Basis for Dosing Time-Dependent Changes in the Antiviral Activity of Interferon-alpha  in Mice

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Vol. 294, Issue 2, 488-493, August 2000

Basis for Dosing Time-Dependent Changes in the Antiviral Activity of Interferon- $alpha$ in Mice¹

Shigehiro Ohdo, De-Sheng Wang, Satoru Koyanagi, Hiroshi Takane, Kouichi Inoue, Hironori Aramaki, Eiji Yukawa and Shun Higuchi

Department of Clinical Pharmacokinetics, Division of Pharmaceutical Science, Graduate School, Kyushu University (S.O., D.-S.W., S.K., H.T., K.I., E.Y., S.H.); and Department of Molecular Biology, Daiichi College of Pharmaceutical Sciences (H.A.), Fukuoka, Japan

	Abstract

Top Abstract Introduction Materials and Methods Results Discussion References

The influence of dosing time on the pharmacological effect (antiviral activity) of interferon- $alpha$ (IFN- $alpha$ ), and the pharmacologicaland pharmacokinetic mechanisms, were investigated in ICR malemice under a 12-h light/dark cycle (lights on from 7:00 AM to7:00 PM). 2'-5'Oligoadenylate synthetase activity in plasma at24 h after IFN- $alpha$ (10 MI.U./kg, i.v.) injection, as an index ofantiviral activity, was significantly higher for injections givenat 9:00 AM than for injections given at 9:00 PM (P < .05). Theuptake of [³H]thymidine by lymphocytes after 24-h incubation with IFN- $alpha$ , asan index of lymphocyte-stimulating effect, was significantly higherin cells obtained at 9:00 AM than in the cells obtained at 9:00PM (P < .01). The number of receptors per cell and the expressionof interferon-stimulated gene factor in lymphocytes after 24-hincubation with IFN- $alpha$ were significantly higher in the cells obtainedat 9:00 AM than at 9:00 PM (P < .05). A significant dosing time-dependentdifference was demonstrated for the pharmacokinetic parametersof IFN- $alpha$ , which showed higher clearance for injections given at9:00 PM than for those at 9:00 AM (P < .05). The metabolism ofIFN- $alpha$ was significantly higher in kidney obtained at 9:00 PM thanat 9:00 AM (P < .05). These findings support that choosing themost appropriate time of day for administration of IFN- $alpha$ , associatedwith the rhythmicity of IFN- $alpha$ receptor function and IFN- $alpha$ pharmacokinetics,may increase the antiviral activity in experimental and clinicalsituations.

	Introduction

Top Abstract Introduction Materials and Methods Results Discussion References

A large number of physiological rhythms are controlled by the central nervous system, hormone secretion, and so on (Thomsonet al., 1980; Kafka et al., 1981; Naber et al., 1981). Also, manydrugs vary in potency and/or toxicity according to the time inthe circadian cycle when they are administered (Walker and Owasayo,1974; Frederickson et al., 1977; Ohdo et al., 1988, 1990, 1991,1995b, 1996, 1997b, 1998).

Interferons, which belong to a group of cytokines, have been widely used as antiviral and antitumor agents in humans. However,interferons cause unavoidable adverse effects such as fever, fatigue,headache, rigors, and myalgias. One approach to increasing theefficiency of pharmacotherapy is the administration of drugs attimes at which they are most effective and/or best tolerated.Certainly, use of a chronopharmacological strategy can improvethe effects and reduce the toxicity of drugs. Administration ofinterferon- $alpha$ (IFN- $alpha$ ) to cancer patients is better tolerated inthe evening than in the morning, although the pharmacologicaleffectiveness of IFN- $alpha$ has not been examined (Abrams et al., 1985;Iacobelli et al., 1995). There are significant dosing time-dependentdifferences reported in antitumor and myelosuppressive activityof IFN- $alpha$ in mice (Koren and Fleischmann, 1993; Koren et al., 1993).Also, the rhythmic changes of fever and antiviral activity inducedby IFN- $alpha$ were examined in mice (Koyanagi et al., 1997; Ohdo etal., 1997a), but the mechanism was not investigated indetail.

