Rofecoxib [Vioxx, MK-0966; 4-(4'-Methylsulfonylphenyl)-3-phenyl-2-(5H)-furanone]: A Potent and Orally Active Cyclooxygenase-2 Inhibitor. Pharmacological and Biochemical Profiles

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Vol. 290, Issue 2, 551-560, August 1999

Rofecoxib [Vioxx, MK-0966; 4-(4'-Methylsulfonylphenyl)-3-phenyl-2-(5H)-furanone]: A Potent and Orally Active Cyclooxygenase-2 Inhibitor. Pharmacological and Biochemical Profiles

C.-C. Chan, S. Boyce, C. Brideau, S. Charleson, W. Cromlish, D. Ethier, J. Evans, A. W. Ford-Hutchinson, M. J. Forrest, J. Y. Gauthier, R. Gordon, M. Gresser, J. Guay, S. Kargman, B. Kennedy, Y. Leblanc, S. Leger, J. Mancini, G. P. O'Neill, M. Ouellet, D. Patrick, M. D. Percival, H. Perrier, P. Prasit, I. Rodger, P. Tagari, M. Therien, P. Vickers, D. Visco, Z. Wang, J. Webb, E. Wong, L.-J. Xu, R. N. Young, R. Zamboni and D. Riendeau

Departments of Pharmacology, Biochemistry and Molecular Biology, and Medicinal Chemistry, Merck Frosst Centre for Therapeutic Research, Kirkland, Quebec, Canada (C.-C.C., C.B., S.C., W.C., D.E., J.E., A.W.F.-H., J.Y.G., R.G., M.G., J.G., S.K., B.K., Y.L., S.L., J.M., G.P.O., M.O., M.D.P., H.P., P.P., I.R., P.T., M.T., P.V., Z.W., E.W., L.-J.X., R.N.Y., R.Z., D.R.); Department of Pharmacology, Merck Research Laboratories, Harlow, UK (S.B., J.W.); Department of Pharmacology, Merck Research Laboratories, Rahway, New Jersey (M.J.F., D.V.); and Safety Assessment, Merck Research Laboratories, West Point, Pennsylvania (D.P.)

	Abstract

Top Abstract Introduction Experimental Procedures Results Discussion References

The discoveries that cyclooxygenase (COX)-2 is an inducible form of COX involved in inflammation and that COX-1 is the majorisoform responsible for the production of prostaglandins (PGs)in the gastrointestinal tract have provided a rationale for thedevelopment of specific COX-2 inhibitors as a new class of anti-inflammatoryagents with improved gastrointestinal tolerability. In the presentstudy, the preclinical pharmacological and biochemical profilesof rofecoxib [Vioxx, also known as MK-0966, 4-(4'-methylsulfonylphenyl)-3-phenyl-2-(5H)-furanone],an orally active COX-2 inhibitor, are described. Rofecoxib isa potent inhibitor of the COX-2-dependent production of PGE₂ inhuman osteosarcoma cells (IC₅₀ = 26 ± 10 nM) and Chinese hamsterovary cells expressing human COX-2 (IC₅₀ = 18 ± 7 nM) with a 1000-foldselectivity for the inhibition of COX-2 compared with the inhibitionof COX-1 activity (IC₅₀ > 50 µM in U937 cells and IC₅₀ > 15 µMin Chinese hamster ovary cells expressing human COX-1). Rofecoxibis a time-dependent inhibitor of purified human recombinant COX-2(IC₅₀ = 0.34 µM) but caused inhibition of purified human COX-1in a non-time-dependent manner that could only be observed ata very low substrate concentration (IC₅₀ = 26 µM at 0.1 µM arachidonicacid concentration). In an in vitro human whole blood assay, rofecoxibselectively inhibited lipopolysaccharide-induced, COX-2-derivedPGE₂ synthesis with an IC₅₀ value of 0.53 ± 0.02 µM compared withan IC₅₀ value of 18.8 ± 0.9 µM for the inhibition of COX-1-derivedthromboxane B₂ synthesis after blood coagulation. Using the ratioof the COX-1 IC₅₀ values over the COX-2 IC₅₀ values in the humanwhole blood assay, selectivity ratios for the inhibition of COX-2of 36, 6.6, 2, 3, and 0.4 were obtained for rofecoxib, celecoxib,meloxicam, diclofenac, and indomethacin, respectively. In severalin vivo rodent models, rofecoxib is a potent inhibitor of carrageenan-inducedpaw edema (ID₅₀ = 1.5 mg/kg), carrageenan-induced paw hyperalgesia(ID₅₀ = 1.0 mg/kg), lipopolysaccharide-induced pyresis (ID₅₀ =0.24 mg/kg), and adjuvant-induced arthritis (ID₅₀ = 0.74 mg/kg/day).Rofecoxib also has a protective effect on adjuvant-induced destructionof cartilage and bone structures in rats. In a ⁵¹Cr excretion assay for detection of gastrointestinal integrityin either rats or squirrel monkeys, rofecoxib has no effect atdoses up to 200 mg/kg/day for 5 days. Rofecoxib is a novel COX-2inhibitor with a biochemical and pharmacological profile clearlydistinct from that of current nonsteroidal anti-inflammatory drugsand represents a new therapeutic class of anti-inflammatory agentsfor the treatment of the symptoms of osteoarthritis and rheumatoidarthritis with improved gastrointestinaltolerability.

	Introduction

Top Abstract Introduction Experimental Procedures Results Discussion References

Cyclooxygenases (COXs) are bifunctional hemoproteins that catalyze the bisoxygenation of arachidonic acid to prostaglandin(PG)H₂, which serves as the common precursor for the synthesisof PGs, prostacyclins, and thromboxanes (TBXs), collectively knownas prostanoids. It is now well established that COXs exist astwo isoforms that catalyze the same reaction but differ in termsof regulation of expression (see reviews in Vane and Botting,1995; Smith and DeWitt, 1996). The constitutive isoform COX-1is responsible for the production of PGs involved in prostanoid-mediatedphysiological functions such as gastric cytoprotection, maintenanceof renal homeostasis, and maintenance of normal platelet functions.A second isoform, COX-2, has been identified and has been demonstratedto be highly expressed in response to inflammatory or mitogenicstimuli. Thus, it is proposed that COX-2 is responsible for theproduction of PGs associated with inflammatory conditions. Itis well documented in the literature that the mechanism of actionof nonsteroidal anti-inflammatory drugs (NSAIDs) involves inhibitionof COX (Vane, 1971). The therapeutic actions of these compounds,such as their anti-inflammatory, analgesic, and antipyretic effects,can be explained by inhibition of PG formation. On the other hand,it is also well known that NSAIDs have mechanism-based side effects(Allison et al., 1992; Murray and Brater, 1993; Schafer, 1995)that limit the dose of NSAIDs in patients. The discovery of asecond isoform of COX has provided the rationale for the developmentof specific COX-2 inhibitors as a novel class of anti-inflammatorycompounds compared with current NSAIDs, which inhibit both COX-1and COX-2 with similar potency (Meade et al., 1993; Brideau etal., 1996). It is hypothesized that a specific COX-2 inhibitorwill achieve therapeutic efficacy in osteoarthritis and pain managementwhile avoiding the serious side effects, in particular, gastrointestinalulceration related to COX-1 inhibition observed with NSAIDs. Thishypothesis is supported by data with a number of COX-2 selectiveinhibitors that have shown efficacy in animal models of pain,inflammation, pyresis, and superior gastrointestinal tolerabilitycompared with NSAIDs (Futaki et al., 1993; Seibert et al., 1994;Chan et al., 1995; Riendeau et al., 1997b). Rofecoxib (Vioxx,also known as MK-0966) is a novel and highly selective COX-2 inhibitorthat has been shown to be efficacious in the treatment of osteoarthritis,comparable to NSAIDs (Fig. 1) (Ehrich et al., 1998a,b; 1999) andis currently in the final stage of development. In the presentstudy, the preclinical pharmacological and biochemical profilesof rofecoxib are described and are discussed with respect to clinicalfindings.

