Hepatic Uptake of the Magnetic Resonance Imaging Contrast Agent Gadoxetate by the Organic Anion Transporting Polypeptide Oatp1

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Vol. 290, Issue 1, 153-157, July 1999

Hepatic Uptake of the Magnetic Resonance Imaging Contrast Agent Gadoxetate by the Organic Anion Transporting Polypeptide Oatp1¹

Jessica E. van Montfoort , Bruno Stieger, Dirk K. F. Meijer, Hanns-J. Weinmann, Peter J. Meier and Karin E. Fattinger

Division of Clinical Pharmacology and Toxicology, Department of Medicine, University Hospital, Zürich, Switzerland (J.E.V.M., B.S., P.J.M., K.E.F.); Liver Research Center, Groningen Institute of Drug Studies, Groningen, the Netherlands (J.E.V.M., D.K.F.M.); and Contrast Media Research, Schering AG, Berlin, Germany (H.J.W.)

	Abstract

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Gadoxetate is a new hepatobiliary magnetic resonance imaging contrast agent. It is specifically taken up by hepatocytes, andits uptake can be inhibited by the coadministration of bromosulfophthalein,suggesting an involvement of one or several of the cloned organicanion transporting polypeptides Oatp1, Oatp2, and/or OATP. Inthis study, we demonstrated saturable uptake of gadoxetate byOatp1 cRNA-injected Xenopus laevis oocytes (K_m ~ 3.3 mM). In contrast,gadoxetate was not taken up by Oatp2 or OATP cRNA-injected oocytes.Oatp1-mediated gadoxetate uptake (100 µM) could be inhibited by10 µM bromosulfophthalein (45%), 200 µM taurocholate (92%), 100µM rifamycin SV (97%), and 100 µM rifampicin (51%). These resultsshow that gadoxetate is a low-affinity substrate of Oatp1. Oatp1-mediatedgadoxetate transport demonstrated a similar apparent K_m valueand cis-inhibition pattern as previously determined in rats invivo, indicating that Oatp1 is significantly involved in gadoxetateuptake into ratliver.

	Introduction

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Gadoxetate (gadolinium-ethoxybenzyl-diethylenetriamine-pentaacetic acid, disodium salt; Fig. 1) is a new hepatobiliary magneticresonance imaging contrast agent based on the extracellular fluidmarker gadopentetate [gadolinium-diethylenetriamine-pentaaceticacid (Magnevist)]. The introduction of the lipophilic ethoxybenzylmoiety to gadopentetate resulted in liver-specific contrast enhancementdue to specific uptake into hepatocytes and biliary excretionof gadoxetate (Vogl et al., 1996). Gadoxetate is in phase IIIof clinical trials and has been evaluated for the detection ofliver metastases, hepatocellular carcinomas, hemangiomas, andcholestasis (Schuhmann-Giampieri et al., 1992; Ni et al., 1994;Vogl et al., 1996; Reimer et al., 1997; Schmitz et al., 1997).

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Fig. 1. Chemical structure of gadoxetate (gadolinium-ethoxybenzyldiethylenetriamine-pentaacetic acid, disodium salt).

Gadoxetate is highly water soluble and exhibits low protein binding (10%) (Weinmann et al., 1991). The substance has a highin vivo complex stability (Schuhmann-Giampieri et al., 1992),and there apparently is no biotransformation (Weinmann et al.,1991). In rats, 70% of the dose undergoes hepatobiliary excretion,whereas 30% of the dose is excreted in the urine (Weinmann etal., 1991). Gadoxetate exhibits nonlinear pharmacokinetics dueto saturability of the hepatobiliary excretion. Renal excretionis linear, and its clearance value is similar to the value forglomerular filtration in rats (Schuhmann-Giampieri et al., 1993b).Experiments in which either the common bile duct or the renalblood vessels were ligated showed that dysfunction of liver orkidney may be fully compensated by the remaining alternative eliminationpathway (Muhler et al., 1994).