IFN- $alpha$ elicits antitumor and antiviral activity by binding to a specific receptor on the cell surface (Alexander et al., 1986;Kumar and Korutla, 1995). Furthermore, IFN- $alpha$ elicits transcriptionof various genes through activation of interferon-stimulated genefactor (ISGF), via binding to specific receptor. IFN- $alpha$ is quicklyeliminated from the body via several pathways. The main routeof excretion is via the kidneys (Bino et al., 1982). IFN- $alpha$ ispresumably filtered by glomeruli and taken up into tubules whereinit is metabolized. In this study, the dosing time-dependent changein antiviral activity induced by IFN- $alpha$ was examined in mice. Themechanisms underlying this phenomenon were investigated in termsof chronopharmacodynamics, the rhythmicity of receptor function,and chronopharmacokinetics, the rhythmicity of IFN- $alpha$ metabolisminkidney.

	Materials and Methods

Top Abstract Introduction Materials and Methods Results Discussion References

Animals and Chemicals. Male ICR mice (5 weeks old) were purchased from Charles River Japan Inc. (Kanagawa, Japan). Mice were housed 10 per cage ina light-controlled room (lights on from 7:00 AM to 7:00 PM) ata room temperature of 24 ± 1°C and a humidity of 60 ± 10% withfood and water ad libitum. All mice adapted to their light/darkcycle for 2 weeks before the experiments. IFN- $alpha$ (Sumiferon) wassupplied by Sumitomo Seiyaku Co. (Osaka, Japan). The drug supplywas given within the time period from manufacture before expiration.Adequate stability studies had been conducted on the given lot.IFN- $alpha$ was diluted with sterilized saline to adjust the concentrationto 2 MI.U./ml. The volume of injection was 0.05 ml/10 g of bodyweight. The drug solutions were used within 30 min after preparationto avoid decreasing their biological activity. The complete mediumused in this study consisted of RPMI 1640 supplemented with 10%heat-inactivated fetal bovine serum (FBS; Irvine Scientific, SantaAna, CA), 0.5% penicillin, and 0.5%kanamycin.

2'-5'Oligoadenylate Synthetase (2'-5'OAS) Activity in Plasma. To examine the 2'-5'OAS activity induced by IFN- $alpha$ , groups of eight mice were i.v. injected with 10 MI.U./kg of IFN- $alpha$ or sterilizedsaline in the first half of the light phase (9:00 AM) or in thefirst half of the dark phase (9:00 PM). The dosage of IFN- $alpha$ wasselected based on preliminary experiments in a previous study(Koyanagi et al., 1997). Blood samples were drawn by cardiac punctureat 24 h after IFN- $alpha$ injection and placed into microtubes containing10 µl of EDTA (4%) solution. Plasma samples were obtained aftercentrifugation at 3000 rpm for 3 min and then stored at $-$ 20°Cuntil assay. The plasma 2'-5'OAS activity was determined by radioimmunoassay(2-5A kit; Eiken, Tokyo,Japan).

IFN- $alpha$ Stimulating Effect on Lymphocytes. To study the IFN- $alpha$ stimulating effect on lymphocytes, blood from groups of six mice was taken with a 1-ml syringe at 9:00AM or 9:00 PM, and placed into microtubes containing 30 µl ofEDTA (4%). The blood lymphocytes were isolated by density gradientseparation medium (Lympholyte-M; Cedarlane Laboratory Ltd., Ontario,Canada) and treated with hemolysis buffer (Tris-ammonium chloridebuffer, 0.83% ammonium chloride/Tris buffer = 9:1, pH = 7.65)at 37°C for 5 min to get rid of the red cells. The remaining cellswere counted by trypan blue dye exclusion and resuspended to 1× 10⁵ viable cells/ml in complete medium. IFN- $alpha$ was diluted with sterilizedsaline consisting of 1% BSA (Sigma Chemical Co., St. Louis, MO)to adjust the concentration to 1 × 10⁴, 1 × 10⁵, and 1 × 10⁶ I.U./ml. Lymphocyte suspension (1 ml) was immediately transferredinto microtubes. IFN- $alpha$ solution (final concentration: 0, 100,1,000, 10,000 I.U./ml) and [³H]thymidine (10 µl, 25 µCi/ml) were added to each sample. Thecell suspensions were incubated at 37°C for 24 h in humidifiedair containing 5% CO₂. After incubation, cells were harvestedby centrifugation at 10,000 rpm, washed three times in completemedium, and transferred to scintillation vials containing 10 mlof aqueous counting scintillant (ACS II; Amersham Pharmacia BiotechLtd., Little Chalfont, Buckinghamshire, UK). The uptake of [³H]thymidine by lymphocytes was quantitated by a liquid scintillationcounter (LSC-1000; Aloka Co., Mitaka, Tokyo,Japan).

