Transport of Quinolone Antibacterial Drugs by Human P-Glycoprotein Expressed in a Kidney Epithelial Cell Line, LLC-PK1

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Vol. 282, Issue 2, 955-960, 1997

Transport of Quinolone Antibacterial Drugs by Human P-Glycoprotein Expressed in a Kidney Epithelial Cell Line, LLC-PK₁¹

Tatsuya Ito, Ikuko Yano, Kumiko Tanaka and Ken-Ichi Inui

Department of Pharmacy, Kyoto University Hospital, Faculty of Medicine, Kyoto University, Sakyo-ku, Kyoto 606-01, Japan

	Abstract

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The purpose of this study was to characterize the transport mechanisms involved in the renal tubular secretion of quinolones.The contribution of P-glycoprotein to the transport of quinoloneswas elucidated using a kidney epithelial cell line, LLC-PK₁, andits transfectant derivative cell line, LLC-GA5-COL150, which expresseshuman P-glycoprotein on the apical membrane. The transcellulartransport of levofloxacin, a quinolone antibacterial drug, fromthe basolateral to apical side was increased in LLC-GA5-COL150compared with that in LLC-PK₁ monolayers. The apparent Michaelisconstant and maximum velocity values for the saturable transcellulartransport of levofloxacin from the basolateral to apical sidein LLC-GA5-COL 150 monolayers were 3.0 mM and 45 nmol/mg proteinper 15 min, respectively. The increased basolateral-to-apicaltransport in LLC-GA5-COL150 monolayers was completely inhibitedby cyclosporin A and quinidine to the level observed in LLC-PK₁monolayers. In addition, 3 mM levofloxacin inhibited the basolateral-to-apicaltransport of daunorubicin in LLC-GA5-COL150 monolayers. The basolateral-to-apicaltransport of another quinolone antibacterial drug, DU-6859a, inLLC-GA5-COL150 monolayers greatly exceeded than that in LLC-PK₁monolayers, and was inhibited by levofloxacin. These findingssuggest that quinolone antibacterial drugs are transported byP-glycoprotein, and that P-glycoprotein may contribute at leastin part to the renal tubular secretion of quinolones.

	Introduction

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Quinolone antibacterial drugs are frequently used to treat various bacterial infections. Most quinolone antibacterial drugsare zwitterions at physiological pH, and are excreted into urinevia renal tubular secretion. Probenecid has been shown to decreasethe renal clearance of cinoxacin, norfloxacin and ciprofloxacin(Rodriguez et al., 1979; Shimada et al., 1983; Sörgel and Kinzig,1993). Cimetidine has been shown to decrease the renal clearanceof temafloxacin and enoxacin (Sörgel et al., 1992; Misiak etal., 1993). These findings suggested that quinolone antibacterialdrugs undergo tubular secretion as either acids or bases (Sörgeland Kinzig, 1993). Levofloxacin, a zwitterion at physiologicalpH, also undergoes renal tubular secretion in man (Kamiya et al.,1992). We have shown that ofloxacin, a racemate of levofloxacinand its optical enantiomer, potently inhibits the H⁺-dependent tetraethylammonium uptake in renal brush-border membranevesicles (Okano et al., 1990). We have also shown that levofloxacinpotently inhibits the apical H⁺/organic cation antiporter expressed in the kidney epithelialcell line LLC-PK₁, and that the transcellular transport of levofloxacinwould be mediated by systems that are distinct from those involvedin tetraethylammonium transport (Ohtomo et al., 1996). The detailsof the transport mechanisms for quinolones have yet to be elucidated.

P-glycoprotein, which is a 170- to 180-kDa membrane glycoprotein, has been extensively investigated with regard to the multidrugresistance phenomenon in tumor cells (Gottesman and Pastan, 1988;Endicott and Ling, 1989). P-glycoprotein functions as an ATP-dependentdrug-efflux pump, thereby actively excreting a variety of structurallyunrelated anticancer drugs out of cells thus producing resistance.P-glycoprotein is also found in normal tissues such as on thebrush-border membranes of proximal tubules of the kidney, thebile canalicular membranes of hepatocytes, the apical membranesof mucosal cells in the intestine and the luminal membranes ofendothelial cells in the blood-brain barrier sites (Cordon-cardoet al., 1989; Thiebaut et al., 1987). In our laboratory, the renalsecretion of the commonly used drug digoxin by P-glycoproteinwas elucidated using LLC-PK₁ cells transfected with human MDR1cDNA, LLC-GA5-COL150 cells, which overexpress human P-glycoproteinon the apical membranes (Tanigawara et al., 1992).

