Molecular and Physiological Evidence for Multifunctionality of Carnitine/Organic Cation Transporter OCTN2

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Vol. 59, Issue 2, 358-366, February 2001

Molecular and Physiological Evidence for Multifunctionality of Carnitine/Organic Cation Transporter OCTN2

Rikiya Ohashi, Ikumi Tamai, Jun-ichi Nezu, Hiroko Nikaido, Noriyoshi Hashimoto, Asuka Oku, Yoshimichi Sai, Miyuki Shimane, and Akira Tsuji

Faculty of Pharmaceutical Sciences (R.O., I.T., Y.S., A.T.) and Institute for Experimental Animals, Faculty of Medicine (H.N., N.H.), Kanazawa University, Kanazawa, Japan; Core Research for Evolutional Science and Technology, Japan Science and Technology Corporation, Kawaguchi, Japan (I.T., Y.S., A.T.); and Chugai Research Institute for Molecular Medicine Inc., Ibaraki, Japan (J.N., A.O., M.S.)

	Abstract

Top Abstract Introduction Experimental Procedures Results Discussion References

OCTN2 is an Na⁺-dependent transporter for carnitine, which is essential for fatty acid metabolism, and its functional defectleads to fatal systemic carnitine deficiency (SCD). It also transportsthe organic cation tetraethylammonium (TEA) in an Na⁺-independent manner. Here, we studied the multifunctionality ofOCTN2, by examining the transport characteristics in cells transfectedwith mouse OCTN2 and in juvenile visceral steatosis (jvs) micethat exhibit a SCD phenotype owing to mutation of the OCTN2 gene.The physiological significance of OCTN2 as an organic cation transporterwas confirmed by using jvs mice. The embryonic fibroblasts fromjvs mice exhibited significantly decreased transport of [¹⁴C]TEA. Pharmacokinetic analysis of [¹⁴C]TEA disposition demonstrated that jvs mice showed decreasedtissue distribution and renal secretory clearance. In transportexperiments using OCTN2-expressing cells, TEA and carnitine showedmutual trans-stimulation effects in their transport, implyinga carnitine/TEA exchange mechanism. In addition, Na⁺ affected the affinity of carnitine for OCTN2, whereas Na⁺ is unlikely to be involved in TEA transport. This is the firstmolecular and physiological demonstration of the operation ofan organic cation transporter in renal apical membrane. The resultsare consistent with the physiological coupling of carnitine reabsorptionwith the secretion of organiccations.

	Introduction

Top Abstract Introduction Experimental Procedures Results Discussion References

Organic cations such as tetraethylammonium (TEA) are distributed into various tissues and excreted into urine by specifictransport systems in kidney. Previous studies suggested that organiccations are excreted by potential-dependent OCT transporters andby an organic cation/H⁺ antiporter across the renal epithelial basolateral and apicalmembranes, respectively (Zhang et al., 1998; Koepsell et al.,1999; Sweet and Pritchard, 1999), whereas no apically expressedtransporters have been molecularly identified. We have isolatedand characterized the new family of organic cation transporters,OCTN. The first member of the OCTN family, OCTN1, cloned fromhuman fetal liver, transports organic cations such as TEA in apH-dependent manner (Tamai et al., 1997; Yabuuchi et al., 1999).The second member, OCTN2, transports physiologically importantcarnitine in an Na⁺-dependent manner, as well as organic cations in an Na⁺-independent manner (Tamai et al., 1998; Wu et al., 1998, 1999;Ohashi et al., 1999). OCTN2 is present in various tissues, includingkidney, skeletal muscle, heart, placenta, and others (Tamai etal., 1998). In 1988, the homozygous mutant mice, named juvenilevisceral steatosis (jvs) mice, which exhibit cardiac hypertrophy,lipid accumulation in the liver, and hyperammonemia, (Koizumiet al., 1988; Horiuchi et al., 1993) were found with several histologicalchanges (Koizumi et al., 1988; Narama et al., 1997) and alterationof carnitine disposition (Yokogawa et al., 1999a). The significanceof OCTN2 as the carnitine transporter was clearly demonstratedusing jvs mice, which exhibit the phenotype of systemic carnitinedeficiency (SCD) caused by mutation of the OCTN2 gene (Leu352Arg)(Hashimoto et al., 1998; Lu et al., 1998; Nezu et al., 1999; Yokogawaet al., 1999c). However, no precise studies on organic cationtransport by mouse OCTN2 have been done, and the physiologicaland pharmacological relevance of OCTN2 as an organic cation transporterremains to be clarified. Furthermore, the mechanism of the multifunctionalityof OCTN2, transporting carnitine and organic cations in Na⁺-dependent and independent manners, respectively, is unclear.Because the jvs mice have genetically mutated OCTN2 and completelylack carnitine transport activity, they are expected to be usefulto evaluate a contribution of OCTN2 as an organic cationtransporter.

In the present study, we studied the multifunctionality of OCTN2 and the significance of OCTN2-mediated tissue distributionand renal excretion of the organic cation TEA by comparing thedispositions in wild type and jvs mice, as well as by examiningtransport in OCTN2-expressingcells.