Iodination of IFN- $alpha$ . IFN- $alpha$ was iodinated using a solid-phase lactoperoxidase kit (ICN Pharmaceuticals, Inc., Irvine, CA). All operations were carriedout at room temperature. HCl (0.01 N) was added to neutralizethe 1 mCi of Na¹²⁵I (Amersham Pharmacia Biotech Ltd.) contained in the reactionvial, after which 10 µl of IFN- $alpha$ (1 µg/µl) (Pepro Tech EC Ltd.,London, UK) was added. The lactoperoxidase was dissolved in 25µl of distilled water, and added to the vial of radioiodine. Hydrogenperoxide (3%, 5 µl) was added to the vial and repeated four timesevery 10 min to initiate the reaction. Radioiodinated IFN- $alpha$ wasseparated from reactants with a PD-10 column (Amersham PharmaciaBiotech Ltd.), pre-equilibrated with 25 ml of phosphate buffer(pH 7.5) containing 0.1% BSA, using 0.05 M phosphate buffer (pH7.5) containing 0.5% BSA, as an elution buffer. The radioactivitywas determined by measuring the radioactivity of the precipitatethat was not dissolved by 10% trichloroacetic acid (TCA). Theconcentration of ¹²⁵I-IFN- $alpha$ in the eluting fraction was determined by enzyme-linkedimmunosorbent assay (ELISA) (IFN- $alpha$ immunoassay kit; BioSourceInternational Inc., Irvine, CA). The ¹²⁵I-IFN- $alpha$ was used within 1 month to avoidradiolysis.

IFN- $alpha$ Receptor Assay. To examine the IFN- $alpha$ bound to lymphocytes, blood was drawn from groups of six mice and rinsed with ice-cold PBS at 9:00 AMor 9:00 PM. The lymphocytes were isolated by the method describedabove. The cells were resuspended to 1 × 10⁶ cells/ml in complete medium. The binding experiments were performedat 4°C for 2 h with gentle shaking in a total volume of 200 µlof complete medium containing 0.2% BSA, various concentrationsof ¹²⁵I-IFN- $alpha$ , and 1 × 10⁶ lymphocytes in the microtubes. Sodium azide (0.1%) was also addedto prevent receptor internalization. Protamine sulfate (10 µg/ml;Wako Pure Chemical Industries, Ltd., Osaka, Japan) was added toprevent nonspecific binding, and 2.5 mM CaCl₂ was also added toimprove the binding. After incubation, cells were resuspended,transferred into 200 µl of FBS, and centrifuged at 10,000 rpmfor 1 min. The medium and FBS were then aspirated, the tube tipcontaining bound ligand was cut, and the radioactivity was determinedusing a gamma counter (ARC-360; Aloka Co.). Nonspecific bindingwas determined in the presence of an at least 250-fold excessof unlabeled IFN- $alpha$ . Specific binding was defined as nonspecificbinding subtracted from total binding. The data were plotted accordingto the method of Scatchard (1949). A molecular weight of 20,000was assumed for the calculation of the receptor number per celland the dissociation constant (K_d).

