Multispecific Organic Anion Transporter Is Responsible for the Biliary Excretion of the Camptothecin Derivative Irinotecan and its Metabolites in Rats

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Vol. 281, Issue 1, 304-314, 1997

Multispecific Organic Anion Transporter Is Responsible for the Biliary Excretion of the Camptothecin Derivative Irinotecan and its Metabolites in Rats¹

Xiao-Yan Chu, Yukio Kato, Kayoko Niinuma, Ken-Ichi Sudo, Hideo Hakusui and Yuichi Sugiyama

Faculty of Pharmaceutical Sciences, University of Tokyo, Tokyo, Japan (X.-Y.C., Y.K., K.N., Y.S.), and Drug Metabolism and Analytical Chemistry Research Center, Developmental Research Laboratories, Daiichi Pharmaceutical Co., Ltd., Tokyo, Japan (K.-I.S., H.H.)

	Abstract

Top Abstract Introduction Materials & Methods Results Discussion References

Irinotecan, 7-ethyl-10-[4-(1-piperidino)-1-piperidino]-carbonyloxycamptothecin (CPT-11), is a potent anticancer drug thatis increasingly used in chemotherapy. A frequent limiting sideeffect involves gastrointestinal toxicity (diarrhea), which isthought to be related to the biliary excretion of CPT-11 and itsmetabolites. Accordingly, the biliary excretion mechanisms forboth the lactone and carboxylate forms of CPT-11 and its metabolites,SN-38 and its glucuronide (SN38-Glu), were investigated usingSprague-Dawley (SD) rats and Eisai hyperbilirubinemic rats (EHBR),with the latter being mutant rats with a genetic deficiency ofthe canalicular multispecific organic anion transporter. Afteri.v. administration of CPT-11, the biliary excretion clearance,defined as the biliary excretion rate normalized to the hepaticconcentration, of both the lactone and carboxylate forms of SN38-Gluwas much lower in EHBR. The biliary excretion clearance for thecarboxylate form of both CPT-11 and SN-38 was also substantiallysmaller in EHBR and showed marked saturation with increasing doseonly in SD rats. On the other hand, the biliary excretion clearancefor the lactone forms of CPT-11 and SN-38 showed only a minimaldifference in EHBR, compared with SD rats. These results suggestthat, for the carboxylate form of CPT-11 and SN-38 and the carboxylateand lactone forms of SN38-Glu, there exists a specific transportsystem at the bile canalicular membrane that is deficient in EHBR.To confirm this hypothesis, the uptake of these substrates byisolated hepatic canalicular membrane vesicles (CMV) was examined.ATP-dependence was clearly observed for the uptake of these fourcompounds by CMV prepared from SD rats but not by CMV from EHBR.In addition, the compounds inhibited the ATP-dependent uptakeof S-(2,4-dinitrophenyl) glutathione by CMV from SD rats, in aconcentration-dependent manner. These results suggest that thebiliary excretion of the carboxylate forms of CPT-11 and SN-38and the carboxylate and lactone forms of SN38-Glu is mediatedby the multispecific organic anion transporter, which is deficientin EHBR.

	Introduction

Top Abstract Introduction Materials & Methods Results Discussion References

CPT, a plant alkaloid isolated from a tree found in China (Camptotheca accuminata), is a novel antitumor agent that exertsits activity exclusively by inhibition of topoisomerase I (Kimet al., 1992; Slichenmyer et al., 1993; Tanizawa et al., 1994).However, clinical evaluation of CPT was discontinued due to itsunpredictably severe toxicity and poor water-solubility. Recently,several semisynthetic analogs of CPT have been developed (Miyasakaet al., 1981; Nagata, et al., 1987). Irinotecan (CPT-11) is awater-soluble analog of CPT that was discovered in an attemptto identify derivatives with greater water-solubility and antitumoractivity than CPT (Hertzberg et al., 1989). CPT-11 acts as a prodrugthat undergoes deesterification in vivo to yield SN-38, a metabolitethat is 1000-fold more potent than the parent compound in vitro(Kawato et al., 1991; Kojima et al., 1993).

CPT-11 shows potent anticancer activity in many types of human tumor cells, including small-cell and non-small-cell lung cancers,malignant lymphoma, cervical cancer, ovarian cancer and colorectalcancer (Ohno et al., 1990; Negoro et al., 1991; Sasaki et al.,1995a). It has undergone phase I and II clinical trials in severalcountries. The major toxic effects of CPT-11 are myelosuppressionand gastrointestinal toxicity, especially unpredictable, severediarrhea (Araki et al., 1993). Such intestinal toxicity, however,exhibits large interpatient variability (Rothenberg et al., 1993;Rowinsky et al., 1994; Sasaki et al., 1995b), the mechanisms forwhich are currently unknown. One postulated mechanism for thetoxicity of CPT-11 is related to the biliary excretion of itsmetabolites. After the administration of CPT-11, the active metaboliteSN-38 is formed by deesterification. SN-38 is further conjugatedto SN38-Glu in the liver and mainly excreted via the bile duct,followed by deconjugation by intestinal microflora to regenerateSN-38, which may cause diarrhea (Kaneda et al., 1990). However,the biliary excretion mechanism of CPT-11 and its metaboliteshas not been identified.

CPT-11 and its metabolites have an $alpha$ -hydroxy- $delta$ -lactone ring, which undergoes reversible hydrolysis at a rate that dependson many factors, including pH, ionic strength and protein concentration(Fassberg and Stella, 1992; Burke and Mi, 1994; Rivory and Robert,1994) (fig. 1). The lactone form is essential for the activityof SN-38, and the lactone-hydrolyzed form (carboxylate form) exhibitsonly minimal topoisomerase I-inhibitory activity (Slichenmyeret al., 1993). At physiological pH, however, the lactone formis unstable and the equilibrium favors hydrolysis to open thelactone ring and yield the carboxylate form. Under acidic conditions,the reverse reaction, with formation of the lactone, is favored.Similar reactions also occur with CPT-11 and SN38-Glu (fig. 1).Among these six compounds, anionic charges are present on thecarboxylate forms of CPT-11 and SN-38 and the carboxylate andlactone forms of SN38-Glu. Recently, it has been proposed thatthe hepatic cMOAT, which is expressed on the bile canalicularmembrane, transports several types of organic anions into thebile as a primary active transport system (Ishikawa et al., 1990;Nishida et al., 1992; Sathirakul et al., 1993, 1994; Shimamuraet al., 1994; Pikula et al., 1994; Yamazaki et al., 1996). Therefore,the four CPT-11-related compounds with an anionic charge may berecognized by the cMOAT. In this study, the biliary excretionmechanisms of both the carboxylate and lactone forms of CPT-11and its metabolites were investigated in rats. EHBR derived fromSD rats were used for this purpose; EHBR are genetically deficientwith respect to cMOAT on the bile canalicular membrane (Fernandez-Checaet al., 1992; Takenaka et al., 1995a). The biliary excretion ofCPT-11 and its metabolites was compared in SD rats and EHBR invivo. The isolated bile CMV from SD rats and EHBR were also usedfor the transport study of CPT-11 and its metabolites.

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Fig. 1. Chemical structures of the lactone and carboxylate forms of CPT-11 and its metabolites SN-38 and SN38-Glu.

