Transport of [3H]Losartan across Isolated Perfused Rabbit Proximal Tubule

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Vol. 290, Issue 1, 38-42, July 1999

Transport of [³H]Losartan across Isolated Perfused Rabbit Proximal Tubule

Richard M. Edwards, Elwood J. Stack and Walter Trizna

Department of Renal Pharmacology, SmithKline Beecham Pharmaceuticals, King of Prussia, Pennsylvania

	Abstract

Top Abstract Introduction Materials and Methods Results Discussion References

The transport of the angiotensin II receptor antagonist losartan and its interaction with organic anion transport were examinedin the isolated perfused rabbit proximal tubule. Losartan reversiblyinhibited the secretion of para-aminohippurate (PAH) in a concentration-dependentmanner (IC₅₀ = 15 ± 0.5 µM). Other angiotensin II receptor antagonistsalso inhibited PAH secretion with similar potencies: eprosartan,11 ± 2.3 µM; irbesartan, 17 ± 2.2 µM; and valsartan 3 ± 0.6 µM.[³H]Losartan was secreted by the proximal tubule by a saturableand probenecid-sensitive mechanism. The affinity of losartan forthe organic anion transporter (K_m = 12.3 ±1.8 µM) was significantlygreater than that of PAH (K_m = 88.5 ± 10.7 µM). [³H]Losartan secretion was stimulated in the presence of $alpha$ -ketoglutarate,suggesting that losartan, like PAH, enters the cell in exchangefor a dicarboxylate. These results demonstrate that losartan andprobably other nonpeptide angiotensin II receptor antagonistsare secreted by an organic anion transporter that is similar to,if not identical with, the classic PAHtransporter.

	Introduction

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The nonpeptide angiotensin II receptor antagonists represent a new class of drugs with therapeutic use in hypertension andpossibly other cardiovascular disorders (MacFayden and Reid, 1994).Losartan was the first of this group of compounds to be approvedfor the management of hypertension (Johnston, 1995). As a class,the angiotensin II receptor antagonists are highly protein boundand are anions at physiological pH (Csajka et al., 1997). Themetabolism and elimination of the angiotensin II receptor antagonistsare varied. For example, some angiotensin II receptor antagonistsare extensively metabolized in the liver, generating active and/orinactive metabolites, which are eliminated in the bile or by thekidney (e.g., losartan and irbesartan) (Csajka et al., 1997),whereas others undergo little metabolism and are excreted in thebile and urine largely as unchanged drug (e.g., eprosartan) (Coxet al., 1996). In most cases, however, some proportion of theadministered dose appears unchanged in the urine (Csajka et al.,1997), suggesting that these molecules may be secreted by therenal organic anion transporter. Evidence that these moleculesmay interact with renal organic anion transport comes from studiesshowing that losartan increased uric acid excretion and loweredplasma levels of uric acid in both healthy subjects (Nakashimaet al., 1992) and hypertensive patients (Tsunoda et al., 1993).Subsequent studies demonstrated that losartan and, to a much lesserextent, EXP3174, the active metabolite of losartan, and eprosartaninhibited urate/anion exchange in proximal tubule brush bordermembrane vesicles from rat (Edwards et al., 1996) and human (Roch-Ramelet al., 1997)kidney.

Although the above studies showed that losartan could interact with organic anion reabsorption, little direct evidence existsas to whether losartan and other angiotensin II receptor antagonistscan interact with organic anion secretion and whether this classof compounds is secreted by the renal organic anion transporter.Therefore, the purposes of this study were to examine the interactionof angiotensin II receptor antagonists, principally losartan,with renal organic anion secretion and to characterize the transportof [³H]losartan across the proximaltubule.

	Materials and Methods

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Preparation and Perfusion of Isolated Tubules. Isolated tubules were perfused in vitro according to previously published methods (Edwards and Grantham, 1983). Male New ZealandWhite rabbits (2.5-3 kg) were anesthetized with i.v. pentobarbital,and a kidney was removed. Thin slices were cut and stored in chilleddissection solution consisting of 14 mM KCl, 44 mM K₂HPO₄, 14mM KH₂PO₄, 8 mM NaHCO₃, 160 mM sucrose, and 0.1% BSA, pH 7.4.Proximal tubule S2 segments were dissected, transferred to a temperature-controlledchamber, and mounted onto micropipettes. In most experiments,the tubules were bathed and perfused with Dulbecco's modifiedEagle's medium (DMEM), supplemented with 25 mM NaHCO₃ and equilibratedto pH 7.4 with 95% O₂/5% CO₂. In some experiments, the bath andperfusion solutions consisted of a HEPES-buffered solution thatcontained 116 mM NaCl, 25 mM HEPES, 5 mM KCl, 2 mM NaH₂PO₄, 1mM MgSO₄, 1.8 mM CaCl₂, 10 mM sodium acetate, 8.3 mM glucose,and 5 mM alanine, pH 7.4.