Western Blotting of ISGF. To examine the expression of ISGF in lymphocytes, blood was drawn from groups of three mice at 9:00 AM or 9:00 PM. The lymphocyteswere isolated by the method described above. The cells were resuspendedto 1 × 10⁵ viable cells/ml in complete medium. IFN- $alpha$ solution (final concentration:1000 I.U./ml), 10 µl each, were added to each sample. The cellsuspensions were incubated at 37°C for 24 h in humidified aircontaining 5% CO₂. After incubation, cells were harvested by centrifugationat 10,000 rpm. Cells were washed twice with buffer (25 mM Tris-HCl,150 mM NaCl, pH 8.0) and lysed in lysis buffer (50 mM Tris-HCl,pH 8.0, 120 mM NaCl, 0.5% Nonidet P-40, 100 mM NaF, 200 µM Na₂V₂O₅,1 mM phenylmethylsulfonyl fluoride, 10 µg of leupeptin/ml) for15 min on ice. The lysates were centrifuged at 4°C for 15 min.Cell lysates containing 30 µg of total protein were resolved by10% SDS-polyacrylamide gel electrophoresis, and transferred ontonitrocellulose. The membrane was reacted with the anti-p91 monoclonalantibody (Stat1; N terminus, Transduction Laboratories, Lexington,KY). The antibody cross-reacts with Stat1 (91 kDa) expressingcells in human, dog, mouse, chick, and frog. For detection ofthe antigen-antibody complex on the membrane, an alkaline phosphatase-conjugatedantibody was used as a secondary reagent, and visualized with3,3',5,5'-tetramethylbenzidine substrate. The intensity was assessedby using the NIH Image program on a Macintosh computer. Plotsof ISGF set the mean value of control at 9:00 AM at100.

IFN- $alpha$ Concentration in Plasma. To study the plasma IFN- $alpha$ concentrations over time, groups of six mice were i.v. injected with 10 MI.U./kg of IFN- $alpha$ at 9:00AM or 9:00 PM. Blood samples were collected by orbital sinus collectionat 0.167, 0.5, 1, 2, 3, and 4 h after IFN- $alpha$ injection. Plasmasamples were obtained after centrifugation at 3000 rpm for 3 minand stored at $-$ 20°C until assay. Plasma IFN- $alpha$ concentrations weredetermined by an ELISA kit (IFN- $alpha$ immunoassay kit; BioSource InternationalInc.). The titer was expressed in international units per milliliter,and the detection limit for the sample was 10 I.U./ml.

IFN- $alpha$ Metabolism in Renal Samples. To study IFN- $alpha$ renal metabolism, kidneys were removed from groups of six mice. Renal slices were cut and placed in 1 ml of0.05% BSA-Krebs-Ringer solution (37°C, 95% O₂, 5% CO₂) at 9:00AM or 9:00 PM. Renal slices were preincubated for 30 min, and1000 I.U. of ¹²⁵I-IFN- $alpha$ was added to each tube. At 0, 20, 40, and 60 min afterincubation, a 30-µl sample was transferred to 300 µl of PBS or300 µl of 10% TCA. The PBS or TCA solutions were centrifuged at10,000 rpm for 1 min, and 300 µl of supernatant was used for detectionby a gamma counter. The radioactivity of TCA-soluble fractionwas calculated as follows: % = ([the radioactivity of TCA-solublefraction at each time $-$ the radioactivity of TCA-soluble fractionat 0 min]/[the radioactivity of PBS solution at the correspondingtime (total radioactivity)]) × 100. The residual activity of IFN- $alpha$ was assayed by ELISA.

Statistical Analysis. Pharmacokinetic parameters were calculated by moment analysis. ANOVA and Tukey's test were used for multiple comparisons.Student's t test was used for comparisons between twogroups.

	Results

Top Abstract Introduction Materials and Methods Results Discussion References

Influence of Dosing Time on 2'-5'OAS Activity in Plasma. The influence of IFN- $alpha$ dosing time on 2'-5'OAS activity in plasma is shown in Fig. 1. 2'-5'OAS activity in plasma showed nosignificant difference between mice injected with saline at 9:00AM and 9:00 PM. 2'-5'OAS activity in plasma at 24 h after IFN- $alpha$ (10 MI.U./kg, i.v.) injection was significantly higher for injectionsgiven at 9:00 AM than for those at 9:00 PM (P < .05). 2'-5'OASactivity in plasma after IFN- $alpha$ injection at 9:00 AM increasedsignificantly compared with that after saline injection at 9:00AM (P < .01).

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Fig. 1. Influence of dosing time on the plasma 2'-5'OAS activity at 24 h after IFN- $alpha$ (10 MI.U./kg, i.v.) injection at 9:00 AM or 9:00 PM. *P < .05; **P < .01 when compared with the saline group, or between the two dosing times.

, saline; $black-square$ , IFN- $alpha$ .