	Materials and Methods

Top Abstract Introduction Materials & Methods Results Discussion References

Materials

CPT-11, SN-38 and SN38-Glu were obtained from Daiichi Pharmaceutical Co. Ltd. (Tokyo, Japan) and the Yakult Honsha Co. Ltd.(Tokyo, Japan). The lactone and carboxylate forms of CPT-11, SN-38and SN38-Glu were produced by dissolving the compounds in 50 mMphosphate buffer at pH 3.0 or 9.0 and leaving them overnight.The conversion of the lactones into carboxylates or carboxylatesinto lactones was virtually complete (>99%), as determined byHPLC. CPT, as an internal standard, was obtained from Sigma ChemicalCo. (St. Louis, MO). [³H]DNP-SG (50.0 µCi/nmol) was synthesized according to the methoddescribed previously (Kobayashi et al., 1990). All other chemicalswere commercial products and of analytical grade. Male SD ratsweighing 250 to 300 g were purchased from Nisseizai (Tokyo, Japan),and male EHBR weighing 250 to 300 g were supplied by Eisai Laboratories(Gifu, Japan).

In Vivo Study

The SD rats and EHBR underwent cannulation of the femoral vein and artery using PE50 polyethylene tubing (inner diameter,0.58 mm; outer diameter, 0.965 mm; Becton Dickinson & Co., Parsippany,NJ), and the bile duct was cannulated with PE10 polyethylene tubing(inner diameter, 0.28 mm; outer diameter, 0.61 mm; Becton Dickinson)under light anesthesia with ether. After the operation, the ratswere kept in Bollman cages, with free access to food and water.The temperatures of the rats were monitored and found to remainconstant during the experiment. CPT-11 was dissolved in distilledwater with sonication and then diluted with 9% NaCl to give afinal NaCl concentration of 0.9%. After i.v. injection of 10 or40 mg/kg levels of the lactone form of CPT-11 (1 ml/250 g b.wt.),approximately 0.5 ml of blood was collected at 5 min, 30 min,2 hr, 4 hr and 8 hr, transferred to centrifuge tubes containing5 µl of 10 mM diisopropyl fluorophosphate dissolved in dimethylsulfoxide,kept on ice during the sampling period and finally centrifugedat 4°C. The plasma (0.2 ml) obtained was frozen under liquid N₂immediately after harvesting. Bile samples were collected at 0to 1, 1 to 2, 2 to 4, 4 to 6 and 6 to 8 hr; urine samples werecollected spontaneously. To avoid conversion of the lactone andcarboxylate forms of CPT-11 and its metabolites during sampling,bile and urine samples were collected every 2 hr, kept on iceduring sampling and frozen immediately in liquid N₂ when samplingwas complete. At 8 hr, the rats were sacrificed, and the liverswere removed and immediately frozen in liquid N₂. Concentrationsof both the lactone and carboxylate forms of CPT-11 and its metaboliteswere determined by HPLC, as described below. The urine samplesobtained up to 8 hr were combined, and the total volume was determinedbefore HPLC determination.

In Vitro Uptake by CMV

CMV were prepared from male SD rats and EHBR as described previously (Kobayashi et al., 1990). The CMV were resuspended in250 mM sucrose containing 50 mM Tris-HCl (pH 7.4), frozen in liquidN₂ and stored at $-$ 100°C until use. The purity of the preparedCMV was evaluated by determining the activities of Mg⁺⁺-ATPase and alkaline phosphatase, according to the methods ofScharschmidt et al. (1979) and Yachi et al. (1989), respectively.The activity of prepared CMV was also checked by measuring theATP-dependent uptake of standard substrates, [³H]taurocholate (1 µM) and [³H]DNP-SG (1 µM; 0.1 µM labeled and 0.9 µM unlabeled), at 37°Cfor 2 min.

Uptake of the carboxylate and lactone forms of CPT-11 and its metabolites. The incubation medium for the uptake studies contained 0.25 M sucrose, 10 mM Tris-HCl (pH 7.4), 10 mM MgCl₂, 5 mM ATP, 10mM creatine phosphate and 100 µg/ml creatine phosphokinase. Controlexperiments were performed without the addition of ATP. The uptakestudy was performed at 37°C. After preincubation for 2 min, 5µl of the carboxylate or lactone form of CPT-11 or its metabolites,which had been diluted with incubation medium to give a finalpH of 7.4, was added to give a final ligand concentration of 50µM. After preincubation for an additional 1 min, uptake was startedby the addition of vesicles to give a final protein concentrationof 1 mg/ml; the final incubation volume was 20 µl. At designatedtimes, transport was terminated by addition of 1 ml of ice-coldstop solution, followed immediately by filtration through premoistened0.45-µm HA Millipore filters (catalog no. HAWP 02500; MilliporeCorp., Bedford, MA), which were subsequently washed twice withan additional 5.0 ml of ice-cold stop solution. The stop solutioncontained 10 mM Tris-HCl (pH 7.4), 0.25 M sucrose and 0.1 M NaCl.Filters were dried, cut into small pieces and frozen immediatelyunder liquid N₂ for HPLC analysis. The nonspecific binding ofdrugs to the filters was also determined without CMV, and valuesfor the CMV uptake were obtained by subtracting this nonspecificbinding from the apparent uptake. Such nonspecific binding tothe filter, normalized by the protein amount in the equivalentvolume of incubation mixture with CMV, was 927 ± 57 and 893 ±50 pmol/mg protein for the lactone form of CPT-11 in the presenceand absence of ATP; 582 ± 9 and 554 ± 35 pmol/mg protein for thecarboxylate form of CPT-11 in the presence and absence of ATP;10.8 ± 5.5 and 9.09 ± 3.63 pmol/mg protein for the carboxylateform of SN-38 in the presence and absence of ATP; 19.5 ± 2.8 and22.1 ± 0.7 pmol/mg protein for the lactone form of SN38-Glu inthe presence and absence of ATP; 11.7 ± 0.9 and 12.4 ± 1.4 pmol/mgprotein for the carboxylate form of SN38-Glu in the presence andabsence of ATP; and 2.57 ± 0.55 and 2.47 ± 0.31 pmol/mg proteinfor [³H]DNP-SG in the presence and absence of ATP.

Effect of the lactone and carboxylate forms of CPT-11 and its metabolites on the uptake of [³H]DNP-SG. For transport studies involving the effect of the lactone and carboxylate forms of CPT-11 and its metabolites on the uptakeof [³H]DNP-SG, 1.0 µM [³H]DNP-SG was used. After preincubation at 37°C for 2 min, theinhibitor was added and a further preincubation for 1 min wasallowed. Inhibitor concentrations used were 0.03, 0.1, 0.3, 1,10 and 500 µM for the lactone and carboxylate forms of SN38-Glu;1, 50 and 500 µM for the lactone form of CPT-11; 0.3, 1, 10, 30,50 and 500 µM for the carboxylate form of CPT-11; and 1, 10, 30,50 and 500 µM for the carboxylate form of SN-38. After preincubation,the CMV obtained from SD rats was added to give a final proteinconcentration of 0.5 mg/ml. The final incubation volume was 20µl. After incubation for 2 min, the reaction was terminated asdescribed above. Radioactivity retained on the filter was determinedusing a liquid scintillation counter.