	Experimental Procedures

Top Abstract Introduction Experimental Procedures Results Discussion References

Materials. [Methyl-³H]acetyl-L-carnitine hydrochloride (65 Ci/mmol) and L-[methyl-³H]carnitine hydrochloride (85 Ci/mmol) were purchased from MoravekBiochemicals Inc. (Brea, CA). [1-¹⁴C]Tetraethylammonium bromide (2.4 mCi/mmol), [N-methyl-³H]1-methyl-4-phenylpyridinium acetate (MPP) (82 Ci/mmol), [N-methyl-³H]verapamil hydrochloride (78.6 Ci/mmol) and [glycyl-2-³H]p-aminohippurate (2.45 Ci/mmol) were from New England Nuclear(Boston, MA). [Pyridinyl-5-³H]pyrilamine (28 Ci/mmol) was from Amersham Pharmacia Biotech(Buckinghamshire, UK). Other reagents, including cefazolin sodium,were obtained from Sigma Chemical Co. (St. Louis, MO), Wako PureChemical Industries (Osaka, Japan), and Nacalai Tesque, Inc. (Kyoto,Japan) and used without further purification. HEK 293 cells wereobtained from Japanese Cancer Research Resources Bank (Tokyo,Japan).

Studies of Uptake and Efflux by Fibroblasts and HEK 293 Cells Expressing Mouse OCTN2. Primary cultured fibroblasts from homozygous jvs and normal C57BL/6J embryos were prepared and cultured as described previously(Hashimoto et al., 1998). Briefly, the cells obtained were culturedin Dulbecco's modified Eagle's medium supplemented with 5% fetalcalf serum (Life Technologies, Tokyo, Japan) on plastic disksin humidified 5% CO₂ at 37°C and used for uptake experiments.In the transport measurement, the cells cultured on plastic diskswere incubated with transport medium (Hanks' balanced salt solution)containing a radiolabeled test compound to initiate the uptakestudy. After an appropriate time, the disks were washed threetimes with ice-cold Hanks' balanced salt solution, solubilizedwith 1 N NaOH, and the radioactivity was measured in a liquidscintillation counter after neutralization with HCl and additionof liquid scintillation fluid, Clear-sol I (NacalaiTesque).

For transport studies in HEK 293 cells expressing mouse OCTN2, the full-length wild-type or jvs mouse OCTN2 cDNA, subclonedinto the BamHI sites of the expression vector pcDNA3 and the construct,pcDNA3/mouse OCTN2, was transfected into HEK 293 cells by meansof the calcium phosphate precipitation method as described previously(Tamai et al., 1997

). The cells were cultivated in Dulbecco'smodified Eagle's medium containing 10% fetal calf serum, penicillinand streptomycin in a humidified incubator at 37°C under 5% CO₂.After 24-h cultivation of the cells in the 15-cm dishes, pcDNA3/OCTN2or pcDNA3 vector alone (Mock) was transfected by adding 10 µgof the plasmid DNA per dish. At 48 h after transfection, the cellswere harvested with a rubber policeman, washed twice, and suspendedin the transport medium containing 125 mM NaCl, 4.8 mM KCl, 5.6mM D-glucose, 1.2 mM CaCl₂, 1.2 mM KH₂PO₄, 1.2 mM MgSO₄, and 25mM HEPES, pH 7.4. In an uptake measurement, the cell suspensionwas mixed with transport medium containing a radiolabeled testcompound to initiate the uptake study. In the trans-stimulateduptake experiments, the cells were preloaded with TEA for 30 minand subsequently uptake of [³H]carnitine by the cells was measured. At appropriate times, 100-or 200-µl aliquots of the mixture were withdrawn and the cellswere separated from the transport medium by centrifugation ina microtube containing a mixture of silicon oil and liquid paraffinwith a density of 1.03 and 3 N KOH. The resultant cell pelletswere solubilized in 3 N KOH, neutralized with HCl, and the associatedradioactivity was measured in a liquid scintillation counter.In the trans-stimulated efflux experiments, the cells were preloadedwith [¹⁴C]TEA for 30 min at 37°C. Then, the cells were spun down (0°C,7,000g, 8 sec), suspended in ice-cold transport medium, and washedtwice at 0°C. The cells were again suspended in the transportmedium containing test compounds, and efflux was initiated at37°C. At appropriate times, 100-µl aliquots of the mixture werewithdrawn and the cell-associated radioactivity was measured asdescribed above. Cellular protein content was determined accordingto the method of Bradford using a Bio-Rad protein assay kit (BioRad,Hercules, CA) and bovine serum albumin as the standard (Bradford,1976

). For Na⁺-free experiments, the obtained cells were suspended in Na⁺-free medium, in which Na⁺ was replaced isotonically with N-methyl-D-glucamine (NMG).

Animal Experiments. All the animal experiments were performed according to the Guidelines for the Care and Use of Laboratory Animals in Takara-machCampus of Kanazawa University. Jvs mice, originally found amongmice of the C3H.OH strain (Koizumi et al., 1988), and controlwild mice C3H/HeJ (Japan SLC, Hamamatsu, Japan) were used forthe following studies. By mating heterozygous male mice with heterozygousfemale mice, we obtained homozygous mutants (jvs/jvs). Eight-week-oldjvs male mice (jvs/jvs) and normal male C3H/Hej mice (+/+) wereused to study the disposition of TEA after overnight starvation.Mice were anesthetized with pentobarbital and were bolus-injectedwith 8.8 mg/kg of [¹⁴C]TEA via the jugular vein. [³H]Inulin was simultaneously injected with [¹⁴C]TEA to evaluate glomerular filtration rate (GFR). Serial bloodsamples were collected from the intraorbital venous plexus usingheparinized capillary tubes at designated time intervals in individualmice during the experiment. Urine samples were collected by washingthe bladder with saline (0.5 ml) at designated times through acatheter. For determination of the apparent tissue-to-plasma concentrationratio (K_p), the mice were decapitated at 4 h after a single intravenousinjection of [¹⁴C]TEA. The tissues were quickly excised, rinsed well with ice-coldsaline, blotted to dryness, and weighed. Plasma and urine sampleswere mixed with scintillation fluid for quantitation. Tissue samples(0.05-0.2 g) were dissolved in 1 ml of Soluene-350 (Packard Inc.,Meriden, CT) by incubation at 50°C for 3 h. The dissolved sampleswere mixed with scintillation fluid, neutralized with 1 N HCl,and the associated radioactivity was measured. In the same mannerwith TEA, cefazolin at a dose of 20 mg/kg was intravenously injectedto mice and the concentration of cefazolin in plasma and urinewas measured by high-performance liquid chromatography. The usedcolumn and mobile phase for high-performance liquid chromatographyanalysis of cefazolin were TSKgel ODS-80Ts (4.6 × 150 mm; Tosoh,Tokyo, Japan) and acetonitrile/water containing 10 mM ammoniumacetate (15:85),respectively.

