-perfused group (1.0 ± 0.2 µg/ml). Perfusionof LTC₄ (1 ~ 10 µg/ml) caused a concentration-dependent increasein dye exudation that showed a maximal response at 3 µg/ml LTC₄(table 1). On the other hand, perfusion of PGD₂ or PGF₂into the nasal cavity did not induce greater dye exudation thanoccurred in the vehicle group perfused with 1% ethanol (table1).

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Fig. 1. Increase in nasal vascular permeability induced by perfusion of U-46619 or histamine through the nasal cavity of normal guineapigs. A) Vehicle (2% ethanol, $square$ ) or U-46619 at 0.1 ( $open circle$ ), 1 ( $triangle$ ),10 ( $black-square$ ) or 100 µg/ml ( $black-triangle$ ) was perfused during Period 2. B) Vehicle(saline, $square$ ) or histamine at 3 ( $open circle$ ), 10 ( $black-square$ ), 30 ( $black-triangle$ ) or 100 µg/ml( $bullet$ ) was perfused during Period 2. Each point represents the meanfor 6 to 8 animals, and vertical bars represent the standard error.* P < .05, ** P < .01, compared with the vehicle-perfused group(Dunnett's test).

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TABLE 1
Changes in nasal vascular permeability induced by perfusion of various stimulants through the nasal cavity of normal guineapigs
LTC₄, PGD₂ or PGF₂ in solution was perfused through the nasal cavity for 10 min. The dye concentration in the perfusateduring the first 10 min after perfusion of the stimulants (Period3) is shown. Each value represents the mean ± S.E. for 5 or 6animals.

Changes in intranasal pressure. Aerosol inhalation of U-46619 (10 ~ 100 µg/ml) into the nasal cavity caused a concentration-dependent increase in intranasalpressure. The response to 30 µg/ml U-46619 continued to rise until15 min after inhalation ended, but the response to 100 µg/ml U-46619peaked from 5 to 10 min after inhalation ended (fig. 2A). TheAUCs for the increase in intranasal pressure from 0 to 15 minafter inhalation of 30 and 100 µg/ml U-46619 were 75.0 ± 25.8(P < .05) and 102.9 ± 28.5 cm H₂O · min (P < .01), respectively,and were significantly greater than in the vehicle group, whichinhaled 2% ethanol (18.0 ± 5.8 cm H₂O · min). Inhalation of histaminealso caused an increase in intranasal pressure, which was alreadyincreased at the end of inhalation and plateaued 10 to 15 minafter inhalation ended (fig. 2B). The AUCs for the increase inintranasal pressure from 0 to 15 min after inhalation of 100 and1000 µg/ml histamine were 110.4 ± 21.9 (P < .05) and 124.8 ± 24.4cm H₂O · min (P < .01), respectively, and were significantly greaterthan in the vehicle group, which inhaled saline (24.9 ± 6.6 cmH₂O · min). Inhalation of LTC₄ (0.3 ~ 3 µg/ml) caused a concentration-dependentincrease in intranasal pressure that showed a maximal responseat 1 µg/ml LTC₄ (table 2). After aerosol inhalation of PGD₂ orPGF₂, on the other hand, intranasal pressure fell in comparisonwith the vehicle group, which inhaled 3% ethanol (table 2).

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Fig. 2. Increase in intranasal pressure induced by inhalation of U-46619 or histamine into the nasal cavity of normal guinea pigs.A) The aerosol of vehicle (2% ethanol, $square$ ) or U-46619 at 10 ( $black-square$ ),30 ( $black-triangle$ ) or 100 µg/ml ( $bullet$ ) was inhaled into the nasal cavity for3 min. B) The aerosol of vehicle (saline, $square$ ) or histamine at 10( $black-square$ ), 100 ( $black-triangle$ ) or 1000 µg/ml ( $bullet$ ) was inhaled into the nasal cavityfor 3 min. Each point represents the mean for 4 to 6 animals,and vertical bars represent the standard error. * P < .05, ** P< .01, compared with the vehicle-inhalation group (Dunnett's test).

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TABLE 2
Changes in intranasal pressure induced by inhalation of various stimulants into the nasal cavity of normal guinea pigs
AUC (0-15 min) (cm H₂O · min) = area under the response curve for the increase in intranasal pressure from 0 to 15 min afterinhalation ended. LTC₄, PGD₂ or PGF₂ aerosol was inhaledinto the nasal cavity for 3 min. Each value represents the mean± S.E. for 3 to 9 animals.