Time Dependence of Lymphocyte Stimulating Effect. The stimulating effects of IFN- $alpha$ on lymphocytes are shown in Fig. 2. At the concentrations of 0, 100, 1,000, or 10,000 I.U./mlof IFN- $alpha$ , the uptake of [³H]thymidine by lymphocytes after 24-h incubation was significantlyhigher in the cells obtained at 9:00 AM than at 9:00 PM (P < .01).The uptake of [³H]thymidine by lymphocytes after 24-h incubation in the cellsobtained at 9:00 AM was significantly higher in the IFN- $alpha$ (1,000or 10,000 I.U./ml) group as compared with the saline group (P< .05).

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Fig. 2. Time-dependent difference in the stimulating effect of IFN- $alpha$ in lymphocytes prepared at 9:00 AM (

) or 9:00 PM ( $black-square$ ). The uptake of [³H]thymidine by lymphocytes after 24-h incubation with IFN- $alpha$ was used as an index of lymphocyte-stimulating effect of IFN- $alpha$ . *P < .05; **P < .01 when compared between the two groups.

Time Dependence of IFN- $alpha$ Receptor Function. The specific binding of ¹²⁵I-IFN- $alpha$ at concentrations of 5, 10, 20, or 30 ng/ml (1 ng = 300 I.U., expressed in nanograms per milliliterto estimate easily the parameters of IFN- $alpha$ receptor) was significantlyhigher in the cells obtained at 9:00 AM than in the cells obtainedat 9:00 PM (P < .05, Fig. 3A). The specific binding of ¹²⁵I-IFN- $alpha$ at other concentrations showed no significant time-dependentdifference. The specific binding data were replotted by the methodof Scatchard as shown in Fig. 3B. The number of receptors percell, calculated from the intercept of the Scatchard plot on theabscissa, was significantly larger in cells obtained at 9:00 AMthan at 9:00 PM (P < .05, Table 1). The apparent K_d value didnot differ significantly between cells obtained at 9:00 AM and9:00 PM.

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Fig. 3. Time-dependent difference of IFN- $alpha$ receptor in lymphocytes prepared at 9:00 AM ( $open circle$ ) or 9:00 PM (

). A, binding isotherms. B, Scatchard analysis. *P < .05 when compared between the two groups.

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TABLE 1
Time-dependent difference of IFN- $alpha$ receptor in lymphocytes prepared at 9:00 AM or 9:00 PM
Values show the mean ± S.E. of six mice. Statistical significance is compared between the two groups.

Time-Dependent Expression of ISGF in Lymphocytes. The expression of ISGF in lymphocytes is shown in Fig. 4. The expression of ISGF in lymphocytes after 24-h incubation withsaline showed no significant difference between the cells obtainedat 9:00 AM and 9:00 PM. The expression of ISGF in lymphocytesafter 24-h incubation with IFN- $alpha$ (1000 I.U./ml) was significantlyhigher in the cells obtained at 9:00 AM than at 9:00 PM (P < .05).The expression of ISGF in lymphocytes after 24-h incubation inthe cells obtained at 9:00 AM was significantly higher in theIFN- $alpha$ group as compared with the saline group (P < .05).

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Fig. 4. Time-dependent difference in the expression of ISGF in lymphocytes stimulated for 24 h with IFN- $alpha$ (1000 I.U.) at 9:00 AM or 9:00 PM. The expression of ISGF was determined by Western blot analysis. *P < .05 when compared with the saline group or between the two dosing times.

, saline; $black-square$ , IFN- $alpha$ .

Influence of Dosing Time on IFN- $alpha$ Concentration in Plasma. Plasma IFN- $alpha$ concentrations after IFN- $alpha$ (10 MI.U./kg, i.v.) injection decayed biphasically over time (Fig. 5). IFN- $alpha$ concentrationsat 2, 3, and 4 h after IFN- $alpha$ injection were significantly higherfor injections given at 9:00 AM than for those at 9:00 PM (P <.05). Clearance (CL) was significantly higher in mice injectedwith IFN- $alpha$ at 9:00 PM than in those injected at 9:00 AM (P < .05,Table 2). Area under the concentration-time curve, t_1/2, andmean residence time were significantly larger in mice injectedwith IFN- $alpha$ at 9:00 AM than at 9:00 PM (P < .05).