The biliary excretion of gadoxetate is inhibited by the coadministration of bromosulfophthalein (BSP), which is attributedto a decreased liver uptake of gadoxetate (Clement et al., 1992).This finding suggests that one or several of the polyspecificorganic anion transporting polypeptides (Oatps) are involved inthe uptake of gadoxetate. The first member of the Oatp gene family,Oatp1, has been isolated from rat liver using expression cloningin Xenopus laevis oocytes on the basis of Na⁺-independent BSP uptake (Jacquemin et al., 1994). In additionto BSP, Oatp1 also mediates the uptake of a wide variety of structurallyunrelated compounds, including taurocholate and conjugated andneutral steroids (Kullak Ublick et al., 1994; Bossuyt et al.,1996). Oatp2 has been cloned from rat brain but also is expressedin the liver (Noe et al., 1997). It has a similar substrate specificityas Oatp1, but as a unique feature, Oatp2 mediates high-affinityuptake of the cardiac glycoside digoxin. OATP has been clonedfrom human liver. Its substrate specificity is similar to therat Oatps, although it has lower transport capacities for bileacids and organic anions (Meier et al., 1997). In this study,we investigated whether one or several of the Oatps can mediatethe hepatic uptake of gadoxetate with similar characteristicsas in intactliver.

	Experimental Procedures

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Materials. Radiolabeled [¹⁵³Gd]gadoxetate (107.51 MBq/mg) and unlabeled gadoxetate were kindly provided by Schering AG (Berlin, Germany)(Schuhmann-Giampieri et al., 1992). [³H]Estrone-3-sulfate (53 Ci/mmol) and [³H]digoxin (15 Ci/mmol) were obtained from Du Pont-New EnglandNuclear (Boston, MA). All other chemicals were of analytical gradeand were readily available from commercialsources.

Uptake Studies in X. laevis Oocytes. In vitro synthesis of Oatp1, Oatp2, and OATP cRNA was performed as described previously (Kullak Ublick et al., 1994, 1995;Noe et al., 1997). X. laevis oocytes were prepared (Hagenbuchet al., 1990) and cultured overnight at 18°C. Healthy oocyteswere microinjected with 1 ng of Oatp1, 5 ng of Oatp2, and/or 2.5ng of OATP cRNA and cultured for 3 days in a medium containing88 mM NaCl, 2.4 mM NaHCO₃, 1 mM KCl, 0.3 mM Ca(NO₃)₂, 0.41 mMCaCl₂, 0.82 mM MgSO₄, 0.05 mg/ml gentamycin, and 15 mM HEPES,pH 7.6. The uptake medium consisted of 100 mM NaCl, 2 mM KCl,1 mM CaCl₂, 1 mM MgCl₂, and 10 mM HEPES, pH 7.5. The oocytes wereprewashed in the uptake medium and then incubated at 25°C in 100µl of the uptake medium containing the indicated substrate concentrations.Water-injected oocytes were used as controls for unspecific uptakeof the substrate. After the indicated time intervals, uptake wasstopped by the addition of 6 ml of ice-cold uptake medium. Theoocytes were washed twice with 6 ml of ice-cold uptake medium,and the oocyte-associated radioactivity of [¹⁵³]gadoxetate was determined in a Packard Cobra Auto-Gamma counter(Canberra Packard, Zürich, Switzerland). In the case of the positivecontrols [³H]estrone-3-sulfate and [³H]digoxin, each oocyte was dissolved in 0.5 ml of 10% SDS and5 ml of scintillation fluid (Ultima Gold; Canberra Packard), andthe oocyte-associated radioactivity was determined in a Tri-Carb2200 CA liquid scintillation analyzer (Canberra Packard). To determinethe kinetic constants for Oatp1-mediated gadoxetate uptake, anonlinear curve-fitting program was used (Systat 6.0.1; SPSS Inc.,Chicago, IL) using a simple Michaelis-Menten model (v = V_max[S]/(K_m+ [S])). In the cis-inhibition studies, the inhibitors bromosulfophthalein(BSP; sodium salt) and taurocholate (sodium salt) were dissolvedin the incubation buffer. Because of their low water solubility,the inhibitors rifamycin SV (sodium salt) and rifampicin weredissolved in dimethyl sulfoxide and subsequently diluted 1:100in the incubation medium to the desired concentration. As a control,Oatp1 cRNA-injected oocytes were also incubated in 1% dimethylsulfoxide and showed normal gadoxetateuptake.

Statistical Analysis. Uptake results are given as mean ± S.D. Statistical significance was determined using the Mann-Whitney U test (Systat 6.0.1,SPSS Inc., Chicago,IL).

	Results

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The uptake of gadoxetate (5 µM) was measured in Oatp1, Oatp2, and OATP cRNA-injected X. laevis oocytes. As illustrated inFig. 2, only Oatp1 cRNA-injected oocytes mediated significantgadoxetate uptake. The gadoxetate uptake was approximately 22-foldhigher in Oatp1 cRNA-injected oocytes compared with water-injectedcontrol oocytes. Gadoxetate uptake by Oatp2 and OATP cRNA-injectedoocytes was not different from water-injected control oocytes.Proper expression of the carriers in the oocytes was controlledwith the positive controls estrone-3-sulfate (0.2 µM) for Oatp1and OATP and digoxin (0.8 µM) for Oatp2, respectively (Meier etal., 1997) (data not shown).