Data Analysis. Uptake of [³H]carnitine or [¹⁴C]TEA by in vitro experiments was usually expressed as the cell-to-medium concentration (C/M) ratio(in microliters per milligram of protein) obtained by dividingthe uptake amount by the concentration of test compound in themedium. The K_m values of carnitine and TEA were 22.1 µM and 215µM (Tamai et al., 2000), respectively, and concentrations of [³H]carnitine (10 nM) and [¹⁴C]TEA (50-100 µM) used in each experiment were low enough to beevaluated by the C/M ratio compared with K_m values. Pharmacokineticparameters such as the area under the plasma concentration-timecurve (AUC), the elimination rate constant (k_e), the steady-statedistribution volume (Vdss) and the total body clearance (CL_tot)were estimated according to model-independent moment analysisor compartment analysis using WinNonlin (SCI, Cary, NC). GFR wasestimated in terms of inulin clearance. The renal clearance (CLr)and renal secretory clearance (CLs) were calculated by using theequations CLr = X / AUC and CLs = CLr $-$ GFR, where X is the urinaryexcretion amount of [¹⁴C]TEA. All data are expressed as mean ± S.E.M. and statisticalanalysis was performed by using Student's t test, with p < 0.05as the criterion ofsignificance.

	Results

Top Abstract Introduction Experimental Procedures Results Discussion References

Transport of [¹⁴C]TEA and [³H]Carnitine in Embryonic Fibroblasts from Wild-Type and jvs Mice. Fig. 1, A and B, show the uptakes of [³H]carnitine and [¹⁴C]TEA by embryonic fibroblasts from wild-type and jvs mice. Uptakeof [¹⁴C]TEA by fibroblasts from jvs mice was significantly lower thanthat by the cells from normal mice, as was also the case for [³H]carnitine. Furthermore, after preincubation of fibroblasts with[¹⁴C]TEA, the efflux transport of [¹⁴C]TEA was measured (Fig. 1C). The efflux rate of [¹⁴C]TEA from wild-type fibroblasts was larger than that of jvs fibroblasts.The apparent rapid efflux of TEA from jvs mice-derived fibroblastsat the initial stage represents release of the cell-surface adsorbed[¹⁴C]TEA, because further decrease in cell-associated radioactivitywas not observed. These findings demonstrated that TEA is bidirectionallytransported in mouse embryonic fibroblasts and OCTN2 plays a rolein the transport of TEA as well as carnitine.

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Fig. 1. Uptakes of [³H]carnitine (A) and [¹⁴C]TEA (B) and efflux of [¹⁴C]TEA (C) by embryonic fibroblasts from wild-type ( $open circle$ , open columns) and jvs (

, closed columns) mice. Uptakes of [³H]carnitine (10 nM) and [¹⁴C]TEA (50 µM) by fibroblasts were measured at 37°C and pH 7.4. In the [¹⁴C]TEA efflux study, cells were preloaded by incubating with 300 µM [¹⁴C]TEA for 60 min at 37°C. The effluxes of [¹⁴C]TEA were measured at 37°C and pH 7.4. *, Significantly different from the uptake by wild-type fibroblasts by Student's t test (p < 0.05). **, Significantly different from the content of [¹⁴C]TEA at 0 min by Student's t test (p < 0.05). The results are shown as means ± S.E.M. of four determinations.

Transport of [¹⁴C]TEA and [³H]Carnitine by Wild-Type and jvs OCTN2-Expressing HEK 293 Cells. To compare the transport activities for carnitine and TEA via mouse OCTN2, we examined the uptakes of carnitine and TEA byHEK 293 cells transfected with cDNA of the wild-type OCTN2 andthe mutated OCTN2 found in jvs mice. In the jvs-derived OCTN2-expressingcells, uptake of [³H]carnitine and [¹⁴C]TEA were both negligible, whereas wild-type OCTN2 exhibitedsignificant increase of transport in usual transport medium containingNa⁺ (Fig. 2A). When the uptakes by wild-type OCTN2-expressing cellswere examined in the presence and absence of Na⁺ (Fig. 2B), [¹⁴C]TEA uptake was maintained in the absence of Na⁺, whereas [³H]carnitine uptake was disappeared. Accordingly, OCTN2 does notrequire Na⁺ for the transport of TEA, and the mutation in jvs OCTN2 (Leu352Arg)commonly leads to loss of transport activities of TEA and carnitine(Nezu et al., 1999).