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Fig. 1. Structure of rofecoxib.

	Experimental Procedures

Top Abstract Introduction Experimental Procedures Results Discussion References

In Vitro Biochemical and Pharmacological Assays

Inhibition Studies with Recombinant Human COX-1 and COX-2. Microsomal preparations of recombinant human COX-1 and COX-2 were prepared from a vaccinia virus-COS-7 cell expression system(O'Neill et al., 1994) Recombinant human COX-1 and COX-2 wereexpressed in baculovirus-Sf9 cells, and enzymes were purifiedas described previously (Ouellet and Percival, 1995; Cromlishand Kennedy, 1996). Enzymatic activity was monitored continuouslyby either a fluorescence assay measuring the appearance of theoxidized form of the reducing agent cosubstrate homovanillic acidor by oxygen consumption (Ouellet and Percival, 1995). The HPLCassay for the assessment of inhibition of purified COX-1 by rofecoxibwith 0.1 µM arachidonic acid substrate concentration, the determinationof the stoichiometry of the complex between COX-2 and rofecoxib,the dissociation rate constant of the enzyme-inhibitor complexby recovery of enzymatic activity, and the recovery of intactrofecoxib from that complex were all performed as described previously(Riendeau et al., 1997b). The solvent system for the HPLC analysisof rofecoxib was 15:85 MeOH/aqueous potassium phosphate (1 g/liter),with elution by a linear gradient of 15 to 75% MeOH over 25 minwith detection at 275 nm on a Novapak C18 column (Waters, Milford,MA).

Spectrophotometric Assay of Recombinant Human COX-2. Enzymatic activity of the purified COX-2 was measured using a chromogenic assay based on the oxidation of N,N,N',N'-tetramethyl-p-phenylenediamine(TMPD) during the reduction of PGG₂ to PGH₂ (Copeland et al.,1994). The assay mixture (180 µl) contains 100 mM sodium phosphate,pH 6.5, 1 µM hematin, 1 mg/ml gelatin, 2 to 5 µg/ml of purifiedCOX-2, and 4 µl of the test compound in dimethyl sulfoxide (DMSO).The assay was also performed in the presence of the detergentGenapol X-100 (CalBiochem, San Diego, CA) at a final concentrationof 2 mM. The mixture was preincubated at room temperature (22°C)for 15 min before initiation of the enzymatic reaction by theaddition of 20 µl of a solution of 1 mM arachidonic acid and 1mM TMPD in assay buffer (without enzyme or hematin). For assaysin the presence of Genapol, the arachidonic acid and TMPD solutionwas prepared in 50% aqueous ethanol. The enzyme activity was measuredby estimation of the initial velocity of TMPD oxidation over thefirst 36 s of the reaction as followed from the increase in absorbancyat 610 nm. A low rate of nonenzymatic oxidation was observed inthe absence of COX-2 and was subtracted before the calculationof the percentage ofinhibition.

Whole-Cell Assays with Osteosarcoma Cells (COX-2) and U937 Cells (COX-1). The human osteosarcoma cell line has been shown to selectively express COX-2 by reverse transcription-polymerase chain reactionand immunoblot analysis, whereas undifferentiated human lymphomaU937 cells selectively express COX-1. The production of PGE₂ bythese cells after arachidonic acid challenge was used as an indexof cellular COX-2 and COX-1 activity, respectively. Rofecoxibwas preincubated for 5 to 15 min with the cells under serum-freeconditions [Hanks' balanced salt solution (HBSS)] before a 10-minstimulation with 10 µM arachidonic acid and measurement of PGE₂production as described previously (Wong et al., 1997). COX activityin each cell line is defined as the difference in PGE₂ concentrationsin samples incubated in the presence or absence of arachidonicacid.

Whole-Cell Assays with Transfected Chinese Hamster Ovary (CHO) Cells Expressing COX-1 and COX-2. Stably transfected CHO cells expressing human COX-1 and COX-2 were cultured and assayed for the production of PGE₂ after stimulationby arachidonic acid as described previously (Kargman et al., 1996).Cells (0.3 × 10⁶ cells in 200 µl) were preincubated in HBSS containing 15 mM HEPES,pH 7.4, with 3 µl of the test drug or DMSO vehicle for 15 minat 37°C before challenge with arachidonic acid. Cells were challengedfor 15 min with an arachidonic acid solution [10% ethanol (v/v)in HBSS] to yield final concentrations of 10 µM arachidonic acidin the CHO[COX-2] assay and of 0.5 µM arachidonic acid in theCHO[COX-1] assay. In the absence of addition of exogenous arachidonicacid, levels of PGE₂ in samples from CHO[COX-1] were <30 pg PGE₂/10⁶ cells. In the presence of 0.5 µM exogenous arachidonic acid,levels of PGE₂ in samples from CHO[COX-1] cells increased to 260to 1500 pg PGE₂/10⁶ cells. After stimulation with 10 µM exogenous arachidonic acid,levels of PGE₂ in samples from CHO[COX-2] cells increased from<120 to 700 to 1600 pg PGE₂/10⁶ cells. Compounds were typically tested at eight concentrationsin duplicate using 3-fold serial dilutions in DMSO. COX activityin the absence of test compounds is determined as the differencein PGE₂ levels of cells challenged with arachidonic acid versusthe PGE₂ levels in cells mock-challenged with ethanolvehicle.