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Fig. 2. Comparison of Oatp1-, Oatp2-, and OATP-mediated gadoxetate uptake by X. laevis oocytes. X. laevis oocytes were injected with 1 ng of Oatp1, 5 ng of Oatp2, and 2.5 ng of OATP cRNA. After 3 days in culture, uptake of 5 µM gadoxetate was measured at 60 min (see Experimental Procedures). Data represent the mean ± S.D. of 14 to 16 oocyte uptake measurements in one representative preparation of two separate oocyte preparations. *Significantly different from water control (Mann-Whitney U test, p < .001).

In time-course experiments, the uptake of gadoxetate by Oatp1 was measured during 60 min at the lowest (5 µM) and the highest(10 mM) concentration used in all uptake experiments (Fig. 3).Oatp1-mediated gadoxetate uptake increased linearly during atleast 60 min at both concentrations. In all subsequent experimentsdesigned to determine the kinetic parameters for Oatp1-mediatedgadoxetate uptake, the oocytes were incubated for 20 min withincreasing substrate concentrations.

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Fig. 3. Time course of gadoxetate uptake in Oatp1 cRNA injected X. laevis oocytes. X. laevis oocytes were injected with 1 ng of Oatp1 cRNA. After 3 days in culture, the time courses for 5 µM (A) and 10 mM (B) gadoxetate were measured (see Experimental Procedures). Data are expressed as mean ± S.D. of 9 to 15 oocyte uptake measurements.

Uptake of gadoxetate by Oatp1 was saturable and yielded an apparent K_m value of 3.3 ± 0.4 mM (mean ± S.E.) and a V_max valueof 544 ± 33 fmol/oocyte/min (Fig. 4).

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Fig. 4. Kinetics of gadoxetate uptake in Oatp1 cRNA-injected X. laevis oocytes. X. laevis oocytes were injected with 1 ng of Oatp1 cRNA. After 3 days in culture, uptake of gadoxetate was measured at 20 min (see Experimental Procedures) at increasing substrate concentrations. The solid line represents uptake differences between Oatp1 cRNA- and water-injected oocytes. Data are expressed as mean ± S.D. of 10 to 12 oocyte uptake measurements in two separate oocyte preparations.

Experiments with rats in vivo showed that BSP inhibited liver uptake of gadoxetate (Clement et al., 1992). Hepatic uptakeof gadoxetate was also effectively blocked by the anions rifamycinand bilirubin (Weinmann et al., 1996). Based on these in vivoinhibition data, a series of cis-inhibition studies were performedto further confirm the importance of Oatp1 in liver uptake ofgadoxetate (Fig. 5). An excess of 10 mM cold gadoxetate inhibitedOatp1-mediated uptake of gadoxetate (100 µM) by 79 ± 8% (mean± S.D.). The known Oatp1 substrates BSP (10 µM) and taurocholate(200 µM) inhibited gadoxetate uptake by 45 ± 11% and 92 ± 13%,respectively. Gadoxetate uptake by Oatp1 was also inhibited byboth rifamycin SV (100 µM) and its clinically more relevant derivative,rifampicin (100 µM), to the extents of 97 ± 9% and 51 ± 15%, respectively.

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Fig. 5. The cis-inhibition of gadoxetate uptake in Oatp1 cRNA-injected X. laevis oocytes. X. laevis oocytes were injected with 1 ng of Oatp1 cRNA. After 3 days in culture, uptake of gadoxetate (100 µM) was measured at 20 min (see Experimental Procedures) in the absence (control) and the presence of 10 mM gadoxetate (Gadox.), 10 µM BSP, 200 µM taurocholate (TC), 100 µM rifamycin SV (Rif.SV), and 100 µM rifampicin (Rifamp.). Data are expressed as mean ± S.D. of 13 or 14 oocyte uptake measurements. *Significantly different from water control (Mann-Whitney U test, p < .001).