After the initiation of perfusion, the bath temperature was gradually increased to 37°C, and the tubule was allowed to equilibratefor at least 15 min. Throughout the experiment, bath solutionwas pumped through the chamber at 0.4 ml/min, and the tubuleswere perfused by gravity at a rate of 10 to 15 nl/min. Each experimentconsisted of an initial control period followed by various experimentalperiods as described in Results. After warming and equilibrationat 37°C, the bath solution was changed to one containing [³H]para-aminohippurate (PAH) or [³H]losartan with varying amounts of unlabeled substrate. Afterat least 10 min, two to four timed collections of perfusate weremade over the ensuing 15 to 20 min, with a constant volume constrictionpipette for measurement of control secretion rates. The bath wasthen changed to various experimental conditions as depicted inResults, and after a 10-min equilibration period, two to fourcollections were made as described above. Preliminary experimentsshowed that PAH or losartan secretion was stable for at least2 h, and therefore, attempts were made to complete experimentswithin this timeframe.

The secretory (bath to lumen) fluxes of (J_PAH) and losartan (J_LOS) were calculated as described by Edwards and Grantham (1983)

<UP>J<SUB>PAH or LOS</SUB></UP>=(V<SUB><UP>c</UP></SUB>C<SUB><UP>c</UP></SUB>)<UP>/</UP>(<UP>SA</UP>)(L)

(1)

where V_c is the fluid collection rate (in nl/min), C_c is the concentration of [³H]PAH or [³H]losartan in the collected fluid (in cpm/nl), SA is the specificactivity of [³H]PAH or [³H]losartan, and L is the tubule length (in mm). In each experiment,a secretory flux for a given experimental period was determinedby averaging the two to four collections made during that period.The secretion of PAH or losartan is expressed as fmol/min/mm oras a percentage of control values. In a limited number of experiments,the lumen-to-bath flux of [³H]losartan was measured. In these experiments, tubules were superfusedat a rate of 0.4 ml/min with DMEM-NaHCO₃ and perfused with thesame solution containing 15 µCi/ml [³H]losartan and unlabeled losartan at a final concentration of50 µM. The lumen-to-bath flux (J_l-b) was measured by the rateof appearance of [³H]losartan in the continuously collected bath medium accordingto:

<UP>J<SUB>l−b</SUB></UP>=<UP>cpm<SUB>b</SUB>/</UP>(<UP>SA</UP>)(t)(L)

(2)

where cpm_b represents the counts collected in the bath, SA is the specific activity of [³H]losartan in the perfusate, t is the collection time, and L isthe tubule length. For each tubule, J_l-b was determined from theaverage of three 10-mincollections.

The results are expressed as mean ± S.E.M. and were analyzed by Student's t test or ANOVA followed by Dunnett's test for multiplecomparisons. A value of p < .05 was considered to be statisticallysignificant. The n values refer to the number of tubules. Saturationand competition curves were analyzed by nonlinear regression analysis(GraphPAD Software, San Diego,CA).

Chemicals. [³H]PAH (specific activity, 1.28 Ci/mmol) and [³H]losartan (DuP 753; specific activity, 43.9 Ci/mmol) were obtained from NewEngland Nuclear (Boston, MA). Losartan, eprosartan, valsartan,and irbesartan were provided by the Department of Medicinal andSynthetic Chemistry (SmithKline Beecham Pharmaceuticals, Kingof Prussia, PA). All other reagents were from Sigma Chemical Co.(St. Louis,MO).

	Results

Top Abstract Introduction Materials and Methods Results Discussion References

Initial experiments were conducted to determine whether losartan could cis-inhibit PAH transport as would be expected if anorganic anion competed for the same transporter as PAH. As shownin Fig. 1, losartan rapidly and reversibly inhibited PAH secretionby isolated perfused proximal tubules. In the presence of 10 µM[³H]PAH, J_PAH during the control period was 382 ± 4.9 fmol/min/mm.The addition of 10 µM losartan to the bath significantly (p =.0003) inhibited PAH secretion by approximately 40% to 232 ± 3.5fmol/min/mm. On removal of losartan, PAH secretion returned tocontrol values: 359 ± 9.6 fmol/min/mm. The inhibitory effect oflosartan, as well as the other nonpeptide angiotensin II receptorantagonists (eprosartan, valsartan, and irbesartan), was concentrationdependent (Fig. 2). The concentrations of the antagonists neededto inhibit PAH secretion by 50% were 15 ± 0.5 µM for losartan,11 ± 2.3 µM for eprosartan, 3 ± 0.6 µM for valsartan, and 17 ±2.2 µM for irbesartan. Valsartan was significantly (p < .05) morepotent than the other angiotensin II receptor antagonists in inhibitingPAH secretion.