Whole-Cell Assay for Rat COX-2 in Sf9 Insect Cells. Rat COX-2 cellular activity was assayed using a procedure based on the arachidonic acid-dependent production of PGE₂ by baculovirus-infectedSf9 cells expressing rat COX-2 (Cromlish and Kennedy, 1996). Theassay for the production of PGE₂ by arachidonic acid-stimulatedcells was performed as described for the CHO[COX-2] cells using10 µM arachidonic acid, a 10-min reaction time, and a total of2 × 10⁵ cells (infected plus noninfected cells) per well (final volumeof 200 µl). The production of PGE₂ by Sf9 [rat COX-2] cells increased3- to 19-fold after stimulation with 10 µM arachidonic acid tovalues of 4.0 to 8.1 ng PGE₂/10⁶ total cells. Inhibitors, tested at eight concentrations using3-fold serial dilutions of the highest inhibitor concentrationin DMSO, were preincubated for 15 min before arachidonic acidchallenge.

Human, Rat, and Dog Microsomal COX Assays. Whole kidneys (1-10 g of tissue) were suspended in 50 mM potassium phosphate buffer, pH 7.1, containing 0.1 M NaCl, 2 mM EDTA,and 1 mM phenylmethylsulfonyl fluoride (homogenization buffer).Samples were then homogenized for 2 min on ice using a hand-heldtissue homogenizer (Biospec Products, Inc., Bartlesville, OK)at maximum setting, after which they were sonicated for 10 s usinga microultrasonic cell disrupter (Kontes, Vineland, NJ). Tissuehomogenates were then centrifuged at 100,000g for 1 h at 4°C.The 100,000g microsomal pellet was resuspended in homogenizationbuffer and was sonicated (2 × 10 s) on ice. The resulting human,rat, and dog kidney microsomal suspensions diluted to proteinconcentrations of approximately 6, 10, and 12 mg/ml, respectively.Aliquots of microsomal preparations were stored at $-$ 80°C and thawedon ice immediately beforeassays.

Rofecoxib was preincubated at room temperature for 5 or 15 min with a microsomal preparation from rat, dog, or human kidneys.The preincubation buffer contained 0.1 M Tris·HCl, pH 7.4, 10mM EDTA, 0.5 mM phenol, 1 mM reduced glutathione, 1 µM hematin,and a protein concentration of 0.12 mg/ml. Arachidonic acid wasthen added to a final concentration of 2 µM, and the samples werefurther incubated at room temperature for 40 min. After the incubationperiod, the reaction was terminated by the addition of 25 µl of1 N HCl with mixing. Samples were neutralized by the additionof 25 µl of 1 N NaOH before analysis of the amount PGE₂ by radioimmunoassay.Assays were performed in duplicate or triplicate. Control reactionmixtures contained ethanol vehicle instead of arachidonic acid.In the absence of the addition of arachidonic acid, levels ofPGE₂ in samples from human, dog, and rat kidney microsomes wereapproximately 1.5 ng/mg protein, 0.1 ng/mg protein, and 6.7 ng/mgprotein, respectively. In the presence of arachidonic acid, levelsof PGE₂ in these preparations increased to approximately 4.2 ng/mgprotein, 1.2 ng/mg protein, and 22 ng/mg protein, respectively.COX activity in the absence of test compounds is defined as thedifference between PGE₂ levels in samples incubated in the presenceof arachidonic acid or ethanolvehicle.

Assay of U937 Microsomal COX-1 at Low Arachidonic Acid Concentration. The activity of human COX-1 in a microsomal preparation from U937 cells was assayed at low arachidonic acid concentration(Riendeau et al., 1997a). Rofecoxib was preincubated with themicrosomal preparation (protein concentration of 0.12 mg/ml) for15 min at room temperature in 0.1 M Tris · HCl, pH 7.4, 10 mMEDTA, 0.5 mM phenol, 1 mM reduced glutathione, and 1 µM hematin.After preincubation, arachidonic acid was added to a final concentrationof 0.1 µM, and the samples were further incubated for 40 min beforequantification of PGE₂ by radioimmunoassay. COX activity in theabsence of rofecoxib was determined as the difference in PGE₂levels of microsomes incubated with arachidonic acid versus thePGE₂ levels in microsomes incubated with ethanolvehicle.

TBX B₂ and 12-Hydroxyeicosatetraenoic Acid (12-HETE) Production by Calcium Ionophore-Activated Human Platelets. Washed human platelets in HBSS buffered with 15 mM HEPES, pH 7.4, were preincubated at a final concentration of 4 × 10⁷ cells/ml (0.2-0.25 ml) in the absence or presence of the inhibitor(from a 125-fold concentrated solution in DMSO) for 2 min beforestimulation with 2 µM calcium ionophore A23187 for TBX₂ and 12-HETEproduction (Riendeau et al., 1994).

Inhibition of Leukotriene B (LTB)₄ Production by Human Polymorphonuclear (PMN) Leukocytes. Rofecoxib was preincubated with PMN leukocytes prepared from human blood from consenting volunteers (5 × 10⁵ cells/ml) in HEPES (15 mM)-buffered HBSS, pH 7.4, for 2 min at37°C. The cells were then challenged with 10 µM calcium ionophoreA23187, and the reaction was terminated after 5 min by the additionof cold methanol. The production of LTB₄ by human PMN leukocyteswas determined by radioimmunoassay. The effect of rofecoxib wasdetermined using a five-point titration over the concentrationrange of 0.31 to 25 µM. The percentage of inhibition was determinedfrom the difference in LTB₄ production by ionophore-challengedcells incubated in the presence of rofecoxib or with the DMSOvehicle.

Leukocyte 15-Lipoxygenase Assay. Rofecoxib was incubated at concentrations ranging from 0.7 to 20 µM with partially purified 15-lipoxygenase from human leukocytesin 0.05 M sodium phosphate, pH 6.3, 24 µg/ml phosphatidylcholine,and 20 µM arachidonic acid. After a 10-min incubation at roomtemperature, the reaction was quenched with acetonitrile and analyzedby reverse phase-HPLC on a C18 column eluted with acetonitrile/water/trifluoroacetic(60:40:0.1) for the quantification of 15-hydroperoxyeicosatetraenoicacid.

Human Whole Blood Assay. The assay was done using identical procedures as reported previously (Brideau et al., 1996). Briefly, for the COX-2 assay,fresh heparinized human whole blood was incubated with lipopolysaccharide(LPS) from Escherichia coli at 100 µg/ml and with 2 µl of vehicle(DMSO) or a test compound for 24 h at 37°C. PGE₂ levels in theplasma were measured using radioimmunoassay after deproteination.For the COX-1 assay, an aliquot of fresh blood was mixed witheither DMSO or a test compound and was allowed to clot for 1 hat 37°C. TBX₂ levels in the serum were measured using an enzymeimmunoassay after deproteination. The effects of rofecoxib, celecoxib,meloxicam, diclofenac, and indomethacin were examined under thesame experimentalconditions.