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Fig. 2. Uptakes of TEA and carnitine by HEK 293 cells transfected with cDNA of wild-type and jvs-mutant OCTN2. Uptakes of [³H]carnitine (10 nM) and [¹⁴C]TEA (50 µM) by the cells were measured for 10 or 30 min, respectively, at 37°C and pH 7.4. (A) Uptakes of carnitine (left) and TEA (right) by cells transfected with the pcDNA vector alone (Mock,

) and the plasmid vector containing cDNA for wild-type OCTN2 (

) and jvs-mutant OCTN2 ( $black-square$ ) in transport buffer containing Na⁺. *, Significantly different from the uptake by jvs-mutant OCTN2-transfected cells by Student's t test (p < 0.05). (B) Uptakes of carnitine (left) and TEA (right) by cells transfected with the pcDNA vector alone (Mock

) and the plasmid vector containing cDNA for wild-type OCTN2 (

), were measured in the absence ( $-$ Na⁺) or presence (+Na⁺) of Na⁺ in the transport buffer. In the absence of Na⁺, Na⁺ was replaced with N-methyl-D-glucamine. *, Significantly different from the uptake by Mock cells by Student's t test (p < 0.05). The results are shown as mean ± S.E.M. of three determinations.

Na⁺-Dependent Inhibition of OCTN2-Mediated [¹⁴C]TEA Uptake by Carnitine. We next examined the inhibitory effect of various concentrations of carnitine on the OCTN2-mediated uptake of [¹⁴C]TEA in the presence and absence of extracellular Na⁺ (Fig. 3). The reduction of [¹⁴C]TEA uptake by carnitine was concentration-dependent, being significantlygreater in the presence of Na⁺. Accordingly, Na⁺ seems to influence the affinity of carnitine for OCTN2.

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Fig. 3. Na⁺-dependent inhibition by carnitine of TEA uptake by OCTN2-expressing HEK 293 cells. The uptakes of [¹⁴C]TEA (100 µM) were measured for 30 min at 37°C in transport buffer, pH 7.4, in the presence of various concentrations of carnitine. The results show the expressed-OCTN2 specific uptake obtained by subtracting the uptake by Mock cells from that by the OCTN2-expressing cells in the presence ( $black-square$ ) or absence (

) of Na⁺ in the transport buffer. Uptake in the absence of Na⁺ was determined by replacing Na⁺ with N-methyl-D-glucamine. The results are shown as means ± S.E.M. of three determinations.

Mutual trans-Stimulation Effects on TEA and Carnitine Transport by OCTN2. To examine the functional coupling of the transport of TEA and carnitine, trans-stimulation effects via OCTN2 were measured.Based on the Na⁺ dependence of carnitine transport and the physiological concentrationof Na⁺, trans-stimulation effects were evaluated by measuring influxand efflux transports of carnitine and TEA, respectively. Afterpreloading of OCTN2-expressing HEK 293 or Mock cells with TEAat 100 µM, 500 µM, or 1 mM, the uptake of a tracer concentrationof [³H]carnitine was evaluated in the presence or absence of Na⁺ (Fig. 4, A and B). In Mock cells, a higher concentration of TEA(1 mM) was used to keep the intracellular TEA concentration ata level similar to that in OCTN2-expressing cells and a similarlevel of TEA uptake at 500 µM, which showed significant effecton carnitine uptake, by OCTN2-expressing cells. When OCTN2-expressingcells were preloaded with TEA, uptake of [³H]carnitine was significantly increased compared with that bythe cells without preloading. The extent of the increment wasdependent on the concentration of TEA preloaded, with a higheruptake at higher concentrations of preloaded TEA (Fig. 4A). Inthe absence of Na⁺, however, no stimulation of the uptake of [³H]carnitine by TEA was observed (Fig. 4B). Thus, efflux of TEAseems to facilitate the Na⁺-dependent carnitine influx.

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Fig. 4. Trans-stimulation of [³H]carnitine uptake (A, B) and [¹⁴C]TEA efflux (C) by OCTN2-expressing HEK 293 cells. In trans-stimulation of [³H]carnitine uptake, OCTN2-expressing (shown as OCTN2) or Mock (shown as Mock) cells were preloaded with 0, 100, 500 µM or 1 mM TEA for 30 min. Subsequently, uptakes of 10 nM [³H]carnitine were measured in the presence (A) or absence (B) of Na⁺ in the transport buffer. In trans-stimulation of [¹⁴C]TEA efflux, cells were preloaded by incubating with 100 (OCTN2-expressing cells, solid lines) or 200 µM (Mock, broken line) [¹⁴C]TEA for 30 min at 37°C (C). The effluxes of [¹⁴C]TEA were measured in the absence (

as control) or presence of 250 µM carnitine ( $open circle$ ), 10 mM TEA ( $triangle$ ) or 1 mM quinidine (

). The results are shown as means ± S.E.M. of three determinations. *, Significantly different from control of OCTN2-mediated uptake by Student's t-test (p < 0.05). **, Significantly different from control of OCTN2-mediated efflux by Student's t test (p < 0.05).

After preincubation of OCTN2-expressing and Mock cells with [¹⁴C]TEA, the efflux transport of [¹⁴C]TEA was measured in the presence and absence of carnitine inthe extracellular medium (Fig. 4C). The efflux rate of [¹⁴C]TEA was higher in OCTN2-expressing cells than in Mock cells.In the presence of a strong inhibitor of OCTN2, quinidine (Ohashiet al., 1999

; Table 2), the efflux rate of [¹⁴C]TEA in OCTN2-expressing cells was decreased level comparablewith that in Mock cells, confirming that [¹⁴C]TEA is exported from the cells via OCTN2. In the presence of250 µM carnitine, which is a normal urinary level (Leschke etal., 1984

), in the extracellular medium, significantly enhancedefflux of [¹⁴C]TEA was observed in OCTN2-expressing cells, whereas such aneffect was not observed in the Mock cells (data not shown). Additionof 10 mM unlabeled TEA to the extracellular efflux medium enhancedthe OCTN2-mediated efflux of [¹⁴C]TEA at the initial 1 min, whereas 2 min after initiation ofefflux, the efflux rate of [¹⁴C]TEA was retarded compared with the control. This result canbe explained by assuming that the unlabeled TEA added to the extracellularefflux medium was gradually taken up by the cells and exertedan inhibitory effect on [¹⁴C]TEA efflux in the same manner as observed in the case of quinidine.Accordingly, these results suggest that OCTN2-mediated TEA effluxis linked with influx of carnitine, as well as TEA itself, byan exchange transportmechanism.