P-glycoprotein is localized on the brush-border membranes of the normal proximal tubular cells in the kidney, and has widesubstrate specificity. We hypothesized that P-glycoprotein maycontribute to the renal tubular secretion of quinolone antibacterialdrugs. We studied the transport of levofloxacin and another newquinolone, DU-6859a, using LLC-GA5-COL150 cells. Our results suggestthat quinolone antibacterial drugs are transported by P-glycoproteinand that P-glycoprotein may contribute at least in part to therenal tubular secretion of quinolones.

	Materials and Methods

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Cell culture. LLC-GA5-COL150 cells established previously in our laboratory (Tanigawara et al., 1992; Ueda et al., 1992) and LLC-PK₁ cells(ATCC, CRL-1392) as host cells were maintained by serial passagein plastic culture dishes. Complete medium consisted of Dulbecco'smodified Eagle's medium supplemented with 10% fetal calf serumwithout antibiotics, and 150 ng/ml colchicine was added to themedium for LLC-GA5-COL150 cells. Monolayers were grown under anatmosphere of 5% CO₂-95% air at 37°C, and were subcultured every6 to 7 days using 0.02% EDTA and 0.05% trypsin (Saito et al.,1992). In general, the plastic dishes (100 mm) were inoculatedwith 1 × 10⁶ cells in 10 ml of complete culture medium. For the transportstudies, LLC-GA5-COL150 and LLC-PK₁ cells were seeded on polycarbonatemembrane filters (3-µm pores, 4.71 cm² growth area) inside Transwell cell culture chambers (Costar,Cambridge, MA) at a cell density of 5 × 10⁵ and 3 × 10⁵ cells/cm², respectively. Transwell chambers were placed in 35-mm wellsof tissue culture plates with 2.6 ml of outside medium (basolateralside) and 1.5 ml of inside medium (apical side). Fresh mediumwas replaced every 2 days, and the cells were used on the 7thday after seeding. In our study, LLC-GA5-COL150 and LLC-PK₁ cellswere used between passages 7 and 16, and between passages 217and 227, respectively.

Transport and cellular accumulation measurements. Transcellular transport and accumulation of [¹⁴C]levofloxacin, [³H]daunorubicin, and [¹⁴C]DU-6859a were measured using monolayer cultures grown in Transwellchambers (Saito et al., 1992). The composition of incubation mediumwas as follows: 145 mM NaCl, 3 mM KCl, 1 mM CaCl₂, 0.5 mM MgCl₂,5 mM D-glucose, 5 mM HEPES (pH 7.4). The pH of the medium wasadjusted with a solution of NaOH. Six hours before the transportexperiments, the culture medium was replaced with fresh colchicine-freeculture medium. After removal of the culture medium from bothsides of the monolayers, the cell monolayers were preincubatedwith 2 ml of incubation medium in each side for 15 min at 37°C.Then, 2 ml of incubation medium containing the radioactive substratewere added to either the basolateral or apical side, 2 ml of nonradioactiveincubation medium was added to the opposite side and the monolayerswere incubated for specified periods at 37°C. D-[³H]Mannitol (5 µM, 37 kBq/ml), a compound that is not transportedby the cells, was used to calculate the paracellular fluxes andthe extracellular trapping of [¹⁴C]levofloxacin (5 µM, 5.4 kBq/ml) and [¹⁴C]DU-6859a (5 µM, 3.8 kBq/ml). [¹⁴C]Sucrose (21.2 µM, 3.6 kBq/ml) was used to calculate the paracellularfluxes and the extracellular trapping of [³H]daunorubicin (100 nM, 17.1 kBq/ml). For transport measurements,aliquots (50 µl) of the incubation medium on the other side weretaken at specified times, and the radioactivity was counted.

For accumulation studies, the medium was removed by aspiration at the end of the incubation period, and the monolayers wererapidly washed twice with 2 ml of ice-cold incubation medium oneach side. The filters with monolayers were detached from chambers,the cells on the filters were solubilized with 0.5 ml of 1 N NaOHand the radioactivity in aliquots of 50 µl were counted. The radioactivityof the collected medium and the solubilized cell monolayers wasdetermined in 3 ml of ACS II (Amersham International, Buckinghamshire,UK) by liquid scintillation counting.