In Vivo Assays

All procedures used in the in vivo assays were approved by the Animal Care Committees or Institutional Animal Care and UseCommittee at the Merck Frosst Centre for Therapeutic Research(Kirkland, Quebec, Canada), Merck, Sharp & Dohme NeuroscienceResearch Centre (Harlow, UK), and Merck Research Laboratories(Rahway, NJ) according to guidelines established by the CanadianCouncil on Animal Care, the British Home Office, and the U.S.Department of Agriculture and National Institutes of Health,respectively.

The following assays were done using identical procedures as described previously (Chan et al., 1995); these studies includedcarrageenan-induced rat paw edema assay, carrageenan-induced ratpaw hyperalgesia assay, endotoxin-induced pyresis in rats, and⁵¹Cr fecal excretion in rats and squirrel monkeys. Additional studiesare describedbelow.

Rat Adjuvant-Induced Arthritis (AIA) Model. AIA was induced in six groups of 10 rats (female Lewis, 144-172 g, 7 weeks old), each by an intradermal injection of 0.5 mgof Mycobacterium butyricum in light mineral oil in the left hindfoot pad as described previously (Fletcher et al., 1998). Tenrats were not injected and served as nonadjuvant controls. Bodyweights, radiographs, and foot volumes of the noninjected (secondary)paws were determined on various days (0, 14, and 21). Rofecoxib(0.1, 0.3, 1.0, and 3.0 mg/kg/day p.o.; 0.05, 0.15, 0.5, and 1.5mg/kg b.i.d.), indomethacin (1 mg/kg/day p.o.; 0.5 mg/kg b.i.d.),and appropriate vehicles were started on day 0 and continued throughoutthe experiment. Rats were euthanized by carbon dioxide inhalationon day 21. The thymus and spleen of all rats were removed andweighed. To assess tibiotarsal joint integrity, radiographic scoreswere assigned according to an adaptation of a previously describedmethod (Clark et al., 1979) by a radiologist who was blinded totreatment. Two-factor ("treatment" and "time") ANOVA with repeatedmeasures on "time" were applied to the percent changes for bodyweight and foot volumes and to the rank-transformed radiographictotal scores. A post hoc Dunnett's test was conducted to comparethe effect of treatments to vehicle. A one-way ANOVA was appliedto the thymic and spleen weights, followed by the Dunnett's test,to compare the effect of treatments tovehicle.

Ex Vivo Whole Blood Assay in Anesthetized Dogs. Fasted normal male laboratory beagles were anesthetized and bronchially intubated. After 15-min stabilization, a blood samplewas collected into anticoagulant, and a bolus dose of either vehicle(80% PEG 200 in distilled water), diclofenac (0.1 mg/kg), or rofecoxib(0.05, 0.1, or 0.2 mg/kg) was administered i.v., followed by acontinuous infusion of either vehicle, diclofenac (2.5 µg/kg/min),or rofecoxib (0.8-8 µg/kg/min). Additional blood samples wereobtained 1 and 4 h after the beginning of the infusion and wereincubated with LPS from E. coli (100 µg/ml) for 2 h at 37°C. Arachidonicacid dissolved in 30% ethanol in PBS, or the latter vehicle wasthen added (final arachidonic acid concentration of 100 µM) to500-µl aliquots and incubated for 30 min. Prostanoid productionwas terminated by rapid centrifugation and methanolic extractsof plasma were prepared [plasma/MeOH 1:4 (v/v)]. The PGE₂ contentof dilutions of these extracts was then measured by specific radioimmunoassay.Postdose inhibition of arachidonic acid-induced PGE₂ productionwas calculated by comparison with predosevalues.

Statistics

Results are expressed as mean ± S.E.M. Unless otherwise specified, differences between vehicle control and treatment groupswere tested using one-way ANOVA, followed by multiple comparisonby the Dunnett's test. A value of P < .05 was considered statisticallysignificant. Dose-response curves for percent inhibition werefitted by a four-parameter logistic function using a nonlinearleast-squares regression. IC₅₀ or ID₅₀ was derived by interpolationfrom the fitted four-parameterequation.

Materials

The following compounds were synthesized by the Medicinal Chemistry Department at Merck Frosst Centre for Therapeutic Research:rofecoxib, celecoxib (Penning et al., 1997), meloxicam. Sourcesof other compounds were: diclofenac, flurbiprofen, naproxen, LPS(Sigma-Aldrich, Oakville, Ontario, Canada); indomethacin (Merck,Sharp & Dohme Canada, Kirkland, Quebec,Canada).

	Results

Top Abstract Introduction Experimental Procedures Results Discussion References

In Vitro Studies

Selective Inhibition of COX-2 by Rofecoxib in Intact Cell Assays. Rofecoxib is a potent inhibitor of COX-2 in a variety of cell-based assays (IC₅₀ = 18-46 nM) and shows a 1000-fold selectivityfor the inhibition of COX-2 compared with COX-1 (Table 1). Rofecoxibinhibited the arachidonic acid-dependent production of PGE₂ byosteosarcoma cells (COX-2) with an IC₅₀ value of 26 ± 10 nM (n= 5). No significant decrease in the potency of rofecoxib wasobserved in the presence of 1% human, dog, or rat serum. The IC₅₀value for the inhibition of arachidonic acid-dependent productionof PGE₂ by U937 cells (COX-1) was >50 µM (n = 4). Similarly, rofecoxibwas a potent inhibitor of recombinant human COX-2 expressed instably transfected CHO cells (IC₅₀ = 18 ± 7 nM, n = 6) and was>800-fold less potent as an inhibitor of human COX-1 in stablytransfected CHO cells (IC₅₀ > 15 µM, n = 3). Rofecoxib was alsofound to be an inhibitor of rat COX-2 in a Sf9 whole-cell assaywith a potency (46 ± 9 nM, n = 3) similar to that obtained forindomethacin (18 nM, n = 2). The data for rofecoxib and indomethacinare summarized in Table 1 and indicate that although indomethacinis a potent inhibitor of both COX-1 and COX-2 in cell-based assays,rofecoxib is a potent and selective inhibitor of human COX-2 incell-based assays.