Effect of seratrodast and azelastine on U-46619- and histamine-induced responses. Seratrodast (0.3, 1 and 3 mg/kg p.o.) given 1 hr before 3 µg/ml U-46619 perfusion dose-dependently inhibited the U-46619-inducedincrease in dye exudation by 41, 67 (P < .01) and 71% (P < .01),respectively (table 3). Azelastine (1 mg/kg p.o.) significantlyinhibited the histamine (100 µg/ml)-induced increase in dye exudationby 84% (P < .05) (table 3). Seratrodast (0.01, 0.03 and 0.1 mg/kgp.o.) given 1 hr before 30 µg/ml U-46619 inhalation dose-dependentlysuppressed the U-46619-induced increase in intranasal pressureby 17, 55 and 79% (P < .01), respectively (table 4). Azelastine(1 mg/kg p.o.) significantly inhibited the histamine (1000 µg/ml)-inducedincrease in intranasal pressure by 62% (P < .05) (table 4). Thesedrugs did not affect the time course of the U-46619- or histamine-inducedresponses.

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TABLE 3
Effects of seratrodast and azelastine on the U-46619- and histamine-induced increase in nasal vascular permeability in normalguinea pigs
Normal guinea pigs were challenged by perfusion of U-46619 (3 µg/ml) or histamine (100 µg/m) through the nasal cavity. Thedrug or 5% gum arabic (control) was administered p.o. 1 hr beforeU-46619 or histamine perfusion. The increases in dye concentrationin the perfusate during Period 3 are shown. Each value representsthe mean ± S.E. for 4 or 6 animals.

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TABLE 4
Effects of seratrodast and azelastine on the U-46619- and histamine-induced increase in intranasal pressure in normal guineapigs
AUC (0-15 min) (cm H₂O · min) = area under the response curve for the increase in intranasal pressure from 0 to 15 min afterinhalation ended. Normal guinea pigs were challenged by inhalationof U-46619 (30 µg/ml) or histamine (1000 µg/ml) aerosol into thenasal cavity. The drug or 5% gum arabic (control) was administeredp.o. 1 hr before U-46619 or histamine inhalation. Each value representsthe mean ± S.E. for 5 to 8 animals.

Exudation of dye induced by antigen challenge in actively sensitized guinea pigs. In guinea pigs actively sensitized by antigen aerosol inhalation, perfusion of OA (0.1 ~ 1%) into the nasal cavity causeda concentration-dependent increase in dye exudation that increasedslightly in Period 2, peaked in Period 3, and decreased graduallythereafter (fig. 3). In the groups challenged with 0.1, 0.3 and1% OA, the dye concentrations in the Period 3 perfusate were 7.0± 1.8, 9.6 ± 1.8 and 19.8 ± 3.7 µg/ml (P < .01), respectively.The response to 1% OA was significantly different from that ofthe saline-perfused group (1.6 ± 0.2 µg/ml). Seratrodast (0.3,3 and 30 mg/kg p.o.) given 1 hr before antigen challenge significantlyreduced the OA (0.3%)-induced increase in exudation of dye by29, 51 (P < .05) and 74% (P < .01), respectively (table 5). Ozagrel(100 mg/kg p.o.) significantly suppressed this OA-induced responseby 52% (P < .05), and azelastine (1 mg/kg p.o.) significantlyreduced it by 69% (P < .01) (table 5). On the other hand, pranlukast(3 and 30 mg/kg p.o.) given 1 hr before antigen challenge didnot reduce the OA-induced increase in dye exudation (table 5).

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Fig. 3. Increase in nasal vascular permeability induced by antigen challenge into the nasal cavity of actively sensitized guinea pigs.Actively sensitized guinea pigs were challenged by perfusion ofsaline ( $square$ ) or 0.1 ( $black-triangle$ ), 0.3 ( $bullet$ ) or 1% OA ( $black-square$ ) through the nasalcavity during Period 2. Each point represents the mean for 5 to9 animals, and vertical bars represent the standard error. * P< .05, ** P < .01, compared with the saline-perfused group (Dunnett'stest).

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TABLE 5
Effects of seratrodast, ozagrel, azelastine and pranlukast on the antigen-induced increase in nasal vascular permeabilityin actively sensitized guinea pigs
Actively sensitized guinea pigs were challenged by perfusion of a submaximal concentration of OA (0.3%) through the nasalcavity. The drug or 5% gum arabic (control) was administered p.o.1 hr before antigen challenge. The increases in dye concentrationin the perfusate during the first 10 min after antigen challenge(Period 3) are shown. Each value represents the mean ± S.E. for7 to 18 animals.

