PREDOMINANT CONTRIBUTION OF ORGANIC ANION TRANSPORTING POLYPEPTIDE OATP-B (OATP2B1) TO APICAL UPTAKE OF ESTRONE-3-SULFATE BY HUMAN INTESTINAL CACO-2 CELLS

Yoshimichi Sai, Yosuke Kaneko, Satsuki Ito, Keisuke Mitsuoka, Yukio Kato, Ikumi Tamai, Per Artursson, and Akira Tsuji

Division of Pharmaceutical Sciences, Graduate School of Natural Science and Technology, Kanazawa University, Kakuma, Kanazawa, Japan (Y.S., Yo.K., S.I., K.M., Yu.K., A.T.); Department of Molecular Biopharmaceutics, Faculty of Pharmaceutical Sciences, Tokyo University of Science, Yamasaki, Noda, Japan (I.T.); and Department of Pharmacy, Uppsala University, Uppsala, Sweden (P.A.)

(Received January 30, 2006; accepted May 17, 2006)

Abstract

Top
Abstract
Materials and Methods
Results
Discussion
References

Human organic anion transporting polypeptide OATP-B (OATP2B1)is a pH-sensitive transporter expressed in the apical membranesof small intestinal epithelial cells. In this study, we haveexamined the contribution of OATP-B to the uptake of [³H]estrone-3-sulfatein Caco-2 cells in comparison with those of its homologs OATP-D(OATP3A1) and OATP-E (OATP4A1). Immunocytochemical study revealedthat OATP-B is expressed in the apical membranes of Caco-2 cells.The uptake of [³H]estrone-3-sulfate by Caco-2 cells was Na⁺-independentand inhibited by several organic anions. It showed biphasicsaturation kinetics with K_m values of 1.81 µM and 1.40mM. The uptake of [³H]estrone-3-sulfate by human embryonic kidney(HEK) 293 cells stably expressing OATP-B (HEK293/OATP-B) wasalso Na⁺-independent and inhibited by several organic anions.The K_m value for estrone-3-sulfate uptake by OATP-B (1.56 µM)was close to that for the high-affinity component observed inCaco-2 cells. The mRNA expression level of OATP-B was higherthan that of OATP-D or OATP-E in Caco-2 cells and in human jejunumbiopsies from healthy volunteers. The values of [³H]estrone-3-sulfateuptake normalized to OATP-B mRNA expression were similar inCaco-2 cells and HEK293/OATP-B cells. The specific activityof OATP-B per mRNA expression was much higher than that of OATP-Dand OATP-E. [³H]Estrone-3-sulfate uptake by membrane vesiclesprepared from HEK293/OATP-B cells exhibited an overshoot phenomenonin the presence of an inwardly directed H⁺ gradient, suggestingthat an H⁺ gradient is the driving force of estrone-3-sulfatetransport by OATP-B. These results suggest that OATP-B is predominantlyresponsible for the apical uptake of estrone-3-sulfate in Caco-2cells.

Organic anion transporting polypeptides (OATP, gene symbol SLC21/SLCO)are expressed in various organs and transport endogenous compounds,such as bile acids, peptides, conjugated metabolites, and thyroidhormones, as well as xenobiotic compounds and clinically usedtherapeutic agents, such as pravastatin, benzylpenicillin, anddigoxin (Hsiang et al., 1999

; Tamai et al., 2000a

; Cui et al.,2001

; Kullak-Ublick et al., 2001

). OATP-A (also called OATP1A2)was first isolated from human liver (Kullak-Ublick et al., 1995

).Other members of the OATP family such as OATP-C (OATP2/LST-1/OATP1B1)(Abe et al., 1999

; Hsiang et al., 1999

), OATP8 (LST-2/OATP1B3)(Konig et al., 2000

; Abe et al., 2001

), OATP-B (OATP2B1), OATP-D(OATP3A1), OATP-E (OATP4A1) (Tamai et al., 2000a

; Adachi etal., 2003

), OATP-F (OATP-1C1) (Pizzagalli et al., 2002

), andprostaglandin transporter PGT (OATP2A1) (Lu et al., 1996

) havealso been identified in human. All of these transporters arethought to be involved in the disposition of anionic compoundsin organs, except for OATP-R (OATP4C1), which was recently clonedand efficiently transports digoxin and ouabain at the basolateralmembranes of proximal tubule cells in the kidney (Mikkaichiet al., 2004

Among them, OATP-B is localized at sinusoidal membrane of hepatocytes,like OATP-C and OATP8, and may play a role in hepatic uptakeof organic anions (Konig et al., 2000; Kullak-Ublick et al.,2001). Compared with OATP-C and OATP8, which are almost exclusivelyexpressed in the liver, the tissue distribution of OATP-B isrelatively ubiquitous (Tamai et al., 2000a). In placenta, OATP-Bis localized at the basolateral membrane of the cytotrophoblastand is suggested to be involved in the transport of steroidhormones between the uterus and fetus (St-Pierre et al., 2002;Ugele et al., 2003). In the mammary gland, OATP-B is expressedin myoepithelium that surrounds the ductal epithelial cellsand is thought to transport estrogens to breast tumors and normaltissues (Pizzagalli et al., 2003). We have shown that OATP-Bis also localized at the brush-border membrane of human small-intestinalepithelial cells and transports estrone-3-sulfate and pravastatinin a pH-dependent manner (Kobayashi et al., 2003; Nozawa etal., 2004).

Because the microenvironment of epithelial cells in the smallintestine is acidic, organic anions had been thought to be absorbedvia the epithelial cells by passive diffusion according to thepH-partition hypothesis (Shiau et al., 1985). However, we establishedthe existence of specific carrier-mediated absorption mechanismsfor organic anions in the small intestine (Tamai et al., 1995,1996, 1999, 2000b). OATP-B recognizes various types of organicanions as substrates and has a unique substrate specificity,with greater affinity for sulfate-conjugated compounds thannonconjugates (Kullak-Ublick et al., 2001; Tamai et al., 2001b).Therefore, recent identification of the pH-sensitive transporterOATP-B on intestinal brush-border membranes may imply a rolein the gastrointestinal absorption of organic anions. OATP-Dand OATP-E are also expressed in the small intestine, as wellas OATP-B, but information on the physiological and pharmacologicalsignificance of OATP-B is still limited.

In the present study, to clarify further the contribution ofOATP-B to the transport of organic anions in the small intestine,we quantified the mRNA expression levels of OATP-B, OATP-D,and OATP-E in human jejunum and human intestinal epithelialcell model Caco-2 cells and examined the subcellular localizationof OATP-B protein in Caco-2 cells. In addition, by comparingthe characteristics of estrone-3-sulfate uptake and the mRNAexpression level of OATP-B in Caco-2 cells and in HEK293 cellsstably expressing OATP-B, we evaluated the relative contributionof OATP-B to the uptake of estrone-3-sulfate from the apicalsurfaces of Caco-2 cells.

Materials and Methods

Top
Abstract
Materials and Methods
Results
Discussion
References

Materials. [³H]Estrone-3-sulfate ammonium salt (1.59 TBq/mmol)was purchased from PerkinElmer Life Science Products, Inc. (Boston,MA). The pcDNA3 vector was obtained from Invitrogen (Carlsbad,CA). HEK293 cells were obtained from the Japanese Cancer ResearchResources Bank (Tokyo, Japan). Caco-2 cells were obtained fromAmerican Type Culture Collection (Manassas, VA). All other reagentswere purchased from Sigma Chemicals (St. Louis, MO) and WakoPure Chemical Industries (Osaka, Japan).

Tissue Samples. Human jejunal mucosa biopsies were obtainedusing a Watson capsule from 13 healthy volunteers (on no medication)aged 21 to 52 years (four females and nine males). Biopsiesand all subsequent procedures were carried out with consentfrom the ethical review board of Huddinge University Hospital(Taipalensuu et al., 2001).