HPLC Analysis

The analysis of the carboxylate and lactone forms of CPT-11 and its metabolites was accomplished by HPLC, as described previously(Rivory and Robert, 1994; Sasaki et al., 1995b), with a modificationthat permitted the simultaneous determination of CPT-11, SN-38and SN38-Glu. Briefly, for the analysis of plasma samples, 50µl of ice-cold 50 mM phosphate buffer (pH 6.0) was added to 200µl of plasma, followed by the addition of 50 µl of the ice-coldlactone form of CPT, as an internal standard, and 450 µl of methanol.The mixture was vortex-mixed for 10 sec and centrifuged at 4°Cfor 5 min. Then 70 µl of 50 mM phosphate buffer (pH 6.0) was addedto 100 µl of supernatant, and the mixture was injected immediatelyonto the HPLC column, followed by determination of only the lactoneforms, because of large interference peaks around the retentiontimes of the carboxylate forms. Total (sum of lactone and carboxylateforms) drug was determined as the lactone in the same manner,except that 70 µl of 0.3 M HCl was added instead of 50 mM phosphatebuffer, to ensure complete lactonization of the drug. The carboxylateform of the drug was determined by subtraction of the lactoneform from the total drug concentration. Bile and urine sampleswere diluted with 50 mM phosphate buffer (pH 6.0), and liver samples(0.5 g) were homogenized with 3 ml of methanol/50 mM phosphatebuffer (pH 6.0) (7:3, v/v) for the analysis of the lactone andtotal concentrations in the same way. Because there were no interferingpeaks in the samples from the in vitro CMV uptake study, the lactoneand carboxylate forms of the drugs were determined simultaneouslyby using the method for the lactone form determination describedabove. In the uptake study, the conversion of the lactone andcarboxylate forms of the drug on the filter and in the mediumduring the experiment was <5%, as determined by HPLC. Therefore,only the total concentration of drugs was determined when analyzingfilter and medium samples. Briefly, for the analysis of filtersamples, 250 µl of ice-cold 50 mM phosphate buffer (pH 6.0) wasadded to the filter, followed by 50 µl of the ice-cold lactoneform of CPT, as an internal standard, and 450 µl of methanol.The mixture was vortex-mixed for 1.5 min, to extract the drugson the filter, and was centrifuged at 4°C for 5 min. Then, 70µl of 0.3 M HCl was added to 100 µl of supernatant, and the mixture(50 µl) was injected onto the HPLC column, followed by determinationof only the total form of the drugs. The medium samples were dilutedwith 50 mM phosphate buffer (pH 6.0) to give a total volume of250 µl, followed by the addition of 50 µl of the ice-cold lactoneform of internal standard and 450 µl of methanol. The mixturewas vortex-mixed for 10 sec and centrifuged at 4°C for 5 min.Then, 70 µl of 0.3 M HCl was added to 100 µl of supernatant, andthe mixture was injected onto the HPLC column for drug determination.

The HPLC system consisted of an Hitachi L-6300 pump, a Tosoh TSK Gel ODS-80Ts (150 × 4.6 mm inner diameter) column with aTSK Guardgel ODS-80Ts guard column, an Hitachi AS-4000 autosamplerand an Hitachi F-1050 fluorescence detector. The excitation andemission settings for the in vivo analysis were 375 and 545 nm,respectively. The limits of detection, in terms of the amountof sample injected onto the HPLC column, were 0.2, 0.03 and 0.4pmol for the lactone forms of CPT-11, SN-38 and SN38-Glu, respectively.In the CMV uptake study, the excitation and emission settingswere 370 and 430 nm for CPT-11 and SN38-Glu and 380 and 556 nmfor SN-38, respectively. The limits of detection were 0.0074,0.01 and 0.0044 pmol for the lactone forms of CPT-11, SN-38 andSN38-Glu, respectively. The operation of the HPLC system was controlledby an Hitachi D-6100 HPLC manager. The mobile phase consistedof solvent A of acetonitrile/tetrahydrofuran/0.9 mM 1-heptanesulfonicacid sodium salt in 50 mM phosphate buffer (pH 6.0) (8:4:88) andsolvent B of acetonitrile/5 mM 1-heptanesulfonic acid sodium saltin 50 mM phosphate buffer (pH 6.0) (30:70). The total elutiontime was 22 min, with 100% solvent A from 0 to 7 min, 100% solventB from 7.1 to 16 min and 100% solvent A from 16.1 to 22 min. Theflow rate was 0.9 ml/min.

Data Analysis

The AUC_(0-8hr) for the lactone and carboxylate forms of CPT-11 and its metabolites was calculated by the trapezoidalrule. CL_bile,p was calculated from the following equation:

CLbile,p<IT>=X</IT>bile(0-8hr)<IT>/</IT>AUC(<IT>0–8</IT>hr) (1)

where X_bile(0-8hr) is the cumulative amount excreted into bile over 0 to 8 hr. CL_bile,h, defined as biliary excretionrate divided by the hepatic concentration of the drug, was calculatedfrom the following equation:

CLbile,h<IT>=V</IT>bile(<IT>8</IT>hr)<IT>/X</IT>liver(<IT>8</IT>hr) (2)

where V_bile(8hr) and X_liver(8hr) are the biliary excretion rate and hepatic concentration at 8 hr, with dimensions of milligramper minute per kilogram and milligram per gram of liver, respectively.V_bile(8hr) was approximated by the following equation:

Vbile(<IT>8</IT>hr)<IT>≅X</IT>bile(<IT>6–8</IT>hr)<IT>/120 </IT>min (3)

where X_bile(6-8hr) is the amount of drug excreted into the bile duct from 6 to 8 hr. Thus, the CL_bile,h calculatedhas the dimensions of grams of liver per minute per kilogram.It was assumed that 1 g of liver is equivalent to 1 ml and, therefore,the CL_bile,h has the dimensions of milliliter per minute per kilogram.

C_bile/C_liver was calculated from the following equation:

Cbile<IT>/C</IT>liver<IT>=C</IT>bile(<IT>8</IT>hr)<IT>/X</IT>liver(<IT>8</IT>hr) (4)

where C_bile(8hr) is the drug concentration in bile at 8 hr and approximated by the following equation:

Cbile(<IT>8</IT>hr)<IT>≅C</IT>bile(<IT>6–8</IT>hr)<IT>=V</IT>bile(<IT>6–8</IT>hr)<IT>/Q</IT>bile(<IT>6–8</IT>hr) (5)

where V_bile(6-8hr) is the rate of drug excreted into the bile duct from 6 to 8 hr. Q_bile(6-8hr) is the bile flowrate from 6 to 8 hr.

The CL_r was calculated from

CLr<IT>=X</IT>urine(<IT>0–8</IT>hr)<IT>/</IT>AUC(<IT>0–8</IT>hr) (6)

where X_urine(0-8hr) is the cumulative amount excreted into urine from 0 to 8 hr.

The inhibition constant (K_i) values for evaluating the inhibitory effect of CPT-11 and its metabolites on the uptake of [³H]DNP-SG by CMV from SD rats were obtained by fitting the followingequation to the data:

V(+I)<IT>/V</IT>(−I)<IT>=1/1+</IT>(<IT>I/K</IT><IT>i</IT>) (7)

where V_(+I) and V_(I) represent the transport velocity in the presence and absence of inhibitor, respectively;I is the inhibitor concentration. This equation was derived basedon the assumption of competitive inhibition and the fact thatthe [³H]DNP-SG concentration (1 µM) is much lower than the K_m value(71 µM) (Akerboom et al., 1991) for DNP-SG uptake.

Statistical Method

The results are shown as means ± S.E. for the number of determinations. Dunnett's test was used to determine the significanceof differences between the means of two groups, with P < .01 andP < .05 as the minimum levels of significance.

