Prediction of in Vivo Hepatic Metabolic Clearance of YM796 from in Vitro Data by Use of Human Liver Microsomes and Recombinant P-450 Isozymes

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Vol. 282, Issue 2, 909-919, 1997

Prediction of in Vivo Hepatic Metabolic Clearance of YM796 from in Vitro Data by Use of Human Liver Microsomes and Recombinant P-450 Isozymes

Takafumi Iwatsubo , Hiroshi Suzuki, Noriaki Shimada, Kan Chiba, Takashi Ishizaki, Carol E. Green, Charles A. Tyson, Tsuyoshi Yokoi, Tetsuya Kamataki and Yuichi Sugiyama

Drug Metabolism Laboratories, Yamanouchi Pharmaceutical Co., Ltd., 1-1-8, Azusawa, Itabashi-ku, Tokyo, 174, Japan (T.I.), Faculty of Pharmaceutical Sciences, The University of Tokyo, 7-3-1, Hongo, Bunkyo-ku, Tokyo 113, Japan (H.S., Y.S.), Research and Development Division, Daiichi Pure Chemicals Co., Ltd., 3-13-5, Nihombashi, Chuo-ku, Tokyo, 103, Japan (N.S.), Laboratory of Biochemical Pharmacology and Biotoxicology, Faculty of Pharmaceutical Sciences, Chiba University, 1-33, Yayoi-cho, Inage-ku, Chiba, 263, Japan (K.C.), Department of Clinical Pharmacology, International Medical Center of Japan, 1-21-2, Toyama, Shinjuku-ku, Tokyo, 162, Japan (T.I.), Toxicology Laboratory, SRI International, Menlo Park, California (C.E.G., C.A.T.) and Division of Drug Metabolism, Faculty of Pharmaceutical Sciences, Hokkaido University, W-6, N-12, Kita-ku, Sapporo 060, Japan (T.Y., T.K.)

	Abstract

Top Abstract Introduction Materials & Methods Results Discussion References

The metabolic rate of (S)-( $-$ )-2,8-dimethyl-3-methylene-1-oxa-8-azaspiro [4,5] decane-L-tartarate monohydrate (YM796), an antidementiaagent, was determined by use of 12 different human liver microsomalsamples. The metabolism of YM796 was shown to consist of threecomponents; one high-affinity (K_m1 = 1.67 µM), one low-affinity(K_m2 = 654 µM) and a nonsaturable component. Good correlationswere observed between the individual CYP3A4 content in 12 differenthuman liver microsomal samples and kinetic parameters such asCL_int,
all, the high-affinity component clearance (V_max1/K_m1)and the low-affinity component clearance (V_max2/K_m2).Anti-human CYP3A4/5 antibodies inhibited the metabolism of YM796at 1 µM by up to 75%. In addition, ketoconazole, an inhibitorof CYP3A4, inhibited YM796 metabolism by >90%. The metabolic clearanceof YM796 in each of the 12 human liver microsomal samples wassuccessfully predicted from the kinetic parameters obtained withthe recombinant microsomes by taking into consideration the CYP3A4content in each microsomal sample. Based on the CL_{int, all} estimatedfrom the in vitro experiments, the area under the plasma concentration-timecurve after oral administration (AUC_oral) of YM796 was also predictedby taking into account the hepatic blood flow rate (Q_h), the unboundfraction of YM796 in human plasma (f_p) and the fraction absorbedfrom the gut. In addition, AUC_oral was determined in six healthymale volunteers. The predicted AUC_oral was similar to the observedvalue in vivo, which suggests that the in vitro metabolism dataobtained with human liver microsomes are useful for quantitativelypredicting human liver metabolism in vivo and that recombinantmicrosomes are also available when the particular isozyme is almostcompletely responsible for the metabolism of the drug, the variationin P-450 content of human liver is known and the experimentalconditions such as the amount of CYP reductase and cytochromeb₅are carefully optimized to mimic the activity found in nativemicrosomes, as for YM796.

	Introduction

Top Abstract Introduction Materials & Methods Results Discussion References

It is of clinical importance to predict hepatic and renal clearances in humans because many drugs are eliminated from thebody predominantly by these pathways. There have been many successfulattempts to predict renal clearance (CL_r) in humans by applyingthe method for animal scaling based on data derived from animalexperiments (Dedrick, 1974; Boxenbaum, 1982; Sawada et al., 1984).On the other hand, the application of the animal scaling methodto the prediction of hepatic clearance (CL_h) is limited becauseof large interspecies differences in the metabolic clearances(Boxenbaum, 1980).

An alternative method has been proposed by Rane et al. (1977) and Wilkinson (1987) to predict hepatic metabolic clearancefrom in vitro metabolism data in rats by use of liver microsomesor isolated hepatocytes by taking into account parameters suchas Q_h and the unbound fraction of drug in blood (f_b). We havealso successfully predicted the in vivo metabolic clearances inrats for 14 drugs reported to be metabolized by CYP (Sugiyamaet al., 1988; Sugiyama and Iwatsubo, 1994). Houston (1994) comparedthe intrinsic metabolic clearances (CL_int) for many drugs estimatedfrom in vitro experiments with rat liver microsomes and isolatedrat hepatocytes with the CL_intvalues calculated from in vivopharmacokinetic data, and found good predictability, althoughthe CL_intseemed to be slightly underestimated in liver microsomes.In particular, the CL_int estimated by use of isolated hepatocytescorrelated well with in vivo CL_int for various drugs exhibitinga 4 order magnitude of difference in CL_int.

A predictability assessment of an in vivo kinetic (i.e., clearance) behavior from the correspondent in vitro data would thusalso be very useful for the human situation, particularly in viewof the increasing availability of human liver specimens. We havedescribed a method for predicting in vivo hepatic metabolic clearancefrom in vitro metabolism data and have suggested that this "invitro/in vivo scaling" method is also useful in humans for variousdrugs which are metabolized by P-450 in the liver, based on thewealth of in vitro and in vivo literature data on metabolism (Iwatsuboet al., 1996). In this respect, we have also indicated that severalimportant factors should be considered to increase the predictability(Iwatsubo et al., 1997). In addition, as an in vitro alternativeto human liver microsomes, it is possible to use recombinant microsomesprepared from cells expressing the human CYP isozyme (recombinantsystem) to predict an in vivo metabolic clearance.