Cell Culture. HEK293 cells were routinely grown in Dulbecco'smodified Eagle's medium containing 10% fetal calf serum (LifeTechnologies, Gaithersburg, MD), benzylpenicillin, and streptomycinsulfate in a humidified incubator at 37°C and 5% CO₂. HEK293cells were transfected with OATP-B subcloned into pcDNA3 orpcDNA3 vector alone according to the calcium phosphate precipitationmethod (Tamai et al., 2000a). To obtain HEK293 cells stablyexpressing OATP-B, cells grown on a 60-mm dish were transfectedwith 2 µg of plasmid encoding OATP-B. On the next day,the transfected cells were plated at a density of 2 x 10⁵ cells/dish(100 mm). The cells were cultured in the presence of 1 mg/mlG418 (Sigma), and single colonies were isolated at day 14. Theexpression of OATP-B was screened by measuring the uptake of[³H]estrone-3-sulfate. The established cells stably expressingOATP-B were named HEK293/OATP-B, and the cells expressing pcDNA3were named HEK293/Mock cells. To obtain HEK293 cells transientlyexpressing OATP-B, OATP-D, and OATP-E, each cDNA subcloned intopcDNA3 was transfected into HEK293 cells according to the calciumphosphate precipitation method (Tamai et al., 2000a). Determinationof mRNA expression and transport activity was performed at 2days after the transfection.

Caco-2 cells were cultured as described previously (Tavelinet al., 2002) with minor modifications. Caco-2 cells were routinelygrown in Dulbecco's modified Eagle's medium containing 10% fetalcalf serum (Life Technologies), benzylpenicillin, and streptomycinsulfate in 75-cm² flasks in a humidified incubator at 37°Cunder 10% CO₂. When the cells reached confluence, they wereplated on 2-cm² multiwell dishes at a density of 5 x 10⁵ cells/well,and the medium was changed at 3 h after plating. The cells werecultured for 14 to 15 days before use for each experiment.

RT-PCR Analysis. Total RNAs from HEK293/OATP-B, HEK293/Mock,and Caco-2 cells were purified using an RNeasy Mini Kit (QIAGEN,Valencia, CA) according to the manufacturer's instructions.After treatment of total RNA with DNase I, first strand cDNAwas prepared from 5 µg of total RNA and amplified usingOATP-B-specific primer pairs (5'-TCAAGCTGTTCGTTCTGTGC-3' and5'-GTGTTCCCCACCTCGTTGAA-3'). These primers correspond to nucleotidepositions 321 to 340 (sense) and 474 to 455 (antisense) of OATP-BcDNA. PCR reaction was run for 30 cycles of 94°C for 30s, 55°C for 30 s, and 72°C for 30 s. PCR products wereseparated by 2% agarose gel electrophoresis, followed by stainingwith ethidium bromide.

Immunoblot and Immunocytochemical Study of OATP-B in HEK293/OATP-Band Caco-2 Cells. Immunoblotting and Immunocytochemical stainingwere performed as described previously (Nozawa et al., 2002)with minor modifications. Rabbit polyclonal anti-OATP-B antiserumwas prepared in our previous study using a synthesized carboxyl-terminalpolypeptide of OATP-B with the amino acid sequence CLVSGPGKKPEDSRVas the epitope (Nozawa et al., 2002). This sequence is specificfor OATP-B, being absent in both OATP-D and OATP-E. The specificityof this antibody was confirmed in our previous study (Nozawaet al., 2002). Caco-2 cells were cultured on 15-mm micro coverglasses and fixed with 10% formalin in PBS(–), 100% methanolon ice, and 0.1% Triton X-100 in PBS(–) at room temperature.The cells were incubated for 1 h with polyclonal anti-OATP-Bantiserum diluted 1:1000 in PBS(–) containing 0.1% bovineserum albumin or rabbit normal IgG. At the same time, monoclonalanti-Na⁺/K⁺-ATPase antibody diluted at 1:200 was mixed withthe primary antibodies. After having been washed with PBS(–),the cells were incubated with Alexa Fluoro 594 goat anti-rabbitIgG and Alexa Fluoro 488 goat anti-mouse IgG (Molecular Probes,Inc., Eugene, OR) as the secondary antibodies for 30 min. Then,they were mounted in VECTASHIELD mounting medium (Vector Laboratories,Burlingame, CA) and examined with a confocal laser scanningmicroscope LSM510 (Carl Zeiss GmbH, Jena, Germany).

Transport Experiments in HEK293 Cells and Caco-2 Cells. HEK293/OATP-Band HEK293/Mock cells were cultured for 3 days on 15-cm dishes.They were harvested and suspended in an incubation medium [125mM NaCl, 4.8 mM KCl, 5.6 mM D-glucose, 1.2 mM CaCl₂, 1.2 mMKH₂PO₄, 12 mM MgSO₄, and 25 mM HEPES-Tris (pH 7.4)]. The cellsuspension was preincubated at 37°C for 20 min in the incubationmedium (pH 7.4) and then centrifuged, and the resultant cellpellets were mixed with the uptake medium (pH 6.0 or 7.4) containinga test compound to initiate uptake. The uptake medium containedthe same constituents as the suspension medium except for 25mM MES in place of HEPES and was adjusted to pH 6.0 with Tris.In Na⁺-free medium, NaCl was replaced with lithium chloride,potassium chloride, rubidium chloride, choline chloride, orN-methyl-D-glucamine (NMG) chloride. At appropriate times, aliquotsof the mixture were withdrawn, and the cells were separatedfrom the uptake medium by centrifugal filtration through a layerof a mixture of silicone oil (SH550; Toray Dow Corning Co.,Tokyo, Japan) and liquid paraffin (Wako Pure Chemical Industries)with a density of 1.03. Each cell pellet was solubilized in3 N KOH and then neutralized with HCl. The cell-associated radioactivitywas measured with a liquid scintillation counter using Cleasol-Ias a liquid scintillation fluid (Nacalai Tesque, Kyoto, Japan).

Caco-2 cells were cultured on 2-cm² multiwell dishes for 14to 15 days, and then the transport experiments were performed.The cells were washed with incubation medium [137 mM NaCl, 5.4mM KCl, 25 mM D-glucose, 0.95 mM CaCl₂, 0.44 mM KH₂PO₄, 0.81mM MgSO₄, and 10 mM HEPES-Tris (pH 7.4)]. The cells were preincubatedat 37°C for 10 min in the incubation medium (pH 7.4), thenthe medium was aspirated, and the uptake medium (pH 6.0 or 7.4)containing a test compound was added. Uptake medium containedthe same constituents as the incubation medium except for 10mM MES instead of HEPES and was adjusted to pH 6.0 with Tris.In Na⁺-free medium, NaCl was replaced with lithium chloride,potassium chloride, rubidium chloride, choline chloride, orNMG chloride. At the designated times, the uptake medium wasaspirated, and the cells were washed with ice-cold incubationmedium (pH 7.4). Each cell monolayer was solubilized in 5 NNaOH and then neutralized with HCl. The cell-associated radioactivitywas measured with a liquid scintillation counter using Cleasol-Ias a liquid scintillation fluid.

The content of protein in each cell was measured by the methodreported by Bradford (1976) using a Bio-Rad (Hercules, CA) proteinassay kit. Initial uptake of [³H]estrone-3-sulfate was determinedat 2 min in both cell lines.