	Results

Top Abstract Introduction Materials & Methods Results Discussion References

Plasma concentration-time profiles of CPT-11 and its metabolites. The plasma concentration-time profiles for the lactone and carboxylate forms of CPT-11, SN-38 and SN38-Glu after i.v. injectionof the lactone form of CPT-11 to SD rats and EHBR are shown infigures 2, 3 and 4, respectively. In the time period immediatelyafter i.v. injection, CPT-11 was mainly present in plasma as thelactone form in both SD rats and EHBR; subsequently, the carboxylateform of CPT-11 appeared gradually in plasma (fig. 2). In SD rats,the AUC_(0-8hr) of the lactone form of CPT-11 exhibited nonlinearitywith increasing dose, whereas minimal saturation could be observedin EHBR (table 1). The plasma concentration of the active metaboliteSN-38 was much lower than that of the parent drug CPT-11 (fig.3). Similarly, with CPT-11, the carboxylate form of SN-38 appearedgradually in plasma with time (fig. 3). At a dose of 10 mg/kg,the disappearance of the carboxylate form of SN-38 in plasma ofSD rats was much faster than in EHBR, whereas the difference inthe disappearance curve of the carboxylate form of SN-38 was minimalat 40 mg/kg for the SD and EHBR strains (fig. 3). The AUC_(0-8hr)for the carboxylate form of SN-38 differed markedly between SDrats and EHBR (0.0474 ± 0.0081 µg·hr/ml and 0.339 ± 0.078 µg·hr/mlfor SD rats and EHBR, respectively) at 10 mg/kg but was very similarfor the two strains at 40 mg/kg (0.249 ± 0.064 µg·hr/ml and 0.245± 0.060 µg·hr/ml for SD rats and EHBR, respectively) (table 2).The plasma disappearance of both the lactone and carboxylate formsof SN38-Glu was also slower in EHBR at 10 mg/kg, compared withthat in SD rats (fig. 4). On the other hand, at the higher dose(40 mg/kg), similar concentration-time profiles were obtainedfor both the carboxylate and lactone forms of SN38-Glu with eachstrain (fig. 4). The difference in AUC_(0-8hr) for both thecarboxylate and lactone forms of SN38-Glu between SD rats andEHBR was much more marked at the lower dose (10 mg/kg) than atthe higher dose (40 mg/kg) (table 3).

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Fig. 2. Plasma concentration-time curves for the lactone (A and B) and carboxylate (C and D) forms of CPT-11 after i.v. administrationof the lactone form of CPT-11 (10 and 40 mg/kg) in SD rats (Aand C) and EHBR (B and D) with bile cannulation. Each data pointrepresents the mean ± S.E. of three different rats. $black-square$ , lactoneform at 10 mg/kg; $square$ , carboxylate form at 10 mg/kg; $bullet$ , lactoneform at 40 mg/kg; $open circle$ , carboxylate form at 40 mg/kg.

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Fig. 3. Plasma concentration-time curves for the lactone (A and B) and carboxylate (C and D) forms of SN-38 after i.v. administrationof the lactone form of CPT-11 (10 and 40 mg/kg) in SD rats (Aand C) and EHBR (B and D) with bile cannulation. Each data pointrepresents the mean ± S.E. of three different rats. $black-square$ , lactoneform at 10 mg/kg; $square$ , carboxylate form at 10 mg/kg; $bullet$ , lactoneform at 40 mg/kg; $open circle$ , carboxylate form at 40 mg/kg.

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Fig. 4. Plasma concentration-time curves for the lactone (A and B) and carboxylate (C and D) forms of SN38-Glu after i.v. administrationof the lactone form of CPT-11 (10 and 40 mg/kg) in SD rats (Aand C) and EHBR (B and D) with bile cannulation. Each data pointrepresents the mean ± S.E. of three different rats. $black-square$ , lactoneform at 10 mg/kg; $square$ , carboxylate form at 10 mg/kg; $bullet$ , lactoneform at 40 mg/kg; $open circle$ , carboxylate form at 40 mg/kg.

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TABLE 1
Pharmacokinetic parameters of lactone and carboxylate forms of CPT-11 after i.v. administration of CPT-11 (10 and 40 mg/kg)in SD rats and EHBR
All values are given as the mean ± S.E. of three different experiments.

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TABLE 2
Pharmacokinetic parameters of lactone and carboxylate forms of SN-38 after i.v. administration of CPT-11 (10 and 40 mg/kg)in SD rats and EHBR
All values are given as the mean ± S.E. of three different experiments.

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TABLE 3
Pharmacokinetic parameters of lactone and carboxylate forms of SN38-Glu after i.v. administration of CPT-11 (10 and 40 mg/kg)in SD rats and EHBR
All values are given as the mean ± S.E. of three different experiments.

Biliary excretion of CPT-11 and its metabolites. The biliary excretion of CPT-11 and its metabolites was measured up to 8 hr in SD rats and EHBR after i.v. injection of thelactone form of CPT-11 (figs. 5 and 6). The bile flow rate wasnot significantly affected by i.v. injection of CPT-11 in eitherSD rats or EHBR. The pharmacokinetic parameters obtained are listedin tables 1, 2 and 3. For the carboxylate form of CPT-11, withincreasing dose, clear saturation of biliary excretion was observedin SD rats, whereas no apparent saturation was found in the EHBR(fig. 5, C and D). As for the lactone form of CPT-11, saturationwas also observed but in both SD rats and EHBR (fig. 5, A andB). As shown in figure 6, SN-38 was mainly excreted into bileas the carboxylate form both in SD rats and EHBR. The cumulativeamount of the carboxylate form of SN-38 excreted into bile exhibitedalmost no change even with increasing dose in SD rats (table 2),showing a clear saturation. On the other hand, such nonlinearitywas not observed in EHBR (table 2). In SD rats, clear saturationof biliary excretion for both the lactone and carboxylate formsof SN38-Glu was observed with increasing dose (fig. 6). On theother hand, in EHBR, the biliary excretion of the lactone andcarboxylate forms of SN38-Glu was not so clear, compared withSD rats (fig. 6).

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Fig. 5. Biliary excretion of the lactone (A and B) and carboxylate (C and D) forms of CPT-11 after i.v. administration of CPT-11 (10and 40 mg/kg) in SD rats (A and C) and EHBR (B and D). Each datapoint represents the mean ± S.E. of three different rats. $black-square$ , lactoneform at 10 mg/kg; $square$ , carboxylate form at 10 mg/kg; $bullet$ , lactoneform at 40 mg/kg; $open circle$ , carboxylate form at 40 mg/kg.

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Fig. 6. Biliary excretion of the lactone (A and B) and carboxylate (C and D) forms of SN-38 and SN38-Glu after i.v. administrationof the lactone form of CPT-11 (10 and 40 mg/kg) in SD rats (Aand C) and EHBR (B and D). Each data point represents the mean± S.E. of three different rats. $black-square$ , lactone form of SN-38 at 10mg/kg; $square$ , carboxylate form of SN-38 at 10 mg/kg; $bullet$ , lactone formof SN-38 at 40 mg/kg; $open circle$ , carboxylate form of SN-38 at 40 mg/kg; $black-diamond$ , lactone form of SN38-Glu at 10 mg/kg; $diamond$ , carboxylate form ofSN38-Glu at 10 mg/kg; $black-triangle$ , lactone form of SN38-Glu at 40 mg/kg; $triangle$ , carboxylate form of SN38-Glu at 40 mg/kg.

Estimation of CL_bile,p and CL_bile,h. The CL_bile,p value of both the lactone and carboxylate forms of CPT-11 exhibited nonlinearity in SD rats. Moreover, the saturationof CL_bile,p for the carboxylate form of CPT-11 was more markedthan that of the lactone form (table 1). In contrast, no clearsaturation could be observed for CL_bile,p of the lactone or carboxylateform of CPT-11 in EHBR. The CL_bile,h was reduced for the carboxylateform of CPT-11 as the dose increased only in SD rats; no nonlinearitycould be observed in EHBR. The reduction in CL_bile,h for the lactoneform of CPT-11 was minimal with increasing dose in both SD ratsand EHBR. The absolute value of the CL_bile,h for the carboxylateform of CPT-11 was much larger than that of the lactone form inSD rats, especially at the lower dose (10 mg/kg). In addition,at 10 mg/kg, the CL_bile,h of the carboxylate form of CPT-11 inSD rats was larger than that in EHBR; at the higher dose, thedifference was smaller (table 1). Similar results were also observedfor the CL_bile,p and CL_bile,h of SN-38 (table 2). A reductionin CL_bile,h with increasing dose was not observed for the lactoneform of SN-38 but was present for the carboxylate form in SD rats.The CL_bile,h value for the carboxylate form of SN-38 was largerin SD rats than in EHBR, especially at the lower dose. In contrast,no marked difference was found for the lactone form of SN-38 inCL_bile,h between SD rats and EHBR (table 2). For SN38-Glu, theCL_bile,h value of both the lactone and carboxylate forms was clearlylower in EHBR than in SD rats. In SD rats, the CL_bile,h valueof the carboxylate form was larger than that of the lactone format 10 mg/kg, and saturation was more marked for the carboxylateform than for the lactone form (table 3).