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TABLE 1
Potency and selectivity of rofecoxib in in vitro assays

Inhibition Studies with Purified COX-2 and COX-1. The kinetic mechanism of inhibition of COX-1 and COX-2 by rofecoxib was investigated using microsomal and purified recombinanthuman enzymes. Rofecoxib inhibits the COX activity of purifiedhuman COX-2 (spectrophotometric assay), with IC₅₀ values of 0.34(n = 2) and 0.40 µM (n = 2) for the assays performed in eitherthe absence or presence of the detergent Genapol X-100, respectively.The compound is approximately equipotent to indomethacin in thisassay (Table 1). The level of inhibition of purified COX-2 byrofecoxib was dependent on the preincubation period of enzymeand drug before initiation of the reaction with arachidonic acid.Increased concentrations of rofecoxib result in a faster rateof onset of inhibition (Fig. 2A). Analysis of the data in termsof a two-step mechanism of inhibition (Ouellet and Percival, 1995;Riendeau et al., 1997b) gave a value for the second order rateconstant for the onset of inhibition of COX-2 by rofecoxib of0.0036 ± 0.0024 µM¹ s¹. A similar time-dependent inhibition by rofecoxib was observedusing microsomal COX-2, and an IC₅₀ value of 0.13 µM was obtainedafter a 15-min preincubation period. In contrast, the inhibitionof COX-1 by rofecoxib is non-time-dependent. Microsomal COX-1was inhibited approximately 15% by 10 µM rofecoxib in fluorescenceassays performed without preincubation and using an initial arachidonicacid concentration of 20 µM. No increase in inhibition was observedwith up to 15-min preincubation of enzyme and inhibitor. Higherlevels of inhibition of purified COX-1 could only be observedin assays performed in the presence of very low concentrationsof arachidonic acid (0.1 µM). Under these conditions, an IC₅₀value of 26 ± 6 µM (n = 11) was obtained for rofecoxib.

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Fig. 2. A, time-dependent inhibition of purified human COX-2 by rofecoxib. Purified human COX-2 (0.08 µg) was preincubated for different periods of time with 0.5 µM (

) or 8 µM (

) rofecoxib before the initiation of the reaction with arachidonic acid and measurement of the remaining activity by the fluorescence assay. The lines represent the fit of the data to a single exponential. The activity of the vehicle-treated control (2.5 rfu/s) remained constant throughout the experiment. B, recovery of activity of rofecoxib-inhibited COX-2 by dialysis. Purified human COX-2 (0.07 mg) was pretreated for 60 min with 1.2 mol equivalents rofecoxib before dialysis against 10,000 volumes of buffer. Aliquots were removed at intervals, and the recovery of enzyme activity of the rofecoxib-treated COX-2 (

) or vehicle-treated control (

) was measured using the oxygen consumption assay.

Both active COX-2 and intact inhibitor could be recovered after time-dependent inhibition, demonstrating that the inhibitionof COX-2 by rofecoxib was not due to the irreversible covalentinactivation of the enzyme. The recovery of active enzyme wasdemonstrated in an experiment in which purified COX-2 was inhibitedwith a small excess of rofecoxib and then dialyzed against a largeexcess of buffer. The results (Fig. 2B) show that the enzyme activityrecovers after inhibition in a first order manner with a T_1/2of 9 ± 2 h and that after a dialysis period of 23 h, close to100% of the original activity has been recovered. In the secondexperiment, purified COX-2 was treated with 1 Eq of rofecoxibfor 30 min. After this time, the enzyme was 91% inhibited comparedwith a vehicle-treated control. The enzyme-inhibitor complex wasthen denatured, and any released inhibitor was extracted fromthe protein by treatment with organic solvent. HPLC of the extractshowed a single peak at the same retention time as that of authenticrofecoxib with quantitative recovery compared with an identicallytreated no-enzyme control. These results therefore are consistentwith the noncovalent nature of the tight complex between COX-2and rofecoxib. Time-dependent and reversible inhibition couldalso be demonstrated in CHO[COX-2] cells (data not shown). Thestoichiometry of the enzyme-inhibitor complex was determined bya titration in which aliquots of purified COX-2 (3.4 µM) weretreated with 0 to 6 µM rofecoxib and the remaining COX activitywas measured after a 30-min preincubation period. A linear decreasein enzyme activity with increasing inhibitor concentration wasobtained (results not shown), with the maximal inhibition observed(94%) occurring at concentrations of rofecoxib of more than 3.2µM. This result is therefore consistent with the formation ofan enzyme-inhibitor complex having 1:1stoichiometry.

Effect of Rofecoxib on Human, Dog, and Rat Microsomal COX Activities. Rofecoxib is a time-dependent inhibitor of human recombinant COX-2 in microsomal assays with an IC₅₀ value of 130 nM aftera 15-min preincubation. In human, dog, and rat kidney microsomepreparations (COX-1), rofecoxib was substantially less potentwith IC₅₀ values of 14, >30, and >30 µM, respectively. An incompleteinhibition of PGE₂ production in human kidney microsomes by rofecoxibwas observed at doses of rofecoxib exceeding the IC₅₀ value (maximuminhibition of 67-86%), probably due to the limited water solubilityof the compound under the assay conditions. Data are summarizedin Table 1 and compared with those obtained with indomethacin,which is a potent inhibitor of PGE₂ synthesis by the three differentkidney microsomal preparations. Thus rofecoxib is a weak or totallyineffective inhibitor of PGE₂ production by microsomes from human,rat, or dog kidneys, at concentrations 30 to 100 times higherthan those required for the inhibition by indomethacin, in agreementwith the selectivity of inhibition of rofecoxib for COX-2.

Inhibition of Microsomal COX-1 from U937 Cells at Low Arachidonic Acid Concentration. The effect of rofecoxib on COX-1 was determined using a sensitive assay based on the production of PGE₂ by U937 cell microsomesafter incubation with a low, subsaturating concentration of arachidonicacid (0.1 µM). Potent nonselective inhibitors, such as indomethacin,show IC₅₀ values in the low nanomolar range in this assay (Table1). Rofecoxib inhibited the production of PGE₂ by U937 cell microsomesin the assay at low arachidonic acid concentration with an IC₅₀value of 2.0 ± 0.5 µM (n =7).

Effect of Rofecoxib on TBX₂ and 12-HETE Synthesis by Human Platelets. The production of TBX₂ by Ca²⁺ ionophore-stimulated human platelets was used to further evaluate the potency of inhibitors atblocking COX-1-mediated prostanoid production. In this assay,indomethacin and diclofenac were potent inhibitors (IC₅₀ = 2-4nM) of TBX₂ production. Rofecoxib had no significant effect (<15%inhibition) on the production of TBX₂ and 12-HETE by calcium ionophore-challengedhuman platelets (IC₅₀ > 20 µM; n = 5 with two different plateletpreparations).

Human Whole Blood COX-1 and COX-2 Assay. The results are summarized in Table 2. Rofecoxib is a potent inhibitor of human whole blood COX-2 activity with an IC₅₀ valueof 0.53 ± 0.02 µM. Using the ratio of the COX-1 IC₅₀ value overthe COX-2 IC₅₀ value, selectivity ratios for the inhibition ofCOX-2 of 36, 6.6, 2, 3, and 0.4 were obtained for rofecoxib, celecoxib,meloxicam, diclofenac, and indomethacin, respectively. Thus, rofecoxibhas the highest selectivity among this panel of compounds whentested under the same experimental conditions.