Quantitative RT-PCR Analysis. Quantification of the mRNAs codingfor OATP-B, OATP-D, and OATP-E was performed as described previously(Naruhashi et al., 2002) by using LightCycler technology (RocheDiagnostics, Indianapolis, IN). Total RNA was prepared as describedbelow. The cDNA from 5 µg of RNA was used for OATP-B-,OATP-D-, or OATP-E-specific PCR. Primer sets were as follows:OATP-B primers (5'-TCAAGCTGTTCGTTCTGTGC-3' and 5'-GTGTTCCCCACCTCGTTGAA-3'),OATP-D primers (5'-CTGCAACAGCACGAATCTCA-3' and 5'-AGGGATGAAGCCCAACAAAC-3'),and OATP-E primers (5'-GAATACTAGGGGGCATCCCG-3' and 5'-GACGCCCAGCACCTTGTACA-3'),which produce 154-, 265-, and 170-base pair amplicons, respectively.The PCR programs were as follows: OATP-B, initial denaturationat 95°C for 10 min, followed by 50 cycles of denaturationat 95°C for 0 s and combined annealing extension at 56°Cfor 0 s, 72°C for 6 s. OATP-D, initial denaturation at 95°Cfor 10 min, followed by 50 cycles of denaturation at 95°Cfor 0 s and combined annealing extension at 56°C for 0 s,72°C for 10 s. OATP-E, initial denaturation at 95°Cfor 10 min, followed by 50 cycles of denaturation at 95°Cfor 0 s and combined annealing extension at 56°C for 0 s,72°C for 7 s. Each sample of cDNA was diluted with salmonsperm DNA to three different concentrations (i.e., 1, 4, and16 ng/µl) for quantification. The standard curve for thereal-time PCR analysis was generated by using gel-purified PCRproducts that had been quantified by measuring the UV absorbance(A₂₆₀) and diluted with salmon sperm DNA to 1 x 10¹ to 1 x 10⁸copy/µl. The copy number was calculated based on the conversionformulas: 1 A₂₆₀ unit of ssDNA = 33 µg/ml H₂O; averagemolecular mass of cDNA = number of bases x 330 Da. The efficiencyof the reverse-transcription was assumed to be 100%. mRNA expressionis given as the copy number per unit RNA amount (copy per nanogramof total RNA).

Transport Experiments in Membrane Vesicles. The membrane vesicleswere prepared essentially as described previously (Tamai etal., 2001a). In brief, HEK293/OATP-B or HEK293/Mock cells werecultured in the presence of 1 mg/ml G418. The confluent cellswere harvested, washed, suspended in 25 ml of buffer I [10 mMNaCl, 1.5 mM MgCl₂, 0.02 mM phenylmethanesulfonyl fluoride,and 10 mM HEPES-Tris (pH 7.4)], and placed on ice for 30 min.The cells were disrupted using a Nitrogen Bomb (Parr 4635) at700 psi, homogenized, and separated by sucrose gradient centrifugation,and membrane vesicles were finally obtained as a pellet aftercentrifugation at 100,000g for 3 h. The final pellet was suspendedin buffer II [250 mM sucrose, 0.02 mM phenylmethanesulfonylfluoride, and 10 mM HEPES-Tris (pH 7.4)] and stored at –80°Cuntil it was used. The content of protein in each preparationwas measured by using a Bio-Rad protein assay kit. Transportstudies were performed by a rapid filtration technique at 37°C.Membrane vesicles stored at –80°C were thawed rapidlyat 37°C and kept on ice. After the vesicles had been preincubatedfor 20 min at 37°C, 10 µl of the membrane vesiclesuspension containing 10 µg of protein was mixed with90 µl of solution containing the test compound in bufferIII [250 mM sucrose and 10 mM MES-Tris (pH 6.0) or HEPES-Tris(pH 7.4)] to initiate uptake reactions. The uptake was terminatedby diluting the mixture with 1 ml of buffer IV [260 mM sucrose,0.1 mM estrone-3-sulfate, and 10 mM HEPES-Tris (pH 7.4)] at4°C, and the mixture was immediately filtered through amembrane filter (GVWP02500, 0.22-µm pore size; Millipore)that had been presoaked with a 0.1 mM estrone-3-sulfate solutionovernight and washed three times with buffer IV. The radioactivityretained on the membrane filter was quantitated with a liquidscintillation counter. The background radioactivity was evaluatedby mixing an ice-cold [³H]estrone-3-sulfate solution with membranevesicles that had previously been diluted with ice-cold bufferIV, immediately followed by filtration.

Data Analysis. All data are expressed as means ± S.E.M.unless otherwise noted, and statistical analysis was performedwith Student's t test, taking p < 0.05 as the criterion ofsignificance. Cell-to-medium (C/M) or vesicle-to-medium (V/M)ratio was obtained by dividing the cellular or vesicular uptakeamount (mol/mg protein), respectively, by the concentrationof test compound in the medium (moles per liter). Kinetic parameterswere estimated using either of the following equations, whichconsist of one or two saturable Michaelis-Menten componentscombined with a nonsaturable component:

Formula

Formula
where V, S,V_max, K_m, and k_ns represent the initial uptake velocity, substrateconcentration, maximum uptake velocity, Michaelis constant,and nonsaturable uptake clearance, respectively. The fittingwas performed by nonlinear least-squares regression analysisusing the MULTI program (Yamaoka et al., 1981). Validity ofthe model was verified based on Akaike's Information Criterion.

Results

Top
Abstract
Materials and Methods
Results
Discussion
References

mRNA Expression Levels of OATP-B, OATP-D, and OATP-E in HumanJejunum and Caco-2 Cells. We quantitatively investigated themRNA expression levels of OATPs in the human jejunum using biopsysamples from 13 healthy volunteers and Caco-2 cells (Table 1).Real-time quantitative PCR analysis was performed three timesat different dilutions for each sample. The mRNA expressionlevel of OATP-B was much higher than that of OATP-D or OATP-Ein human jejunum (p < 0.05) and in Caco-2 cells. The mRNAexpression level of villin, an epithelial cell-specific gene,was also measured to evaluate the relative content of epithelialcells. The villin-normalized mRNA expression level of OATP-Bin human jejunum varied 9-fold from the lowest to the highestlevel, suggesting that there is considerable variation amongindividuals.

View this table:
[in this window]
[in a new window]

TABLE 1 mRNA expression level of OATP-B, OATP-D, OATP-E, and villin in human jejunal biopsy sample and Caco-2 cells examined by quantitative real-time PCR analysis

Subcellular Localization of OATP-B in Caco-2 Cells. OATP-B islocalized at apical membranes of enterocytes in human smallintestine (Nozawa et al., 2004). In the present study, therefore,localization of OATP-B in Caco-2 cells was examined using anti-OATP-Bantibody. OATP-B was localized at the apical surface of Caco-2cells, as shown by red staining in Fig. 1. In the control experimentwith rabbit normal IgG, the signal was negligible (Fig. 1).Na⁺/K⁺-ATPase, a marker protein known to be localized at thebasal membrane of intestinal epithelial cells, was stained green,and there was no crossover signal with OATP-B (Fig. 1). Thesedata suggest that OATP-B is predominantly localized at the apicalmembrane of Caco-2 cells.

View larger version (50K):
[in this window]
[in a new window]

FIG. 1. Confocal laser scanning microscopic analysis of immunocytochemical localization of OATP-B protein in Caco-2 cells. A, immunocytochemical detection of OATP-B (red) and Na⁺/K⁺-ATPase (green) in Caco-2 cell monolayers was performed using anti-OATP-B antibody (a–c) or rabbit normal IgG (d–f) and anti-Na⁺/K⁺-ATPase antibody (a–f) as a basolateral marker. Images (x–y sections) were taken through Caco-2 cell monolayers from the apical to basal surfaces: at the apical surface (a and d), 5.1 µm below the apical surface (b and e), and 11 µm below the apical surface (c and f) of the monolayers. The scale bar represents 10 µm. B, side view (x–z reconstruction) showing localization of OATP-B and Na⁺/K⁺-ATPase in each monolayer. The upper and lower sides of the images represent the apical and basal cell membranes, respectively. a, double staining with anti-OATP-B and anti-Na⁺/K⁺-ATPase antibodies; b, double staining with rabbit normal IgG and anti-Na⁺/K⁺-ATPase antibody. The secondary antibodies used were Alexa 488-labeled goat anti-mouse IgG and Alexa 594-labeled goat anti-rabbit IgG.

Effect of Extracellular pH on Uptake of [³H]Estrone-3-sulfateby HEK293/OATP-B and Caco-2 Cells. We compared the transportcharacteristics of OATP-B and those of Caco-2 cells to examinethe possible involvement of this transporter in the uptake ofestrone-3-sulfate by Caco-2 cells. For this purpose, we haveestablished a cell line stably expressing OATP-B (HEK293/OATP-B).The expression of OATP-B was examined by RT-PCR and Westernblot analysis. A band corresponding to OATP-B was observed inCaco-2 and HEK293/OATP-B cells, but not in HEK293/Mock cells(Fig. 2A). The expression of OATP-B protein was also observedin Caco-2 and HEK293/OATP-B cells (Fig. 2B).