Pharmacokinetic Analysis of [¹⁴C]TEA in Wild-Type and jvs Mice. Pharmacokinetic characteristics of TEA after intravenous administration to wild-type and jvs mice were compared. The timeprofiles of plasma concentration and cumulative urinary excretionof radioactivity of [¹⁴C]TEA are shown in Fig. 5, A and B. The radioactivities in plasmaand urine can largely be ascribed to intact [¹⁴C]TEA, because Mintun et al. (1980) reported that 96% of [¹⁴C]TEA was excreted in urine as an intact form after i.v. administrationin rats. Marked difference in plasma concentration-time curvesat the elimination phase (i.e., 30 min and after) were observedbetween the two types of mice (Fig. 5A). By the compartment analysis,the rate constant of elimination phase in jvs mice was significantlydecreased compared with wild-type mice (wild-type, 0.116 ± 0.01min¹; jvs, 0.059 ± 0.006 min¹; p < 0.05), whereas the rate constants of distribution phasewere not changed between wild-type and jvs mice (wild-type, 0.195± 0.105 min¹; jvs, 0.229 ± 0.040 min¹, p > 0.05). The difference of the slopes at the linear terminalphase suggested that jvs mice have a lower elimination rate thanwild-type mice. The cumulative urinary excretion of radioactivityin jvs mice was significantly lower than that of wild-type micefrom 60 min after administration (Fig. 5B). Pharmacokinetic parametersof [¹⁴C]TEA were calculated from these results. The AUC from time 0to infinity for jvs mice (919 ± 86 µg/min/ml) was significantlyincreased in comparison with that of wild-type mice (553 ± 43µg/min/ml, p < 0.05). GFR, which was estimated from inulin clearance,and the renal clearance (CLr) of TEA were 9.78 ± 0.86 ml/min/kgand 16.0 ± 0.8 ml/min/kg in wild-type mice and 6.34 ± 0.68 ml/min/kgand 9.77 ± 1.19 ml/min/kg for jvs mice, respectively. Based onthese values, the renal secretory clearances (CLs), which representthe renal capability for active secretion of TEA, were evaluatedto be 6.22 ± 0.42 ml/min/kg and 3.43 ± 0.77 ml/min/kg for wild-typeand jvs mice, respectively, showing a 45% decrease in jvs micecompared with wild-type mice. GFR in jvs mice was lower than thatin wild mice, so the renal function of jvs mice was partiallyimpaired. To evaluate the alteration of other epithelial functionthan OCTN2 in jvs mice, the pharmacokinetic characteristics ofcefazolin were evaluated after intravenous administration to wild-typeand jvs mice. Cefazolin is an anionic cephalosporin antibioticthat is not metabolized in the body and mainly excreted into theurine (Brogard et al., 1978; Yamazaki et al., 1981; Tsuji et al.,1983). Furthermore, the mechanisms responsible for the excretionof cefazolin are glomerular filtration and active tubular secretion,which is mediated by organic anion transport system in humansand several animals, including mice (Nightingale et al., 1975;Tsuchiya et al., 1978; Kasher et al., 1983; Tsuji et al., 1985;Takano et al., 1989; Hori et al., 1993). The time profiles ofplasma concentration and cumulative urinary excretion of intactcefazolin are shown in Figs. 6A and 6B and they were very similarbetween the two types of mice. Furthermore, pharmacokinetic parametersof cefazolin calculated were comparable without significant differencesbetween wild-type and jvs mice. For example, the AUC from time0 to infinity for wild-type and jvs mice were 4151 ± 443 µg/min/mland 3586 ± 216 µg/min/ml, respectively. The CLr and CLs valuesof cefazolin were 4.39 ± 0.71 ml/min/kg and 2.83 ± 0.49 ml/min/kg,respectively, in wild-type mice and 5.31 ± 0.34 ml/min/kg and4.41 ± 0.37 ml/min/kg, respectively, for jvs mice. Based on theseobservations, renal secretory transport activity of organic anionsseemed to be maintained in jvs mice. Accordingly, the observeddecrease in CLs of TEA in jvs mice should be ascribed mainly tothe loss of specific secretory activity by OCTN2 for TEA.

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Fig. 5. Plasma concentration (A) and cumulative urinary excretion (B) of [¹⁴C]TEA after intravenous administration to wild and jvs mice. [¹⁴C]TEA was intravenously administered at a dose of 8.8 mg/kg to wild-type ( $open circle$ ) and jvs mice (

). *, Significantly different from wild-type mice by Student's t test (p < 0.05). The results are shown as means ± S.E.M. of four to five mice.

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Fig. 6. Plasma concentration (A) and cumulative urinary excretion (B) of cefazolin after intravenous administration to wild and jvs mice. Cefazolin was intravenously administered at a dose of 20 mg/kg to wild-type ( $open circle$ ) and jvs mice (

). The results are shown as means ± S.E.M. of three to four mice.