Protein assay. The protein contents of the cell monolayers solubilized in 1 N NaOH were determined by the method of Bradford (1976) usinga Bio-Rad Protein Assay Kit (Bio-Rad Laboratories, Richmond, CA)with bovine $gamma$ -globulin as a standard. The protein contents ofLLC-GA5-COL150 and LLC-PK₁ monolayers were 0.7 to 0.8, and 1.0to 1.2 mg/filter, respectively.

Statistical analysis. Statistical analysis was performed by non-paired t test or Scheffé's F test when multiple comparisons were needed. Differenceswere considered significant when P < .05.

Materials. D-[³H]Mannitol (828.8 GBq/mmol), [¹⁴C]sucrose (170.0 MBq/mmol), and [³H]daunorubicin (170.2 GBq/mmol) were purchased from Du Pont-NewEngland Nuclear Research Products (Boston, MA). [¹⁴C]Levofloxacin (1.07 GBq/mmol), [¹⁴C]DU-6859a (769 MBq/mmol), unlabeled levofloxacin and DU-6859awere kindly supplied by Daiichi Seiyaku Co. (Tokyo, Japan) (fig.1). Cyclosporin A was a gift from Sandoz Pharmaceutical, Co. Ltd.(Tokyo, Japan). Cimetidine, colchicine, quinidine, tetraetylammoniumand p-aminohippurate were purchased from Nacalai Tesque, Inc.(Kyoto, Japan). All other chemicals used were of the highest purityavailable.

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Fig. 1. Chemical structures of levofloxacin and DU-6859a.

	Results

Top Abstract Introduction Materials & Methods Results Discussion References

Transcellular transport and cellular accumulation of levofloxacin. We first measured the transcellular transport and cellular accumulation of levofloxacin (100 µM) by LLC-GA5-COL150 and LLC-PK₁monolayers. The basolateral-to-apical flux rate of levofloxacinby LLC-PK₁ monolayers was larger than that in the opposite direction(fig. 2A). The basolateral-to-apical transport of levofloxacinwas significantly increased (P < .01) in LLC-GA5-COL150 comparedwith that in LLC-PK₁ monolayers. The cellular accumulation oflevofloxacin from the basolateral side in LLC-GA5-COL150 monolayerswas significantly increased (P < .05) at 15 and 30 min comparedwith that in LLC-PK₁ monolayers. The cellular accumulation oflevofloxacin from the apical side in LLC-GA5-COL150 monolayerswas significantly decreased (P < .01) compared with that in LLC-PK₁monolayers (fig. 2B).

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Fig. 2. Transcellular transport (A) and cellular accumulation (B) of levofloxacin by LLC-GA5-COL150 and LLC-PK₁ monolayers. LLC-GA5-COL150(solid symbols) and LLC-PK₁ (open symbols) monolayers were incubatedat 37°C with 100 µM [¹⁴C]levofloxacin added either to the apical ( $black-triangle$ , $triangle$ ) or basolateral( $bullet$ , $open circle$ ) side of monolayers. After incubation, the appearance ofradioactivity on the opposite side and accumulation were measured.Each point represents the mean ± S.E. of at least three monolayers.* P < .05, ** P < .01, significant difference from LLC-PK₁ monolayers(open symbols).

Concentration dependence of levofloxacin transcellular transport. We next examined the transcellular transport of varying concentrations of levofloxacin by LLC-GA5-COL150 monolayers. Figure3 shows the results of kinetic analysis of the transcellular transportof levofloxacin from the basolateral to apical side by LLC-GA5-COL150monolayers as a function of substrate concentration ranging from0.05 to 5 mM. The transport rates were estimated at 15 min becausefindings were linear on incubation up to 60 min (fig. 2A). Therelationship between concentration and the basolateral-to-apicalflux rate in LLC-GA5-COL150 monolayers approached saturation.We evaluated the apparent kinetic parameters by nonlinear leastsquares regression analysis according to the sum of the saturabletransport indicated by Michaelis-Menten equation and the nonsaturabletransport. The apparent Michaelis constant (K_m) and maximum velocity(V_max) values for the saturable transport of levofloxacin were3.0 mM and 45 nmol/mg protein per 15 min, respectively.