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Fig. 1. Time course of the reversible inhibition of [³H]PAH secretion (J_PAH) by losartan in the proximal tubule. During the control and recovery periods, the bath contained 10 µM [³H]PAH. Losartan (10 µM) was added to the bath at the indicated time (10-30 min). Results are the mean ± S.E.M. of four tubules.

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Fig. 2. Effects of losartan, eprosartan, valsartan, and irbesartan on [³H]PAH secretion (J_PAH). Concentration of [³H]PAH was 10 µM. Results are expressed as a percent of control J_PAH, which was 365 ± 35 fmol/min/mm. Each point is the mean ± S.E.M. of three or four tubules.

The previous experiments demonstrated that losartan could inhibit PAH secretion, suggesting that it interacted with the PAHtransporter. To determine whether losartan itself was transported,additional experiments examined the transport of [³H]losartan. The addition of 10 µM [³H]losartan to the bath resulted in a J_LOS of 598 ± 54 fmol/min/mm.Probenecid, a classic inhibitor of the organic anion transporter,produced a concentration-dependent inhibition of losartan secretion(Fig. 3), with half-maximal inhibition occurring at a concentrationof 17.9 ± 4.0 µM. PAH was much less effective in inhibiting [³H]losartan secretion, with an IC₅₀ value of 0.9 ± 0.2 mM. Figure4 shows the relationship between the bath concentration of [³H]losartan and J_LOS. The bath-to-lumen transport of [³H]losartan was clearly saturable. Double reciprocal plots revealedan apparent affinity (K_m) of 12.3 ± 1.8 µM and a maximal transportrate (V_max) of 1490 ± 22 fmol/min/mm (n = 3). For comparison,similar experiments were performed with [³H]PAH (Fig. 5). Apparent K_m and V_max values for PAH were 88.5± 10.7 µM and 3939 ± 561 fmol/min/mm, respectively, values similarto those previously reported for J_PAH in the rabbit S2 segment(Shimomura et al., 1981). The apparent K_m value and the V_max valuefor losartan were significantly different from the correspondingvalues for PAH (p = .002 and p = .01, respectively). The datashown in Figs. 4 and 5 represent total bath-to-lumen fluxes ofPAH and losartan, which are composed of both active and passivecomponents. In preliminary experiments, we measured the secretionof PAH and losartan over the same concentration range as shownin Figs. 4 and 5 in the presence of 5 mM probenecid to block activesecretion (Shimomura et al., 1981). Under these conditions, bothPAH and losartan passive fluxes were similar and never exceeded6% of the total flux at any substrate concentration, and therefore,we did not correct for the passive component.

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Fig. 3. Effects of probenecid and PAH on [³H]losartan secretion (J_LOS). Concentration of [³H]losartan was 10 µM. Results are expressed as a percent of control J_LOS, which was 598 ± 10.6 fmol/min/mm. Each point is the mean ± S.E.M. of four tubules.

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Fig. 4. [³H]Losartan secretion (J_LOS) as a function of bath losartan concentration. Top, J_LOS was measured in the presence of increasing concentrations of losartan added to the bath (5-500 µM). Bottom, double reciprocal plot of the data. Apparent K_m and V_max values were 12.3 ± 1.8 µM and 1490 ± 22 fmol/min/mm, respectively (n = 3).

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Fig. 5. [³H]PAH secretion (J_PAH) as a function of bath PAH concentration. Top, J_PAH was measured in the presence of increasing concentrations of PAH added to the bath (5-500 µM). Bottom, double reciprocal plot of the data. Apparent K_m and V_max values were 88.5 ± 10.7 µM and 3939 ± 561 fmol/min/mm, respectively (n = 3).

In four tubules, the lumen-to-bath flux of [³H]losartan was measured. When perfused with 50 µM losartan, the lumen-to-bathflux amounted to 54 ± 11.1 fmol/min/mm and was unaffected by 1mM probenecid (53.5 ± 3.3 fmol/min/mm). This represented only4.6% of the bath-to-lumen flux of losartan measured at the sameconcentration (1164 ± 77 fmol/min/mm).