In the present study, with (S)-( $-$ )-2,8-dimethyl-3-methylene-1-oxa-8-azaspiro [4,5] decane-L-tartarate monohydrate (YM796),which is being developed for the treatment of dementia, as a modelcompound, we have shown that the CYP3A4 isozyme is responsiblefor the metabolism of YM796. We have examined the availabilityof the recombinant system of human CYP isozymes as an alternativeto human liver microsomes by comparing the estimated and correctedmetabolic clearances based on the CYP3A4 content in both systemsand also assessed the predictive validity of in vivo metabolicclearances from in vitro metabolic data.

	Materials and Methods

Top Abstract Introduction Materials & Methods Results Discussion References

Chemicals and reagents. YM796 and [¹⁴C]YM796 were synthesized by Yamanouchi Pharmaceutical Co., Ltd (Tokyo, Japan) and by Amersham International (Buckinghamshire,UK), respectively. 6 $beta$ -Hydroxytestosterone and ketoconazole werepurchased from Sigma Chemical Co. (St. Louis, MO). Acetonitrile,methanol and other reagents of analytical grade were purchasedfrom Wako Pure Chemical Industries, Ltd (Osaka, Japan). NADP,glucose 6-phosphate and glucose-6-phosphate dehydrogenase wereobtained from Boehringer Mannheim (Mannheim, Germany). Microsomalpreparations of recombinant human CYP enzymes expressed by thehuman B lymphoblastoid cell line, AHH-1 (recombinant microsomes),were purchased from Gentest Corp. (Woburn, MA). Twelve human livermicrosomes (H-19, H-35, H-36, H-38, H-50, H-51, H-56, H-57, H-62,H-66, H-67 and H-84) with large variations in the CYP3A4 contentwere selected and generous gifts for the in vitro metabolism experimentsamong 26 different microsomes prepared from human livers storedin the human liver bank of SRI International (Menlo Park, CA).Antibodies to human CYP3A4/5 were also a generous gift from InternationalMedical Center of Japan (Tokyo, Japan).

YM796 metabolism in human liver microsomes or recombinant human CYP isozymes. YM796 and [¹⁴C]YM796 (1 µM; specific activity, 40 mCi/mmol) were incubated with a reaction mixture (0.25 ml) consisting of 25µg human liver MS protein and an NADPH-generating system (0.33mM NADP, 8 mM glucose 6-phosphate, 0.1 U/ml glucose-6-phosphatedehydrogenase, 6 mM MgCl₂) in 100 mM potassium phosphate buffer(pH 7.4). Incubation conditions used for microsomes from B lymphoblastoidcells expressing the different recombinant human CYP isozymeswere similar to those used for human liver microsomes, exceptfor the quantity of microsomes. In the metabolism studies witheach of the recombinant human CYP isozymes, the quantity of MSprotein was adjusted to the amount of CYP isozyme similar to thatreported for human liver microsomes. Enzyme reactions were initiatedby adding 25 µl of the NADPH-generating system as mentioned above.After incubation at 37°C in a shaking water bath for 2 min, thereaction was terminated by adding 250 µl methanol, and then thereaction mixture was centrifuged at 10,000 × g for 5 min and analiquot of supernatant was spotted onto silica-gel plates (E.Merck, Darmstadt, Germany) to separate metabolites from the parentdrug by TLC with use of chloroform/methanol/27% ammonia (100:10:1)as a mobile phase. Experiments were performed in triplicate. YM796concentrations to estimate the kinetic parameters were from 1to 1000 µM. The quantitation of metabolites was performed withBAS-2000 equipment (Fuji-film, Tokyo, Japan).

Immunoinhibition study. Human liver microsomes (H-35) at a final concentration of 0.1 mg/ml were preincubated for 30 min at room temperature withincreasing amounts of antibodies (from 1 to 4 mg/mg MS protein)for human CYP3A4/5 or preimmunoglobulin G obtained from rabbits.The final YM796 concentration was 1 µM.

Inhibition study. As an inhibitor of human CYP3A4, ketoconazole was used to assess if it would have an inhibitory effect on YM796 metabolism.Assays were performed with human liver microsomes (H-35) underthe optimal conditions above. Final YM796 concentrations wereset at 1 and 1000 µM, whereas ketoconazole concentrations rangedfrom 0.01 to 10 µM.

Purification of NADPH-cytochrome P-450 reductase and cytochrome b₅. NADPH-cytochrome P-450 reductase was purified from rat liver microsomes to a specific activity of 23 U/mg protein by the methodof Yasukochi and Masters (1976) with minor modifications. Cytochromeb₅ was purified from rat liver microsomes to a specific contentof 28 nmol/mg protein by the method reported previously (Kamatakiet al., 1981).

Effects of NADPH-cytochrome P-450 reductase and cytochrome b₅ on YM796 metabolism in recombinant microsomes for human CYP3A4. Under the conditions described above, the effects of NADPH-cytochrome P-450 reductase and cytochrome b₅ on YM796 metabolismin recombinant microsomes expressing human CYP 3A4 were estimatedby use of increasing amounts of NADPH-cytochrome P-450 reductase(5-40 U/nmol P-450) or cytochrome b₅ (0.5-8.0 nmol/nmol P-450).Before the addition of the substrate and the NADPH-generatingsystem, the recombinant microsomes were preincubated with NADPH-cytochromeP-450 reductase or cytochrome b₅ at 37°C for 10 min. The finalYM796 concentration was 1 µM. As a positive control, the effectsof NADPH-cytochrome P-450 reductase and cytochrome b₅on testosterone-6 $beta$ -hydroxylaseactivity were also examined. Incubation conditions were essentiallythe same as those used for YM796 metabolism as described previously,except that the time used was 10 min. The final testosterone concentrationwas 250 µM. The 6 $beta$ -hydroxytestosterone was determined by an HPLC-UVabsorbance method as reported elsewhere (Yoshimoto et al., 1995).Nitrazepam was used as an internal standard. The HPLC column usedwas a CAPCELL PAK C18 SG 120 column (250 × 4.6 mm internal diameter,Shiseido Co., Ltd., Tokyo, Japan). The mobile phase for the 6 $beta$ -hydroxytestosteroneassay was a 60:40 (v/v) mixture of methanol and 0.05 M potassiumphosphate buffer (pH 3.4) and delivered at a flow rate of 1.0ml/min.