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Fig. 3. Kinetic analysis of concentration dependence of levofloxacin transcellular transport for LLC-GA5-COL150 monolayers. LLC-GA5-COL150monolayers were incubated for 15 min at 37°C with varying concentrationsof [¹⁴C]levofloxacin added to the basolateral side. After incubation,the appearance of radioactivity on the opposite side and accumulationwere measured. The solid and dotted lines represent the estimatedoverall and nonsaturable transport, respectively. The inset showsEadie-Hofstee plots of levofloxacin transcellular transport aftercorrection for nonsaturable transport. V, transcellular transportrate (nmol/mg protein per 15 min); S, substrate concentration(mM).

Inhibitory effects of P-glycoprotein modulators on levofloxacin transport. The inhibitory effects of P-glycoprotein modulators on the transcellular transport of levofloxacin were examined. As shownin figure 4, the transcellular transport of levofloxacin in LLC-GA5-COL150monolayers was significantly inhibited by 5 and 10 µM cyclosporinA (P < .05) and 50 µM quinidine (P < .01), and was decreased tothe level observed in LLC-PK₁ monolayers. The transcellular transportof levofloxacin by LLC-PK₁ monolayers was not affected by theseP-glycoprotein modulators. Cimetidine, tetraethylammonium andp-aminohippurate did not influence the transcellular transportof levofloxacin by LLC-GA5-COL150 or LLC-PK₁ monolayers. CyclosporinA and quinidine were used as 1% ethanol solutions, which did notaffect the transcellular transport of levofloxacin (data not shown).

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Fig. 4. Effect of various drugs on the transcellular transport of levofloxacin by LLC-GA5-COL150 (A) and LLC-PK₁ (B) monolayers. Themonolayers were incubated for 60 min at 37°C with 100 µM [¹⁴C]levofloxacin added to the basolateral side in the absence orpresence of various drugs. Cyclosporin A (5 µM, 10 µM), quinidine(50 µM) and ionic drugs (2.5 mM) were added into the medium onboth sides of the cell monolayers during preincubation and incubationperiods. After incubation, the appearance of radioactivity onthe opposite side and accumulation were measured. Each columnrepresents the mean ± S.E. of three monolayers. * P < .05; ** P< .01, significant difference from control.

Inhibitory effect of levofloxacin on daunorubicin transport. We have shown that daunorubicin, an anticancer drug, is transported by P-glycoprotein in LLC-GA5-COL150 monolayers (Tanakaet al., 1996). To further characterize the interaction of levofloxacinwith P-glycoprotein, the inhibitory effect of levofloxacin onthe transport of daunorubicin was examined. As shown in figure5A, the transcellular transport of daunorubicin from the basolateralto apical side was inhibited by 3 mM levofloxacin, while transportin the opposite direction was not affected. The cellular accumulationof daunorubicin from both sides was increased, because levofloxacininhibited the expulsion of daunorubicin across the apical membranesvia P-glycoprotein (fig. 5B).

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Fig. 5. Effect of levofloxacin on the transcellular transport and cellular accumulation of daunorubicin by LLC-GA5-COL150 monolayers.A, The monolayers were incubated for 60 min at 37°C with 100 nM[³H]daunorubicin added to either the apical ( $black-triangle$ , $triangle$ ) or basolateralside ( $bullet$ , $open circle$ ) in the absence (open symbols) or presence (solid symbols)of 3 mM levofloxacin. Levofloxacin was added into the medium onboth sides of the cell monolayers during preincubation and incubationperiods. After incubation, the appearance of radioactivity onthe opposite side was measured. B, After a 60-min transport measurement,accumulation was determined in the absence (open columns) or presence(dotted columns) of levofloxacin. Each point or column representsthe mean ± S.E. of three monolayers. * P < .05, significant differencefrom each open column.