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TABLE 2
IC₅₀ values of rofecoxib, celecoxib, meloxicam, diclofenac, and indomethacin in human whole blood COX-1 and COX-2 assays

Other In Vitro Selectivity Studies. In a series of selectivity studies, rofecoxib had no effect on LTB₄ biosynthesis by calcium ionophore-challenged PMN leukocytes(IC₅₀ > 25 µM, n = 3) and no effect on the activity of human leukocyte15-lipoxygenase (IC₅₀ > 20 µM, n = 2; Table 1). Additionally,no detectable activities of rofecoxib were noted in a diversearray of receptor or enzyme assays performed by a contract laboratory(MDS Panlabs, Seattle,WA).

In Vivo Studies

Carrageenan-Induced Rat Paw Edema Assay. The administration of rofecoxib 1 h before injection of carrageenan inhibited the edema response dose-dependently with anID₅₀ value of 1.5 ± 0.1 mg/kg (Fig. 3A). In the control group,the paw volume increased by 1.1 ± 0.02 ml (n = 30) 3 h after injectionof carrageenan. The potency of rofecoxib was comparable to thatof indomethacin (ID₅₀ = 2.0 ± 0.2 mg/kg).

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Fig. 3. Inhibitory effect of rofecoxib or indomethacin in rodent models of inflammation, pain, and pyresis. A, carrageenan-induced paw edema assay (n = 10-30 rats/dose group). B, LPS-induced pyresis (n = 5-15 rats/dose group). C, carrageenan-induced hyperalgesia (n = 8-16 rats/dose group). The percentage of inhibition or hyperalgesia was calculated from the difference between a treated group and the vehicle control. *P < .05 versus vehicle control. Vertical bars show S.E.M.

Endotoxin-Induced Pyresis in Rats. The injection of LPS (0.36 mg/kg i.p.) resulted in an increase of 2.26 ± 0.11°C (n = 15) in rectal temperature 7 h postinjection(compared with the saline-injected group). The administrationof rofecoxib at the plateau of temperature elevation (5 h) reversedthe LPS-induced pyrexia in a dose-dependent manner (ID₅₀ = 0.24± 0.07 mg/kg, Fig. 3B). Rofecoxib was about 5-fold more potentthan indomethacin (ID₅₀ = 1.07 ± 0.16 mg/kg).

Carrageenan-Induced Rat Paw Hyperalgesia. Intraplantar injection of carrageenan (4.5 mg) induced marked paw edema and hyperalgesia to mechanical compression of theinflamed hind paw. Oral administration of rofecoxib (ID₅₀ = 1.0mg/kg) or indomethacin (ID₅₀ = 1.5 mg/kg) 1 h before the testreversed the carrageenan-induced hyperalgesia dose-dependently(Fig. 3C).

AIA in Rats. Rofecoxib significantly reduced paw swelling, thymus weights, and radiographic total scores in rats with AIA. The efficacyof rofecoxib was similar to that produced by an effective doseof indomethacin (1 mg/kg/day). Rofecoxib reduced the secondarypaw volume with an ID₅₀ value of 0.7 mg/kg/day (Fig. 4). Indomethacin(1 mg/kg/day) inhibited the paw swelling by 82% in this experiment.The total radiographic scores of the secondary paw in the vehicle-treated,adjuvant-injected animals were significantly greater than thatin the control, nonadjuvant-injected animals. Animals that receivedrofecoxib at 1 and 3 mg/kg/day or indomethacin at 1 mg/kg/dayshowed a significant attenuation of radiographic changes at bothdays 14 and 21 (Fig. 5). At the end of the study, a general necropsywas performed, and abdominal, peritoneal, and thoracic cavitieswere normal in all rats.

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Fig. 4. Inhibition by rofecoxib of secondary paw swelling in rats with AIA. Rofecoxib was administered orally daily for 21 days after induction of arthritis in female Lewis rats via intraplantar injection of Mycobacterium butyricum. Contralateral paw (secondary paw) volumes were measured before and at days 14 (A) and 21 (B) after induction of arthritis. The percentage of inhibition was calculated from the difference between a treated group and the vehicle control. N = 10 rats/dose group. Vertical bars show S.E.M.

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Fig. 5. Total radiographic scores of rats with AIA treated with either rofecoxib or indomethacin. Rofecoxib or indomethacin (Indo, 1 mg/kg/day) was administered orally daily for 21 days after the induction of arthritis in female Lewis rats via intraplantar injection of M. butyricum. Total radiographic scores of the secondary paw were derived from examination of lateral radiographs obtained before and at days 14 (A) and 21 (B) after induction of arthritis. N = 10 rats/dose group. *P < .05 versus vehicle control. Vertical bars show S.E.M. Cont, control noninjected animals; Veh, adjuvant-injected animals treated with drug vehicle.

Ex Vivo Whole Blood Assay in Anesthetized Dogs. Infusion of vehicle had no significant effect on the ex vivo biosynthesis of LPS-stimulated dog whole blood over the 4-h periodof the experiment. In contrast, diclofenac infused at 2.5 µg/kg/minreduced the ex vivo biosynthesis of PGE₂ in LPS-stimulated dogwhole blood (4 h) to 12% of predose values (88 ± 2% inhibition;Fig. 6). Rofecoxib was also active against ex vivo PGE₂ formationof LPS-stimulated dog whole blood, showing dose-dependent inhibitionof 37 ± 12, 64 ± 6, and 75 ± 0.3% after 4-h infusion with 0.8,2.5, and 8 µg/kg/min, respectively.

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Fig. 6. Inhibition of arachidonic acid-induced PGE₂ formation in LPS-stimulated dog whole blood ex vivo by rofecoxib or diclofenac. Rofecoxib or diclofenac was infused in anesthetized dogs, and whole blood PGE₂ generation in response to exogenous arachidonic acid (100 µM) was measured at time zero and 1 and 4 h after dosing. The percentage of predose values are shown. n = 2 to 11 dogs/dose group. Vertical bars show S.E.M.

