Broad-Spectrum Antiviral Activity of the IMP Dehydrogenase Inhibitor VX-497: a Comparison with Ribavirin and Demonstration of Antiviral Additivity with Alpha Interferon

doi:10.1128/AAC.44.4.859-866.2000

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Antimicrobial Agents and Chemotherapy, April 2000, p. 859-866, Vol. 44, No. 4
0066-4804/00/$04.00+0
Copyright © 2000, American Society for Microbiology. All rights reserved.

Broad-Spectrum Antiviral Activity of the IMP Dehydrogenase Inhibitor VX-497: a Comparison with Ribavirin and Demonstration of Antiviral Additivity with Alpha Interferon

W. Markland,^* T. J. McQuaid, J. Jain, and A. D. Kwong

Vertex Pharmaceuticals Inc., Cambridge, Massachusetts 02139-4242

Received 13 July 1999/Returned for modification 3 November 1999/Accepted 3 January 2000

	ABSTRACT

Top Abstract Introduction Materials and Methods Results Discussion References

The enzyme IMP dehydrogenase (IMPDH) catalyzes an essential step in the de novo biosynthesis of guanine nucleotides, namely,the conversion of IMP to XMP. The major event occurring in cellsexposed to competitive IMPDH inhibitors such as ribavirin or uncompetitiveinhibitors such as mycophenolic acid (MPA) is a depletion of theintracellular GTP and dGTP pools. Ribavirin is approved as aninhaled antiviral agent for treatment of respiratory syncytialvirus (RSV) infection and orally, in combination with alpha interferon(IFN- $alpha$ ), for the treatment of chronic hepatitis C virus (HCV)infection. VX-497 is a potent, reversible uncompetitive IMPDHinhibitor which is structurally unrelated to other known IMPDHinhibitors. Studies were performed to compare VX-497 and ribavirinin terms of their cytotoxicities and their efficacies againsta variety of viruses. They included DNA viruses (hepatitis B virus[HBV], human cytomegalovirus [HCMV], and herpes simplex virustype 1 [HSV-1]) and RNA viruses (respiratory syncytial virus [RSV],parainfluenza-3 virus, bovine viral diarrhea virus, Venezuelanequine encephalomyelitis virus [VEEV], dengue virus, yellow fevervirus, coxsackie B3 virus, encephalomyocarditis virus [EMCV],and influenza A virus). VX-497 was 17- to 186-fold more potentthan ribavirin against HBV, HCMV, RSV, HSV-1, parainfluenza-3virus, EMCV, and VEEV infections in cultured cells. The therapeuticindex of VX-497 was significantly better than that of ribavirinfor HBV and HCMV (14- and 39-fold, respectively). Finally, theantiviral effect of VX-497 in combination with IFN- $alpha$ was comparedto that of ribavirin with IFN- $alpha$ in the EMCV replication system.Both VX-497 and ribavirin demonstrated additivity when coappliedwith IFN- $alpha$ , with VX-497 again being the more potent in this combination.These data are supportive of the hypothesis that VX-497, likeribavirin, is a broad-spectrum antiviralagent.

	INTRODUCTION

Top Abstract Introduction Materials and Methods Results Discussion References

Cells require adequate nucleotide levels which are made available for nucleic acid synthesis via two distinct mechanisms:the salvage pathway and de novo synthesis. Using the salvage pathway,cells recycle nucleosides and nucleobases, whereas with de novosynthesis, the purine or pyrimidine ring systems of the nucleotidesare assembled in a stepwise manner (17). Different cell typesrely on the two pathways of nucleotide biosynthesis to variousdegrees. Cells that proliferate relatively rapidly, such as lymphocytes,rely more on the de novo pathway because they require more nucleotidesthan can be provided by the salvage pathway (1).

IMP dehydrogenase (IMPDH; EC 1.1.1.205) catalyzes the rate-limiting step in the de novo biosynthesis of guanine nucleotides,the NAD⁺-dependent conversion of IMP to XMP. XMP is aminated in the nextbiosynthesis step to form GMP. It is crucial for many cellularmetabolic and synthetic processes. Two isoforms of human (andmouse) IMPDH (isoforms I and II) have been identified, with eachcontaining 514 amino acids, and they share 84% sequence identity.Forms I and II of human and mouse IMPDHs have 97 and 99% sequenceidentities, respectively. The native enzyme exists as a homotetramerwith a subunit molecular mass of 56 kDa. X-ray crystal structuresof mycophenolic acid (MPA) (26), ribavirin monophosphate (27),and an IMP analogue together with an NAD analogue (3) in complexwith IMPDH have been determined. Inhibition of IMPDH reduces thelevel of intracellular guanine nucleotides required for adequateRNA and DNA synthesis. Therefore, IMPDH inhibitors have potentialantiproliferative, antiviral, and antiparasitic effects (25,36).

The pharmacologic effects of IMPDH inhibition have been exploited by a number of marketed products. MPA is a potent, uncompetitiveIMPDH inhibitor. Its ester prodrug, mycophenolate mofetil (CellCept),has been approved for use for the prevention of acute rejectionin kidney (for a review, see reference 29) and heart (15)transplant recipients when used in combination with steroids andcyclosporine A. Ribavirin (Virazole, Rebetol) is a nucleosideanalog which, following intracellular phosphorylation, is a competitiveIMPDH inhibitor. Ribavirin is approved as an inhaled antiviralagent for treatment of respiratory syncytial virus (RSV) infectionand, orally in combination with alpha interferon (IFN- $alpha$ ), forthe treatment of chronic hepatitis C virus (HCV)infection.