View larger version (33K):
[in this window]
[in a new window]

FIG. 2. RT-PCR and Western blot analysis of OATP-B in HEK293/OATP-B, HEK293/Mock, and Caco-2 cells. A, RT-PCR using specific primers for OATP-B was performed with total RNA prepared from HEK293/OATP-B (lanes 1 and 2), HEK293/Mock (lane 3 and 4), and Caco-2 cells (lanes 5 and 6). Reverse transcription was performed in the presence (lanes 1, 3, and 5) or absence (lanes 2, 4, and 6) of reverse transcriptase. PCR products were separated by 2% agarose gel electrophoresis, followed by staining with ethidium bromide. B, crude membrane fraction was prepared from HEK293/OATP-B (lane 1) and Caco-2 (lanes 2 and 3) cells followed by treatment with peptide N-glycosidase F to remove sugar modification (lanes 1 and 3). Each of the protein samples was subjected to SDS-polyacrylamide gel electrophoresis and immunoblotting using anti-OATP-B antibody. M, molecular mass marker.

First, the pH dependence of [³H]estrone-3-sulfate uptake wascompared between HEK293/OATP-B and Caco-2 cells. [³H]Estrone-3-sulfateuptake by HEK293/OATP-B cells was much higher than that by HEK293/Mockcells, and the uptake was higher at pH 6.0 than at pH 7.4 (Fig. 3, A and B).Unlabeled estrone-3-sulfate (100 µM) decreased the uptakeof [³H]estrone-3-sulfate in HEK293/OATP-B cells (p < 0.05)to the level of HEK293/Mock cells (Fig. 3, A and B). On theother hand, [³H]estrone-3-sulfate uptake by Caco-2 cells wasalso inhibited by unlabeled estrone-3-sulfate (4 mM) (p <0.05), and the uptake at pH 6.0 tended to be higher than thatat pH 7.4, although the pH dependence was not great (Fig. 3, C and D).

View larger version (27K):
[in this window]
[in a new window]

FIG. 3. Time course of uptake of [³H]estrone-3-sulfate by HEK293/OATP-B, HEK293/Mock, and Caco-2 cells. Uptake of [³H]estrone-3-sulfate (4.7 nM) by HEK293/OATP-B or HEK293/Mock cells over 10 min was measured at 37°C in the uptake medium at pH 6.0 (A) or pH 7.4 (B) after preincubation for 20 min at 37°C in the incubation medium (pH 7.4). Uptake of [³H]estrone-3-sulfate (4.7 nM) by Caco-2 cells over 30 min was measured at 37°C in the uptake medium at pH 6.0 (C) or pH 7.4 (D) after preincubation for 10 min at 37°C in the incubation medium (pH 7.4). Closed and open circles represent the uptake in the absence or presence of unlabeled (100 µM for HEK293 and 4 mM for Caco-2 cells) estrone-3-sulfate, respectively. Closed and open triangles represent the corresponding values for HEK293/Mock cells (A and B). Each result represents the mean ± S.E.M. (n = 4). *, significantly different from the value measured in the presence of unlabeled estrone-3-sulfate (p < 0.05).

Effect of Extracellular Cations on Uptake of [³H]Estrone-3-sulfateby HEK293/OATP-B and Caco-2 Cells. The absence of Na⁺ dependenceis a well known characteristic of transport mediated by OATP-B.Therefore, we examined the Na⁺ dependence to see whether thetransport characteristics of Caco-2 cells matched those of OATP-B.Extracellular Na⁺ was replaced with other cations (Li⁺, K⁺,Rb⁺, choline⁺, and NMG⁺), and the uptake of [³H]estrone-3-sulfatewas examined (Fig. 4). Replacement of extracellular cationshad little effect on the uptake of [³H]estrone-3-sulfate inboth cell lines. Uptake was slightly decreased with cholineand NMG, and this is consistent with the properties of otherOATP family members (Hagenbuch and Meier, 2003

View larger version (21K):
[in this window]
[in a new window]

FIG. 4. Effects of extracellular cations on uptake of [³H]estrone-3-sulfate by HEK293/OATP-B (A) and Caco-2 (B) cells. A, HEK293/OATP-B cells were preincubated for 20 min at 37°C in the incubation medium (pH 7.4). Uptake of [³H]estrone-3-sulfate (4.7 nM) over 2 min was then measured at 37°C by incubating cells in the uptake medium at pH 6.0. The results were normalized by the uptake in the presence of Na⁺ after correcting for the uptake by HEK293/Mock cells. Each result represents the mean ± S.E.M. (n = 4). B, Caco-2 cells were preincubated for 10 min at 37°C in the incubation medium (pH 7.4). Uptake of [³H]estrone-3-sulfate (4.7 nM) over 2 min was then measured at 37°C by incubating cells in the uptake medium at pH 6.0. The results were normalized by the uptake in the presence of Na⁺. Each result represents the mean ± S.E.M. (n = 3). *, significantly different from the control (p < 0.05).

Kinetic Analysis of [³H]Estrone-3-sulfate Uptake by HEK293/OATP-Band Caco-2 Cells. Initial uptake rates of estrone-3-sulfateby HEK293/OATP-B cells at concentrations ranging from 4.7 nMto 15 µM exhibited saturation (Fig. 5A). Eadie-Hofsteeplots showed a single straight line, the K_m and V_max valuesbeing 1.56 ± 0.10 µM and 1.15 ± 0.04 nmol/mgprotein/2 min, respectively (Fig. 5B). The K_m value is similarto those reported by others (2–9 µM; Tamai et al.,2001b

; Pizzagalli et al., 2003

). On the other hand, biphasicsaturation kinetics was observed when the initial uptake ofestrone-3-sulfate by Caco-2 cells was examined at concentrationsranging from 4.7 nM to 4 mM (Fig. 5, C and D), suggesting thepresence of two kinetically distinct saturable components. TheK_m values of the high- and low-affinity sites were 1.81 ±0.94 µM and 1.40 ± 0.01 mM, and the V_max valueswere 0.134 ± 0.011 and 24.5 ± 1.1 nmol/mg protein/2min, respectively (Fig. 5, C and D). By comparing the valuesof the V_max/K_m ratio for high- and low-affinity sites, the contributionof the high-affinity site to overall uptake clearance was estimatedto be approximately 4 times larger than that of the low-affinitysite at low concentrations.

View larger version (29K):
[in this window]
[in a new window]

FIG. 5. Concentration dependence of uptake of [³H]estrone-3-sulfate by HEK293/OATP-B, HEK293/Mock, and Caco-2 cells. A, uptake of estrone-3-sulfate at various concentrations for 2 min was measured at pH 6.0 and 37°C in HEK293/OATP-B (closed circles) and HEK293/Mock (open circles) cells. Dotted and solid lines represent nonsaturable uptake observed in HEK293/Mock cells and saturable uptake mediated by OATP-B, respectively, both of which were obtained from nonlinear least-squares regression analysis as described under Materials and Methods. Each result represents the mean ± S.E.M. (n = 4). B, OATP-B-mediated uptake of estrone-3-sulfate at various concentrations at pH 6.0 is shown as an Eadie-Hofstee plot. The straight line was obtained by fitting based on nonlinear least-squares regression analysis. C, uptake of estrone-3-sulfate at various concentrations for 2 min was measured at pH 6.0 and 37°C. Dotted and solid lines represent the nonsaturable and saturable uptake, respectively, obtained from nonlinear least-squares regression analysis of the total uptake (closed circles). Each result represents the mean ± S.E.M. (n = 3). D, saturable uptake of estrone-3-sulfate is shown as an Eadie-Hofstee plot. The straight line was obtained by fitting based on nonlinear least-squares regression analysis.