Protein binding of YM796 in human plasma. To 2-ml aliquots of human plasma, 20 µl of phosphate-buffered isotonic solution containing [¹⁴C]YM796 were added to give concentrations of 0.5, 50 and 2500µM. After incubation for 30 min at 37°C, a 50-µl aliquot was takenfrom each plasma sample to measure the total plasma concentrationand the remainder was transferred to a ultrafiltration tube (UltrafreeCL, Millipore Corp., Bedford, MA). The tubes were centrifugedfor 15 min (1,000 × g at 37°C), and then a 50-µl aliquot of filtratewas removed to measure the unbound plasma concentration. Aliquotsof plasma and filtrated samples were subjected to liquid scintillationcounting with 10 ml of liquid scintillator.

Blood-to-plasma concentration ratio (R_B) of YM796 in humans. R_B of YM796 was determined with heparinized whole blood (Lin et al., 1982). To 1-ml aliquots of human blood preincubated at37°C, 20-µl aliquots of phosphate-buffered isotonic solution containing[¹⁴C]YM796 were added to give concentrations of 0.5, 50 and 2500µM. After incubation for 5 min at 37°C, the blood samples werecentrifuged for 5 min at 1,500 × g, and then aliquots of plasmawere subjected to liquid scintillation counting with 10 ml ofliquid scintillator.

Prediction of AUC or F_h of YM796 under linear conditions in humans from in vitro metabolic data. CL_h under linear conditions was calculated by use of the CL_{int, all} values obtained from in vitro studies. The following equationsbased on the dispersion model (Roberts and Rowland, 1986a; Sugiyamaet al., 1988) were used:

CLh<IT>=Q</IT>h(<IT>1−</IT>Fh) (1)

Fh<IT>=</IT><FR><NU><IT>4a</IT></NU><DE>(<IT>1+a</IT>)<IT>2</IT>exp{(<IT>a−1</IT>)<IT>/2</IT>DN}<IT>−</IT>(<IT>1−a</IT>)<IT>2</IT>exp{<IT>−</IT>(<IT>a+1</IT>)<IT>/2</IT>DN}</DE></FR> (2)

where

a=(1+4RN<IT> · </IT>DN)<IT>1/2</IT> (3)

in which

RN<IT>=</IT>(fp<IT>/</IT>RB)<IT> · </IT>CLint,all<IT>/Q</IT>h (4)

CL_{int, all} is calculated from the K_mand V_max values obtained in vitro as follows:

CLint,all<IT>=</IT><LIM><OP>∑</OP><LL><IT>i</IT></LL></LIM><FR><NU><IT>V</IT>max<IT>,i</IT></NU><DE><IT>K</IT><IT>m,i</IT></DE></FR> (5)

The CL_{int, all} values estimated from the in vitro experiments with human liver microsomes were expressed per gram of liverby taking into account the mass recovery of CYP (Iwatsubo et al.,1996, 1997). A Q_h value of 0.95 ml/min/g liver (Bischoff et al.,1971; Dedrick et al., 1973; Montandon et al., 1975) and a dispersionnumber (D_N) of 0.17 (Roberts and Rowland, 1986b; Iwatsubo et al.,1996, 1997) were used for all calculations of CL_h. The f_p andR_B values of YM796 used for equation 4 were 0.700 (±0.002) and1.11 (±0.07) obtained at YM796 concentrations ranging from 0.5to 2500 µM, respectively. Thus, the oral clearance (CL_oral) wascalculated from equation 6 by use of the CL_h and F_h values underlinear conditions as estimated above, together with the CL_r value(72.7 ml/min) obtained from the urinary excretion data for theparent drug in humans.

CLoral<IT>=</IT>(CLh<IT>+</IT>CLr<IT>+</IT>Fh<IT> · </IT>CLg)<IT>/</IT>(Fa<IT> · </IT>Fg<IT> · </IT>Fh) (6)

where F_a, F_g and CL_g represent the fraction absorbed from the intestinal tract, intestinal availability and clearance forintestinal metabolism, respectively. Taking into considerationthe results obtained from the experiments in rats showing thatthe fraction of unchanged YM796 absorbed from the intestinal tract,estimated from the difference in plasma concentrations betweenthe circulating arterial blood and portal vein blood after administrationof YM796 into the intestinal loop, was close to unity and thefact that YM796 was not metabolized by microsomes from the smallintestine, we assumed that F_a·F_g was unity and CL_g was negligible(close to 0) for all calculations in the present study.