The C_bile/C_liver of the carboxylate forms of CPT-11, SN-38 and SN38-Glu in SD rats showed obvious saturation when the dosewas increased from 10 mg/kg to 40 mg/kg; on the other hand, thiswas not the case for the lactone forms (tables 1, 2 and 3).In addition, the C_bile/C_liver of the carboxylate forms of CPT-11,SN-38 and SN38-Glu and the lactone form of SN38-Glu in EHBR ata dose of 10 mg/kg was significantly lower than that in SD rats(tables 1, 2 and 3).

Urinary excretion of CPT-11 and its metabolites. Nonlinearity was observed in the CL_r of the carboxylate forms of CPT-11, SN-38 and SN38-Glu only in SD rats, whereas no clearsaturation in the CL_r could be observed for those compounds inEHBR. In addition, the lactone forms of CPT-11, SN-38 and SN38-Glushowed a minimal reduction in CL_r with increasing dose in bothSD rats and EHBR (tables 1, 2 and 3).

Characterization of CMV. The Mg⁺⁺-ATPase enrichment factor was 67.6 ± 9.1 (mean ± S.E., n = 3) and 72.7 (mean value, n = 2) in CMV from SD rats and EHBR,respectively, compared with the corresponding activity in liverhomogenate. The alkaline phosphatase enrichment factor was 80.9± 7.8 (mean ± S.E., n = 3) and 76.4 (mean value, n = 2) in SDrats and EHBR, respectively. The ATP-dependent uptake of [³H]taurocholate was 186 ± 2 and 153 ± 10 pmol/2 min/mg protein(mean ± S.E. of three different experiments) and that of [³H]DNP-SG was 178 ± 19 and 0.1 pmol/2 min/mg protein in SD ratsand EHBR, respectively.

Study of uptake of CPT-11 and its metabolites by CMV from SD rats and EHBR. The uptake by CMV from SD rats was markedly stimulated by ATP for the carboxylate and lactone forms of SN38-Glu and the carboxylateforms of CPT-11 and SN-38 (fig. 7). The uptake showed linearityover at least 2 min. No ATP-dependence was found in the uptakeof the lactone form of CPT-11. Due to the low solubility of thelactone form of SN-38 and the detection limit for SN-38 (approximately0.01 pmol), uptake of the lactone form of SN-38 could not be determined.The uptake by CMV prepared from EHBR was also examined (fig. 8).Compared with SD rats, the ATP-dependent uptake by CMV from EHBRwas greatly impaired in the case of the lactone and carboxylateforms of SN38-Glu and the carboxylate forms of CPT-11 and SN-38.A minimal ATP-dependence was found for the uptake of the lactoneform of CPT-11 by CMV from EHBR.

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Fig. 7. ATP-dependent uptake of the lactone and carboxylate forms of CPT-11 and its metabolites by CMV obtained from SD rats. CMVwere incubated in the presence of ligand (50 µM) with ( $black-square$ ) or without( $square$ ) ATP (5 mM) and an ATP-regenerating system. Data are means± S.E. of three preparations. A, lactone form of SN38-Glu; B,carboxylate form of SN38-Glu; C, lactone form of CPT-11; D, carboxylateform of CPT-11; E, carboxylate form of SN-38.

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Fig. 8. ATP-dependent uptake of the lactone and carboxylate forms of CPT-11 and its metabolites by CMV obtained from SD rats (A) andEHBR (B). CMV were incubated in the presence of substrate (50µM) with ( $black-square$ ) or without ( $square$ ) ATP (5 mM) and an ATP-regeneratingsystem. The uptake time was 2 min.

, ATP-dependent uptake foreach compound. Data are means ± S.E. of three preparations. *P< .05, **P < .01 for the difference in uptake between SD ratsand EHBR, by Dunnett's test.

Effect of the lactone and carboxylate forms of CPT-11 and its metabolites on the uptake of [³H]DNP-SG by CMV from SD rats. The effects of the lactone and carboxylate forms of CPT-11 and its metabolites on the ATP-dependent uptake of [³H]DNP-SG are shown in figure 9. DNP-SG uptake was significantlyinhibited by the carboxylate and lactone forms of SN38-Glu andthe carboxylate forms of SN-38 and CPT-11, whereas the lactoneform of CPT-11 had little effect on the uptake of DNP-SG (fig.9). The K_i values were 1.03 ± 0.05, 1.62 ± 0.05, 18.3 ± 3.6 and96.6 ± 8.4 µM for the carboxylate form of SN38-Glu, the lactoneform of SN38-Glu and the carboxylate forms of SN-38 and CPT-11,respectively.

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Fig. 9. Effect of the carboxylate and lactone forms of CPT-11 and its metabolites on ATP-dependent uptake of [³H]DNP-SG (1 µM) by CMV obtained from SD rats. Data are means ±S.E. of three preparations. $square$ , lactone form of CPT-11; $black-square$ , carboxylateform of CPT-11 (K_i = 96.6 ± 8.4 µM); $open circle$ , carboxylate form of SN-38(K_i = 18.3 ± 3.6 µM); $bullet$ , carboxylate form of SN38-Glu (K_i = 1.03± 0.05 µM); $black-triangle$ , lactone form of SN38-Glu (K_i = 1.62 ± 0.05 µM).

	Discussion

Top Abstract Introduction Materials & Methods Results Discussion References

Although CPT-11 is a potent and novel anticancer drug, a severe side effect (diarrhea) has been observed in some patientsduring its clinical use. To understand the mechanism for thisside effect, it is important to clarify the pharmacokinetics ofCPT-11. The pharmacokinetics of CPT-11 in both humans and animalshave been widely studied (Ohe et al., 1992; Rothenberg et al.,1993). Nonlinear pharmacokinetics of CPT-11 in rats were previouslyreported (Kaneda and Yokokura, 1990; Atsumi et al., 1991), showingthat CPT-11 and its metabolites recovered from bile during thefirst 24 hr after drug administration accounted for about 50 to60% of total drug disposition. Those data suggested that the eliminationof CPT-11 and its metabolites in rats is mainly via biliary excretion.However, the biliary excretion mechanism of CPT-11 and its metaboliteswas unknown. In addition, most previous studies measured onlytotal (sum of carboxylate and lactone forms) concentrations ofCPT-11 and its metabolites, rather than considering the biliaryexcretion of the individual carboxylate and lactone forms of CPT-11and its metabolites. In this study, we systematically examinedthe biliary excretion of the carboxylate and lactone forms ofCPT-11 and its metabolites in normal rats and EHBR, to clarifythe biliary excretion mechanism involved.