Inhibitory Effects of Various Compounds on Uptake of [³H]Estrone-3-sulfateby HEK293/OATP-B and Caco-2 Cells. To compare substrate recognitionspecificity between Caco-2 and HEK293/OATP-B cells, the inhibitoryeffects of various compounds were examined. In addition to estrone-3-sulfate,OATP-B can transport BSP (sulfobromophthalein), DHEAS (dehydroepiandrosteronesulfate), pravastatin, and benzylpenicillin (Tamai et al., 2000a;Kullak-Ublick et al., 2001; Nozawa et al., 2004). Therefore,the IC₅₀ values of those four compounds were examined. The [³H]estrone-3-sulfateuptake by HEK293/OATP-B and Caco-2 cells was strongly inhibitedby BSP and DHEAS, both of which are sulfate conjugates (Fig. 6,Table 2). Pravastatin and benzylpenicillin also inhibited theuptake of [³H]estrone-3-sulfate in both HEK293/OATP-B and Caco-2cells (Fig. 6). The IC₅₀ values for DHEAS, pravastatin, andbenzylpenicillin were similar in HEK293/OATP-B and Caco-2 cells,whereas that for BSP exhibited a 10-fold difference (Table 2).These IC₅₀ values are not very different from the reported K_mvalues for transport of BSP (0.7 µM), DHEAS (9 µM),and pravastatin (2 mM) by OATP-B (Kullak-Ublick et al., 2001;Pizzagalli et al., 2003; Nozawa et al., 2004). In addition,the uptake of [³H]estrone-3-sulfate was inhibited by severalorganic anions and monocarboxylic acids but not by organic cationsexcept cimetidine (Fig. 7). The inhibition profiles were similarfor HEK293/OATP-B and Caco-2 cells (Fig. 7).

View larger version (25K):
[in this window]
[in a new window]

FIG. 6. Inhibitory effect of BSP (open circles), DHEAS (closed circles), pravastatin (open squares), and benzylpenicillin (closed squares) on uptake of [³H]estrone-3-sulfate by HEK293/OATP-B and Caco-2 cells. A, HEK293/OATP-B cells were preincubated for 20 min at 37°C in the incubation medium (pH 7.4). Uptake of [³H]estrone-3-sulfate (4.7 nM) was then measured for 2 min at 37°C by incubating cells in the uptake medium at pH 6.0. The results are shown as a percentage of control uptake after correcting for the uptake by HEK293/Mock cells. Each result represents the mean ± S.E.M. (n = 4). B, Caco-2 cells were preincubated for 10 min at 37°C in the incubation medium (pH 7.4). Uptake of [³H]estrone-3-sulfate (4.7 nM) over 2 min was then measured at 37°C by incubating cells in the uptake medium at pH 6.0. The results are shown as percentage of control uptake. Each result represents the mean ± S.E.M. (n = 3).

View this table:
[in this window]
[in a new window]

TABLE 2 IC₅₀ values for the inhibitory effects of typical substrates of OATP-B on uptake of [³H]estrone-3-sulfate by HEK293/OATP-B and Caco-2 cells

View larger version (27K):
[in this window]
[in a new window]

FIG. 7. Inhibitory effect of various compounds on uptake of [³H]estrone-3-sulfate by HEK293/OATP-B and Caco-2 cells. A, HEK293/OATP-B cells were preincubated for 20 min at 37°C in the incubation medium (pH 7.4). Uptake of [³H]estrone-3-sulfate (4.7 nM) was then measured for 2 min at 37°C or 4°C by incubating cells in the uptake medium at pH 6.0. The results are shown as a percentage of control uptake after correcting for the uptake by HEK293/Mock cells. Each result represents the mean ± S.E.M. (n = 4). B, Caco-2 cells were preincubated for 10 min at 37°C in the incubation medium (pH 7.4). Uptake of [³H]estrone-3-sulfate (4.7 nM) over 2 min was then measured at 37°C or 4°C by incubating cells in the uptake medium at pH 6.0. The results are shown as a percentage of control uptake. Each result represents the mean ± S.E.M. (n = 3). *, significantly different from the control (p < 0.05). DIDS, 4,4'-diisothiocyanostilbene-2–2'-disulfonic acid.

Transport of [³H]Estrone-3-sulfate Observed in Caco-2 CellsCan Be Accounted for by OATP-B's Expression Level and IntrinsicTransport Activity. To know whether OATP-B can account for theobserved [³H]estrone-3-sulfate transport activity in Caco-2cells, we next examined 1) the mRNA copy number of OATP-B inCaco-2 cells and 2) the linearity of the relationship betweenOATP-B mRNA expression level and [³H]estrone-3-sulfate transportactivity. HEK293 cells were transiently transfected with differentamounts of OATP-B cDNA plasmids, and using the same batch oftransfectants, the relationship between mRNA expression andinitial uptake clearance of [³H]estrone-3-sulfate was examined(Fig. 8). The transport activity in HEK293 cells was increased(9.75–348 µl/mg protein/min) with increase in thetransfected amount of OATP-B cDNA (1–20 µg/culturedish) (Fig. 8). A double logarithmic plot of initial uptakeclearance of [³H]estrone-3-sulfate versus mRNA expression ofOATP-B in HEK293 cells was linear within the range of 3200 to91,800 copy/ng total RNA (Fig. 8). Based on this correlation,OATP-B mRNA expression in Caco-2 cells (9030 copy/ng total RNA)can account for approximately 20 to 30 µl/mg protein/minof initial uptake clearance, which was close to the actual uptakeactivity observed in Caco-2 cells [17.2 µl/mg protein/min,Fig. 8, broken line; and the V_max/K_m value of the high-affinitysite (37.0 µl/mg protein/min, Fig. 5, C and D)]. Moreover,as Caco-2 cells express OATP-D (34.9 copy/ng total RNA) andOATP-E (154 copy/ng total RNA) (Table 1), the contributionsof those transporters to the [³H]estrone-3-sulfate uptake werealso assessed. When HEK293 cells were transfected with plasmidencoding OATP-D cDNA, the [³H]estrone-3-sulfate uptake by thecells was as small as the nonsaturable endogenous transportactivity of nontransfected HEK293 cells (3.02 µl/mg protein/min),although 69,200 copy/ng total RNA of OATP-D mRNAs was expressedin the transfected cells (Fig. 8, triangle). In the case ofOATP-E transfection, the uptake activity and mRNA expressionlevel were 10.8 µl/mg protein/min and 30,200 copy/ng totalRNA, respectively (Fig. 8, square). The uptake activity of OATP-E-transfectedcells was much smaller than that via OATP-B, even when the mRNAexpression levels for both OATPs were comparable (Fig. 8). Consideringthe relatively low transport activity per mRNA copy in HEK293cells and the very low mRNA expression level in Caco-2 cells,neither OATP-D nor OATP-E can be a major transporter for [³H]estrone-3-sulfateuptake in Caco-2 cells. These results suggest that OATP-B, butnot OATP-D or OATP-E, is the predominant contributor to estrone-3-sulfateuptake by Caco-2 cells.

View larger version (18K):
[in this window]
[in a new window]

FIG. 8. Initial uptake clearance of [³H]estrone-3-sulfate and mRNA expression of OATP-B, OATP-D, and OATP-E in Caco-2 cells and HEK293 cells expressing OATP-B, OATP-D, and OATP-E. Initial uptake clearance of [³H]estrone-3-sulfate (4.7 nM) and mRNA expression level of OATP-B (circles), OATP-D (triangle), or OATP-E (square) were measured in HEK293 cells transiently transfected with OATP-B, OATP-D, or OATP-E cDNA in various amounts of plasmid. For comparison, uptake clearance of [³H]estrone-3-sulfate in Caco-2 cells is shown as a broken line. mRNA expression levels of OATP-B, OATP-D, or OATP-E in Caco-2 cells are shown with arrows: (B), (D), or (E), respectively. The gray bar represents nonsaturable transport of [³H]estrone-3-sulfate in Caco-2 and HEK293 cells.