Tissue Distribution of [¹⁴C]TEA in Wild-Type and jvs Mice. We examined the tissue distribution of TEA in vivo. The values of tissue-to-plasma concentration ratio (K_p) of [¹⁴C]TEA at 4 h after intravenous administration in wild-type andjvs mice are summarized in Table 1 and compared with those ofcarnitine that have been reported previously (Yokogawa et al.,1999a). The K_p values of TEA in brain, lung, liver, and spleenin jvs mice were significantly lower than those in wild-type mice.In kidney, however, the K_p value of jvs mice (25.0 ± 4.6) wassignificantly higher than that of wild-type mice (9.89 ± 1.16).The K_p values of other tissues were not significantly changedbetween wild-type and jvs mice. The specific increase of K_p valuesin kidney may be explained by the decrease of renal apical secretorytransport activity and the decrease of K_p values in other tissuesmay be explained by the decreased tissue uptake activities.

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TABLE 1
Tissue-to-plasma concentration ratio (K_p) of [¹⁴C]TEA in wild-type and jvs mice
K_p values were obtained 4 h after intravenous administration of [¹⁴C]TEA at a dose of 8.8 mg/kg in wild-type and jvs mice. Each value represents the mean ± S.E.M. of four or five mice.

Inhibition and Transport of Various Compounds in OCTN2-Expressing HEK 293 Cells. To confirm the specificity of OCTN2, the inhibitory effects of various endogenous compounds and xenobiotics on L-[³H]carnitine uptake by OCTN2-expressing cells were examined (Table2). Endogenous cations such as choline, acetylcholine, serotonin,dopamine, norepinephrine, and thiamine showed significant inhibitoryeffects (p < 0.05), whereas guanidine, N¹-methylnicotinamide, epinephrine and histamine, and such organicanions as $alpha$ -ketoglutarate and p-aminohippuric acid were not inhibitory.Furthermore, cationic xenobiotics such as MPP, acetyl- $beta$ -methylcholine,pyrilamine, diphenhydramine, procainamide, lidocaine, quinidine,and verapamil demonstrated significant inhibitory effects.

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TABLE 2
Inhibitory effects of several endogenous compounds and xenobiotics on carnitine uptake by OCTN2-expressing HEK 293 cells
The uptake of [³H]carnitine was measured for 3 min at 37°C in Na⁺-containing transport buffer, pH 7.4, containing each compound. Each value represents the mean ± S.E.M. of three determinations. The data represent the difference in uptakes by Mock and OCTN2-expressing HEK293 cells.

To explore the possible substrates of OCTN2, we measured uptakes of several compounds by OCTN2-expressing cells. Uptakes weremeasured at 5 or 30 min, depending on the tested compounds. Asshown in Table 3, [³H]carnitine and its acyl-derivative [³H]acetyl-L-carnitine were good substrates for OCTN2. Althoughthe background uptake observed in Mock cells was rather high,[³H]verapamil, which is a potent inhibitor of carnitine uptake byOCTN2 (Table 2), exhibited significantly increased uptake inOCTN2-expressing cells. [³H]Pyrilamine, a moderate inhibitor of carnitine transport, wasalso transported by OCTN2. Furthermore, uptake of [³H]MPP, which is a weak inhibitor of OCTN2-mediated carnitine uptake,was slightly but significantly increased, whereas the organicanion [³H]p-aminohippuric acid, which had no inhibitory effect on carnitinetransport, was not transported.

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TABLE 3
Transport of carnitine and various organic cations by OCTN2-expressing HEK 293 cells
The uptakes of [³H]carnitine (10 nM), [³H]acetyl-L-carnitine (7.7 nM), [³H]verapamil (12 nM), [³H]pyrilamine (50 nM), [¹⁴C]TEA (104 µM), [³H]MPP (12 nM), and [³H]PAH (408 nM) in OCTN2-expressing HEK 293 cells were measured for 5 or 30 min at 37°C in Na⁺-containing transport buffer, pH 7.4. Each value represents the mean ± S.E.M. of three experiments by the same batch of transfected cells. C/M ratio was obtained by dividing uptake amount by the concentration of [¹⁴C]TEA in the uptake medium. Net uptake represents the difference in the uptakes between OCTN2-expressing and Mock cells.

	Discussion

Top Abstract Introduction Experimental Procedures Results Discussion References

Cationic xenobiotics and endogenous metabolic products are eliminated through kidney, liver, and intestine by transportersthat exhibit broad substrate specificity (Pritchard and Miller,1993; Oude Elferink et al., 1995; Hunter and Hirst, 1997). Inrenal epithelial cells, membrane potential-dependent organic cationtransporters (OCTs) are functional at basolateral membrane (Zhanget al., 1998; Koepsell et al., 1999; Sweet and Pritchard, 1999),but the apical membrane transporters, which were suggested tobe proton or organic cation/organic cation exchange transporter(s),have not been clearly identified. We found that OCTN1, which showslow structural similarity with OCTs, is strongly expressed inkidney and transports cationic compounds (Tamai et al., 1997;Yabuuchi et al., 1999). Subsequently, we (Tamai et al., 1998;Ohashi et al., 1999) and Wu et al. (1998, 1999) have isolatedand characterized OCTN2 as an organic cation and high-affinityNa⁺-dependent carnitine transporter in human and rat. Because OCTNstransport organic cations as well as carnitine, they may contributein part to the tissue distribution and renal excretion of organiccations (Wu et al., 1998). However, the relevance of OCTNs toorganic cation transport remains uncertain, because of the absenceof an in vivo evaluation of them. In jvs mice, which show theSCD phenotype (Koizumi et al., 1988), there is a functional defectof OCTN2 owing to a single mutated amino acid residue (L352R)of OCTN2, and the physiological significance of OCTN2 as the carnitinetransporter was clearly demonstrated in vivo (Lu et al., 1998;Nezu et al., 1999). In the present study, we studied the roleof OCTN2 in the transport of organic cations and the relationshipof this with carnitine transport, by means of molecular and invivo pharmacokinetical analyses using jvsmice.