Ribavirin is a broad-spectrum antiviral agent with activity against at least 12 DNA-containing viruses and 40 RNA-containingviruses (4, 6, 22, 24). Three different mechanisms forthe antiviral activity of ribavirin have been proposed (11).One proposed mechanism is the inhibition of viral RNA transcriptionand/or elongation. It has been observed that ribavirin triphosphateinhibits vesicular stomatitis virus RNA polymerase (9, 31),La Crosse encephalitis virus polymerase (2, 31), reovirustranscriptase (22), and influenza virus polymerase (8, 33)transcription. Inhibition of the viral RNA polymerase elongationreaction has been proposed for reovirus (22) and influenza virus(33). A second proposed mechanism involves inhibition of theformation of a guanine pyrophosphate "cap" on the 5' end of viralmRNA by viral mRNA guanylyltransferase. This effect has been observedin vaccinia virus mRNA (12), and the cause of this effect inSindbis virus mutants resistant to MPA and ribavirin was mappedto a viral gene coding for RNA guanylyltransferase (23). However,the major event occurring in cells exposed to ribavirin and structurallyrelated compounds such as 5-ethynyl-1- $beta$ -D-ribofuranosylimidazole-4-carboxamide,tiazofurin, and selenazofurin is a depletion of the intracellularGTP and dGTP pools as a result of the inhibition of IMPDH (fora review, see reference 4). Thus, the antiviral effects ofribavirin and other IMPDH inhibitors can be reversed by the exogenousaddition of guanosine but not other nucleosides (6, 34).These results strongly suggest that, analogous to the cytostaticeffect of IMPDH inhibitors on rapidly proliferating lymphocyteand tumor cell lines, the de novo rather than the salvage pathwayof GTP synthesis may be critical in the supply of precursors forviral RNA and DNA synthesis. Since the antiviral and cytostaticeffects of IMPDH inhibitors are established under different conditions(with resting cell monolayers and exponentially growing cells,respectively), they are not mutuallyexclusive.

IMPDH inhibitors have also been shown to potentiate the effect of purine nucleoside analogs which are inhibitors of humanimmunodeficiency virus (13) and herpesvirus replication (19).This potentiation is thought to occur via a more efficient phosphorylationof the nucleoside analog that arises from a depletion of dGTPpools by IMPDH inhibition, resulting in an enhancement of antiviralactivity (5).

VX-497 (molecular weight, 452.5) is a selective, highly potent, reversible, and uncompetitive inhibitor of the two isoformsof human IMPDH (K_is, 10 and 7 nM for isoforms I and II, respectively),being structurally unrelated to other known IMPDH inhibitors andsuitable for oral dosing. Vertex Pharmaceuticals is conductingphase III clinical trials to evaluate VX-497 as a possible treatmentfor psoriasis or for chronic hepatitis caused by HCV. The aimsof the studies described herein were to determine the antiviraleffect of VX-497 against a variety of viruses, to compare thisactivity to that of ribavirin, and to determine the combined antiviraleffect of VX-497 with IFN- $alpha$ . VX-497 had a consistently greaterantiviral effect than ribavirin in almost all of the assaysperformed.

	MATERIALS AND METHODS

Top Abstract Introduction Materials and Methods Results Discussion References

Compounds. VX-497 (Fig. 1) is a low-molecular-mass (452.5 Da) phenyloxazole derivative (chemical name, (S)-N-3-[3-(3-methoxy-4-oxazol-5-yl-phenyl)-ureido]-benzyl-carbamicacid tetrahydrofuran-3-yl-ester). It was stored frozen in dimethylsulfoxide as a 50 mM stock. Ribavirin (1- $beta$ -D-ribofuranosyl-1H-1,2,4-triazole-3-carboximide;Virazole) was obtained from Sigma (catalog no. R9644) and wasstored frozen as a 500 mM stock in dimethyl sulfoxide. IFN- $alpha$ (mouse,recombinant) was obtained from Calbiochem (catalog no. 407293)as a frozen solution in water. L929 cells (mouse fibroblast CCL-1cells [American Type Culture Collection]) were maintained in Eagleminimal essential medium containing 10% fetal bovine serum, nonessentialamino acids, sodium pyruvate, and L-glutamine. Poly(dI-dC) wasobtained from Pharmacia.

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FIG. 1. Chemical structure of VX-497.

Antiviral and cell growth analyses. The antiviral activities of VX-497 and ribavirin were tested against a variety of DNA viruses (hepatitis B virus [HBV], humancytomegalovirus [HCMV], and herpes simplex virus type 1 [HSV-1])and a variety of RNA viruses (RSV, parainfluenza-3 virus, bovineviral diarrhea virus [BVDV], Venezuelan equine encephalomyelitisvirus [VEEV], dengue virus, yellow fever virus [YFV], coxsackieB3 virus, influenza A virus, and murine encephalomyocarditis virus[EMCV]). These studies either were performed at Vertex Pharmaceuticalsor were contracted to ViroMed Laboratories Inc. (Minneapolis,Minn.), Southern Research Institute (Frederick, Md.), or AdvancedBiotechnologies Inc. (Columbia, Md.). While the conditions andassays used for each virus differed, the conditions for the ribavirinand VX-497 comparison were identical in each case and were performedin a blinded manner. The appropriate cells were trypsinized, counted,and seeded into 96-well plates. At confluence, serial dilutionsof test compounds and test compound combinations were added tothe cells, followed by the addition of a predetermined multiplicityof infection for each virus. Appropriate viral, cell, growth medium,and compound cytotoxicity controls were contained within eachplate. Each datum point is the average of three determinations.(Standard deviations were, on average, approximately 10% of themean, with a range typically no more than 20% of the mean.) Atan appropriate postinfection time point, an aliquot of the mediumfrom each well was taken (where indicated) and was stored forviral yield determinations or PCR analysis. Each datum point isthe average of three determinations. Table 1 shows the resultsfor a single experiment performed by the contracted commercialanalysts or in-house, as indicated. Duplications of any work andthe mean and standard deviations or range of results are presentedin the footnotes to Table 1, where appropriate. The antiviralmethodology for each virus including cell type, cytopathic effect(CPE), plaque reduction, or viral yield is indicated in the footnotesto Table 1.