Transport of [³H]Estrone-3-sulfate by OATP-B Depends on an H⁺-Gradient.Uptake of [³H]estrone-3-sulfate by membrane vesicles expressingOATP-B was examined. In the presence of an inwardly directedH⁺-gradient (pH_out/pH_in = 6.0:7.4), the uptake of [³H]estrone-3-sulfateby OATP-B vesicles was much higher than that by Mock vesicles(p < 0.05) and showed an overshoot phenomenon (Fig. 9A).The overshoot uptake was not observed in the presence of anH⁺-ionophore, FCCP (Fig. 9A). In the absence of the H⁺-gradient(pH_out/pH_in = 7.4:7.4), no overshoot uptake of [³H]estrone-3-sulfatewas observed in both OATP-B or Mock vesicles (Fig. 9B). Theosmolarity of the medium was changed (290–1090 mOsm/kg)by increasing the concentration of sucrose, and the uptake of[³H]estrone-3-sulfate in the steady state was examined. Uptakeof [³H]estrone-3-sulfate at 120 min by membrane vesicles preparedfrom OATP-B- and mock-transfected HEK293 cells decreased linearlyas the reciprocal of medium osmolarity decreased, suggestingthat [³H]estrone-3-sulfate is taken up into an intravesicularspace (data not shown).

View larger version (16K):
[in this window]
[in a new window]

FIG. 9. Effect of an H⁺-gradient on uptake of [³H]estrone-3-sulfate by membrane vesicles obtained from HEK293/OATP-B and HEK293/Mock. Membrane vesicles obtained from HEK293/OATP-B (circles) or HEK293/Mock cells (triangles) were preincubated for 10 min at 37°C in the transport buffer (pH 7.4). Uptake of [³H]estrone-3-sulfate (47 nM) was then measured over 120 min at pH 6.0 (A) or pH 7.4 (B) in the absence (closed symbols) or presence (open symbols) of 50 µM FCCP. Each point represents the mean and S.E.M. (n = 3). *, significantly different from mock vesicles (p < 0.05).

	Discussion

Top Abstract Materials and Methods Results Discussion References

Although OATP-B is known to be localized at apical membranesof human small intestinal epithelial cells, it has not yet beenclarified whether this transporter plays physiological/pharmacologicalroles as an uptake mechanism in the intestinal absorption ofits substrates or not. In this study, we characterized the estrone-3-sulfateuptake at the apical membranes of human intestinal Caco-2 cellsand compared it with the OATP-B-mediated transport. The expressionof OATP-B in Caco-2 cell was clarified by RT-PCR and Westernblot analysis (Fig. 2). OATP-B was localized at the apical membraneof Caco-2 cells (Fig. 1). The present findings, as well as theprevious observation that OATP-B is localized at the brush-bordermembrane of human enterocytes (Kobayashi et al., 2003

), supportthe hypothesis that OATP-B plays an important role in the uptakeof its substrates at the luminal membranes of the small intestine.The characteristics of estrone-3-sulfate uptake at the apicalmembranes of human intestinal Caco-2 cells were quite similarto those of HEK293/OATP-B cells in terms of 1) the inhibitionprofile by various kinds of organic anions, monocarboxylic acids(Fig. 7), 2) the IC₅₀ values of BSP, DHEAS, pravastatin, andbenzylpenicillin (Fig. 6 and Table 2), 3) the K_m value (Fig. 5),4) the effect of replacement of extracellular cations (Fig. 4),and 5) the specific activity per mRNA expression (Fig. 8). OATP-Bwas the most abundant transporter among the OATPs expressedin the small intestine and Caco-2 cells (Table 1 and Fig. 8).All of these data suggested that OATP-B plays a predominantrole in the uptake of estrone-3-sulfate at the luminal membranesof the small intestine.

There was a marked difference in the expression levels of OATPsbetween human jejunum and Caco-2 cells. There are several possibleexplanations for the difference. First, the relative contentof epithelial cells in the human biopsy samples could be lowerthan that in Caco-2 cell samples: since OATPs are expressedonly in the absorptive epithelial cells, contamination of nonepithelialcells in the biopsy sample would decrease the apparent expressionlevel of OATPs. However, since the expression levels of villin,an epithelial cell-specific gene, are comparable in the biopsysample (661 copy/ng total RNA) and in Caco-2 cells (925 copy/ngtotal RNA), contamination seems unlikely to account for thedifference. Second, up-regulation or down-regulation of OATPseither in Caco-2 cells or in the biopsy samples may explainthe difference. Indeed, there was a severalfold variation inthe expression level of OATP-B among our Caco-2 cell cultures(data not shown), even though the [³H]estrone-3-sulfate uptakeactivity and OATP-B mRNA expression level were well correlated.Third, mRNAs of OATPs are not evenly distributed longitudinallyalong the intestine, so for instance, mRNA expression of OATP-Bin the jejunum could be lower than in other parts. For example,mRNA and protein expression of the Na⁺-dependent bile acid transporterASBT is restricted to the terminal ileum (Saeki et al., 1999;Stelzner et al., 2000). Recently, Sun et al. (2002) examinedgene expression of several transporters and metabolic enzymes,such as cytochrome P450, in Caco-2 cells and found that it differedfrom the expression profile in human small intestine. In addition,expression of constitutive genes in Caco-2 cells could dependon the culture conditions. Further in vivo and in vitro analysesare necessary to examine these possibilities.

The transport by OATP-B is pH-sensitive, with the uptake ofestrone-3-sulfate, pravastatin, DHEAS, taurocholic acid, andfexofenadine being increased at acidic pH compared with neutralpH (Kobayashi et al., 2003; Nozawa et al., 2004). In this study,the uptake of estrone-3-sulfate by HEK293/OATP-B cells was alsohigher at pH 6.0 than at pH 7.4 (Fig. 3). Because OATP-B-mediatedtransport was reported to be inhibited by the proton-ionophoreFCCP, protons may be a candidate for the driving force of transportby OATP-B (Nozawa et al., 2004). To clarify whether or not theproton gradient is indeed the driving force for OATP-B, we hereperformed transport studies using membrane vesicles expressingOATP-B (Fig. 9). An overshoot phenomenon, which was inhibitedby FCCP, was observed in the presence of an inwardly directedgradient of protons, suggesting that estrone-3-sulfate uptakeis driven, at least in part, by the proton gradient. This characteristiccould be favorable for OATP-B to play a physiological role inthe uptake of substrates at the intestinal lumen.

The pH dependence of estrone-3-sulfate uptake by Caco-2 cellswas not large compared with that seen in HEK293/OATP-B cells(Figs. 3 and 4). There are several possible reasons for sucha difference. First, some other transport mechanism may alsoexist in the apical membranes of Caco-2 cells and could be involvedin uptake of estrone-3-sulfate. We examined the expression andpossible involvement of OATP-D and OATP-E, both of which areexpressed in the small intestine and Caco-2 cells (Tamai etal., 2000a; Fig. 8 and Table 1). HEK293 cells transfected withOATP-D and OATP-E exhibited much lower estrone-3-sulfate uptakethan did the cells transfected with OATP-B (Fig. 8): the expressionlevels of OATP-D and OATP-E transiently transfected in HEK293cells were approximately 1000- and 400-fold higher, respectively,than in Caco-2 cells, whereas uptake of estrone-3-sulfate waslower than that observed in Caco-2 cells in each case (Fig. 8).These results suggest that OATP-D and OATP-E do not contributesubstantially to apical uptake of estrone-3-sulfate by Caco-2cells. Another possible reason for the discrepancy in pH dependencebetween HEK293/OATP-B and Caco-2 cells may be a difference inthe microclimate pH in the vicinity of OATP-B proteins in Caco-2cells. An isoform of Na⁺/H⁺ exchanger, NHE3, is expressed inthe apical membrane of Caco-2 cells (Janecki et al., 1998).This protein could release protons close to OATP-B, resultingin a constant supply of protons as a driving force of OATP-B.Indeed, NHE3 affects transport activity of oligopeptide transporterPEPT1 by supplying a driving force at the apical membrane ofCaco-2 cells (Walker et al., 1998; Thwaites et al., 2002; Watanabeet al., 2005).