Gastrointestinal Studies in Rats. Figure 7 shows that acute dosing of diclofenac or indomethacin at 10 mg/kg caused a significant increase in fecal ⁵¹Cr excretion in a 48-h period after the injection of ⁵¹Cr-labeled red blood cells in rats. In contrast, rofecoxib at100 mg/kg was without effect. In chronic dosing studies, administrationof diclofenac at 3 mg/kg b.i.d. for 5 days resulted in a significantincrease in fecal ⁵¹Cr excretion. In chronic dosing studies with indomethacin at 3mg/kg, one of five animals died of gastrointestinal side effectsafter 4 days of dosing. The remaining four animals showed overtclinical symptoms (loss of appetite, loss of body weight, constipation,jaundice), and ⁵¹Cr excretion experiments could not be performed. In contrast,oral dosing of rofecoxib at 100 mg/kg b.i.d. for 5 days had noeffect on fecal ⁵¹Cr excretion. In a separate study, oral dosing of rofecoxib at300 mg/kg/day for 2 weeks did not produce gastrointestinal lesions,whereas it has been reported previously that a single oral doseof indomethacin, flurbiprofen, or piroxicam at 3 to 10 mg/kg producedclear visible gastric lesions (Chan et al., 1995).

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Fig. 7. Effects of acute or chronic (5 days b.i.d.) dosing of rofecoxib, diclofenac, or indomethacin on gastrointestinal integrity in rats. Test compound was administered orally, followed immediately by i.v. injection of ⁵¹Cr-labeled red blood cells (20 µCi/rat) obtained from a donor rat. Fecal ⁵¹Cr excretion was collected for 48 h and was expressed as a percentage of injected dose. N = 4 to 8 rats/dose group. *P < .05 versus vehicle control. Vertical bars show S.E.M.

Gastrointestinal Studies in Squirrel Monkey. Figure 8 shows that chronic oral dosing of diclofenac (1 mg/kg b.i.d. for 4 days) or naproxen (5 mg/kg b.i.d. for 5 days)resulted in a significant enhancement in fecal ⁵¹Cr excretion. In comparison, rofecoxib at 100 mg/kg b.i.d. for5 days administered in either 1% methocellulose or 5% Tween 80vehicle had no significant effect compared with the vehicle controlgroup. Neither rofecoxib nor diclofenac had any effect on 24-hfecal mass; however, naproxen at 5 mg/kg significantly increased24-h fecal mass compared with the control group.

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Fig. 8. Effects of chronic dosing of rofecoxib (100 mg/kg b.i.d), diclofenac (1 mg/kg b.i.d.), or naproxen (5 mg/kg b.i.d) for 5 days on gastrointestinal integrity in squirrel monkeys. Fecal ⁵¹Cr (as a percentage of injected dose) was measured in groups of 3 to 10 squirrel monkeys after 4 to 5 days of b.i.d. treatment with vehicle, diclofenac, naproxen, or rofecoxib. *P < .05 versus vehicle control. Vertical bars show S.E.M.

	Discussion

Top Abstract Introduction Experimental Procedures Results Discussion References

Potency and Selectivity of COX-2 Inhibition. The present study demonstrates that rofecoxib is a highly selective inhibitor of COX-2 in a number of in vitro assays. Themechanism of inhibition of COX activity by rofecoxib is very similarto those reported with the COX-2-selective inhibitors DuP-697,NS-398, and DFU (Copeland et al., 1994; Ouellet and Percival,1995; Riendeau et al., 1997b) and is consistent with the inhibitionof COX-2 by rofecoxib occurring via a two-step time-dependentmechanism leading to the formation of a tightly bound inhibitedcomplex. In contrast, the weak inhibition of COX-1 by rofecoxibis competitive and non-time-dependent. These results contrastwith potent nonselective COX inhibitors such as indomethacin andflurbiprofen, which are time-dependent inhibitors of bothisoforms.

Rofecoxib caused little or no inhibition of prostanoid synthesis (IC₅₀ > 15-50 µM) in several COX-1-mediated in vitro assays.A lower IC₅₀ value of 2 µM was obtained in the U937 microsomalassay in which the accumulation of PGE₂ is measured after incubationwith a low, subsaturating concentration of the arachidonic acidsubstrate. This assay has been reported to give IC₅₀ values thatcorrelate with those of other COX-1 assays, but it has been reportedto be more sensitive to inhibition. For comparison, the IC₅₀ valueof rofecoxib is similar to that of L-745,337 (IC₅₀ = 2.8 µM) butmuch higher that those of NS-398 (IC₅₀ = 0.3 µM), meloxicam (IC₅₀= 0.14 µM), DuP 697 (IC₅₀ = 7 nM), or celecoxib (IC₅₀ = 52 nM;Riendeau et al., 1997a

). These results indicate that rofecoxibshows a selectivity for the inhibition of COX-2 in vitro evenunder conditions of limiting arachidonic acid availability favoringthe inhibition of COX-1 (i.e., IC₅₀ = 2 µM for rofecoxib againstmicrosomal COX-1 at low arachidonic acid concentration versus0.1-0.4 µM for COX-2 at saturating arachidonicacid).

The human whole blood COX-1 and COX-2 assays provide an additional and a more relevant measure of COX-2 inhibition selectivityunder a pathophysiological environment rich in plasma proteinand cells (Patrignani et al., 1994

; Brideau et al., 1996

). Othervariations of the human whole blood/cell assays have been reportedand have been used to show the efficacy of selective and specificCOX-2 inhibitors (Grossman et al., 1995

; Young et al., 1996

).In the present study, using the ratio of the COX-1 IC₅₀ valueover the COX-2 IC₅₀ value as an index for selectivity, the followingCOX-2 selectivity ratio was obtained: rofecoxib > celecoxib >meloxicam $congruent$ diclofenac > indomethacin, showing that rofecoxibhas the highest COX-2 selectivity when tested under the same experimentalcondition.

Rofecoxib inhibited dose-dependently the LPS-stimulated-, COX-2-derived PGE₂ synthesis in human whole blood in single or multipleoral dosing studies (Ehrich et al., 1996

, 1999

; Depre et al.,1998

). COX-1-derived serum TBX₂ in clotting whole blood was notinhibited even at doses of up to 1000 mg. This is in contrastto indomethacin, which inhibited both TBX₂ generation and LPS-stimulatedPGE₂ synthesis at therapeutic doses (Ehrich et al., 1999

). TheCOX-2 specificity of rofecoxib was also demonstrated in a humangastric biopsy study in which COX-1-derived gastric PGE₂ or PGF₂was inhibited by indomethacin (10 µM) but not by rofecoxib (upto 3.3 µM; Cryer et al., 1996

). Thus, at the clinical dose rangeof 12.5 to 25 mg (see below), rofecoxib inhibits only COX-2, butnot COX-1, activities in either human whole blood or gastric tissues,fulfilling the requirement for a COX-2-specific agent (Brookset al., 1999

) and in agreement with the results of the preclinicalstudies.