Increase in intranasal pressure induced by antigen challenge in actively sensitized guinea pigs. In guinea pigs actively sensitized by antigen aerosol inhalation, aerosol inhalation of OA (0.1 ~ 3%) into the nasal cavitycaused a concentration-dependent increase in intranasal pressurethat plateaued at 5 to 10 min after antigen challenge (fig. 4).In the groups challenged with 0.1, 0.3, 1 and 3% OA, the increasesin intranasal pressure 10 min after antigen challenge were 2.2± 1.3, 5.6 ± 1.1, 10.7 ± 2.2 (P < .01) and 10.5 ± 2.1 cm H₂O (P< .05), respectively; two of these values were significantly higherthan in the group that inhaled saline (1.9 ± 0.7 cm H₂O). Seratrodast(0.3, 3 and 30 mg/kg p.o.) given 1 hr before antigen challengedose-dependently reduced the OA (3%)-induced increase in intranasalpressure by 11, 27 and 48% (P < .05), respectively (fig. 5; table6). Azelastine (1 mg/kg p.o.) reduced this OA-induced increasein intranasal pressure, but the value of the AUC did not reachstatistical significance (fig. 5; table 6). Pranlukast (3 and30 mg/kg) given 1 hr before antigen challenge did not inhibitthe OA-induced increase in intranasal pressure (table 6).

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Fig. 4. Increase in intranasal pressure induced by antigen challenge into the nasal cavity of actively sensitized guinea pigs. Activelysensitized guinea pigs were challenged with aerosol inhalationof saline ( $square$ ) or 0.1 ( $black-triangle$ ), 0.3 ( $bullet$ ), 1 ( $black-square$ ) or 3% OA ( $triangle$ ) into thenasal cavity. Each point represents the mean for 4 or 5 animals,and vertical bars represent the standard error. * P < .05, ** P< .01, compared with the saline-inhalation group (Dunnett's test).

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Fig. 5. Effects of seratrodast and azelastine on the antigen-induced increase in intranasal pressure in actively sensitized guineapigs. Actively sensitized guinea pigs were challenged by inhalationof a 3% OA aerosol into the nasal cavity. Seratrodast ( $bullet$ ) andazelastine ( $black-triangle$ ) were administered p.o. at 30 and 1 mg/kg, respectively,1 hr before antigen challenge. Each point represents the meanfor seven animals, and vertical bars represent the standard error.* P < .05, ** P < .01, compared with the control group ( $open circle$ ) (Dunnett'stest).

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TABLE 6
Effects of seratrodast, azelastine and pranlukast on the antigen-induced increase in intranasal pressure in actively sensitizedguinea pigs
AUC (0-25 min) (cm H₂O · min) = area under the response curve for the increase in intranasal pressure from 0 to 25 min afterantigen challenge. Actively sensitized guinea pigs were challengedby inhalation of a 3% OA aerosol into the nasal cavity. The drugor 5% gum arabic (control) was administered p.o. 1 hr before antigenchallenge. Each value represents the mean ± S.E. for 7 to 10 animals.

Decrease in area of the nasopharyngeal airway induced by antigen challenge in actively sensitized guinea pigs. The nasopharyngeal airway was observed by MRI after antigen challenge in actively sensitized guinea pigs. As shown in figure6, the mucosa surrounding the nasopharyngeal airway was observedas an area with a high signal intensity. When compared with thesaline-challenged group, the OA-challenged group showed swellingof the mucosa, and the cross-sectional area of the airway lumenwas significantly reduced by 32 (P < .05) or 33% (P < .01) (fig.6, A and B; table 7). Seratrodast (30 mg/kg p.o.) given 1 hrbefore antigen challenge significantly suppressed the decreasein the area of the airway lumen by 48% (P < .05) (fig. 6C; table7). Azelastine (1 mg/kg p.o.) significantly inhibited the decreasein the area of the airway lumen by 67% (P < .05) (table 7).

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Fig. 6. Representative T₁-weighted transverse slice from an actively sensitized guinea pig after saline (panel A) or antigen (panelsB and C) challenge. A) Nasopharyngeal airway (arrow) and nasalmucosa (arrowhead) from a saline-challenged animal. B) Swellingof the nasal mucosa (arrowheads) and a decrease in the area ofthe nasopharyngeal airway (arrow) are seen after antigen challenge.C) Seratrodast (30 mg/kg) was administered p.o. 1 hr before antigenchallenge. Inhibition of the swelling of the nasal mucosa (arrowhead)and the inhibition of the decrease in the area of the nasopharyngealairway (arrow) are seen.