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Fig. 5. Influence of dosing time on plasma IFN- $alpha$ concentrations after IFN- $alpha$ (10 MI.U./kg, i.v.) injection at 9:00 AM ( $open circle$ ) or 9:00 PM (

). *P < .05 when compared between the two groups.

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TABLE 2
Influence of IFN- $alpha$ dosing time on the pharmacokinetic parameters after IFN- $alpha$ (10 MI.U./kg, i.v.) injection at 9:00 AM or 9:00 PM
Values show the mean ± S.E. of six mice. Statistical significance is compared between the two groups.

Time-Dependent Metabolism in Isolated Renal Slices. The metabolism of ¹²⁵I-IFN- $alpha$ (1000 I.U./ml) in renal slices is shown in Fig. 6. The radioactivity of TCA-soluble fraction at60 min after incubation was significantly higher in renal slicesobtained at 9:00 PM than at 9:00 AM (P < .05, Fig. 6A). The residualactivity of IFN- $alpha$ , analyzed by ELISA, at 60 min after incubationwas significantly higher in renal slices obtained at 9:00 AM thanat 9:00 PM (P < .05, Fig. 6B).

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Fig. 6. Time-dependent difference of IFN- $alpha$ metabolism in renal slices taken at 9:00 AM ( $open circle$ ) or 9:00 PM (

). A, radioactivity of degraded IFN- $alpha$ in TCA-soluble fraction. B, residual activity of undegraded IFN- $alpha$ assayed by ELISA. *P < .05 when compared between the two groups.

	Discussion

Top Abstract Introduction Materials and Methods Results Discussion References

The antiviral activity of interferon is due, at least in part, to the 2'-5'OAS system (Baglioni, 1979). Plasma 2'-5'OAS activityis used as an index of the antiviral effect of interferon in patientswith hepatitis. 2'-5'OAS activity in plasma at 24 h after IFN- $alpha$ injection was significantly higher for injections given at 9:00AM than for injection at 9:00 PM, although it showed no significanttime-dependent difference between mice injected with saline at9:00 AM and 9:00 PM. This finding confirms previous observationswith higher activity in the latter half of the dark phase andformer half of the light phase, and lower activity in the latterhalf of the light phase and former half of the dark phase (Koyanagiet al., 1997). To clarify the mechanisms underlying the dosingtime-dependent antiviral activity induced by IFN- $alpha$ , the amountof [³H]thymidine uptake by lymphocytes was used as an index of thestimulating effects of IFN- $alpha$ on lymphocytes. The uptake of [³H]thymidine by lymphocytes after 24-h incubation with IFN- $alpha$ wassignificantly higher in the cells obtained at 9:00 AM than inthe cells obtained at 9:00 PM. This finding corresponded wellto the dosing time-dependent antiviral activity of IFN- $alpha$ . A higherresponse of lymphocytes to IFN- $alpha$ was observed at 9:00 AM thanat 9:00 PM. Because IFN- $alpha$ also modifies pituitary-adrenal function(Roosth et al., 1986), the secretion of corticosterone by IFN- $alpha$ may vary depending on dosingtime.

IFN- $alpha$ elicits antiviral activity by binding to a specific receptor on cell surface (Aguet and Mogensen, 1983; Zoon and Arnheiter,1984), and is partially lymphocyte-mediated (Alexander et al.,1986). The number of IFN- $alpha$ receptors per lymphocyte was significantlylarger in cells obtained at 9:00 AM than at 9:00 PM. The nextquestion is whether the increase in IFN- $alpha$ receptor number is functionallysignificant. IFN- $alpha$ exerts its biological effect presumably byinducing the expression of a series of IFN-induced genes. ISGF,a transcriptional activator, is considered a positive regulatorin the biological action of IFN- $alpha$ (Kumar and Korutla, 1995). Theexpression of ISGF was significantly higher in cells obtainedat 9:00 AM than at 9:00 PM. This result can partly explain thetime-dependent antiviral activity of IFN- $alpha$ in terms of pharmacology.The number of IFN- $alpha$ receptor binding sites increases concomitantlywith an increase in IFN-signaling, when the proportion of cellsin the S (DNA synthesis) phase increases in leukemia (Tamura etal., 1997). This might be true in the case of this study. Certainly,the proportion of cells in the S phase was significantly higherin lymphocytes obtained at 9:00 AM than at 9:00 PM (9:00 AM, 6.7± 1.3%; 9:00 PM, 1.8 ± 0.3%, n = 5, mean ± S.E., P < .05). Itshould be clarified in the future why IFN- $alpha$ receptor expressionvaries with cell cycledistribution.