AUC of YM796 after oral administration in humans. Six healthy male volunteers were enrolled in the study and admitted to the Kitasato University School of Medicine. The protocolhad been approved by the Institutional Review Board and writtenconsent been obtained from each of the subjects before the study.All subjects were given YM796 orally in a capsule form (lactosetriturated powder) at a dose of 5 mg (14.3 µmol). Blood sampleswere collected from the antecubital vein with a heparinized syringebefore dosing and at 0.5, 1, 2, 3, 4, 6, 8, 10, 12 and 24 h postdose.After centrifugation, plasma was separated and stored at $-$ 20°Cuntil assay. An aliquot of plasma (2.5 ml) was buffered with 0.5ml saturated sodium bicarbonate solution after addition of 0.1ml internal standard aqueous solution, and the resulting mixturewas stirred and applied to a disposable column (Chem Elute, AnalytichemInternational, Harbor City, CA) for liquid-liquid extraction.YM796 was extracted by passing 4 ml dichlorethane through thecolumn twice. The extract was evaporated to dryness under reducedpressure, then the residue was dissolved in 0.5 ml of 0.1 N hydrochloricacid and washed with 8 ml diethylether. After stirring and centrifugation,the upper layer (ether) was discarded. To the aqueous layer, 1ml saturated sodium bicarbonate solution was added and YM796 wasextracted from the resulting mixture by use of 7 ml dichloroethane.After stirring and centrifugation, the aqueous layer was discardedand the organic layer was evaporated to dryness. The residue wasdissolved in chloroform, and a small aliquot (25 µl) was injectedinto the GC-MS-MS system that was performed on a Finnigan MAT(San Jose, CA) TSQ70 triple quadrupole mass spectrometer connectedto the gas chromatograph (Varian 3400). Gas chromatography wasperformed on a phenylmethyl silicone capillary column (DB-17,15 m × 0.25 mm internal diameter, 0.25 µm, J&W Scientific, Folsom,CA). The column temperature was raised from 50°C to 242°C at arate of 32°C/min. The sheath (nebulizing) gas pressure and auxiliarynitrogen flow were set at 70 p.s.i. (approximately 4.8 × 10⁵ Pa) and 20 ml/min, respectively. Chemical ionization was performedin the reaction gas (methane) at an ionization voltage of 100V. The mass spectrometer was set to admit positively charged protonatedmolecules [M+H]⁺ at m/z 182 (YM796) and m/z 196 (internal standard) via the firstquadrupole filter (Q1) with collision-induced fragmentation inQ2 [collision gas argon, $-$ 25 eV, 1.5 mTorr (approximately 0.20Pa)] and monitoring, via Q3, the production of fragments m/z 96and m/z 110 for YM796 and its internal standard, respectively.Each selected reaction was monitored with a dwell time of 0.2s.

Data analysis. The kinetic data for YM796 metabolism obtained in human liver microsomes and recombinant microsomes for human CYP3A4, respectively,were fitted to the following equations with use of MULTI (Yamaokaet al., 1981).

v=Vmax<IT>1</IT><IT> · S/</IT>(<IT>Km1+S</IT>)<IT>+V</IT>max<IT>2</IT><IT> · S/</IT>(<IT>Km2+S</IT>)<IT>+</IT>CLns<IT> · S</IT> (7)

(8)

Fitting evaluation was carried out based on the Akaike's information criterion value (Akaike, 1969).

In addition, the metabolic clearance in human liver microsomes was predicted from parameters obtained in recombinant microsomesby taking into consideration the CYP3A4 content in both microsomalpreparations and by converting V_max1 and V_{max 2} given as per milligramrecombinant MS protein in equation 8 to V_max1 $'$ and V_max2 $'$ givenas per milligram human liver MS protein with the following equations,respectively:

(9)

<IT>V<SUB>max1</SUB>×</IT><FR><NU>CYP<IT>3</IT>A<IT>4 </IT>content<IT>/</IT>mg human liver MS protein</NU><DE>CYP<IT>3</IT>A<IT>4 </IT>content<IT>/</IT>mg recombinant MS protein</DE></FR>

(10)

<IT>V<SUB>max2</SUB>×</IT><FR><NU>CYP<IT>3</IT>A<IT>4 </IT>content<IT>/</IT>mg human liver MS protein</NU><DE>CYP<IT>3</IT>A<IT>4 </IT>content<IT>/</IT>mg recombinant MS protein</DE></FR>

	Results

Top Abstract Introduction Materials & Methods Results Discussion References

YM796 metabolism in human liver microsomes. Eadie-Hofstee plots for the formation of total metabolites of YM796 in three representative human liver microsomal sampleswhich contain high (H-62; 148 pmol/mg MS protein), moderate (H-51;51.0 pmol/mg MS protein) and low (H-57; 19.7 pmol/mg MS protein)amounts of CYP3A4 are shown in figure 1. For all microsomes, theformation of YM796 metabolites could be described by three components:high-affinity with low-capacity, low-affinity with high-capacityand nonsaturable components. Table 1 summarizes each kineticparameter obtained by fitting analysis for all of 12 microsomesused in the present study. The mean K_m and V_max values for thehigh- and low-affinity components, respectively, were as follows:K_m1 = 1.67 µM and V_max1 = 0.0239 nmol/min/mg MS protein;and K_m2 = 654 µM and V_{max 2} = 1.51 nmol/min/mg MS protein(table 1). The clearance of the nonsaturable component (CL_ns)was 0.00123 ml/min/mg MS protein. Under linear conditions wherethe YM796 concentration was much less than K_m1, the fractionalclearance of each component to CL_{int, all} was 80.4, 13.0 and 6.6%,respectively. When CL_{int, all} was expressed per nanomole of CYP3A4instead of per milligram of MS protein, the CL_{int, all} valuesestimated in the 12 human liver microsomal samples under linearconditions showed smaller interindividual variabilities irrespectiveof more than a 7-fold interindividual difference in CYP3A4 content(table 1).

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Fig. 1. Eadie-Hofstee plots for the formation of total metabolites and major metabolites (M1 and M2) of YM796 in 3 individual humanliver microsomal samples. YM796 (1-1000 µM) was incubated for2 min at 37°C with human liver microsomes (0.1 mg protein/ml)with high (H-62; 148 pmol/mg MS protein), moderate (H-51; 51.0pmol/mg MS protein) and low (H-57; 19.7 pmol/mg MS protein) amountsof CYP3A4. (A) Eadie-Hofstee plots for total metabolite formation;(B) Eadie-Hofstee plots for M1 formation; and (C) Eadie-Hofsteeplots for M2 formation. Note that the scales of both ordinateand abscissa of each figure are different. The closed circlesindicate observed data and the solid lines represent the fittedcurves (equation 13). The dotted lines represent the predictedcurves from the kinetic parameters obtained in the recombinantmicrosomes of human CYP3A4 by considering the content of CYP3A4in each microsomal sample based on equations 8 to 10. The CYP3A4content in the recombinant system was 0.0345 nmol/mg MS protein.