According to the current model of organic anion secretion in the proximal tubule (Shimada et al., 1987; Pritchard, 1988),PAH and other organic anions enter the cell across the basolateralmembrane in exchange for $alpha$ -ketoglutarate ( $alpha$ -KG) moving out ofthe cell down its concentration gradient. The intracellular concentrationof $alpha$ -KG is maintained by intracellular synthesis as well as Na⁺-coupled entry of the dicarboxylate into the cell. Accordingly,exposure of the cells to $alpha$ -KG should stimulate the uptake andsecretion of an organic anion if it is transported by the organicanion/ $alpha$ -KG exchanger. To determine whether losartan transportwas affected by $alpha$ -KG, J_LOS was measured in tubules exposed toincreasing concentrations of $alpha$ -KG added to the bath. For theseexperiments, we used a bicarbonate-free HEPES-buffered solutionin which the effects of $alpha$ -KG are more readily demonstrable (Shpunet al., 1995). As shown in Fig. 6, both PAH and losartan secretionwere stimulated by the addition of $alpha$ -KG to the bathing medium.In the absence of $alpha$ -KG, both J_PAH and J_LOS were markedly reducedcompared with values obtained in previous experiments using DMEM:59.6 ± 7.8 versus 412 ± 19.9 fmol/min/mm for PAH and 95.9 ± 4.8versus 683 ± 50.2 fmol/min/mm for losartan. Significant (p < .05)stimulation of PAH secretion occurred at concentrations of $alpha$ -KGof 10 µM and above, whereas stimulation of losartan secretionwas not observed until a concentration of 30 µM $alpha$ -KG. At 10 µM $alpha$ -KG, J_PAH values (505 ± 91 fmol/min/mm) were similar to thoseobtained in DMEM, whereas 100 µM $alpha$ -KG was required to increaseJ_LOS (616 ± 34.4 fmol/min/mm) to values obtained in DMEM.

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Fig. 6. Effect of $alpha$ -KG on J_PAH and J_LOS. Tubules were perfused and bathed with a HEPES-based buffer in the presence of increasing concentrations of $alpha$ -KG added to the bath. Concentrations of [³H]PAH and [³H]losartan were 10 µM. Results are expressed as a percent of control secretion in the absence of added $alpha$ -KG and were 59.6 ± 7.8 fmol/min/mm for PAH and 95.9 ± 4.8 fmol/min/mm for losartan. Results are mean ± S.E.M. of three tubules for each anion. *p < .05 versus control.

	Discussion

Top Abstract Introduction Materials and Methods Results Discussion References

The renal organic anion transporter or transporters are responsible for the transepithelial movement of a large number ofendogenous substances, as well as numerous xenobiotics (Mollerand Sheikh, 1983). The present study is the first to characterizethe renal tubule secretion of a nonpeptide angiotensin II receptorantagonist, a class of compounds with increasing importance inthe treatment of hypertension (MacFayden and Reid, 1994). Theresults of this study demonstrate that [³H]losartan is secreted by the proximal tubule in a manner similarto the prototypical organic anion, PAH. This conclusion is basedon the observations that losartan and PAH cis-inhibited the secretionof each other, that [³H]losartan secretion was saturable and was inhibited by probenecid,and that [³H]losartan secretion was stimulated by the presence of $alpha$ -KG. Noevidence for a significant reabsorptive flux of losartan wasobtained.