Estrone-3-sulfate is a sulfate-conjugated metabolite of estroneand acts as a carrier of estrogen in plasma and various tissues.Estrone is metabolized to estrone-3-sulfate in the liver, andits metabolites are secreted into bile, reabsorbed into enterocytes,and undergo enterohepatic circulation (Honjo, 1979). Becauseestrone-3-sulfate is likely to exist in ionic form at physiologicalpH, it is thought that carrier-mediated transport systems playa major role in the membrane permeation processes involved.Whereas hepatic uptake of estrogen may be mediated by OATP familymember(s) expressed in the sinusoidal membranes of hepatocytes(König et al., 2000), intestinal uptake of estrogen hasnot been well characterized. The results in this study suggestthat intestinal absorption of estrogen in humans is likely tobe mediated by OATP-B. It is an interesting hypothesis thatintestinal OATP-B not only accepts estrone-3-sulfate as an endogenoussubstrate but also recognizes therapeutic agents such as pravastatinand benzylpenicillin, contributing to their oral absorption(Kobayashi et al., 2003).

In conclusion, we have established that OATP-B is expressedin apical membranes of Caco-2 cells and that it is the predominantcontributor to apical uptake of estrone-3-sulfate, based onthe kinetic parameters of the uptake, the inhibitory profilesof various substrates, and the linear relationship between mRNAexpression levels and transport activity. Interindividual variationin the mRNA expression level of OATP-B in the human jejunumwas large. Genetic polymorphisms of OATP-B were previously found,and there were allelic differences of transport activity forestrone-3-sulfate (Nozawa et al., 2002; Ishikawa et al., 2004).Therefore, further analysis is required to examine the pharmacokineticand/or pharmacodynamic impact of such polymorphisms in OATP-Bto clarify fully the functional importance of this transporterin intestinal transport of endogenous compounds and variousxenobiotics. Recently, citrus juices have been reported to reducethe bioavailability of orally administered fexofenadine. OATP-Bmay be of importance as a target for individualized medicine.

Footnotes

This work was supported in part by a grant-in-aid for scientificresearch from the Ministry of Education, Science, Sports, andCulture of Japan.

Article, publication date, and citation information can be foundat http://dmd.aspetjournals.org.

doi:10.1124/dmd.106.009530.

ABBREVIATIONS: OATP, organic anion transporting polypeptide;HEK, human embryonic kidney; RT-PCR, reverse transcriptase-polymerasechain reaction; PBS, phosphate-buffered saline; MES, 2-(N-morpholino)ethanesulfonicacid; BSP, sulfobromophthalein; DHEAS, dehydroepiandrosteronesulfate; FCCP, carbonylcyanide p-trifluoromethoxyphenyl hydrazone;NMG, N-methyl-D-glucamine.

Address correspondence to: Dr. Ikumi Tamai, Department of Molecular Biopharmaceutics, Faculty of Pharmaceutical Sciences, Tokyo University of Science, 2641 Yamasaki, Noda, Chiba 278-8510, Japan. E-mail: tamai{at}rs.noda.tus.ac.jp

References

Top
Abstract
Materials and Methods
Results
Discussion
References

Abe T, Kakyo M, Tokui T, Nakagomi R, Nishio T, Nakai D, Nomura H, Unno M, Suzuki M, Naitoh T, Matsuno S, and Yawo H (1999) Identification of a novel gene family encoding human liver-specific organic anion transporter LST-1. J Biol Chem 274: 17159–17163.[Abstract/Free Full Text]

Abe T, Unno M, Onogawa T, Tokui T, Kondo TN, Nakagomi R, Adachi H, Fujiwara K, Okabe M, Suzuki T, et al. (2001) LST-2, a human liver-specific organic anion transporter, determines methotrexate sensitivity in gastrointestinal cancers. Gastroenterology 120: 1689–1699.[CrossRef][Medline]

Adachi H, Suzuki T, Abe M, Asano N, Mizutamari H, Tanemoto M, Nishio T, Onogawa T, Toyohara T, Kasai S, et al. (2003) Molecular characterization of human and rat organic anion transporter OATP-D. Am J Physiol 285: F1188–F1197.

Bradford MM (1976) A rapid and sensitive method for the quantitation of microgram quantities of protein utilizing the principle of protein-dye binding. Anal Biochem 72: 248–254.[CrossRef][Medline]

Cui Y, Konig J, Leier I, Buchholz U, and Keppler D (2001) Hepatic uptake of bilirubin and its conjugates by the human organic anion transporter SLC21A6. J Biol Chem 276: 9626–9630.[Abstract/Free Full Text]

Hagenbuch B and Meier PJ (2003) The superfamily of organic anion transporting polypeptides. Biochim Biophys Acta 1609: 1–18.[Medline]

Honjo H (1979) Estrogen metabolism and enterohepatic circulation. Nippon Rinsho 37: 46–52.

Hsiang B, Zhu Y, Wang Z, Wu Y, Sasseville V, Yang WP, and Kirchgessner TG (1999) A novel human hepatic organic anion transporting polypeptide (OATP-2). Identification of a liver-specific human organic anion transporting polypeptide and identification of rat and human hydroxymethylglutaryl-CoA reductase inhibitor transporters. J Biol Chem 274: 37161–37168.[Abstract/Free Full Text]

Ishikawa T, Tsuji A, Inui K, Sai Y, Anzai N, Wada M, Endou H, and Sumino Y (2004) The genetic polymorphism of drug transporters: functional analysis approaches. Pharmacogenomics 5: 67–99.[CrossRef][Medline]

Janecki AJ, Montrose MH, Zimniak P, Zweibaum A, Tse CM, Khurana S, and Donowitz M (1998) Subcellular redistribution is involved in acute regulation of the brush border Na⁺/H⁺ exchanger isoform 3 in human colon adenocarcinoma cell line Caco-2. Protein kinase C-mediated inhibition of the exchanger. J Biol Chem 273: 8790–8798.[Abstract/Free Full Text]

Kobayashi D, Nozawa T, Imai K, Nezu J, Tsuji A, and Tamai I (2003) Involvement of human organic anion transporting polypeptide OATP-B (SLC21A9) in pH-dependent transport across intestinal apical membrane. J Pharmacol Exp Ther 306: 703–708.[Abstract/Free Full Text]

Konig J, Cui Y, Nies AT, and Keppler D (2000) Localization and genomic organization of a new hepatocellular organic anion transporting polypeptide. J Biol Chem 275: 23161–23168.[Abstract/Free Full Text]

Kullak-Ublick GA, Hagenbuch B, Stieger B, Schteingart CD, Hofmann AF, Wolkoff AW, and Meier PJ (1995) Molecular and functional characterization of an organic anion transporting polypeptide cloned from human liver. Gastroenterology 109: 1274–1282.[CrossRef][Medline]

Kullak-Ublick GA, Ismair MG, Stieger B, Landmann L, Huber R, Pizzagalli F, Fattinger K, and Meier PJ (2001) Organic anion-transporting polypeptide B (OATP-B) and its functional comparison with three other OATPs of human liver. Gastroenterology 120: 525–533.[CrossRef][Medline]

Lu R, Kanai N, Bao Y, and Schuster VL (1996) Cloning, in vitro expression, and tissue distribution of a human prostaglandin transporter cDNA(hPGT). J Clin Investig 98: 1142–1149.[Medline]

Mikkaichi T, Suzuki T, Onogawa T, Tanemoto M, Mizutamari H, Okada M, Chaki T, Masuda S, Tokui T, Eto N, et al. (2004) Isolation and characterization of a digoxin transporter and its rat homologue expressed in the kidney. Proc Natl Acad Sci USA 101: 3569–3574.[Abstract/Free Full Text]

Naruhashi K, Sai Y, Tamai I, Suzuki N, and Tsuji A (2002) PepT1 mRNA expression is induced by starvation and its level correlates with absorptive transport of cefadroxil longitudinally in the rat intestine. Pharm Res (NY) 19: 1417–1423.