	Discussion

Top Abstract Introduction Experimental Procedures Results Discussion References

Gadoxetate is a new magnetic resonance imaging contrast agent that is specifically taken up by hepatocytes and excreted intobile (Schuhmann-Giampieri et al., 1992). During preclinical trials,it was shown that the hepatobiliary excretion of gadoxetate inrats was saturable, suggesting carrier-mediated gadoxetate transport.Recently, several transport proteins with broad substrate specificitieshave been cloned. The members of the organic cation transporterfamily (e.g., rOCT1, rOCT2) transport small organic cations (Koepsell,1998; Zhang et al., 1998). The organic anion transporters OAT1and OAT2 mediate mainly the transport of small anionic drugs (molecularweight in the range of 150-350), such as p-aminohippurate, salicylate,and acetylsalicylate (Sekine et al., 1997, 1998; Sweet et al.,1997). In contrast, the Oatps mediate the transport of larger,amphipathic molecules, such as taurocholate and BSP (Meier etal., 1997). Gadoxetate is a rather large (molecular weight 726)dianion, and its hepatic uptake could be inhibited by the coadministrationof BSP (Schuhmann-Giampieri et al., 1992). Furthermore, uptakeof gadoxetate by rat hepatocytes could be inhibited by the anionsbilirubin and rifamycin (Weinmann et al., 1996). These findingssuggested the involvement of one or several of the cloned Oatpsbecause BSP uptake was shown to be mediated by Oatp1 and OATP(Meier et al., 1997). In this study, it was tested whether theuptake of gadoxetate by hepatocytes is mediated by Oatp1, Oatp2,and/orOATP.

This study shows that only Oatp1 cRNA-injected X. laevis oocytes mediated significant gadoxetate uptake activity (Fig. 2).This finding is further proof for the functional differences betweenthe members of the Oatp gene family (Meier et al., 1997). Becausegadoxetate is negatively charged at physiological pH, exclusiveuptake by Oatp1 further supports the preference of Oatp1 for organicanions. In contrast, the unique feature of Oatp2 is high-affinityuptake of the neutral cardiac glycoside digoxin (Noe et al., 1997),whereas OATP exhibits high initial uptake rates for the cationN-(4,4-azo-n-pentyl)-21-deoxyajmalinium and the thrombin inhibitorCRC 220 (Meier et al., 1997).

Oatp1-mediated gadoxetate uptake exhibited saturability with increasing substrate concentrations (Fig. 4). The apparent K_mvalue was 3.3 ± 0.4 mM (mean ± S.E.). Nonlinear pharmacokineticmodeling of the gadoxetate plasma concentration time course andthe urinary and biliary gadoxetate excretion data after i.v. injectionof a gadoxetate bolus (0.5 mmol/kg) in rats yielded a K_m valueof 2.7 ± 1.45 mM (mean ± S.D.) (Schuhmann-Giampieri, 1993a). Thissimilarity between the K_m value of Oatp1-mediated gadoxetate uptakeand the K_m value of fitted in vivo data indicates that Oatp1 issignificantly involved in gadoxetate uptake into rat liver. Thereis no saturation of the hepatobiliary elimination pathway withdiagnostic doses of gadoxetate (0.01-0.03 mmol/kg; Weinmann etal., 1991) because saturation of the hepatobiliary eliminationpathway is reached only with doses of more than 0.5 mmol/kg (Schuhmann-Giampieriet al., 1992). Hence, the involvement of Oatp1 as a low-affinity,high-capacity carrier would be favorable for rapid liver enhancementbecause sufficient amounts of gadoxetate can efficiently be takenup by the hepatocytes. Apart from biliary elimination, gadoxetatemay regurgitate from the hepatocytes into the bloodstream andthen is cleared by the kidney (Muhler et al., 1994). The effluxof gadoxetate back to the blood could also be mediated by Oatp1because it was shown that Oatp1 can mediate bidirectional BSPtransport in stably transfected HeLa cells (Shi et al., 1995).

The cis-inhibition studies further support the hypothesis that Oatp1 is an important uptake carrier for gadoxetate in ratliver. Similar to the in vivo situation (Weinmann et al., 1991;Schuhmann-Giampieri et al., 1992), Oatp1-mediated gadoxetate uptakewas inhibited by BSP and rifamycin SV (Fig. 5). The clinicallymore relevant drug rifampicin also inhibited gadoxetate uptakeby Oatp1. Kullak-Ublick et al. (1994) reported previously thatrifampicin does not alter Oatp1-mediated BSP uptake. In contrast,Oatp1-mediated gadoxetate uptake was substantially inhibited byrifampicin (Fig. 5). The most probable reasons for this apparentinconsistencies are the different affinities of gadoxetate (K_m~ 3.3 mM) and BSP (K_m ~ 1.5 µM) for Oatp1. Thus, it can be expectedthat any inhibitor with an Oatp1 affinity between that of BSPand gadoxetate will affect gadoxetate transport but will havelittle influence on BSPtransport.