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TABLE 7
Effects of seratrodast and azelastine on the antigen-induced decrease in the area of the nasopharyngeal airway in activelysensitized guinea pigs
Actively sensitized guinea pigs were challenged by instillation of 0.3% OA into the nasal cavity. Seratrodast (30 mg/kg),azelastine (1 mg/kg) or 5% gum arabic (control) was administeredp.o. 1 hr before antigen challenge. Each value represents themean ± S.E. for 6 to 8 animals.

Levels of TXB₂ and histamine in the perfusate. Concentrations of TXB₂ and histamine in nasal lavage fluid were measured after antigen challenge in actively sensitized guineapigs. As shown in figure 7, the concentration of TXB₂ in nasalcavity perfusate was increased by intranasal antigen challenge,peaked at Period 2 to Period 3 and gradually decreased thereafter.The concentrations of TXB₂ in the perfusates at Periods 2 and3 were 270.2 ± 62.2 (P < .01) and 269.6 ± 57.6 pg/ml (P < .01),respectively, and were significantly higher than in the saline-challengedgroup (43.8 ± 12.3 pg/ml at Period 2 and 40.7 ± 12.4 pg/ml atPeriod 3). The concentration of histamine was markedly increasedduring Period 2 by antigen challenge and declined rapidly thereafter(fig. 7). The concentration of histamine in the Period 2 perfusatewas 22.5 ± 5.2 ng/ml (P < .01) and was significantly higher thanin the saline-challenged group (0.3 ± 0.1 ng/ml).

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Fig. 7. Levels of thromboxane B₂ and histamine in nasal cavity perfusates of actively sensitized guinea pigs. Actively sensitizedguinea pigs were challenged by perfusion of saline (open symbol)or 0.3% OA (closed symbol) during Period 2. Each point representsthe mean for 7 or 8 animals, and vertical bars represent the standarderror. * P < .05, ** P < .01, compared with the saline-perfusedgroup (unpaired t test).

	Discussion

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In this study, we showed that seratrodast (Ashida et al., 1989; Kurokawa et al., 1994), a selective TXA₂ receptor antagonist,and azelastine (Katayama et al., 1981; Zechel et al., 1981), anantihistamine drug, inhibit increases in both vascular permeabilityof the nasal mucosa and intranasal pressure and reduce swellingof the nasal mucosa induced by antigen challenge. In addition,intranasal challenge with U-46619, a TXA₂ mimetic, and histamineincreased nasal vascular permeability and intranasal pressure.Levels of TXB₂ and histamine in nasal lavage fluid were markedlyincreased after antigen challenge in actively sensitized guineapigs. These results strongly suggest that TXA₂ and histamine playpivotal roles in the increases in both vascular permeability ofthe nasal mucosa and intranasal pressure evoked by antigen challengein this allergic rhinitis model. It has been suggested that histaminemediates antigen-evoked edema of the nasal mucosa in guinea pigs(Mizuno et al., 1991; Shirasaki et al., 1992; Sherwood et al.,1993). To the best of our knowledge, this is the first time thatparticipation of TXA₂ in edema of the nasal mucosa induced byan anaphylactic response has been demonstrated.