The biliary excretion mechanism for the carboxylate and lactone forms of CPT-11, SN-38 and SN38-Glu was investigated in bothin vivo and in vitro CMV studies. Because the carboxylate andlactone forms of SN38-Glu and the carboxylate forms of CPT-11and SN-38 have anionic charges, we hypothesized that the biliaryexcretion of these four compounds is mediated by cMOAT, whichis known to be genetically deficient in EHBR. The observed resultsstrongly support the validity of our hypothesis. First, in SDrats, the CL_bile,h values of the carboxylate forms of CPT-11,SN-38 and SN38-Glu showed obvious saturation when the dose wasincreased from 10 mg/kg to 40 mg/kg. Second, compared with SDrats, the CL_bile,h for the carboxylate and lactone forms of SN38-Gluand the carboxylate forms of CPT-11 and SN-38 in EHBR were markedlyreduced, especially at the lower dose (10 mg/kg). Similarly toCL_bile,h, the C_bile/C_liver showed obvious saturation for the carboxylateforms of CPT-11, SN-38 and SN38-Glu in SD rats (tables 1, 2and 3). The C_bile/C_liver for these three compounds and the lactoneform of SN38-Glu in EHBR at a dose of 10 mg/kg was significantlylower than in SD rats. These results suggest that the biliaryexcretion of these four compounds is by carrier-mediated transport,which is deficient in EHBR. To examine our hypothesis directly,a study of the uptake of the carboxylate and lactone forms ofCPT-11 and its metabolites by CMV isolated from SD rats and EHBRwas performed. For the carboxylate and lactone forms of SN38-Gluand the carboxylate forms of CPT-11 and SN-38, the uptake by CMVin SD rats showed a clear ATP-dependence (fig. 7), whereas theATP-dependent uptake was much lower in CMV obtained from EHBR(fig. 8). On the other hand, no ATP-dependence was found in theuptake of the lactone form of CPT-11 by CMV obtained from eitherSD rats or EHBR. These results indicate that there is a primaryactive transport system on the bile canalicular membrane specificfor the four compounds with anionic charges and this transportsystem is deficient in EHBR. Finally, to add further support toour hypothesis, DNP-SG, which is well known as a representativesubstrate for cMOAT (Akerboom et al., 1991; Takenaka et al., 1995b;Ballatori and Truong, 1995; Yamazaki et al., 1996), was used tostudy the inhibition of DNP-SG uptake by these compounds. Theresults shown in figure 9 show that the uptake of DNP-SG by CMVfrom SD rats is greatly inhibited by the carboxylate and lactoneforms of SN38-Glu and the carboxylate forms of CPT-11 and SN-38.However, no inhibitory effect was found for the lactone form ofCPT-11. This result suggests that the carboxylate and lactoneforms of SN38-Glu and the carboxylate forms of CPT-11 and SN-38share, at least in part, the same transporter as DNP-SG. Thisfinding, therefore, is consistent with the in vivo results withEHBR. Our in vivo and in vitro results, therefore, demonstratethat the biliary excretion of the carboxylate and lactone formsof SN38-Glu and the carboxylate forms of CPT-11 and SN-38 aremediated by the cMOAT located on the bile canalicular membrane,which is genetically deficient in EHBR. Comparison of the inhibitoryefficiency for DNP-SG uptake by CMV, as shown in figure 9, suggeststhat both the carboxylate and lactone forms of SN38-Glu have amuch higher affinity for the DNP-SG transporter than do the carboxylateforms of SN-38 and CPT-11, because their K_i values were much smaller(<2 µM) than those of the carboxylate forms of SN-38 (20 µM) orCPT-11 (100 µM). In addition, for SN38-Glu, the K_i value for itscarboxylate form (1.0 µM) was smaller than that for the lactoneform (1.6 µM), suggesting that the carboxylate form of SN38-Gluhas a relatively higher affinity, compared with its lactone form.A similar finding was also obtained in the in vivo study. Withincreasing dose, saturation in the CL_bile,h for the carboxylateform in SD rats was more obvious than for the lactone form (table3). That is, the CL_bile,h for the carboxylate form of SN38-Gluat 10 mg/kg was much greater than that at 40 mg/kg, whereas thedifference in the CL_bile,h for the lactone form between 10 and40 mg/kg was minimal. This result can be explained if the carboxylateform has a higher affinity (low K_m value) for the transporterthan does the lactone form and, therefore, saturation of its biliaryexcretion can be easily observed. One possible factor in sucha postulated difference in affinity is that, compared with thelactone form of SN38-Glu, there are two anionic charges presentin the carboxylate form of SN38-Glu, and this might result inthe higher affinity for the transporter than is the case withits lactone form.

As shown in figure 8, unlike the lactone and carboxylate forms of CPT-11, the ATP-dependent uptake of both lactone and carboxylateforms of SN38-Glu was partially retained in CMV from EHBR at asubstrate concentration of 50 µM (fig. 8B). This suggests thata primary active transport system, other than the cMOAT deficientin EHBR, is expressed on the bile canalicular membrane in EHBR.Recently, we found that the ATP-dependent uptake of E3040 glucuronidecould also be observed in CMV from EHBR (Niinuma, O. Takenaka,T. Horie, K. Kubayashi, Y. Kato, H. Suzuki and Y. Sugiyama, unpublishedobservations). Thus, it is possible that multiple transport systemsfor organic anions are located on the canalicular membrane. Inaddition, the K_i values obtained by evaluating the inhibitoryeffects of CPT-11 and its metabolites on the ATP-dependent uptakeof DNP-SG were 1.0 and 1.6 µM for the carboxylate and lactoneforms of SN38-Glu, respectively (fig. 9). On the other hand, ATP-dependencewas clearly observed in the uptake of both the carboxylate andlactone forms of SN38-Glu at a substrate concentration of 50 µM(figs. 7 and 8). If these compounds share the same transporter(cMOAT) with DNP-SG, their own uptake by CMV at a concentrationof 50 µM should be almost saturated and no clear ATP-dependentuptake should be observed. Accordingly, we suggest that thereis a multiplicity of biliary excretion systems for both the lactoneand carboxylate forms of SN38-Glu on the bile canalicular membrane.A primary active transporter, other than cMOAT, which is stillmaintained in EHBR, may be responsible for the residual ATP-dependentuptake of these compounds.

The CMV uptake of the carboxylate form of SN-38 also showed ATP-dependence in EHBR. Although the uptake in the presence ofATP (705 ± 31 pmol/mg protein) was significantly higher than theuptake in its absence (523 ± 49 pmol/mg protein), it is stillpossible that the primary active transporter for SN-38 (carboxylateform) might also be expressed on the bile canalicular membranein EHBR, because such a difference in CMV uptake in the presenceor absence of ATP was not so obvious (fig. 8B), nor was thereany significant difference in uptake over 0.5 min in the presenceor absence of ATP (data not shown). In addition, when the concentration-dependenceof SN-38 uptake by CMV prepared from SD rats was examined, onlya single component for the saturation of uptake was found (X.-Y.Chu, Y. Kato and Y. Sugiyama, unpublished observations). Therefore,it is likely that SN-38 (carboxylate form) is recognized onlyby cMOAT and the contribution of the other transporter is minor.