Plasma IFN- $alpha$ concentrations in the elimination phase after IFN- $alpha$ injection were significantly higher for injections givenat 9:00 AM than for those at 9:00 PM. The dosing time-dependentdifference of plasma IFN- $alpha$ concentrations corresponded well tothat of 2'-5'OAS activity induced by IFN- $alpha$ . Therefore, the diurnaldifference of 2'-5'OAS activity induced by IFN- $alpha$ can be explainedin part by that of plasma IFN- $alpha$ concentration. A significant dosingtime-dependent difference was also demonstrated for the pharmacokineticparameters of IFN- $alpha$ , which showed higher CL for the injectionat 9:00 PM than for that at 9:00 AM. The rhythmicity in CL seemsto be closely related to that in plasma IFN- $alpha$ concentration. IFN- $alpha$ concentrations in plasma have been shown to decay biphasicallyafter i.v. injection of IFN- $alpha$ , and the distribution phase lastedfor 1 h after drug injection (Cantell and Pyhara, 1973). IFN- $alpha$ is quickly eliminated from the body via several pathways. Themain route of excretion is via the kidneys (Bino et al., 1982).Renal tubular cells extract and break down many plasma proteins(Strober and Waldmann, 1974). IFN- $alpha$ is also internalized and catabolizedintracellularly in the kidney via receptor-mediated endocytosis(Bocci et al., 1983). Both the renal elimination rate and livermetabolism rate increase during the active period in mice (Ohdoet al., 1995a). The rhythmicity can reflect not only the rhythmicactivity of enzymes in the kidneys and liver, but also the rhythmicrate of blood flow (Labrecque et al., 1988). The rhythmicity ofCL in our study corresponds well to that of blood flow. The bloodflow in humans also increases during active periods (Lemmer andNold, 1991). This data obtained in nocturnally active mice maycorrespond with the data in diurnally active humans, if referredto the species-specific rest-activity cycle. The renal metabolicactivity in vitro was significantly higher in the renal slicesprepared at 9:00 PM than in those prepared at 9:00 AM. The findingin vitro corresponded well to the dosing time-dependent differenceof IFN- $alpha$ pharmacokinetics in vivo. Thus the circadian rhythm inIFN- $alpha$ pharmacokinetics may be caused by the diurnal rhythm ofrenal function. Although the circadian rhythm of receptor-mediatedendocytosis has not yet been investigated, it should be clarifiedin thefuture.

These findings in this mouse model support the concept that choosing the most appropriate time of day for administration ofIFN- $alpha$ associated with the rhythmicity of IFN- $alpha$ receptor functionand renal function may increase the antiviral activity in experimentaland clinicalsituations.

	Acknowledgment

We thank Sumitomo Seiyaku Co. (Osaka, Japan) for the generous supply of IFN- $alpha$ (Sumiferon) for thisexperiment.

	Footnotes

Accepted for publication April 28, 2000.

Received for publication January 4, 2000.

¹ This research was supported by Grant-in-Aid 00223884 for Scientific Research (C) from the Ministry of Education, Science,Sports and Culture, Japan (S.O.), a grant-in-aid from the TokyoBiochemical Research Foundation, a grant-in-aid from the NakatomiFoundation, and a grant-in-aid from Nippon BoehringerIngelheim.

Send reprint requests to: Shigehiro Ohdo, Ph.D., Department of Clinical Pharmacokinetics, Division of Pharmaceutical Science, Graduate School, Kyushu University, 3-1-1, Maidashi, Higashi-Ku, Fukuoka, 812-8582 Japan. E-mail: ohdo{at}shunsan.phar.kyushu-u.ac.jp.

	Abbreviations

IFN- $alpha$ , interferon- $alpha$ ; MI.U., mega international units; ISGF, interferon-stimulated gene factor; 2'-5'OAS, 2'-5'oligoadenylate synthetase; CL, clearance; FBS, fetal bovine serum; TCA, trichloroacetic acid; ELISA, enzyme-linked immunosorbent assay.

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