Anti-inflammatory, Analgesic, and Antipyretic Effects. In established rodent models of acute and chronic inflammation, pain, and fever, rofecoxib was as effective as conventionalNSAIDs with ID₅₀ values ranging from 0.7 to 1.5 mg/kg. In a separatestudy using a nonhuman primate model of pyresis (Chan et al.,1997), the antipyretic effectiveness of rofecoxib was also demonstrated(Schwartz et al., 1999). It should be mentioned that the plasmalevels of rofecoxib at the effective dose range of 1 to 3 mg/kg(<1 µM, Wang et al., unpublished observation) are below the levelrequired to inhibit COX-1. Thus, in accord with previous datareported for other selective COX-2 inhibitors (Chan et al., 1995;Riendeau et al., 1997b), inhibition of COX-2 alone is sufficientto achieve anti-inflammatory, analgesic, and antipyretic effectsin preclinicalmodels.

In a chronic, and more severe, inflammatory model such as the AIA in rats, rofecoxib was effective in reducing paw swellingand thymus weight with efficacy comparable to that of indomethacin.In particular, rofecoxib had a protective effect on adjuvant-induceddestruction of cartilage and bone structures, as measured by acomposite radiographic score, suggesting that rofecoxib has abeneficial effect on prevention of loss of function. A similarobservation has been reported with a COX-2 inhibitor, SC-58125,in this model (Anderson et al., 1996

In a dental pain analgesia study, rofecoxib at single doses of 50 or 500 mg demonstrated full analgesic activity, equivalentto that observed with ibuprofen (400 mg) (Ehrich et al., 1999

).As well, rofecoxib (12.5 or 25 mg) significantly reduced oraltemperature with efficacy comparable to that of ibuprofen (400mg) in patients with fever (Schwartz et al., 1999

). In a 6-weekstudy in patients with knee and hip osteoarthritis, significantefficacy was observed with rofecoxib (up to 50 mg) on the basisof each of three primary endpoints (Ehrich et al., 1998a

) andhealth-related quality of life assessment (Ehrich et al., 1998b

).A 6-month extension study was initiated, and clinical improvementwas sustained in the rofecoxib treatment groups throughout thestudy period, with efficacy comparable to that of diclofenac (Ehrichet al., 1998a

). In contrast to NSAIDs, however, rofecoxib didnot inhibit human whole blood COX-1 activities even at doses morethan 10-fold higher (i.e., 375 mg) than the efficacious dosesof 12.5 to 25 mg (Depre et al., 1998

). These studies clearly demonstratethat clinical efficacy can be achieved with rofecoxib at dosesthat inhibit only COX-2, consistent with preclinical results andin accord with the COX-2hypothesis.

Gastrointestinal Tolerability. It has been shown unequivocally and consistently in experimental models that COX-2 inhibitors do not cause gastric lesionseven at above effective anti-inflammatory doses (Futaki et al.,1993; Seibert et al., 1994; Chan et al., 1995; Riendeau et al.,1997b), in stark contrast to NSAIDs, which induce gastrointestinallesions after a single acute dose. Rofecoxib did not produce anygastric or intestinal lesions after 300 mg/kg/day in a 2-weekoral study in rats. This is echoed by a gastrointestinal integritystudy using ⁵¹Cr-labeled red blood cells as permeability markers. Rofecoxibhad no effect at 200 mg/kg/day for 5 days whereas a 2- to 3-foldincrease in fecal ⁵¹Cr excretion was observed with indomethacin at a single dose of3 mg/kg. Similar gastrointestinal sparing effects were observedwith rofecoxib in squirrel monkeys (Chan et al., 1995; Riendeauet al., 1997b). Using the ED₅₀ values in the rat paw edema assayand the ulcerogenic dose in the rodent study as measures for efficacyand ulcerogenicity, therapeutic index values of more than 200and 0.7 were obtained for rofecoxib and indomethacin,respectively.

In a 7-day endoscopy study of the stomach and duodenum in human subjects, the effect of rofecoxib at a dose (250 mg) of morethan 10-fold the clinically effective dose for the treatment ofosteoarthritis was statistically indistinguishable from the placebocontrol (Lanza et al., 1997

), compared with aspirin or ibuprofen,which produced significant mucosal damage at their clinical doses.This is supported by two gastrointestinal integrity studies usingwell-documented ⁵¹Cr permeability markers similar to those used in the preclinicalmodels mentioned above. Rofecoxib at 25 or 50 mg, a dose two tofour times the clinical dose, had no effect compared with placeboon the urinary recovery of ⁵¹Cr-EDTA in a 7-day study in human subjects (Bjarnason et al.,1998

). Similarly, rofecoxib did not affect ⁵¹Cr-labeled fecal blood loss compared with placebo in a 4-weekstudy (Hunt et al., 1998

). In these studies, indomethacin or ibuprofenproduced statistically significant effect compared with both placeboand rofecoxib. More importantly, rofecoxib was well toleratedin patients with osteoarthritis in a 6-month efficacy study, withno report of clinically important gastrointestinal complicationssuch as upper gastrointestinal bleeding or ulceration (Ehrichet al., 1998a

). This contrasts strongly with current NSAIDs, inwhich case the major cause of withdrawal is gastrointestinalcomplications.

Conclusion. The present study has clearly demonstrated that rofecoxib has equivalent anti-inflammatory, analgesic, and antipyretic activitiescompared with current NSAIDs in preclinical animal models, whilehaving a substantially different gastrointestinal side effectprofile. This is consistent with the clinical data available forrofecoxib when compared with standard NSAIDs. In both preclinicaland clinical studies, highly selective COX-2 inhibitors, suchas rofecoxib, are distinct from current NSAIDs with respect totheir pharmacological profiles. Thus, highly selective COX-2 inhibitorscan be classified as a new class of therapeutic agent for thetreatment of acute and chronic inflammatory conditions, with awell-defined molecular and biochemicaltarget.

	Acknowledgments

We thank Dr. W. R. Widmer (Department of Veterinary Clinical Sciences, Purdue University College of Veterinary Medicine, WestLafayette, IN) for assessment of radiographic scores in the ratadjuvant arthritisstudy.

	Footnotes

Accepted for publication February 22, 1999.

Received for publication December 22, 1998.

Send reprint requests to: Dr. Chi-Chung Chan, Department of Pharmacology, Merck Frosst Centre for Therapeutic Research, P.O. Box 1005, Pointe Claire, Dorval, Quebec, Canada H9R 4P8. E-mail: chi_chung_chan{at}merck.com

	Abbreviations

COX, cyclooxygenase; HBSS, Hanks' balanced salt solution; NSAID, nonsteroidal anti-inflammatory drug; CHO, Chinese hamster ovary; TMPD, N,N,N',N'-tetramethyl-p-phenylenediamine; AIA, adjuvant-induced arthritis; PG, prostaglandin; TBX, thromboxane; 12-HETE, 12-hydroeicosatetraenoic acid; PMN, polymorphonuclear; LTB, leukotriene B; DMSO, dimethyl sulfoxide; LPS, lipopolysaccharide.

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