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TABLE 1
Kinetic parameters for YM796 metabolism in human liver microsomes

At least four different metabolites of YM796 were detectable by TLC for each microsomal sample. The R_f values of YM796 andeach metabolite (M1- M4) were 0.52 and 0.12, 0.19, 0.39 and 0.45,respectively. Two of them (M1 and M2) were major and accountedfor approximately 50 and 30% of the total metabolite formation,respectively (fig. 2). Eadie-Hofstee plots for the formation ofM1 and M2 in the same three human liver microsomal samples asmentioned above are also shown in figure 1. For both metabolites,the metabolic pattern could be described by three components aswell as the total metabolites, and the high-affinity componentaccounted for 80% of the CL_int,
all under linear conditions. TheK_m1 values estimated by fitting analysis for total metabolites,M1 and M2 were 1.94, 2.13 and 2.80 µM for H-51, 1.88, 1.13 and2.09 µM for H-57 and 1.70, 1.03 and 2.16 µM for H-62, respectively,showing no marked difference in the K_m1 values amongmetabolites in each microsomal sample. The contribution of eachcomponent to the CL_{int, all} under the linear conditions was 71.6to 89.2%, 9.9 to 15.0% and 0.8 to 13.7% for total metabolites,78.8 to 90.7%, 5.8 to 11.3% and 3.0 to 10.5% for M1 and 69.6 to90.0%, 3.7 to 14.9% and 1.5 to 15.5% for M2, showing no pronounceddifferences among the metabolites.

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Fig. 2. TLC patterns of YM796 and its metabolites in human liver microsomes. The final YM796 concentrations were 1 µM (A), 30 µM (B)and 1000 µM (C). The ¹⁴C-labeled YM796 concentration was kept constant at 8.88 × 10⁴ dpm/ml (1 µM). All samples were derived from the microsomes fromH-35 subject. R_f values for YM796, M1, M2, M3 and M4 were 0.52,0.12, 0.19, 0.39 and 0.45, respectively.

Identification of CYP isozyme(s) responsible for YM796 metabolism. Significant correlations were obtained between the CYP3A4 content and the CL_{int, all}, the high-affinity component clearance(V_max1/K_m1) or the low-affinity component clearance (V_max2/K_m2)for the 12 human liver microsomal samples as shown in figure 3(r = 0.917, 0.851 or 0.928, respectively). Furthermore, a significantcorrelation with V_max1 or V_max2 was obtained (table 2). Figure4 shows the formation clearance for total metabolites over a widerange of YM796 concentrations in the recombinant human CYP isozymes(i.e., CYP1A2, 2C9, 2D6, 2E1 and 3A4). A high metabolic activitywas observed only with the recombinant CYP3A4. In addition, antibodiesto human CYP3A4/5 inhibited the formation of total metabolitesof YM796 by approximately 75% (fig. 5). Similar inhibitory effectswere observed for the formation of M1 and M2 as well as totalmetabolites. Ketoconazole, an inhibitor of CYP3A4, also inhibitedYM796 metabolism in a concentration-dependent manner, and theinhibition was almost complete at 10 µM (fig. 6). The formationof M1 and M2 was also inhibited in a concentration-dependent mannerby ketoconazole with a complete inhibition at 10 µM.

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Fig. 3. Correlation between CYP3A4 content and overall intrinsic clearance, V_max
1/K_m1 or V_max2/K_m2 obtained fromin vitro metabolic data of YM796 with 12 human liver microsomalsamples. The parameters used here are summarized in table 1.The solid lines represent the linear regression lines, and thecorrelation coefficients (r values) are given.

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TABLE 2
Correlation coefficients between CYP3A4 content and each kinetic parameter

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Fig. 4. Concentration dependence of in vitro metabolic clearances of YM796 in each of the recombinant CYP isozymes. YM796 (1-1000µM) was incubated for 2 min at 37°C with recombinant microsomesexpressing each CYP isozyme. A quantity of MS protein containingan amount of each CYP enzyme similar to the value reported forhuman liver microsomes (Shimada et al., 1994

) was used as follows: $open circle$ , control; $black-square$ , CYP1A2 (4.2 pmol/0.400 mg recombinant MS protein/ml); $black-triangle$ , CYP2C9 (6.0 pmol/0.420 mg recombinant MS protein/ml); $black-diamond$ , CYP2D6(0.5 pmol/0.003 mg recombinant MS protein/ml); $black-down-triangle$ , CYP2E1 (2.2pmol/0.019 mg recombinant MS protein/ml); $bullet$ , CYP3A4 (9.6 pmol/0.275mg recombinant MS protein/ml).

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Fig. 5. Effects of antibodies to human CYP3A4/5 on the formation of total metabolites of YM796 in human liver microsomes. Human livermicrosomes (H-35, 0.1 mg protein/ml) were preincubated for 30min at room temperature with 1 to 4 mg of antibodies to humanCYP3A4/5 or preimmunoglobulin G per mg MS protein. $open circle$ , preimmuneIgG; $bullet$ , anti-human CYP3A4/5 IgG.

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Fig. 6. Effect of ketoconazole on the formation of total metabolites of YM796 in human liver microsomes. YM796 (1 or 1000 µM) wasincubated for 2 min at 37°C with human liver microsomes (H-35,0.1 mg protein/ml) in the absence or presence of ketoconazole(0.01-10 µM). $black-square$ , YM796 1 µM; $bullet$ , YM796 1000 µM.

YM796 metabolism by recombinant human CYP3A4. Eadie-Hofstee plots for the formation of total metabolites of YM796 in the recombinant human CYP3A4 are shown in figure 7.They could be described by two components, one with high affinityand another with a very low affinity. The respective K_m and V_maxvalues were 1.10 µM and 0.0160 nmol/min/mg protein, and 10.9 mMand 8.98 nmol/min/mg protein. The high-affinity component wasmore important under the linear conditions where YM796 concentrationswere much lower than K_m1. The K_m value for the high-affinitycomponent was similar to that obtained with human liver microsomalsamples. With use of the recombinant human CYP3A4, the testosterone-6 $beta$ -hydroxylationactivity increased by about 2- to 3-fold after the addition ofCYP reductase or cytochrome b₅, whereas YM796 metabolism was unaffected(fig. 8).