CPE assay. 3-(4,5-Dimethylthiazol-2-yl)-5-(3-carboxymethylphenyl)-2-(4-sulfophenyl)-2H-tetrazolium salt and phenazine ethosulfate (MTS)(or MTT, MTA, or XTT) reagent was added to each well, and theplate was incubated at 37°C before reading of the formazan levelsin a microplate reader (490 nm). The data were analyzed to generatecell viability profiles and, where indicated, CPE reduction profilesfor each compound and combination. Cell viability was measuredas MTS, MTT, MTA, or XTT conversion relative to that for the cellcontrol. Antiviral activity was measured as MTS, MTT, MTA, orXTT conversion relative to the differential between those forcell and viral controls (CPEreduction).

Virus yield and plaque reduction assays. The virus yield assay was performed with stored aliquots of media from the VX-497, ribavirin, or combination antiviral studies.The aliquots were serially diluted in medium prior to additionto the wells containing confluent cells (in duplicate or triplicate).The virus were allowed to adsorb for 30 min, followed by washingwith phosphate-buffered saline and replacement with serum-containingmedium and incubation overnight. After an appropriate period oftime for plaque formation, stain was added and the plaques werecounted. For the plaque reduction assay, a known amount (in PFU)of virus was allowed to adsorb to the appropriate cell line, followedby washing with phosphate-buffered saline and addition of growthmedium with and without a test compound(s). Following an appropriateperiod of time, the medium was removed, the cells were stained,and plaque size and number wererecorded.

PCR analysis. Virion-associated HBV DNA present in the tissue culture supernatant was amplified by PCR with primers derived from HBV strainayw (16). PCR-amplified DNA was detected in real time by monitoringincreases in fluorescence signals that result from exonucleolyticdegradation of a quenched fluorescent probe molecule followinghybridization of the probe to the amplified HBV DNA. The TaqManprobe molecule, designed with the aid of Primer Express (PE-AppliedBiosystems) software, is complementary to the DNA sequences presentin the HBV DNA region. A total of 3 µl of clarified supernatantwas analyzed directly (without DNA extraction) in a 50-µl PCRmixture. Reagents and conditions used in the quantitative PCRwere performed as described by the manufacturer (PE-Applied Biosystems).The standard curve (for a 1.2-kbp HBV ayw subgenomic fragment)ranged from 10⁶ to 10¹ nominal copy equivalents per PCRmixture.

Reversibility with guanosine. Studies to compare the antiviral and cytotoxic activities of VX-497 and ribavirin were performed in the presence and absenceof 100 µM guanosine to assess whether the antiviral effect wasreversible and, hence, could be attributed to inhibition of IMPDH.The effect of the added guanosine on GTP and dGTP pools in thepresence of guanosine and VX-497 was not measured in these experiments,and the level of guanosine required for reversal of IMPDH inhibitionis cell line dependent. Thus, any decrease in antiviral efficacyof VX-497 in the presence of 100 µM guanosine indicates that IMPDHinhibition is an important component of the antiviral mechanismof action; however, the absence of an effect does not excludeinvolvement of IMPDHinhibition.

Gel shift assay. (i) Cell culture. The murine fibroblast L929 cell line was cultured in Eagle minimal essential medium supplemented with 10% fetal bovine serum,nonessential amino acids, 50 U of penicillin per ml, 50 µg ofstreptomycin per ml, and 2 mM L-glutamine. EMCV was infected at500 PFU/10⁷ L929 cells. Cells were left untreated or were treated with differentconcentrations of murine IFN- $alpha$ alone, VX-497 alone, or combinationsthereof.

(ii) EMSAs. The nucleotide sequences of the oligonucleotides used as probes in the electrophoretic mobility shift assays (EMSAs) were5'-CATGCCTCGGGAAAGGGAAACCGAAACTGAAGCC-3' for probe WT ISRE (interferon-sensitiveresponse element), 5'-CATGCCTCGGGACAGGGACACCGACACTGAAGCC-3' forprobe MUT ISRE (nucleotides that differ from those in the wild-typesequence are underlined), and 5'-CATGTTATGCATATTCCTGTAAGTG-3'for probe WT GAS (gamma interferon-activated sequence). The oligonucleotideswere annealed and end labeled with [ $gamma$ -³²P]ATP and polynucleotide kinase and were purified on 12% acrylamidegels. Small-scale nuclear extracts were made from 10⁷ L929 cells by a modification of the method of Dignam et al. (7).The total protein in nuclear extracts was estimated with the bicinchoninicacid protein assay kit (Pierce). For each EMSA binding reaction,10,000 cpm (~0.2 to 0.5 ng) of end-labeled probe was incubatedwith 6 to 12 µg of nuclear extract in the presence of 2.5 of µgsheared poly(dI-dC). The binding reaction mixtures were incubatedat room temperature for 20 min and were then electrophoresed on4% nondenaturing acrylamide gels at room temperature. The gelswere exposed to a Fuji phosphorimager for quantification of theradioactivity in EMSAbands.