Although seratrodast is a selective TXA₂ receptor antagonist, it also antagonizes the contractile responses of guinea pigtracheal strips to PGD₂ and PGF₂ (Ashida et al., 1989), becausethese prostanoids contract airway smooth muscle by acting on aTX receptor (TP receptor) on the human and guinea pig airway smoothmuscle (Coleman and Sheldrick, 1989; McKenniff et al., 1991).Therefore, to elucidate further the involvement of TXA₂ in theantigen-induced responses in this model, we also studied the effectof ozagrel (Hiraku et al., 1986), a TX synthetase inhibitor, onantigen-induced increases in nasal vascular permeability. Administrationof ozagrel had an inhibitory effect on the antigen-induced increasein nasal vascular permeability. In addition, PGD₂ and PGF₂at relatively high concentrations tended to decrease both nasalvascular permeability and intranasal pressure in normal guineapigs (tables 1 and 2). These results strongly suggest that theinhibitory effect of seratrodast on the increase in nasal vascularpermeability induced by intranasal antigen challenge resultedfrom an antagonistic effect against the TXA₂ released by antigenchallenge and that PGD₂ and PGF₂ were not involved in theantigen-induced responses in this model. Woodward et al. (1990)demonstrated that PGD₂, but not PGF₂, increases conjunctivalmicrovascular permeability and that this response to PGD₂ couldnot be ascribed to the TX receptor because a selective TXA₂ receptorantagonist had no effect on it. Moreover, it has been reportedthat PGD₂ and PGF₂ do not displace the specific binding ofa radiolabeled TXA₂ receptor antagonist to membrane preparationsof pulmonary arterial endothelial cells (Sung et al., 1989). Therefore,it seems likely that there are differences in the affinities ofthese prostanoids for TP receptors in different regions. In additionto these observations, there are differences between tissues inthe effect of TXA₂ on vascular permeability. It has been reportedthat TXA₂ mimetics, including U-46619, increase vascular permeabilityin the conjunctiva (Woodward et al., 1990) and in the lower airway(Lötvall et al., 1992) as well as in the nose, and that theseresponses are inhibited by selective TX receptor antagonists.On the other hand, Woodward et al. (1990) demonstrated that TXA₂mimetics do not increase cutaneous vascular permeability. Nothingthat has been learned to date can readily account for these differentactivities of TXA₂ mimetics and prostaglandins in different regions.Although the notion of heterogeneous subpopulations of TP receptorsis currently being contested, Raychowdhury et al. (1994) havedemonstrated the existence of a family of TP receptors producedby alternative splicing of the carboxyl terminus. Thus these pharmacologicalobservations also seem to suggest the existence of heterogeneouspopulations of TP receptors. However, the ability of divergentcarboxyl tails significantly to influence recognition of TP receptorligands remains a topic for future detailed examination.

Administration of LTC₄ into the nasal cavity also caused increases in nasal vascular permeability and intranasal pressure,as previously reported (Shirasaki et al., 1992), but the maximalresponses to LTC₄ were less than the maximal responses to U-46619or histamine. Administration of pranlukast (Nakagawa et al., 1992;Yamaguchi et al., 1992), a peptide leukotriene receptor antagonist,had little effect on the antigen-induced increases in nasal vascularpermeability and intranasal pressure. In addition, because swellingof the nasal mucosa is caused by increased vascular permeability,we suspect that pranlukast may not inhibit the swelling of thenasal mucosa induced by antigen challenge in this model. Consideredas a whole, these results suggest that peptide leukotrienes, includingLTC₄, hardly contribute at all to these antigen-induced responses,at least in our guinea pig model.

In this study, we found that antigen challenge into the nasal cavity evoked histamine and TXB₂ release into nasal cavity perfusatesthat peaked during Period 2 and from Period 2 to Period 3, respectively,and that this was followed by a transient increase in dye exudationthat peaked during Period 3. In addition, persistent increasesin intranasal pressure and swelling of the nasal mucosa were inducedby antigen challenge in actively sensitized guinea pigs. It iswidely assumed that nasal blockage is caused by swelling of thenasal mucosa induced by both mucosal edema as a result of increasedvascular permeability and dilation of capacitance vessels, leadingto engorgement of blood in the nasal mucosa. However, Sherwoodet al. (1993) reported that antigen-induced swelling of the nasalmucosa was a result of increased vascular permeability in thenasal mucosa of actively sensitized guinea pigs, because oxymetazoline,a vascular decongestant, did not inhibit the swelling. We thereforeconclude that histamine and TXA₂ released by antigen challengebegin to increase nasal vascular permeability when the levelsof these mediators in the nasal mucosa increase to a certain pointand that the lasting increase in intranasal pressure is secondaryto an increase in nasal vascular permeability with leakage ofplasma that leads to prolonged edema of the nasal mucosa.

It is well known that histamine is released from inflammatory cells in response to immunological stimuli earlier than TXA₂,because histamine and TXA₂ are preformed and newly generated mediators,respectively. In the present study, the increased level of histaminein nasal lavage fluid after antigen challenge peaked earlier thanthat of TXB₂ (fig. 7). In addition, histamine and U-46619 requireddifferent times to increase intranasal pressure; intranasal pressurehad already increased at the end of histamine inhalation but graduallyincreased after U-46619 inhalation (fig. 2). Therefore, it seemsthat histamine and TXA₂ are involved in the antigen-induced increasein intranasal pressure at different times. This suspicion is supportedby the observation that azelastine and seratrodast tended to attenuatethe early (0 to 10 min after antigen challenge) and delayed (10to 25 min after antigen challenge) increases, respectively, inintranasal pressure induced by intranasal antigen inhalation inactively sensitized guinea pigs (fig. 5). Although the sourceof the antigen-induced histamine release is suspected to be mastcells, the source of TXA₂ release in the present experiments isunknown. TXA₂ is known to be generated by several types of cells,including macrophages, neutrophils and mast cells (Higgs et al.,1983; Holgate et al., 1984; Schleimer et al., 1983), and any ofthese may be involved.