It has been reported that the diarrhea induced by CPT-11 also occurs in rats and is similar in nature to that in humans (Takasunaet al., 1995a,b). The possible mechanisms for the diarrhea causedby CPT-11 have received a great deal of attention. The diarrheainduced by enterocolitis has been suggested to be caused by highlevels of SN-38 and/or CPT-11 retained for a long period in theintestine (Araki et al., 1993), and the biliary excretion of SN38-Glumay be contributory (Kaneda et al., 1990). One treatment approachbased on this hypothesis would be to reduce the intestinal concentrationof SN-38 by inhibiting the activity of $beta$ -glucuronidase in theintestinal microflora, and baicalin, an inhibitor of $beta$ -glucuronidase,has been reported to ameliorate CPT-11-induced diarrhea in rats(Takasuna et al., 1995b). A biliary index (the product of therelative area ratio of SN-38 to SN38-Glu multiplied by that ofCPT-11 under the plasma concentration-time curve) has been definedand found to be correlated with the degree of diarrhea in humans(Gupta et al., 1994). This study is in agreement with our hypothesisif we consider that lowering the biliary excretion clearance ofSN38-Glu consequently reduces the biliary index; however, we shouldconsider the possibility that interpatient variance in glucuronidationactivity might also affect the biliary index and side effects.Our study gives deeper insight into the biliary excretion mechanismof CPT-11 and its metabolites and also suggests that the biliaryexcretion of SN38-Glu is mediated by cMOAT; therefore, inhibitorsof cMOAT may be candidates for ameliorating CPT-11-induced diarrhea.However, the mechanism for the diarrhea caused by CPT-11 is acomplicated one. In addition to the possible mechanism discussed,there are other pathways that may also contribute to the diarrhealside effect. Indeed, the intestinal secretion of CPT-11 in ratshas been observed (Kaneda and Yokokura, 1990). On the other hand,a recent study in two patients found that the total cumulativebiliary and urine excretion of CPT-11 and its metabolites up to48 hr ranged from 25 to 50% (Lokiec et al., 1995). It is possiblethat CPT-11 can be excreted by another, as yet unidentified, secretionpathway such as intestinal secretion or eliminated by conversioninto other, as yet unidentified, metabolites in humans (Rivoryand Robert, 1995). Therefore, it is possible that several othermechanisms may also be involved in the induction of the diarrhealside effect of CPT-11. As for the validity of our hypothesis andwhether the mechanism for the toxicity of CPT-11 in rats is similarto that in humans, further investigation is needed. In conclusion,the excretion of the carboxylate and lactone forms of SN38-Gluand the carboxylate forms of CPT-11 and SN-38 across the bilecanalicular membrane is mediated by the primary active transporter(cMOAT), which is deficient in EHBR.

	Acknowledgments

We are grateful to the Yakult Honsha Co. Ltd. (Tokyo, Japan) for providing CPT-11, SN-38 and SN38-Glu.

	Footnotes

Accepted for publication December 6, 1996.

Received for publication May 10, 1996.

¹ This study was supported in part by a Grant-in-Aid for Scientific Research provided by the Ministry of Education, Scienceand Culture of Japan.

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

	Abbreviations

AUC, area under the curve; C_bile/C_liver, bile-to-liver concentration ratio; CL_bile,h, biliary excretion clearance defined with respect to the hepatic concentration of the drug; CL_bile,p, biliary excretion clearance defined with respect to the plasma concentration of the drug; CL_r, urinary excretion clearance; cMOAT, canalicular multispecific organic anion transporter; CMV, canalicular membrane vesicle(s); CPT, camptothecin; CPT-11, 7-ethyl-10-[4-(1-piperidino)-1-piperidino]-carbonyloxycamptothecin; DNP-SG, S-(2,4-dinitrophenyl) glutathione; EHBR, Eisai hyperbilirubinemic rat(s); HPLC, high-performance liquid chromatography; SD, Sprague-Dawley; SN38-Glu, SN-38 glucuronide.

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Slichenmyer, W. J., Rowinsky, E. K., Donehower, R. C. and Kaufmann, S. H.: The current status of camptothecin analogues as antitumor agents. J. Natl. Cancer Inst. 85: 271-291, 1993[Abstract/Free Full Text].
Takasuna, K., Kasai, Y., Kitano, Y., Mori, K., Kakihata, K., Hirohashi, M. and Nomura, M.: Study on the mechanisms of diarrhea induced by a new anticancer camptothecin derivative, irinotecan hydrochloride (CPT-11), in rats. Folia Pharmacol. Jpn. 105: 447-460, 1995a.
Takasuna, K., Kasai, Y., Kitano, Y., Mori, K., Kobayashi, R., Hagiwara, T., Kakihata, K., Hirohashi, M., Nomura, M., Nagai, E. and Kamataki, T.: Protective effects of kampo medicines and baicalin against intestinal toxicity of a new anticancer camptothecin derivative, irinotecan hydrochloride (CPT-11), in rats. Jpn. J. Cancer Res. 86: 978-984, 1995b[Medline].
Takenaka, O., Horie, T., Suzuki, H. and Sugiyama, Y.: Different biliary excretion systems for glucuronide and sulfate of a model compound: Study using Eisai hyperbilirubinemic rats. J. Pharmacol. Exp. Ther. 274: 1362-1369, 1995a[Abstract/Free Full Text].
Takenaka, O., Horie, T., Kobayashi, K., Suzuki, H. and Sugiyama, Y.: Kinetic analysis of hepatobiliary transport for conjugated metabolites in the perfused liver of mutant rats (EHBR) with hereditary conjugated hyperbilirubinemia. Pharm. Res. 12: 1746-1755, 1995b[Medline].
Tanizawa, A., Fujimori, A., Fujimori, Y. and Pommier, Y.: Comparison of topoisomerase I inhibition, DNA damage, and cytotoxicity of camptothecin derivatives presently in clinical trials. J. Natl. Cancer Inst. 86: 836-842, 1994[Abstract/Free Full Text].
Yachi, K., Sugiyama, Y., Sawada, Y., Iga, T., Ikeda, Y., Toda, G. and Hanano, M.: Characterization of rose bengal binding to sinusoidal and canalicular plasma membrane from rat liver. Biochim. Biophys. Acta 978: 1-7, 1989[Medline].
Yamazaki, M., Suzuki, H. and Sugiyama, Y.: Recent advances in carrier-mediated hepatic uptake and biliary excretion of xenobiotics. Pharm. Res. 13: 497-513, 1996[Medline].

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				M. J. Zamek-Gliszczynski, K. A. Hoffmaster, J. E. Humphreys, X. Tian, K.-i. Nezasa, and K. L. R. Brouwer Differential Involvement of Mrp2 (Abcc2) and Bcrp (Abcg2) in Biliary Excretion of 4-Methylumbelliferyl Glucuronide and Sulfate in the Rat J. Pharmacol. Exp. Ther., October 1, 2006; 319(1): 459 - 467. [Abstract] [Full Text] [PDF]

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				M. Shimizu, K. Fuse, K. Okudaira, R. Nishigaki, K. Maeda, H. Kusuhara, and Y. Sugiyama CONTRIBUTION OF OATP (ORGANIC ANION-TRANSPORTING POLYPEPTIDE) FAMILY TRANSPORTERS TO THE HEPATIC UPTAKE OF FEXOFENADINE IN HUMANS Drug Metab. Dispos., October 1, 2005; 33(10): 1477 - 1481. [Abstract] [Full Text] [PDF]

				M. N. Tallman, J. K. Ritter, and P. C. Smith DIFFERENTIAL RATES OF GLUCURONIDATION FOR 7-ETHYL-10-HYDROXY-CAMPTOTHECIN (SN-38) LACTONE AND CARBOXYLATE IN HUMAN AND RAT MICROSOMES AND RECOMBINANT UDP-GLUCURONOSYLTRANSFERASE ISOFORMS Drug Metab. Dispos., July 1, 2005; 33(7): 977 - 983. [Abstract] [Full Text] [PDF]

				T. Nozawa, H. Minami, S. Sugiura, A. Tsuji, and I. Tamai ROLE OF ORGANIC ANION TRANSPORTER OATP1B1 (OATP-C) IN HEPATIC UPTAKE OF IRINOTECAN AND ITS ACTIVE METABOLITE, 7-ETHYL-10-HYDROXYCAMPTOTHECIN: IN VITRO EVIDENCE AND EFFECT OF SINGLE NUCLEOTIDE POLYMORPHISMS Drug Metab. Dispos., March 1, 2005; 33(3): 434 - 439. [Abstract] [Full Text] [PDF]