Synergy analysis. Analysis of the antiviral activity of IFN- $alpha$ with ribavirin or IFN- $alpha$ with VX-497 with the EMCV-L929 system was undertaken byusing the independent effects model (Macsynergy II, version 1)(21). In this model values of synergy or antagonism are presentedin synergy volume units, typically as square micromolar percent,for the two compounds and the activity is measured. In this casethe synergy volume unit is micromolar unit percent (micromolarfor ribavirin or VX-497, unit for IFN- $alpha$ , and percent for antiviralactivity). Values under 25 µM unit %, at 95% confidence, shouldbe regarded as insignificant. Values between 25 and 50 µM unit% should be considered minor but significant, while values between50 and 100 µM unit % indicate moderate synergy, with the possibilityof importance in vivo. Values over 100 µM unit % indicate strongsynergy with a probability of importance invivo.

	RESULTS

Top Abstract Introduction Materials and Methods Results Discussion References

VX-497 antiviral efficacy. The effect of VX-497 on virus replication in the assays described above (Table 1) fell into three groups. VX-497 is mostpotent against the first group of viruses, which includes HBV,HCMV, EMCV, and RSV, with 50% inhibitory concentrations (IC₅₀s)of 0.38, 0.80, 1.0, and 1.14 µM, respectively. VX-497 has intermediateantiviral activity against a second group of viruses, which includesHSV-1, parainfluenza-3 virus, BVDV, VEEV, and dengue virus, withIC₅₀s ranging from 6 to 19 µM. VX-497 did not demonstrate antiviralefficacy against the third group of viruses, as measured by itsinability to achieve an IC₅₀ measurement for YFV, coxsackie B3virus, or influenza A virus at 31 µM, the highest concentrationtested.

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TABLE 1. Summary of assays with VX-497 and ribavirin for their antiviral activity and cytotoxicity^a

Antiviral efficacy of ribavirin. The effect of ribavirin on virus replication in the assays described above could also be divided into three groups. Ribavirinis most potent against a first group of viruses, which includesdengue virus and EMCV, with IC₅₀s of 8 and 17 µM, respectively.Ribavirin has intermediate antiviral activity against a secondgroup of viruses, which includes HBV, HCMV, RSV, HSV-1, parainfluenza-3virus, and influenza A virus, with IC₅₀s ranging from 20 to 198µM. Ribavirin did not demonstrate antiviral efficacy, failingto achieve an IC₅₀ at the highest concentration tested (500 µM),for the third group of viruses, namely, coxsackie B3 virus, YFV,andVEEV.

Comparison of VX-497 and ribavirin antiviral potencies. As summarized in Table 2, VX-497 was 10- to 100-fold more potent than ribavirin against HBV, HCMV, RSV, HSV-1, EMCV, parainfluenza-3virus, and VEEV. The only virus against which VX-497 was lesspotent than ribavirin was influenza A virus, against which VX-497had no activity at the highest concentration (31 µM) tested. Table2 also demonstrates that the therapeutic index of VX-497 wasbetter than that of ribavirin for HBV (13.7 versus 2.2) and HCMV(38.8 versus >3.4). The therapeutic index of VX-497 was similarto that of ribavirin for HSV-1, EMCV, and parainfluenza-3 virusbut was three- to fourfold lower for BVDV and RSV.

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TABLE 2. Comparison of antiviral potencies of VX-497 and ribavirin

Effects of VX-497 and ribavirin on HBV replication. More detailed graphs of the results of testing of ribavirin and VX-497 against HBV are presented in Fig. 2a and b, respectively.Against HBV infection in vitro, ribavirin had an IC₅₀ of 44 µMwith a corresponding 50% cytotoxic concentration (CC₅₀) of 96µM, for a therapeutic or selectivity index of approximately 2.In contrast, VX-497 was 100-fold more potent, with an IC₅₀ of380 nM and a corresponding CC₅₀ of 5.2 µM, for a therapeutic indexof 14. The antiviral activity of VX-497 in HepG2.2.2.15 cellswas reversed threefold by the addition of guanosine (Table 1),suggesting that IMPDH inhibition plays a role in the antiviraleffect of VX-497 on an HBV-infected liver cell line in vitro.

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FIG. 2. (a) Effect of ribavirin on viability of HepG2 2.2.15 cells and HBV replication. (b) Effect of VX-497 on viability of HepG2 2.2.15 cells and HBV replication. (c) Effect of ribavirin on viability of Vero cells and HSV-1 replication. (d) Effect of VX-497 on viability of Vero cells and HSV-1 replication. Cell viability (striped bars) is measured (in percent) relative to cell growth in the absence of drug. Antiviral activity (solid bars) is measured (in percent) relative to viral replication in the absence of drug. Results are the means of triplicate determinations, with standard deviations shown.

Effects of VX-497 and ribavirin on HSV-1 replication. In the absence of guanosine, VX-497 was ~26-fold more potent than ribavirin against HSV-1, with an IC₅₀ of 6.3 µM comparedto a ribavirin IC₅₀ of 162 µM (Fig. 2c and d). In the presenceof guanosine, VX-497 had a greater than sixfold reduced antiviralactivity, suggesting a role for IMPDH inhibition in the antiviraleffect on HSV-1 infection in vitro. The effect of guanosine onthe reversal of the antiviral activities of ribavirin and VX-497was also observed in the HSV-1 in vitro infection model (Table1).