Transcellular transport and cellular accumulation of DU-6859a. To elucidate the general contribution of P-glycoprotein for the transport of quinolones, we studied the transport of anotherquinolone antibacterial drug, DU-6859a (100 µM), which is alsomainly excreted via the kidneys in man (Nakashima et al., 1995).The basolateral-to-apical flux rate of DU-6859a by LLC-PK₁ monolayerswas larger than the apical-to-basolateral flux rate (basolateral-to-apical,2.7 ± 0.5; apical-to-basolateral, 1.3 ± 0.5, nmol/mg protein per60 min, mean ± S.E. of three monolayers). The basolateral-to-apicaltransport in LLC-GA5-COL150 greatly exceeded that in LLC-PK₁ monolayers(fig. 6A). The basolateral-to-apical transport of DU-6859a inLLC-GA5-COL150 monolayers was suppressed and the cellular accumulationwas significantly increased (P < .05) by 3 mM levofloxacin (fig.6).

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Fig. 6. Effect of levofloxacin on the transcellular transport and cellular accumulation of DU-6859a by LLC-GA5-COL150 and LLC-PK₁monolayers. A, LLC-GA5-COL150 ( $bullet$ , $black-triangle$ ) and LLC-PK₁ ( $open circle$ ) monolayerswere incubated for 60 min at 37°C with 100 µM [¹⁴C]DU-6859a of 0.1% dimethyl sulfoxide solution added to the basolateralside of monolayers in the absence ( $bullet$ , $open circle$ ) or presence ( $black-triangle$ ) of 3mM levofloxacin. Levofloxacin was added into the medium on bothsides of the cell monolayers during preincubation and incubationperiods. After incubation, the appearance of radioactivity onthe opposite side was measured. B, After a 60-min transport measurement,accumulation was determined in the absence (open column) or presence(dotted column) of levofloxacin by LLC-GA5-COL150 monolayers.Each point or column represents the mean ± S.E. of three monolayers.* P < .05, significant difference from control.

	Discussion

Top Abstract Introduction Materials & Methods Results Discussion References

To investigate the participation of P-glycoprotein in the renal tubular secretion of quinolone antibacterial drugs, we examinedthe transport of levofloxacin and DU-6859a by LLC-GA5-COL150 monolayersthat overexpress P-glycoprotein on the apical membranes. Our resultsclearly indicated that these quinolone antibacterial drugs aretransported by P-glycoprotein, and that P-glycoprotein-mediatedtransport may contribute at least in part to the renal tubularsecretion of quinolones.

The basolateral-to-apical transport of levofloxacin was significantly increased in LLC-GA5-COL150 relative to that in LLC-PK₁monolayers, but the cellular accumulations from the basolateralside were almost same between these two cell lines, although significantlydifferent (fig. 2). In general, most substrates for P-glycoproteinare extensively transported by LLC-GA5-COL150 compared with LLC-PK₁monolayers, accompanied by a decrease in cellular accumulation(Saeki et al., 1993a; Tanaka et al., 1996). Our results may bedue to the characteristics of levofloxacin with low cellular accumulationby LLC-PK₁ monolayers similarly to diltiazem (Saeki et al., 1993b).Therefore, we used the transcellular transport of levofloxacinas an index of P-glycoprotein-mediated transport.

The apparent K_m value for the P-glycoprotein-mediated transport of levofloxacin was 3.0 mM from the kinetic analysis to examinesaturable transcellular transport (fig. 3). Therefore, the affinityof levofloxacin to P-glycoprotein was lower than that of cyclosporinA (Saeki et al., 1993a). The increased transcellular transportof levofloxacin in LLC-GA5-COL150 monolayers was almost completelyinhibited by the P-glycoprotein modulators cyclosporin A and quinidine,and was reduced to the level observed in LLC-PK₁ monolayers. Morethan half of the increased transcellular transport of 100 µM levofloxacinin LLC-GA5-COL150 monolayers were inhibited by only 5 µM cyclosporinA. This result was consistent with the reported apparent K_m valueof cyclosporin A for P-glycoprotein, 8.4 µM (Saeki et al., 1993a).These findings clearly showed that the increased saturable transcellulartransport of levofloxacin by LLC-GA5-COL150 monolayers is mediatedby P-glycoprotein.