The uptake and efflux of [¹⁴C]TEA by embryonic fibroblasts from jvs mice were decreased compared with those by wild mice (Fig.1). Furthermore, the mutated OCTN2 found in jvs mice lacked transportactivity for TEA as well as carnitine (Fig. 2A). These resultssuggest that OCTN2 transports TEA bidirectionally and that jvsmice are suitable to evaluate the OCTN2-mediated organic cationtransport. Because it was reported that P478L and Y211F mutationsof human and rat OCTN2 affected carnitine transport without changein TEA transport activity (Seth et al., 1999), the functionalsite for carnitine on OCTN2 is presumed to be partly shared butnot identical with that of TEA. Based on these observations, theregion of mutation on OCTN2 of jvs mice (L352R) may be essentialin transporting both compounds. Accordingly, we evaluated thesignificance of OCTN2 as an organic cation transporter by usingjvs mice. The disposition of TEA is significantly altered in jvsmice (Fig. 5, A and B; Table 1). The plasma concentration of[¹⁴C]TEA in jvs mice was higher and urinary excretion was delayedcompared with those of wild-type mice. In jvs mice, the GFR estimatedin terms of the clearance of [³H]inulin, which was administered simultaneously with [¹⁴C]TEA, was also lower than that of wild-type mice. These resultsindicated that renal function (glomerular filtration and/or renalblood flow) in jvs mice may be impaired nonspecifically. One reasonfor the decrease of GFR in jvs mice might be severe cardiomyopathy(Horiuchi et al., 1993). Recently, it was demonstrated that therat multispecific organic anion transporter OAT1 mediates therenal secretion of $beta$ -lactam antibiotics, including cefazolin,at the renal basolateral membrane (Jariyawat et al., 1999). Furthermore,mouse and human type-I inorganic phosphate/organic anion transportersare responsible for the urinary secretion of many organic anionssuch as cefazolin at the renal apical membrane (Uchino et al.,2000a,b). So, we examined the effect of cefazolin on the in vitrotransport of carnitine by wild-type and jvs mice fibroblasts andobserved no effect of cefazolin on carnitine uptake (data notshown). In addition, in the present study, the secretory clearanceof cefazolin examined in wild-type and jvs mice was maintained(Fig. 6, A and B). However the renal secretory clearance of [¹⁴C]TEA was significantly low in jvs mice (55% of wild-type mice).So, the decrease in CLs of [¹⁴C]TEA in jvs mice is thought to be specific. Furthermore, theincrease of K_p value of TEA was observed only in kidney (Table1), which is in contrast to the previous observation that theK_p value of [³H]carnitine in kidney of jvs mice was lower than that of wild-typemice (Yokogawa et al., 1999a). In contrast, K_p values of [¹⁴C]TEA in other tissues were decreased in jvs mice compared withthose in wild-type mice (Table 1), which is similar to the observationin [³H]carnitine distribution (Yokogawa et al., 1999). Accordingly,the high K_p value of [¹⁴C]TEA in jvs-mice kidney is specific and can be explained by anincrease of accumulation owing to the decrease in secretory transportacross the apical membrane. From these results, the apparent decreaseof excretion rate of [¹⁴C]TEA into urine can be ascribed to the specific decrease of renalsecretory transport of [¹⁴C]TEA in addition to that of GFR and/or renal blood flow. Furthermore,efflux of [¹⁴C]TEA from the OCTN2-expressing cells was accelerated in the presenceof extracellular TEA, suggesting an exchange transport mechanism.Accordingly, OCTN2 might be one of the organic cation transportersexpressed in the renal apical membrane, possibly an organic cation/organiccationexchanger.

As shown in Table 1, the K_p values of [¹⁴C]TEA in several tissues such as brain, lung, liver and spleen in jvs mice were lowerthan those in wild-type mice, as observed previously in our carnitinestudy (Yokogawa et al., 1999a). However, no significant differencein K_p values of [¹⁴C]inulin, which cannot cross the membrane easily and is a markerof vascular and interstitial fluids, was observed between wild-typeand jvs mice in most tissues (data not shown). The alterationof K_p values in heart, brain and lung is apparently correlatedwith the tissue expression profile of OCTN2 (Tamai et al., 2000).This implies that the OCTN2 contributes at least in part to distributionof TEA in these tissues. The K_p values of [³H]carnitine in the kidney and liver in jvs mice were significantlylower than that of wild-type mice (Yokogawa et al., 1999a) andjvs mice lack in ability of reabsorption of carnitine in kidney(Horiuchi et al., 1994). So, the finding suggested that OCTN2is located on the brush-border membrane in kidney and on the basolateral(sinusoidal) membrane in liver. Therefore, OCTN2 contributes greatlyto the hepatic uptake of [¹⁴C]TEA from blood, which is in accordance with our previous observationin hepatic carnitine transport (Yokogawa et al., 1999b,c). Here,however, the K_p values of [¹⁴C]TEA in lung, heart, liver, kidney, spleen, and gut in jvs miceare unity or above, so TEA is likely to be concentrated by anactive transport system(s) other than OCTN2 (Koepsell et al.,1999). Furthermore, alteration of K_p values of [¹⁴C]TEA was not necessarily correlated with that of [³H]carnitine in a few tissues (Table 1). So, other transporters,such as OCT family and OCTN1, which accept TEA as substrate, maygreatly contribute to the distribution of organic cations in thesetissues.