The finding that the clinically important drug rifampicin inhibits Oatp1-mediated gadoxetate uptake raises the question ofwhether the coadministration of rifampicin could substantiallyreduce gadoxetate-induced liver enhancement. In rats, the structurallyrelated rifamycin significantly inhibited hepatic gadoxetate uptakeat a dose of 30 mg/kg b.wt. (Weinmann et al., 1996). Extrapolationof these results to humans is not yet possible because the transportprotein responsible for gadoxetate uptake into human liver isstill unknown. However, the usual rifampicin dose in men is considerablyless (9 mg/kg b.wt.), and rifampicin serum and hepatic tissueconcentrations in the first hours after administration of therapeuticdoses were reported to be in the range of 1 to 14 µM and 1 to52 µM, respectively (Kiss et al., 1978). Furthermore, rifampicinis bound to serum proteins to an extent of about 80% (Acocella,1978), resulting in a free plasma concentration between 0.2 and3 µM. A rifampicin concentration of 100 µM in the absence of anyserum proteins resulted in a 51% inhibition of Oatp1-mediatedgadoxetate uptake (Fig. 5). Thus, if one assumes that the freeplasma concentration of rifampicin governs uptake inhibition invivo, no substantial reduction of liver enhancement would be expectedafter the administration of therapeutic rifampicindoses.

In contrast to several in vivo observations in which taurocholate and tauroglycocholate did not interfere with hepatic uptakeand biliary excretion of gadoxetate (Clement et al., 1992; Schuhmann-Giampieriet al., 1992, 1993b), taurocholate inhibited Oatp1-mediated gadoxetatetransport into X. laevis oocytes (Fig. 5). This discrepancy arisesbecause in the oocyte experiments, high taurocholate concentrations(200 µM) were used. This value corresponds to four times the apparentK_m value for Oatp1-mediated taurocholate transport (Kullak Ublicket al., 1994). For the in vivo experiments, no data on taurocholateserum concentrations are available. Because bile acids are veryefficiently removed from the circulation, one would expect serumtaurocholate concentrations to be only moderately increased. However,if these concentrations remained below the K_m value for Oatp1-mediatedtaurocholate transport, one would expect gadoxetate uptake tonot be substantiallyinfluenced.

In conclusion, the present study shows that Oatp1 is an important carrier for gadoxetate uptake into rat hepatocytes and thatgadoxetate is a predominant or even specific Oatp1 substrate.Of course, it cannot be definitively excluded that a transporternot included in the present study might additionally mediate hepaticgadoxetate uptake. However, because of the close agreement betweenthe characteristics of Oatp1-mediated gadoxetate transport withprevious in vivo data and the physicochemical properties of gadoxetate,a substantial contribution of other transporters, especially theabove-mentioned OCTs and OATs, seems unlikely. Because the humanOATP does not transport gadoxetate but gadoxetate is concentratedin human liver (Hamm et al., 1995), an Oatp1 analog must alsoexist in human liver. This hypothetical human Oatp1 analog remainsto be identified, cloned, and functionally characterized. Becauseof its Oatp1 specificity and the clear signal obtained in theoocyte system, gadoxetate seems to be a feasible substrate forexpression cloning of the human Oatp1analog.

	Footnotes

Accepted for publication March 11, 1999.

Received for publication January 12, 1999.

¹ This work was supported by the Swiss National Science Foundation Grants 3100-045536.95 and 3200-052190.97. J. van M. was supportedby an Ubbo Emmius scholarship from the University of Groningen.K.F. was supported by a SCORE Career Development Award from theSwiss National Science Foundation. A preliminary report of thisstudy was presented at the 49th Annual Meeting of the AmericanAssociation for the Study of Liver Diseases (AASLD) in Chicago,November 6 through 10, 1998, and published in abstract form [Hepatology(1998) 28:180A).

Send reprint requests to: Dr. K. Fattinger, Division of Clinical Pharmacology and Toxicology, Department of Medicine, University Hospital, CH-8091 Zürich/Switzerland. E-mail: fattinge{at}kpt.unizh.ch

	Abbreviations

BSP, bromosulfophthalein; Oatp, organic anion transporting polypeptide.

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Antibiotic efflux pumps in eukaryotic cells: occurrence and impact on antibiotic cellular pharmacokinetics, pharmacodynamics and toxicodynamics
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Organic Anion-Transporting Polypeptides Mediate Transport of Opioid Peptides across Blood-Brain Barrier
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