				J. Yu, W. D. Shannon, M. A. Watson, and H. L. McLeod Gene Expression Profiling of the Irinotecan Pathway in Colorectal Cancer Clin. Cancer Res., March 1, 2005; 11(5): 2053 - 2062. [Abstract] [Full Text] [PDF]

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				N. Mizuno, T. Niwa, Y. Yotsumoto, and Y. Sugiyama Impact of Drug Transporter Studies on Drug Discovery and Development Pharmacol. Rev., September 1, 2003; 55(3): 425 - 461. [Abstract] [Full Text] [PDF]

				R. H. J. Mathijssen, S. Marsh, M. O. Karlsson, R. Xie, S. D. Baker, J. Verweij, A. Sparreboom, and H. L. McLeod Irinotecan Pathway Genotype Analysis to Predict Pharmacokinetics Clin. Cancer Res., August 1, 2003; 9(9): 3246 - 3253. [Abstract] [Full Text] [PDF]

				K. R. Crews, C. F. Stewart, D. Jones-Wallace, S. J. Thompson, P. J. Houghton, R. L. Heideman, M. Fouladi, D. C. Bowers, M. M. Chintagumpala, and A. Gajjar Altered Irinotecan Pharmacokinetics in Pediatric High-Grade Glioma Patients Receiving Enzyme-inducing Anticonvulsant Therapy Clin. Cancer Res., July 1, 2002; 8(7): 2202 - 2209. [Abstract] [Full Text] [PDF]

				T. Ikegami, L. Ha, K. Arimori, P. Latham, K. Kobayashi, S. Ceryak, Y. Matsuzaki, and B. Bouscarel Intestinal Alkalization As a Possible Preventive Mechanism in Irinotecan (CPT-11)-induced Diarrhea Cancer Res., January 1, 2002; 62(1): 179 - 187. [Abstract] [Full Text] [PDF]

				M. P. Gamcsik, M. S. Kasibhatla, D. J. Adams, J. L. Flowers, O. M. Colvin, G. Manikumar, M. Wani, M. E. Wall, G. Kohlhagen, and Y. Pommier Dual Role of Glutathione in Modulating Camptothecin Activity: Depletion Potentiates Activity, but Conjugation Enhances the Stability of the Topoisomerase I-DNA Cleavage Complex Mol. Cancer Ther., November 1, 2001; 1(1): 11 - 20. [Abstract] [Full Text] [PDF]

				R. H. J. Mathijssen, R. J. van Alphen, J. Verweij, W. J. Loos, K. Nooter, G. Stoter, and A. Sparreboom Clinical Pharmacokinetics and Metabolism of Irinotecan (CPT-11) Clin. Cancer Res., August 1, 2001; 7(8): 2182 - 2194. [Abstract] [Full Text] [PDF]

				M. F. Fromm, H.-M. Kauffmann, P. Fritz, O. Burk, H. K. Kroemer, R. W. Warzok, M. Eichelbaum, W. Siegmund, and D. Schrenk The Effect of Rifampin Treatment on Intestinal Expression of Human MRP Transporters Am. J. Pathol., November 1, 2000; 157(5): 1575 - 1580. [Abstract] [Full Text] [PDF]

				Y. Kato, T. Igarashi, Y. Sugiyama, and A. Nishino Both cMOAT/MRP2 and Another Unknown Transporter(s) Are Responsible for the Biliary Excretion of Glucuronide Conjugate of the Nonpeptide Angiotensin II Antagonist, Telmisaltan Drug Metab. Dispos., October 1, 2000; 28(10): 1146 - 1148. [Abstract] [Full Text] [PDF]

				J. G. Slatter, L. J. Schaaf, J. P. Sams, K. L. Feenstra, M. G. Johnson, P. A. Bombardt, K. S. Cathcart, M. T. Verburg, L. K. Pearson, L. D. Compton, et al. Pharmacokinetics, Metabolism, and Excretion of Irinotecan (CPT-11) Following I.V. Infusion of [14C]CPT-11 in Cancer Patients Drug Metab. Dispos., April 1, 2000; 28(4): 423 - 433. [Abstract] [Full Text]

				H. S. Friedman, W. P. Petros, A. H. Friedman, L. J. Schaaf, T. Kerby, J. Lawyer, M. Parry, P. J. Houghton, S. Lovell, K. Rasheed, et al. Irinotecan Therapy in Adults With Recurrent or Progressive Malignant Glioma J. Clin. Oncol., May 1, 1999; 17(5): 1516 - 1516. [Abstract] [Full Text] [PDF]

				K. Niinuma, Y. Kato, H. Suzuki, C. A. Tyson, V. Weizer, J. E. Dabbs, R. Froehlich, C. E. Green, and Y. Sugiyama Primary active transport of organic anions on bile canalicular membrane in humans Am J Physiol Gastrointest Liver Physiol, May 1, 1999; 276(5): G1153 - G1164. [Abstract] [Full Text] [PDF]

Multispecific Organic Anion Transporter Is Responsible for the Biliary Excretion of the Camptothecin Derivative Irinotecan and its Metabolites in Rats1

Multispecific Organic Anion Transporter Is Responsible for the Biliary Excretion of the Camptothecin Derivative Irinotecan and its Metabolites in Rats¹

				Z.-S. Chen, T. Furukawa, T. Sumizawa, K. Ono, K. Ueda, K. Seto, and S.-I. Akiyama ATP-Dependent Efflux of CPT-11 and SN-38 by the Multidrug Resistance Protein (MRP) and Its Inhibition by PAK-104P Mol. Pharmacol., May 1, 1999; 55(5): 921 - 928. [Abstract] [Full Text]

				X.-Y. Chu, Y. Kato, and Y. Sugiyama Possible Involvement of P-Glycoprotein in Biliary Excretion of CPT-11 in Rats Drug Metab. Dispos., April 1, 1999; 27(4): 440 - 441. [Abstract] [Full Text]

				S. Akhteruzzaman, Y. Kato, A. Hisaka, and Y. Sugiyama Primary Active Transport of Peptidic Endothelin Antagonists by Rat Hepatic Canalicular Membrane J. Pharmacol. Exp. Ther., February 1, 1999; 288(2): 575 - 581. [Abstract] [Full Text]

				X.-Y. Chu, H. Suzuki, K. Ueda, Y. Kato, S.-I. Akiyama, and Y. Sugiyama Active Efflux of CPT-11 and Its Metabolites in Human KB-Derived Cell Lines J. Pharmacol. Exp. Ther., February 1, 1999; 288(2): 735 - 741. [Abstract] [Full Text]

				M. Homma, H. Suzuki, H. Kusuhara, M. Naito, T. Tsuruo, and Y. Sugiyama High-Affinity Efflux Transport System for Glutathione Conjugates on the Luminal Membrane of a Mouse Brain Capillary Endothelial Cell Line (MBEC4) J. Pharmacol. Exp. Ther., January 1, 1999; 288(1): 198 - 203. [Abstract] [Full Text]

				H. Sasabe, Y. Kato, A. Tsuji, and Y. Sugiyama Stereoselective Hepatobiliary Transport of the Quinolone Antibiotic Grepafloxacin and Its Glucuronide in the Rat J. Pharmacol. Exp. Ther., February 1, 1998; 284(2): 661 - 668. [Abstract] [Full Text]

				K. Ito, H. Suzuki, T. Hirohashi, K. Kume, T. Shimizu, and Y. Sugiyama Functional Analysis of a Canalicular Multispecific Organic Anion Transporter Cloned from Rat Liver J. Biol. Chem., January 16, 1998; 273(3): 1684 - 1688. [Abstract] [Full Text] [PDF]