Effects of IFN- $alpha$ , VX-497, and ribavirin on EMCV replication. EMCV, while generally regarded as a mouse virus, has a wide host range, including humans. Infection of the mouse cell lineL929 with EMCV has routinely been used to evaluate and standardizebatches of IFN- $alpha$ and was used in this work as a means of comparingthe antiviral activities of VX-497 and ribavirin when combinedwith IFN- $alpha$ . IFN- $alpha$ demonstrated expected levels of activity againstEMCV, with an IC₅₀ of 0.16 units when measured as a viral yieldreduction (Fig. 3a) or 1.5 units when measured as a reductionin CPE (data not shown). Little if any cytotoxicity was observedfor IFN- $alpha$ in this system. In the absence of guanosine, VX-497was 17-fold more potent than ribavirin against EMCV, with IC₅₀sof 1 and 17 µM, respectively (Fig. 3b and c). In the presenceof 100 µM guanosine, VX-497 had a 14-fold reduction in antiviralactivity and ribavirin had a greater than 29-fold reduction inantiviral activity (Table 1), again suggesting a role for IMPDHinhibition in the antiviral effect.

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FIG. 3. Effects of IFN- $alpha$ (units per 100-µl well) (a), ribavirin (b), and VX-497 (c) on the viability of L929 cells and EMCV replication. Cell viability (striped bars) is measured (in percent) relative to cell growth in the absence of drug. Viral yield (solid bars) is measured (in percent) relative to viral replication in the absence of drug. Results are the means of triplicate determinations, with standard deviations shown.

Combinations of VX-497 and IFN- $alpha$ and of ribavirin and IFN- $alpha$ were tested in the EMCV-L929 system to determine if the antiviralactivities obtained with the single agents could be combined andwhether the resulting activity of the combined pair would be additiveor synergistic. To this end, a series of experiments was performedin which the level of IFN- $alpha$ was fixed (0.2, 0.1, 0.05, and 0 units)and the level of VX-497 (or ribavirin) was titrated into the system.Amounts of IFN- $alpha$ were chosen to be suboptimal (0.2 unit and below)to allow the detection of the antiviral activity of the addedagent. The data are presented as a three-dimensional graph showingchanges in viral yield for each of the combinations of ribavirinwith IFN- $alpha$ (Fig. 4a) and VX-497 with IFN- $alpha$ (Fig. 4b). The cellviability profiles for each compound were not noticeably alteredby the presence of any of the doses of IFN- $alpha$ (data not shown).The reduction in viral yield is correlated with the combinationof ribavirin with IFN- $alpha$ or of VX-497 with IFN- $alpha$ in an additivefashion. Evaluation of the data by using an independent effectsmodel (Macsynergy II, version 1) (21) generated synergy volumesof 33 and 27 µM unit % for the combinations of IFN- $alpha$ with VX-497and of IFN- $alpha$ with ribavirin, respectively. Values in this range(see Materials and Methods), near the threshold of 25 µM unit%, are at the very lower limits of significant synergy. Whilethere may be pockets of marginal synergy or marginal antagonismwithin the combination profiles for both pairs of reagents, areasonable interpretation of the data indicates a general trendtoward additivity. While this additivity is not perfectly quantitative,particularly at saturating levels of either pair, the trend towardadditivity is both apparent and similar for both pairs of reagents.Deviations of individual datum points from the expected linearityfor each dimension within the three-dimensional graph reflectthe experimental errors inherent in such a multistep quantitativeassay for viruses. The principle difference between ribavirinand VX-497 in this assay in which they are used in combinationwith IFN- $alpha$ is their relative potencies, as indicated by the numericalrange of effective drug concentration for each; VX-497 was againthe more potent of the two compounds.

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FIG. 4. Effects of the combination of ribavirin and IFN- $alpha$ (a) or of VX-497 and IFN- $alpha$ on the yield of EMCV in L929 cells. Viral yield is measured (in percent) relative to viral replication in the absence of either drug. Results are the means of triplicate determinations. (Standard deviations were on average 10% of the mean, with a range no more than 20% of the mean.) IFNa, IFN- $alpha$ .

Does VX-497 have an effect on the IFN- $alpha$ signaling pathway? We wished to determine whether VX-497 has any direct or indirect effect on the IFN- $alpha$ signaling pathway. To this end L929 cellsand EMCV-infected L929 cells were treated with IFN- $alpha$ alone andwith IFN- $alpha$ supplemented with VX-497. Nuclear extracts were prepared,normalized for protein concentration, and tested for binding toan interferon-sensitive response element (ISRE) oligonucleotideor, as a control, a gamma interferon-activated sequence (GAS)oligonucleotide. Two radiolabeled ISRE gel-retarded bands (datanot shown) were detected in nuclear extracts of L929 cells (EMCV-infectedor uninfected cells) treated with IFN- $alpha$ (range, 0.01 to 10 unitsper 100-µl well) which were competed by an excess of unlabeledoligonucleotide. No noticeable difference in pattern or intensityof gel-retarded bands (data not shown) was observed when the experimentswere repeated with the addition of VX-497 (range, 100 to 500 nM).This suggests that VX-497 does not alter, positively or negatively,the IFN- $alpha$ signaling pathway in L929 cells and that the antiviraleffect of VX-497 in the EMCV replication system is indeed independent.This is consistent with the simple additivity seen with the IFN- $alpha$ -VX-497combination describedherein.

	DISCUSSION

Top Abstract Introduction Materials and Methods Results Discussion References

The aim of this study was to evaluate the antiviral activity of VX-497 against a variety of viruses in vitro and to compareits potency to that of ribavirin. Ribavirin is an establishedbroad-spectrum antiviral agent which has recently been approvedfor use, in combination with IFN- $alpha$ , for the treatment of chronichepatitis resulting from HCV infection. As a result of this, wealso wished to investigate the potential of combining VX-497 withIFN- $alpha$ . Since there is no adequate in vitro assay for HCV replication,we decided to use EMCV replication in L929 cells (a mouse fibroblastcell line) as a robust and rapid viral assay system in which toperform this comparison. Since this system is routinely used toevaluate and standardize IFN- $alpha$ , it was considered a valid andmeaningful assay for the combinationstudies.