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Fig. 7. Eadie-Hofstee plots for the formation of total metabolites of YM796 in the recombinant system of human CYP3A4. YM796 (1-1000µM) was incubated for 2 min at 37°C with the recombinant humanCYP3A4. A quantity of MS protein containing an amount of CYP enzyme(9.6 pmol/0.275 mg recombinant MS protein/ml) similar to the valuereported for human liver microsomes (Shimada et al., 1994

) wasused. The closed circles indicate observed data, and the solidlines represent the fitted curves. In the inset, the axes areenlarged for the data at lower concentrations (1-100 µM). Thekinetic parameters for the high-affinity component (K_m1and V_max1) were 1.10 µM and 0.0160 nmol/min/mg protein, whereasthe kinetic parameters for the low-affinity component (K_m2and V_max2) were 10.9 mM and 8.98 nmol/min/mg protein, respectively.

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Fig. 8. Effects of cytochrome P-450 reductase or b₅ on testosterone 6 $beta$ -hydroxylation (A and C) and YM796 metabolism (B and D) in therecombinant system. In (A), the amount of NADPH-cytochrome P-450reductase used was 5-40 U/nmol P-450. The incubation time was10 min, and the final testosterone concentration was set at 250µM. In (B), the amount of NADPH-cytochrome P-450 reductase usedwas 5-40 U/nmol P-450. The incubation time was 2 min and, thefinal YM796 concentration was set at 1 µM. In (C), the amountof cytochrome b₅ used was 0.5-8.0 nmol/nmol P-450. The incubationtime was 10 min, and the final testosterone concentration wasset at 250 µM. In (D), the amount of cytochrome b₅ used was 0.5-8.0nmol/nmol P-450. The incubation time was 2 min, and the finalYM796 concentration was set at 1 µM.

Prediction of CL_{int, all} in human liver microsomes from the recombinant data. The intrinsic metabolic clearances were calculated from the kinetic parameters obtained by use of the recombinant human CYP3A4.To predict the intrinsic metabolic clearance for each human livermicrosomal sample, the CYP3A4 content of both the recombinantmicrosomes and individual human liver microsomal samples weretaken into consideration. Shown as the dotted lines in figure1, the predicted values were similar to the observed values despitethe fact that there was more than a 7-fold interindividual differencein the CYP3A4 content of the human liver microsomal samples, whichsuggests that the intrinsic clearance in liver microsomes couldbe predicted with a reasonable accuracy from the correspondentrecombinant data.

Prediction of AUC or F_h of YM796 under the linear conditions in humans from in vitro metabolic data. To correlate the metabolic clearance determined in vitro with that in vivo, f_p and R_B of YM796 were determined. The f_p valueswere almost constant despite the concentrations, being 69.8, 70.2and 70.0% at 0.5, 50 and 2500 µM YM796, respectively. The R_B valueswere 1.10, 1.18 and 1.05 at 0.5, 50 and 2500 µM YM796, respectively,which showed no concentration dependence. The individual dataare summarized in table 1. The CL_{int, all} values obtained forthe 12 human liver microsomal samples were 0.94 ± 0.52 ml/min/gliver (mean ± S.D.). The predicted values of the AUC_oral of YM796corresponding to the aforementioned intrinsic clearances were19.0 ± 14.6 nmol · min/ml (n = 12), which were similar to theobserved values (20.2 ± 7.1 nmol · min/ml, n = 6) (tables 1 and3). The hepatic availabilities were also predicted to be 0.647± 0.152. The coefficient of variation was smaller for CL_int,
allper nanomole of CYP3A4 than that for CL_int,
all per gram of liver(table 1).

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TABLE 3
In vivo observed AUC_oral, predicted AUC_oral and bioavailability based on the in vitro metabolism data

	Discussion

Top Abstract Introduction Materials & Methods Results Discussion References

Eadie-Hofstee plots for the total metabolite formation of YM796 derived from each of the 12 different human liver microsomalsamples showed that multiple metabolic components were responsiblefor the YM796 metabolism. Thus, the following three models wereconsidered for the data fitting: i) one saturable and one nonsaturablecomponent (equation 11), ii) two saturable components (equation12) and iii) two saturable components and one nonsaturable component(equation 13).

v=Vmax<IT> · S/</IT>(<IT>Km+S</IT>)<IT>+</IT>CLns<IT> · S</IT> (11)

v=Vmax<IT>1</IT><IT> · S/</IT>(<IT>Km1+S</IT>)<IT>+V</IT>max<IT>2</IT><IT> · S/</IT>(<IT>Km2+S</IT>) (12)

(13)

When the data obtained with an arbitrary 3 of the 12 human liver microsomal samples (H-35, H-38 and H-62) were fitted tothe three models above, the mean and the standard deviation ofthe calculated Akaike's information criterion were $-$ 8.86 ± 1.83, $-$ 20.9 ± 2.6 and $-$ 23.0 ± 4.2, respectively, which indicates thatequation 13 gave the best fit of the data. Thus, the metabolismdata on YM796 were all analyzed based on the three-component model(equation 13) for each microsomal sample. The contribution of eachcomponent under the linear conditions was 80.4, 13.0 and 6.6%,respectively, with the high-affinity component being the mostimportant (table 1). Even if the data analysis was performedfor individual metabolites (M1 and M2), the contribution of eachcomponent was similar to that found in the total metabolites.The contribution of the high-affinity component was the most importantin all cases, and there were no marked differences in the K_m valuesamong the metabolites. In addition, the inhibition pattern ofM1 and M2 formation by antibodies to human CYP3A4/5 or by ketoconazolewas also very similar to that for the total metabolites, whichsuggests that the formation of the major YM796 metabolites ismediated predominantly by CYP3A4 as the metabolic reaction withalmost the same K_mvalues.