Nozawa T, Imai K, Nezu J, Tsuji A, and Tamai I (2004) Functional characterization of pH-sensitive organic anion transporting polypeptide OATP-B in human. J Pharmacol Exp Ther 308: 438–445.[Abstract/Free Full Text]

Nozawa T, Nakajima M, Tamai I, Noda K, Nezu J, Sai Y, Tsuji A, and Yokoi T (2002) Genetic polymorphisms of human organic anion transporters OATP-C (SLC21A6) and OATP-B (SLC21A9): allele frequencies in the Japanese population and functional analysis. J Pharmacol Exp Ther 302: 804–813.[Abstract/Free Full Text]

Pizzagalli F, Hagenbuch B, Stieger B, Klenk U, Folkers G, and Meier PJ (2002) Identification of a novel human organic anion transporting polypeptide as a high affinity thyroxine transporter. Mol Endocrinol 16: 2283–2296.[Free Full Text]

Pizzagalli F, Varga Z, Huber RD, Folkers G, Meier PJ, and St-Pierre MV (2003) Identification of steroid sulfate transport processes in the human mammary gland. J Clin Endocrinol Metab 88: 3902–3912.[Abstract/Free Full Text]

Saeki T, Matoba K, Furukawa H, Kirifuji K, Kanamoto R, and Iwami K (1999) Characterization, cDNA cloning, and functional expression of mouse ileal sodium-dependent bile acid transporter. J Biochem (Tokyo) 125: 846–851.[Abstract/Free Full Text]

Shiau YF, Fernandez P, Jackson MJ, and McMonagle S (1985) Mechanisms maintaining a low-pH microclimate in the intestine. Am J Physiol 248: G608–G617.[Medline]

Stelzner M, Hoagland V, and Somasundaram S (2000) Distribution of bile acid absorption and bile acid transporter gene message in the hamster ileum. Pflueg Arch Eur J Physiol 440: 157–162.[Medline]

St-Pierre MV, Hagenbuch B, Ugele B, Meier PJ, and Stallmach T (2002) Characterization of an organic anion-transporting polypeptide (OATP-B) in human placenta. J Clin Endocrinol Metab 87: 1856–1863.[Abstract/Free Full Text]

Sun D, Lennernas H, Welage LS, Barnett JL, Landowski CP, Foster D, Fleisher D, Lee KD, and Amidon GL (2002) Comparison of human duodenum and Caco-2 gene expression profiles for 12,000 gene sequences tags and correlation with permeability of 26 drugs. Pharm Res (NY) 19: 1400–1416.

Taipalensuu J, Tornblom H, Lindberg G, Einarsson C, Sjoqvist F, Melhus H, Garberg P, Sjostrom B, Lundgren B, and Artursson P (2001) Correlation of gene expression of ten drug efflux proteins of the ATP-binding cassette transporter family in normal human jejunum and in human intestinal epithelial Caco-2 cell monolayers. J Pharmacol Exp Ther 299: 164–170.[Abstract/Free Full Text]

Tamai I, China K, Sai Y, Kobayashi D, Nezu J, Kawahara E, and Tsuji A (2001a) Na⁺-coupled transport of L-carnitine via high-affinity carnitine transporter OCTN2 and its subcellular localization in kidney. Biochim Biophys Acta 1512: 273–284.[Medline]

Tamai I, Nezu J, Uchino H, Sai Y, Oku A, Shimane M, and Tsuji A (2000a) Molecular identification and characterization of novel members of the human organic anion transporter (OATP) family. Biochem Biophys Res Commun 273: 251–260.[CrossRef][Medline]

Tamai I, Nozawa T, Koshida M, Nezu J, Sai Y, and Tsuji A (2001b) Functional characterization of human organic anion transporting polypeptide B (OATP-B) in comparison with liver-specific OATP-C. Pharm Res (NY) 18: 1262–1269.

Tamai I, Ogihara T, Takanaga H, Maeda H, and Tsuji A (2000b) Anion antiport mechanism is involved in transport of lactic acid across intestinal epithelial brush-border membrane. Biochem Biophys Acta 1468: 285–292.[Medline]

Tamai I, Sai Y, Ono A, Kido Y, Yabuuchi H, Takanaga H, Satoh E, Ogihara T, Amano O, Iseki S, et al. (1999) Immunohistochemical and functional characterization of pH-dependent intestinal absorption of weak organic acids by the monocarboxylic acid transporter MCT1. J Pharm Pharmacol 51: 1113–1121.[CrossRef][Medline]

Tamai I, Takanaga H, Maeda H, Ogihara T, Yoneda M, and Tsuji A (1995) Proton-cotransport of pravastatin across intestinal brush-border membrane. Pharm Res (NY) 12: 1727–1732.

Tamai I, Takanaga H, Maeda H, Yabuuchi H, Sai Y, Suzuki Y, and Tsuji A (1996) Intestinal brush-border membrane transport of monocarboxylic acids mediated by proton-coupled transport and anion antiport mechanism. J Pharm Pharmacol 49: 108–112.

Tavelin S, Grasjo J, Taipalensuu J, Ocklind G, and Artursson P (2002) Applications of epithelial cell culture in studies of drug transport. Methods Mol Biol 188: 233–272.[Medline]

Thwaites DT, Kennedy DJ, Raldua D, Anderson CM, Mendoza ME, Bladen CL, and Simmons NL (2002) H⁺/Dipeptide absorption across the human intestinal epithelium is controlled indirectly via a functional Na⁺/H⁺ exchanger. Gastroenterology 122: 1322–1333.[CrossRef]

Ugele B, St-Pierre MV, Pihusch M, Bahn A, and Hantschmann P (2003) Characterization and identification of steroid sulfate transporters of human placenta. Am J Physiol 284: E390–E398.

Walker D, Thwaites DT, Simmons NL, Gilbert HJ, and Hirst BH (1998) Substrate upregulation of the human small intestinal peptide transporter, hPepT1. J Physiol 507: 697–706.[Abstract/Free Full Text]

Watanabe C, Kato Y, Ito S, Kubo Y, Sai Y, and Tsuji A (2005) Na⁺/H⁺ exchanger 3 affects transport property of H⁺/oligopeptide transporter 1. Drug Metab Pharmacokinet 20: 443–451.[CrossRef][Medline]

Yamaoka K, Tanigawara Y, Nakagawa T, and Uno T (1981) A pharmacokinetic analysis program (MULTI) for microcomputer. J Pharmacobiodyn 4: 879–885.[Medline]

This article has been cited by other articles:

A. S. Kalgutkar, B. Feng, H. T. Nguyen, K. S. Frederick, S. D. Campbell, H. L. Hatch, Y.-A. Bi, D. C. Kazolias, R. E. Davidson, R. J. Mireles, et al.
Role of Transporters in the Disposition of the Selective Phosphodiesterase-4 Inhibitor (+)-2-[4-({[2-(Benzo[1,3]dioxol-5-yloxy)-pyridine-3-carbonyl]-amino}-methyl)-3-fluoro-phenoxy]-propionic Acid in Rat and Human
Drug Metab. Dispos., November 1, 2007; 35(11): 2111 - 2118.
[Abstract] [Full Text] [PDF]

D. T. Thwaites and C. M. H. Anderson
H+-coupled nutrient, micronutrient and drug transporters in the mammalian small intestine
Exp Physiol, July 1, 2007; 92(4): 603 - 619.
[Abstract] [Full Text] [PDF]

This Article

Abstract

Full Text (PDF)

All Versions of this Article:
dmd.106.009530v1
34/8/1423 most recent

Submit a response

Alert me when this article is cited

Alert me when eLetters are posted

Alert me if a correction is posted

Services

Similar articles in this journal

Similar articles in PubMed

Alert me to new issues of the journal

Download to citation manager

Citing Articles

				D. T. Thwaites and C. M. H. Anderson H+-coupled nutrient, micronutrient and drug transporters in the mammalian small intestine Exp Physiol, July 1, 2007; 92(4): 603 - 619. [Abstract] [Full Text] [PDF]