Ribavirin is a competitive inhibitor of IMPDH as ribavirin-5'-monophosphate (K_i = 250 nM). It has demonstrated in vitro activityagainst a broad spectrum of DNA and RNA viruses and has shownclinical efficacy against influenza A and B viruses, RSV, parainfluenzavirus, and Lassa fever virus. It has also been demonstrated tohave antiproliferative activity as well as an ability to inhibitproinflammatory mediators induced by viral infection (20, 30).A side effect of ribavirin is anemia, which results from the accumulationof the triphosphate form of the drug in erythrocytes. Ribavirinhas recently been approved for use in combination with IFN- $alpha$ forthe treatment of HCV-induced hepatitis. Therapeutically, it appearsto act synergistically with IFN- $alpha$ (for a review, see references18 and 32). IFN- $alpha$ has been approved for use in the treatmentof a variety of human malignancies and viral diseases and as animmunomodulator (10, 14). It is currently approved for usein the treatment of chronic viral hepatitis (caused by HBV andHCV) and has been approved for use in combination withribavirin.

In these studies, the antiviral potency of ribavirin was confirmed and the potency of VX-497 was established against a numberof viruses as individual agents. The additive antiviral effectof each agent with IFN- $alpha$ was demonstrated in the L929-EMCV system.For the viruses tested in this study, the activity of VX-497 wasconsistently more potent than that of ribavirin against all virusestested except influenza A virus. The reasons for the improvedantiviral potency of VX-497 can be considered a function of therelative abilities of either compound to inhibit IMPDH. It shouldbe noted that of the variously phosphorylated intracellular formsof ribavirin, only the monophosphate form significantly inhibitsIMPDH. The amount of the monophosphate form as a percentage ofall phosphorylated forms of ribavirin has been measured to bein the range of 5 to 12% in 3T3 cells, 4 to 9% in Vero cells,and 4 to 9% in MA-104 cells (28). This makes the IMPDH-inhibitoryform of ribavirin a minor intracellular component. It is alsointeresting that the relative affinities of VX-497 and ribavirinfor IMPDH are about 35-fold (K_is = 7 and 250 nM, respectively),with VX-497 again being the more potent agent. The greater potencyof VX-497 relative to that of ribavirin in the viral assays demonstratesa similar ratio, having a range of 10- to 100-fold increased potencydepending on the particular viral replication system tested. Therole of IMPDH in the antiviral activities of both compounds isstrengthened by the reversibility of the antiviral effects achievedwith guanosine. While the extent of this reversibility is variableand is probably cell line dependent, it does indicate that GTPpool depletion is an important component of the viral reductionmechanism and is consistent with a mechanism of action involvingthe inhibition of IMPDH. A recent in vitro study (17a) determinedthat HCV and classical swine fever virus NS5B (an RNA template-dependentRNA polymerase and a key component in the viral replicase complex)is selectively and significantly stimulated by high (admittedly,unphysiologically high) levels of GTP. This stimulation is notseen with ATP, CTP, UTP, GDP, or GMP. Perhaps a reduction in physiologicallyrelevant GTP levels that arises, for instance, from IMPDH inhibitioncould account for an antiviral effect invivo.

The additivity of the antiviral effects of VX-497 and IFN- $alpha$ was demonstrated in these studies as a reduction in EMCV replicationand was compared to that of ribavirin and IFN- $alpha$ . Again, VX-497was the more potent of the two agents over the same range of IFN- $alpha$ concentrations tested. The simple additivity seen indicates thatthe antiviral mechanisms elicited by VX-497 and IFN- $alpha$ are independentof each other in this system and likely involve depletion of GTPpools for VX-497 and one of the mechanisms indicated above forIFN- $alpha$ . This viewpoint is consistent with the observation madein the studies presented here that VX-497 had no effect on theIFN- $alpha$ signaling pathway, as determined by gel shift assays withISREoligonucleotides.

In summary, VX-497 exhibits 10- to 100-fold more potency than ribavirin against HBV, HCMV, RSV, HSV-1, parainfluenza 3 virus,EMCV, and VEEV infections in cell culture. These data are supportiveof the hypothesis that VX-497, like ribavirin, is a broad-spectrumantiviral agent. In vitro testing for activity against HCV isproblematic, since a robust in vitro system does not exist forHCV replication. The potential for the use of VX-497 in the treatmentof hepatitis C is premised on the demonstrated clinical activityof ribavirin in the treatment of chronic hepatitis C, particularlyin combination with IFN- $alpha$ , and the demonstrated broad-spectrumantiviral activity of VX-497 shown herein. Since ribavirin's activityagainst HCV may be significantly mediated by IMPDH inhibition,VX-497 may also have activity in the treatment of hepatitis C.We have demonstrated that VX-497 has in vitro antiviral activitythat is comparable or superior to that of ribavirin against anumber of viruses, and we have demonstrated that the additiveantiviral effect of VX-497 and IFN- $alpha$ is similar to but more potentthan that of ribavirin and IFN- $alpha$ . Given the synergistic activityof ribavirin and IFN- $alpha$ in the treatment of HCV infection seenin the clinic, the additive effect of ribavirin or VX-497 withIFN- $alpha$ demonstrated in these studies, and the greater overall potencyof VX-497 relative to that of ribavirin, it is possible that aVX-497-IFN- $alpha$ combination will prove to be a potential alternativetherapy. To this end, phase II clinical trials of VX-497 for thetreatment of HCV infection have recently concluded (the trialswere conducted by Vertex Pharmaceuticals Inc.) (35).