As shown in figure 3, a good correlation was observed between the CL_{int, all} and the CYP3A4 content of each of the 12 livermicrosomal samples, even though there was a greater than 7-folddifference in the interindividual variability in CYP3A4 content.Thus, a large interindividual variability in the capacity of drugmetabolism was suggested in humans. Factors which produce suchinterindividual variability can be classified into an intrinsiccomponent caused by genetic polymorphism, disease or enzyme-inductioncaused by smoking or other environmental factors and an extrinsiccomponent caused by a reduction in the metabolic activity duringstorage or the time to remove the liver from the body. It is veryimportant to discriminate between these two variability factors.If the variability is accounted for by the intrinsic rather thanextrinsic nature, the enzyme activity should be expected to correlatewell with the amount of antigen in a series of liver specimens.In this study, a good correlation was observed between the CL_int,
allof YM796 and the CYP3A4 content, which indicates that the variabilityin the metabolism of YM796 observed among the 12 liver microsomalsamples used might have been predominantly intrinsic in nature.Indeed, good correlations have been observed previously betweenthe CYP3A4 content and metabolic activity in human liver microsomesfor typical substrates of the enzyme such as nifedipine, testosteroneand lidocaine (Sesardic et al., 1988; Imaoka et al., 1990). Thummelet al. (1994) have reported that both the in vitro metabolic clearanceof midazolam estimated by use of S-13 samples prepared from liverbiopsies and the in vivo clearance of the same drug correlatewell with the CYP3A content of the individual livers, independentlyof any large interindividual variability in the metabolic clearance.Furthermore, the absolute values of both in vitro and in vivoclearances were also similar to each other. All of these resultssuggest that it is possible to predict the in vivo clearance ifthe amount of CYP isozyme responsible for the metabolism of adrug is known, and if the interindividual variability in the metabolicclearance is caused predominantly by intrinsic factors.

During development of a new drug, it is important to predict its bioavailability in humans. This is particularly true fordrugs exhibiting a nonlinear bioavailability, such as propranolol(Suzuki et al., 1974). It is also essential to predict nonlinearityat an early stage during the development of a drug because a nonlinearkinetic behavior can generally cause a large interindividual variationin its plasma concentrations. As a method for achieving this end,we proposed a method to predict in vivo clearance from in vitrokinetic parameters (K_m, V_max) (Iwatsubo et al., 1997). In thepresent study, we attempted to estimate AUC_oral of YM796 by predictingthe in vivo CL_oral from the in vitro metabolism data. In predictingthe in vivo CL_h, it is necessary to use a mathematical model todescribe drug concentrations in the liver in vivo. The most frequentlyused are the well-stirred model, parallel-tube model and dispersionmodel. It has been reported that there is little difference inthe predicted values of F_h and CL_h among the models as far aslow-clearance drugs are concerned, whereas pronounced differencesare seen among the models for high-clearance drugs, especiallyin F_h(Rane et al., 1977; Iwatsubo et al., 1997). Although YM796generally is a relatively low-clearance drug in humans, a largeinterindividual variability in the metabolic clearance is observedamong the liver samples. Therefore, in our study, we used thedispersion model which has been reported to predict the hepaticavailability and clearance accurately from in vitro data for manydrugs, despite the extent of clearance in rats (Roberts and Rowland,1986a, b; Sugiyama et al., 1988). Although the most appropriatevalue of D_N will not always be the same for all drugs and betweenrats and humans, a D_N of 0.17 was assumed in the present studybecause the in vivo intrinsic clearance of various types of drugknown to be metabolized by cytochrome P-450, which have been calculatedfrom the literature data involving in vivo pharmacokinetics basedon the dispersion model assuming this D_N value, was similar tothose calculated from in vitro metabolism data reported previously(Iwatsubo et al., 1997). The predicted values of AUC_oral at adose of 0.24 µmol/kg were 19.0 ± 14.6 nmol · min/ml (n = 12),which were similar to the observed values (20.2 ± 7.1 nmol · min/ml,n = 6) (tables 1 and 3). There were interindividual differences(35.1% variation) in the observed values of AUC_oral among thesubjects in vivo. Such interindividual differences have also beenshown for the AUC_oral values (76.8% variation) predicted fromindividual in vitro metabolic clearances (tables 1 and 3). Also,for CL_{int, all} per gram liver and the CYP3A4 content of each microsomalsample, similar variations (55.3% and 64.0%, respectively) wereobserved (table 1). When the CL_{int, all} was expressed per nanomoleof CYP3A4 by taking into account the CYP3A4 content of each livermicrosomal sample, the interindividual difference was greatlyreduced (table 1), which indicates that the interindividual differencein the predicted AUC_oral values would be attributable to a largeinterindividual variation in the CYP3A4 content of the liver used.Because 12 human livers with wide interindividual differencesin CYP3A4 contents were selected in the present study for examiningthe correlation between CYP3A4 contents and the metabolic activities,the results from only 12 livers may not be appropriate to discussthe interindividual variability. We therefore examined the CYP3A4contents and the variabilities with use of the randomly selected26 livers which had been stored at SRI. The mean ± S.D. of CYP3A4contents (n = 26) were 0.072 ± 0.038 nmol/mg MS protein (table3), and the coefficient of variation (52.8%) was smaller thanthat from 12 livers (table 1). These contents and variationswere similar to those (0.096 ± 0.051 nmol/mg MS protein and 53.1%)reported by Shimada et al. (1994) for 60 livers. We then attemptedto predict the mean ± S.D. of the AUC_oral value based on the CYP3A4contents thus obtained and the variation of 26 livers (table 3).In this prediction, the CL_{int, all} (0.275 ml/min/nmol CYP3A4)value obtained from 12 livers was used. The predicted AUC_oralvalue (16.8 ± 9.8) was similar to that (20.2 ± 7.1) obtained fromthe in vivo human study and the predicted variation (58.3%) becamecloser to the variation in vivo (35.1%) (table 3). These analysesindicate that the interindividual variation in CYP3A4 can causesuch large interindividual differences in the plasma concentrationsor AUC of YM796.