Another point of interest is the possible coupling of carnitine influx and TEA efflux. Efflux of TEA from the cells was enhancedby expression of OCTN2, demonstrating that TEA is bidirectionallytransported by OCTN2, which is in accordance with the observationin wild-type fibroblasts. The reduced efflux in the presence ofquinidine confirmed that TEA efflux is mediated by OCTN2, becausequinidine is a strong inhibitor of OCTN2 (Table 2) and is takenup efficiently even by Mock cells (Yabuuchi et al., 1999). Inthe present study, OCTN2-mediated efflux of TEA was enhanced inthe presence of extracellular carnitine. Furthermore, Na⁺-dependent carnitine uptake by the OCTN2-expressing cells wasstimulated by preloaded TEA in a concentration-dependent manner(Figs. 4, A-C). These observations indicate that the influx ofcarnitine and the efflux of TEA are linked and the coupling enhancesthe two transport processes. As shown in Fig. 2B, carnitine transportvia OCTN2 requires Na⁺, whereas TEA transport does not, and Na⁺ affects the affinity for OCTN2 (Fig. 3). From these observations,the molecular mechanism of carnitine/TEA transport via OCTN2 atthe renal apical membrane was postulated as shown in Fig. 7. Becausethe luminal side of the membrane is rich in Na⁺, carnitine is taken up efficiently by the epithelial cells viaOCTN2. When the transporting site is oriented from the outer tothe inner cellular domain by transporting carnitine, the sitewill be inactivated for carnitine transport because of the inside-directedNa⁺ gradient (intracellular low concentration of Na⁺). So, TEA, which is accumulated from the blood by basolateraltransporter OCTs, can be a better substrate and is transportedout of the cells apparently via an exchange mechanism betweencarnitine and TEA. So, the difference of Na⁺ dependence between carnitine and TEA transports determines thedirection under physiological circumstances. A similar findingwas obtained for the y⁺L-type amino acid transport system, which exchanges intracellularcationic amino acid with extracellular neutral amino acid in anNa⁺-dependent manner at the renal epithelial cells (Chillaron etal., 1996; Pfeiffer et al., 1999).

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Fig. 7. Proposed model of the transport mechanisms of carnitine and organic cations by OCTN2. After binding of Na⁺ to the outer surface of OCTN2, the carnitine binding site is activated as shown by the change of the shaded triangle (1) to a square (2) and carnitine is transported into the inner side of the membrane (3 and 4). Because of the presence of the inward-directed Na⁺ gradient, the affinity of carnitine for OCTN2 is reduced on the inner membrane side, and TEA binds to OCTN2 (5 and 6). Subsequently, TEA is transported out of the cells. TEA is transported into cells from the outside in the absence of Na⁺. This model explains the Na⁺ dependence and independence of carnitine and TEA transport, respectively. Furthermore, the two substrates are transported via an exchange mechanism and exhibit a mutual trans-stimulation effect. When the transporter is loaded with carnitine or TEA, it functions more efficiently than the unloaded form, resulting in a trans-stimulation effect. Because carnitine is a zwitterion and TEA is a cation, the anionic moiety of carnitine may require a specific site, which is not involved in TEA binding, on OCTN2. The Na⁺ binding site must be specific to carnitine and was therefore assumed to be located near the binding site of carboxyl group of carnitine, which should not overlap with the TEA binding site.

As summarized in Table 2, various cationic compounds inhibit carnitine transport by OCTN2. In addition, some of them aretransported by OCTN2 (Table 3). Interestingly, among them, carnitineand its structural analog, acetylcarnitine, are transported ina Na⁺-dependent manner, whereas cationic compounds such as TEA shownegligible Na⁺ dependence (Tamai et al., 1998; Wu et al., 1998, 1999; Ohashiet al., 1999). So, those compounds that do not require Na⁺ may be exchanged with carnitine, as observed in the case of TEAefflux, suggesting that reabsorption of carnitine is accompaniedwith accelerated elimination of organic cations and that the secretorytransport of organic cations via OCTN2 energizes reabsorptionof carnitine. The circulating organic cations are concentratedin the epithelial cells by the basolaterally localized OCT transporterand are subsequently secreted into urine across the apical membraneby OCTN2 as one of the apical-type organic cation transportersin the renal tubular epithelialcells.

In conclusion, an involvement of OCTN2 in the tissue distribution and renal secretion of organic cations was demonstratedby using OCTN2-expressing cells and jvs mice. Furthermore, molecularmechanism of multifunctionality of OCTN2 was proposed by hypothesizingan exchange transport of Na⁺-dependent carnitine reabsorption and Na⁺-independent secretion of organiccations.

	Acknowledgments

We thank Dr. H. Uchino and Mr. Y. Yamaguchi for helpful discussions and technicalassistance.

	Footnotes

Received July 7, 2000; Accepted November 11, 2000

This study was partly supported by a Grant-in-Aid for Scientific Research from the Ministry of Education, Science, Sportsand Culture,Japan.

Send reprint requests to: Prof. Akira Tsuji, Ph.D., Department of Pharmacobio-Dynamics, Faculty of Pharmaceutical Sciences, Kanazawa University, 13-1 Takara-machi, Kanazawa 920-0934, Japan. E-mail: tsuji{at}kenroku.kanazawa-u.ac.jp

	Abbreviations

TEA, tetraethylammonium; jvs, juvenile visceral steatosis; SCD, systemic carnitine deficiency; MPP, 1-methyl-4-phenylpyridinium; HEK, human embryonic kidney; NMG, N-methylglucamine; GFR, glomerular filtration rate; AUC, area under plasma concentration-time curve; CLr, renal clearance; CLs, renal secretory clearance; K_p, tissue-to-plasma concentration ratio.

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