	ACKNOWLEDGMENTS

We thank R. A. Byrn for synergy analysis and E. Nimmesgern for input and discussions during the course of this work; the IMPDHChemistry Team (D. M. Armistead, M. C. Badia, R. S. Bethiel, C.A. Frank, P. M. Novak, S. M. Ronkin, and J. O. Saunders) for generatingand providing VX-497; and V. Sato and M. Su for critical readingof themanuscript.

	FOOTNOTES

^* Corresponding author. Mailing address: Vertex Pharmaceuticals Inc., 130 Waverly St., Cambridge, MA 02139-4242. Phone: (617)577-6124. Fax: (617) 577-6210. E-mail: Markland{at}vpharm.com.

REFERENCES

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References

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3. Colby, T. D., K. Vanderveen, M. D. Strickler, G. D. Markham, and B. M. Goldstein. 1999. Crystal structure of human type II inosine monophosphate dehydrogenase: implications for ligand binding and drug design. Proc. Natl. Acad. Sci. USA 96:3531-3536[Abstract/Free Full Text].

4. De Clercq, E. 1993. Antiviral agents: characteristic activity spectrum depending on the molecular target with which they interact, p. 1-55. Academic Press, Inc., New York, N.Y.

5. De Clercq, E. 1995. Trends in the development of new antiviral agents for the chemotherapy of infections caused by herpes viruses and retroviruses. Rev. Med. Virol. 5:149-164.

6. De Clercq, E., M. Cools, J. Balzarini, R. Snoeck, G. Andrei, M. Hosoya, S. Shigeta, T. Ueda, N. Minakawa, and A. Matsuda. 1991. Antiviral activities of 5-ethynl-1- $beta$ -ribofuranosylimidazole-4-carboxamide and related compounds. Antimicrob. Agents Chemother. 35:679-684[Abstract/Free Full Text].

7. Dignam, J. D., R. M. Lebovitz, and R. G. Roeder. 1983. Accurate transcription initiation by RNA polymerase II in a soluble extract from isolated mammalian nuclei. Nucleic Acids Res. 11:1475-1489[Abstract/Free Full Text].

8. Eriksson, B., B. Helgstrand, N. G. Johansson, A. Larsson, A. Misiorny, J. O. Noren, L. Phillipson, K. Stenberg, G. Stening, S. Stridh, and B. Oberg. 1977. Inhibition of influenza virus ribonucleic acid polymerase by ribavirin triphosphate. Antimicrob. Agents Chemother. 11:946-951[Abstract/Free Full Text].

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13. Hartman, N. R., S. A. Gurpreet, D. A. Cooney, H. Mitsuya, S. Kageyama, A. Fridland, S. Broder, and D. G. Johns. 1991. Inhibitors of IMP dehydrogenase stimulate the phosphorylation of the anti-human immunodeficiency virus nucleosides 2',3'-dideoxyadenosine and 2',3'-dideoxyinosine. Mol. Pharmacol. 40:118-124[Abstract].