The present work demonstrates that it may be possible to predict the in vivo metabolic clearance from in vitro human livermicrosomal samples if the CYP isozyme(s) responsible for the metabolismof a drug is identified and its concentration in liver samplesis determined. In the same manner, for drugs which are substratestoward CYP isozyme(s) other than CYP3A4, previous reports suggestthat the metabolic activity of human liver microsomes correlateswell with the liver concentration of the CYP isozyme involved(Sesardic et al., 1988; Shimada et al., 1994; Goldstein et al.,1994). Hence, the method for predicting in vivo clearance usedin this study may also be applicable to isozyme(s) other thanCYP3A4 that are involved in the metabolic pathway(s) of a drug.Furthermore, it may also be possible to estimate the degree ofany intersubject differences in the plasma concentrations or AUCof a drug in vivo based on the range of interindividual variationin the intrinsic metabolic clearance or the liver concentrationof metabolic enzymes.

As shown in figure 7, biphasic metabolite formation kinetic values were observed for YM796 in the recombinant microsomes.One possible explanation for this phenomenon is that in the expressionprocess of CYP3A4, after the correspondent gene was transfectedinto the donor cells, two kinds of conformation were possiblewhere the distance of the binding site for the drug from the surfaceof the membrane of recombinant microsomes was different, resultingin multiplicity in the affinity of the enzyme for the drug. Consideringthat the high-affinity component was more important under linearconditions where YM796 concentrations were much lower than K_m1,and that the K_m value for the high-affinity component was similarto that obtained with human liver microsomal samples, the predictionof in vivo metabolic clearance from in vitro recombinant humanCYP isozymes as an alternative to human liver microsomes may bealso possible in some cases. As shown in figure 1, the predictedvalues for the metabolic clearance in human liver microsomes calculatedfrom kinetic data (K_m, V_max) in the recombinant CYP3A4 by reconcilingthe CYP3A4 content per gram liver were similar to the observedvalues, regardless of a large difference in the absolute CYP3A4content, which thus suggests the usefulness of the recombinantsystem for predicting metabolic clearance in human liver microsomes.This approach for predicting in vivo metabolic clearance fromin vitro metabolism data with human liver microsomes, therefore,may also be applicable to the prediction of in vivo clearancewith recombinant human CYP isozymes if the metabolism of the drugis almost completely caused by the particular isozyme, the variationin P-450 content of human liver is known and the experimentalconditions such as the amount of CYP reductase and cytochromeb₅ are carefully optimized to mimic the activity found in nativemicrosomes, as for YM796.

Attention should be paid to the following points, however, if the recombinant CYP3A4 is used for in vitro metabolism experiments.In the recombinant system, the amounts of enzymes such as CYPreductase and cytochrome b₅ differ from those found in human livers.In most cases, the amounts of these enzymes are less in the recombinantsystem. Therefore, it may be necessary to add these proteins tothe recombinant system to obtain the sufficient metabolic activity.For nifedipine and testosterone, which was used as a positivecontrol in this study, metabolic activity is markedly increasedby the addition of CYP reductase and cytochrome b₅(Nagata etal., 1990; Renaud et al., 1990). In contrast, as shown in figure8, the metabolism of YM796 was unaffected by external P-450 reductaseand cytochrome b₅, although the testosterone metabolism was influencedto a great extent. Thus, attention should be paid to whether themetabolic activity is affected or not by these added enzymes dependingon the substrate drugs used. Recently, a recombinant system expressingsufficient amounts of both CYP reductase and cytochrome b₅, aswell as CYP isozyme, has been developed. This recombinant systemis expected to be helpful in predicting not only metabolic clearancein human liver microsomes but also in vivo CL_h. However, YM796used in the present study is metabolized mostly by CYP3A4 in humansand similar experiments are expected to be carried out soon onseveral drugs to examine whether the prediction of in vivo metabolicclearance from in vitro data obtained by using recombinant humanP-450 isozymes is also possible when the object drug is metabolizedby P-450 isozymes other than CYP3A4 or when the drug is metabolizedby multiple P-450 isozymes, which is a very common situation.

In conclusion, the present study with YM796 as a model drug suggests that it may be possible to predict quantitatively thein vivo metabolic clearance of a target drug from in vitro metabolismexperiments with use of human liver microsomes. In addition, forsome drugs whose metabolism is mediated mainly by a particularhuman P-450 isozyme, like YM796, a recombinant human CYP isozymesystem may also be applicable for predicting in vivo metabolicclearance by taking into account the isozyme content of each liversample after the responsible isozyme is identified.

	Acknowledgments

The authors are most grateful to Drs. M. Murasaki and Y. Otani in Kitasato University School of Medicine for conducting theclinical study of YM796.

	Footnotes

Accepted for publication April 18, 1997.

Received for publication December 6, 1996.

Send reprint requests to: Yuichi Sugiyama, Ph.D., Faculty of Pharmaceutical Sciences, The University of Tokyo, 7-3-1, Hongo, Bunkyo-ku, Tokyo 113, Japan.

	Abbreviations

AUC_oral, area under the plasma concentration-time curve after oral administration; CL_h, hepatic clearance; CL_{int, all}, overall intrinsic metabolic clearance (intrinsic hepatic clearance); CL_ns, intrinsic metabolic clearance for the nonsaturable component; Cl_oral, oral clearance (= dose/AUC_oral); CL_r, renal clearance; CYP, cytochrome P-450; D_N, dispersion number; F_h, hepatic availability; f_p, unbound fraction in human plasma; K_{m, i}, Michaelis-Menten constant for the i-th component of the metabolic reaction; MS, microsomal; Q_h, hepatic blood flow rate; R_B, blood-to-plasma concentration ratio; V_{max, i}, maximal metabolic rate for the i-th component of the metabolic reaction; TLC, thin-layer chromatography; HPLC, high-performance liquid chromatography; GC, gas chromatography; MS-MS, tandem mass spectrometry.

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