We should point out that there are two differences between our guinea pig model and human allergic rhinitis. First, whereasPGD₂ did not increase nasal vascular permeability or intranasalpressure in guinea pigs, instillation of PGD₂ into the human nasalcavity increases nasal airway resistance (Doyle et al., 1990).Second, whereas azelastine inhibited the antigen-induced responsesin this guinea pig model, antihistamine drugs had little or noeffect on nasal blockage in patients with allergic rhinitis (Corradoet al., 1987; Holmberg et al., 1989; Jankowski et al., 1993).Although it is difficult to determine the source of these differencesbetween the effects in humans and in guinea pigs, it may be relatedto the fact that we could not evaluate congestion, which is oneof the major causes of nasal blockage in human allergic rhinitis.The differences may also be attributable in part to differentmethods of using the antihistamine drugs, which were administeredprophylactically and therapeutically. Furthermore, it has beenreported that the immediate response is followed by a late-phaseresponse that begins several hours after intranasal antigen challengein approximately 50% of patients with allergic rhinitis (Dvoraceket al., 1984). In this study, we were concerned with only theimmediate response after antigen challenge in this model. Thismay also have been a cause of the discrepancies. On the otherhand, it has been reported that histamine increases the vascularpermeability of the nasal mucosa (Svensson et al., 1992) and increasesnasal airway resistance (Austin and Foreman, 1994) in humans,whereas the cyclooxygenase inhibitors indomethacin (McLean etal., 1983) and flurbiprofen (Brooks and Karl, 1988) inhibit nasalblockage in patients with allergic rhinitis. High levels of histamine(Naclerio et al., 1983) and TXB₂ (Brown et al., 1987) have beenidentified in the nasal lavage fluid of patients with allergicrhinitis after antigen challenge. In addition, Narita et al. (1996)have shown that BAY u 3405, a TX receptor antagonist, reducesthe biphasic increase in total airway resistance, probably nasalairway resistance, after intranasal antigen challenge in guineapigs. Thus these observations, as well as the results in our guineapig model of allergic rhinitis, suggest that TXA₂ and histaminemay contribute to the development of nasal blockage in allergicrhinitis in humans. However, there is no further evidence to indicatethat TXA₂ and histamine directly participate in the developmentof nasal blockage in human allergic rhinitis in general. It isuncertain whether the findings described in the present paperare applicable to human allergic rhinitis.

In conclusion, we report that U-46619, a TXA₂ mimetic, as well as histamine, increased both nasal vascular permeability andintranasal pressure and that seratrodast and azelastine inhibitedthe increases in nasal vascular permeability and intranasal pressureinduced by intranasal antigen challenge in actively sensitizedguinea pigs. We also demonstrated that TXB₂ and histamine levelsin nasal lavage fluid increased after intranasal antigen challenge.Taken together, these results strongly suggest that TXA₂ and histamineplay important roles in the development of increased nasal vascularpermeability and intranasal pressure evoked by antigen challengein this guinea pig model and that seratrodast may be a usefultool for elucidating the pathophysiological role of TXA₂ in humanallergic rhinitis.

	Acknowledgments

The writers acknowledge the excellent technical assistance of Yumiko Nakai and the expert advice and comments of Yasuo Nagaiin preparing the manuscript.

	Footnotes

Accepted for publication November 11, 1996.

Received for publication April 15, 1996.

Send reprint requests to: Masashi Yamasaki, Pharmaceutical Research Laboratories I, Pharmaceutical Research Division, Takeda Chemical Industries, Ltd., 2-17-85 Jusohonmachi, Yodogawa-ku, Osaka 532, Japan.

	Abbreviations

AUC, area under the response curve; EDTA, ethylenediaminetetraacetic acid disodium salt; LTC₄, leukotriene C₄; MRI, magnetic resonance imaging; OA, ovalbumin; PG, prostaglandin; TX, thromboxane.

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