The occurrence of multidrug resistance is a major obstacle for the treatment of cancer, and identification of clinically usableagents that can effectively reverse multidrug resistance is acurrent issue. We examined the inhibitory effect of levofloxacinon the P-glycoprotein-mediated transport of daunorubicin. Thebasolateral-to-apical transport of daunorubicin was inhibitedby 3 mM levofloxacin, accompanied by a 93% increase in cellularaccumulation (fig. 5). The serum concentration after oral administrationof 200 mg levofloxacin was reported to be 1.2 µg/ml (3.2 µM) atthe peak time in man (Nakashima et al., 1992). Therefore, levofloxacindoes not appear to be a clinically usable agent to reverse P-glycoprotein-associatedmultidrug resistance. Some multidrug-resistant cells overexpressMRP that shares minor sequence homology with P-glycoprotein andis also a member of the ATP-binding cassette transmembrane transporterprotein superfamily (Krishnamachary and Center, 1993). Gollapudiet al. (1995) showed that difloxacin increases the sensitivityof HL-60/AR cells, which overexpress MRP mRNA compared with HL-60cells, to daunorubicin at clinically achievable concentrations.The affinity of quinolones might be different between P-glycoproteinand MRP.

Griffiths et al. (1994) reported the active transepithelial secretion of quinolone derivatives, such as ciprofloxacin andnorfloxacin, from the basolateral to apical side by human intestinalCaco-2 cells. Ciprofloxacin was also studied in the isolated perfusedrat liver, and an active transport mechanism was shown to be involvedin the biliary excretion of this drug (Abadìa et al., 1995).In addition, the accumulation of quinolones into the brain islow, which may be caused either by the relative low influx permeabilityat the blood-brain barrier and blood-cerebrospinal fluid barrierand/or by active efflux at both barriers (Ooie et al., 1996).Considering the distribution of P-glycoprotein in normal tissues,P-glycoprotein might be a common transport system for the eliminationof quinolone antibacterial drugs.

We have shown that levofloxacin potently inhibits the apical H⁺/organic cation antiporter expressed in LLC-PK₁ cells, but thatthe transport of levofloxacin would be mediated by systems thatare distinct from those involved in tetraethylammonium transport(Ohtomo et al., 1996). In this study, levofloxacin and DU-6859awere unidirectionally transported by LLC-PK₁ monolayers, and thebasolateral-to-apical transcellular transport of levofloxacinwas not inhibited by P-glycoprotein modulators, cimetidine, tetraethylammoniumor p-aminohippurate. We considered that there are single or multiplepathways for renal tubular secretion of these quinolone antibacterialdrugs in addition to that via P-glycoprotein. The mechanisms forrenal elimination of quinolones need to be examined further.

In conclusion, our results suggest that quinolone antibacterial drugs are transported by P-glycoprotein and that P-glycoproteinmay contribute at least in part to the renal tubular secretionas well as other elimination processes. The degree to which P-glycoproteincontributes to the in vivo pharmacokinetics of quinolones shouldbe evaluated in future studies.

	Footnotes

Accepted for publication April 7, 1997.

Received for publication January 27, 1997.

¹ This work was supported by a Grant-in-Aid for Scientific Research from the Ministry of Education, Science, and Culture ofJapan and by the Grant-in-Aid from the Tokyo Biochemical ResearchFoundation.

Send reprint requests to: Dr. Ken-ichi Inui, Department of Pharmacy, Kyoto University Hospital, Sakyo-ku, Kyoto 606-01, Japan.

	Abbreviations

HEPES, N-2-hydroxyethylpiperazine-N $'$ -2-ethanesulfonic acid; MRP, multidrug resistance-related protein.

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				Y. Matsuo, I. Yano, T. Ito, Y. Hashimoto, and K.-I. Inui Transport of Quinolone Antibacterial Drugs in a Kidney Epithelial Cell Line, LLC-PK1 J. Pharmacol. Exp. Ther., November 1, 1998; 287(2): 672 - 678. [Abstract] [Full Text]

				C. Østergaard, T. Klitmøller Sørensen, J. Dahl Knudsen, and N. Frimodt-Møller Evaluation of Moxifloxacin, a New 8-Methoxyquinolone, for Treatment of Meningitis Caused by a PenicillinResistant Pneumococcus in Rabbits Antimicrob. Agents Chemother., July 1, 1998; 42(7): 1706 - 1712. [Abstract] [Full Text]

Transport of Quinolone Antibacterial Drugs by Human P-Glycoprotein Expressed in a Kidney Epithelial Cell Line, LLC-PK11

Transport of Quinolone Antibacterial Drugs by Human P-Glycoprotein Expressed in a Kidney Epithelial Cell Line, LLC-PK₁¹