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1.	Allison, A. C., T. Hovi, R. W. E. Watts, and A. D. B. Webster. 1977. The role of de novo purine synthesis in lymphocyte transformation. Ciba Found. Symp. 48:207-224.
2.	Cassidy, L. F., and J. L. Patterson. 1989. Mechanism of La Crosse virus inhibition by ribavirin. Antimicrob. Agents Chemother. 33:2009-2011[Abstract/Free Full Text].
3.	Colby, T. D., K. Vanderveen, M. D. Strickler, G. D. Markham, and B. M. Goldstein. 1999. Crystal structure of human type II inosine monophosphate dehydrogenase: implications for ligand binding and drug design. Proc. Natl. Acad. Sci. USA 96:3531-3536[Abstract/Free Full Text].
4.	De Clercq, E. 1993. Antiviral agents: characteristic activity spectrum depending on the molecular target with which they interact, p. 1-55. Academic Press, Inc., New York, N.Y.
5.	De Clercq, E. 1995. Trends in the development of new antiviral agents for the chemotherapy of infections caused by herpes viruses and retroviruses. Rev. Med. Virol. 5:149-164.
6.	De Clercq, E., M. Cools, J. Balzarini, R. Snoeck, G. Andrei, M. Hosoya, S. Shigeta, T. Ueda, N. Minakawa, and A. Matsuda. 1991. Antiviral activities of 5-ethynl-1- $beta$ -ribofuranosylimidazole-4-carboxamide and related compounds. Antimicrob. Agents Chemother. 35:679-684[Abstract/Free Full Text].
7.	Dignam, J. D., R. M. Lebovitz, and R. G. Roeder. 1983. Accurate transcription initiation by RNA polymerase II in a soluble extract from isolated mammalian nuclei. Nucleic Acids Res. 11:1475-1489[Abstract/Free Full Text].
8.	Eriksson, B., B. Helgstrand, N. G. Johansson, A. Larsson, A. Misiorny, J. O. Noren, L. Phillipson, K. Stenberg, G. Stening, S. Stridh, and B. Oberg. 1977. Inhibition of influenza virus ribonucleic acid polymerase by ribavirin triphosphate. Antimicrob. Agents Chemother. 11:946-951[Abstract/Free Full Text].
9.	Fernandez-Larsson, R., K. O'Connell, E. Koumans, and J. L. Patterson. 1989. Molecular analysis of the inhibitory effect of phosphorylated ribavirin on the vesicular stomatitis virus in vitro polymerase reaction. Antimicrob. Agents. Chemother. 33:1668-1673[Abstract/Free Full Text].
10.	Gale, M., Jr., and M. G. Katze. 1998. Molecular mechanisms of interferon resistance mediated by viral-directed inhibition of PKR, the interferon-induced protein kinase. Pharmacol. Ther. 78:29-46[CrossRef][Medline].
11.	Gilbert, B. E., and V. Knight. 1986. Biochemistry and clinical applications of ribavirin. Antimicrob. Agents and Chemother. 30:201-205[Free Full Text].
12.	Goswami, B. B., E. Borek, and O. K. Sharma. 1979. The broad spectrum antiviral agent ribavirin inhibits capping of mRNA. Biochem. Biophys. Res. Commun. 89:830-836[CrossRef][Medline].
13.	Hartman, N. R., S. A. Gurpreet, D. A. Cooney, H. Mitsuya, S. Kageyama, A. Fridland, S. Broder, and D. G. Johns. 1991. Inhibitors of IMP dehydrogenase stimulate the phosphorylation of the anti-human immunodeficiency virus nucleosides 2',3'-dideoxyadenosine and 2',3'-dideoxyinosine. Mol. Pharmacol. 40:118-124[Abstract].
14.	Jaramillo, M. L., N. Abraham, and J. C. Bell. 1995. The interferon system: a review with emphasis on the role of PKR in growth control. Cancer Invest. 13:327-338[Medline].
15.	Kobashigawa, J., L. Miller, D. Renlund, R. Mentzer, E. Alderman, R. Bourge, M. Costanzo, H. Eisen, G. Dureau, R. Ratkovec, M. Hummel, D. Ipe, J. Johnson, A. Keogh, R. Mamelok, D. Mancini, F. Smart, and H. Valantine. 1998. A randomized active-controlled trial of mycophenolate mofetil in heart transplants. Transplantation. 66:507-515[CrossRef][Medline].
16.	Korba, B. F., and J. L. Gerin. 1992. Use of a standardized cell culture assay to assess activities of nucleoside analogs against hepatitis B virus replication. Antivir. Res. 19:55-70[CrossRef][Medline].
17.	Kornberg, A., and T. A. Baker. 1992. DNA replication, p. 53-100. W. H. Freeman & Co., New York, N.Y.
17a.	Lohmann, V. H. Overton, and R. Bartenschlager. 1999. Selective stimulation of hepatitis C virus and pestivirus NS5B RNA polymerase activity by GTP. J. Biol. Chem. 274:10807-10815[Abstract/Free Full Text].
18.	Main, J., B. McCarron, and H. C. Thomas. 1998. Treatment of chronic viral hepatitis. Antivir. Chem. Chemother. 9:449-460[Medline].
19.	Neyts, J., G. Andrei, and E. De Clercq. 1998. The novel immunosuppressive agent mycophenolate mofetil markedly potentiates the antiherpes activities of acyclovir, gancyclovir, and penciclovir in vitro and in vivo. Antimicrob. Agents Chemother. 42:216-222[Abstract/Free Full Text].
20.	Ning, Q., D. Brown, J. Parodo, M. Cattral, R. Gorczynski, E. Cole, L. Fung, J. W. Ding, M. F. Liu, O. Rotstein, M. J. Phillips, and G. Levy. 1998. Ribavirin inhibits viral-induced macrophage production of TNF, IL-1, the procoagulant fgl2 prothrombinase and preserves Th1 cytokine production but inhibits Th2 cytokine response. J. Immunol. 22:3487-3493.
21.	Prichard, M. N., and C. Shipman. 1992. A three-dimensional model to analyze drug-drug interactions. Antivir. Res. 14:181-206.
22.	Rankin, J. T., S. B. Eppes, J. B. Antczak, and W. K. Joklik. 1989. Studies on the mechanism of the antiviral activity of ribavirin against reovirus. Virology 168:147-158[CrossRef][Medline].
23.	Scheidel, L. M., and V. Stollar. 1991. Mutations that confer resistance to mycophenolic acid and ribavirin on sindbis virus map to the nonstructural protein nsP1. Virology 181:490-499[CrossRef][Medline].
24.	Sidwell, R. W., J. H. Huffman, G. P. Khare, L. B. Allen, J. T. Witkowski, and R. K. Robins. 1972. Broad-spectrum antiviral activity of virazole: 1- $beta$ -D-ribofranosyl-1,2,4-triazole-3-carboxamide. Science 177:705-706[Abstract/Free Full Text].
25.	Silverman Kitchin, J. E., M. Keltz Pomeranz, G. Pak, K. Washenik, and J. L. Shupack. 1997. Rediscovering mycophenolic acid: a review of its mechanism, side effects, and potential uses. J. Am. Acad. Dermatol. 37:445-449[CrossRef][Medline].
26.	Sintchak, M. D., M. A. Fleminh, O. Futer, S. A. Raybuck, S. P. Chambers, P. R. Caron, M. A. Murcko, and K. P. Wilson. 1996. Structure and mechanism of inosine monophosphate dehydrogenase in complex with the immunosuppressant mycophenolic acid. Cell 85:921-930[CrossRef][Medline].
27.	Sintchak, M. D., M. C. Badia, O. Futer, and E. Nimmesgern. 1999. X-ray crystal structure of the antiviral drug ribavirin monophosphate bound to IMP dehydrogenase. Antivir. Res. 41:A56.
28.	Smee, D. F., and J. W. Huggins. 1999. Mode of action of ribavirin against cowpox and monkeypox viruses. Antivir. Res. 41:A52.
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