Despite these similarities, there were quantitative differences in the characteristics of secretion of these two anions acrossthe proximal tubule; chief among these was the much higher affinityof the transporter for losartan (12.3 µM) than for PAH (88.5 µM)and the difference in V_max values. This was also reflected inthe more effective inhibition of PAH secretion by losartan thaninhibition of losartan secretion by PAH. Furthermore, PAH secretionappeared to be more sensitive to the effects of $alpha$ -KG than didlosartan. These latter experiments were conducted in a bicarbonate-free,HEPES-based buffer in which the stimulatory effects of $alpha$ -KG onorganic anion transport are more readily apparent (Shpun et al.,1995). This is presumably due to a reduction in cellular ATP levelsand tricarboxylic cycle intermediates in proximal tubules in theabsence of bicarbonate (Shpun et al., 1995). This is reflectedin the markedly reduced rate of PAH secretion in the absence ofbicarbonate compared with that in the presence of bicarbonateobserved in this and other studies (Dantzler and Evans, 1996).In these metabolically compromised tubules, the addition of exogenous $alpha$ -KG causes a marked increase in organic anion uptake by increasing $alpha$ -KG/organic anion countertransport as well as cellular metabolismin general (Shpun et al., 1995). Similar to observations madein basolateral membrane vesicles (Pritchard, 1988) and renal slices(Pritchard, 1990), $alpha$ -KG produced a biphasic effect on J_PAH. Atconcentrations up to 30 µM, $alpha$ -KG caused a concentration-dependentincrease in J_PAH. This likely reflects both cis- and trans-stimulationof PAH/ $alpha$ -KG exchange, as was also observed for fluorescein secretionin the proximal tubule (Welborn et al., 1998). The J_PAH valuesat 30 µM $alpha$ -KG were similar to those obtained in experiments performedin bicarbonate-containing media. However, at 100 µM $alpha$ -KG, J_PAHwas reduced relative to values obtained at 30 µM, possibly reflectingcompetition with PAH for binding to the transporter or to saturationof the Na⁺/dicarboxylate cotransporter and a reduction in the in>out $alpha$ -KGgradient that drives the $alpha$ -KG/PAH exchanger (Pritchard, 1990).In contrast, losartan secretion was not stimulated until exogenousconcentrations of $alpha$ -KG reached 30 µM and 100 µM $alpha$ -KG was requiredfor J_LOS values to approach those obtained in bicarbonate-containingbuffer. Differences in sensitivity of organic anion transportto $alpha$ -KG have also been observed between urate and PAH transportin pig basolateral membrane vesicles (Werner and Roch-Ramel, 1991).This difference, together with differences in Cl dependence and the rank order potency for inhibition of PAH andurate uptake by various organic anions, led the authors to suggestthat in the pig kidney, urate and PAH uptakes occur via similarbut separate transporters (Werner and Roch-Ramel, 1991). Whetherthe differences in PAH and losartan transport observed in thepresent study represent interaction with different transportersor simply kinetic differences awaits furtherinvestigation.

As a class, the angiotensin II receptor antagonists have high affinity for organic anion transport in the kidney. For example,losartan is 7- to 10-fold more potent than probenecid in inhibitingurate uptake in rat and human brush border membranes (Edwardset al., 1996; Roch-Ramel et al., 1997) and is uricosuric in humans(Nakashima et al., 1992; Tsunoda et al., 1993). In the presentstudy, losartan, eprosartan, and irbesartan inhibited PAH transportwith a potency similar to published values for probenecid (~15µM; Dantzler et al., 1995), whereas valsartan was approximately5-fold more potent than probenecid. The high affinity of thisclass of compounds for the organic anion secretory pathway, ifconfirmed in humans, suggests that these compounds may interferewith the renal excretion of other anionic drugs. However, at thepresent time, we are not aware of any suchreports.

	Acknowledgments

We thank Sue Tirri for administrativeassistance.

	Footnotes

Accepted for publication March 27, 1999.

Received for publication December 22, 1998.

Send reprint requests to: Dr. Richard Edwards, SmithKline Beecham Pharmaceuticals, Department of Renal Pharmacology, UW2521, 709 Swedeland Road, Box 1539, King of Prussia, PA 19406. E-mail: Richard_M_Edwards{at}sbphrd.com

	Abbreviations

PAH, para-aminohippurate; DMEM, Dulbecco's modified Eagle's medium; J_PAH, secretory flux of PAH; J_LOS, secretory flux of losartan; $alpha$ -KG, $alpha$ -ketoglutarate.

	References

Top Abstract Introduction Materials and Methods Results Discussion References

Cox PJ, Bush BD, Gorycki PD, Kuo GY, Kenworthy D, Law DW, Murphy D, Shardlow PC, Taylor A, Upward JW, Compton CH and Murdoch RD (1996) The metabolic fate of eprosartan in healthy volunteers. Exp Tox Pathol 48: 75-82.
Csajka C, Buclin T, Brunner HR and Biollaz J (1997) Pharmacokinetic-pharmacodynamic profile of angiotensin II receptor antagonists. Clin Pharmacokinet 32: 1-29[Medline].
Dantzler WH and Evans KK (1996) Effect of $alpha$ -KG in lumen on PAH transport by isolated perfused rabbit proximal tubules. Am J Physiol 271: F521-F526[Abstract/Free Full Text].
Dantzler WH, Evans KK and Wright SH (1995) Kinetics of interactions of para-aminohippurate, probenecid, cysteine conjugates and n-acetyl cysteine conjugates with basolateral organic anion transporter in isolated rabbit proximal renal tubules. J Pharmacol Exp Ther 272: 663-672[Abstract/Free Full Text].
Edwards RM and Grantham J (1983) Effect of vanadate on fluid absorption and PAH secretion in isolated proximal tubules. Am J Physiol 244: F367-F375.
Edwards RM, Trizna W, Stack EJ and Weinstock J (1996) Interaction of nonpeptide angiotensin II receptor antagonists with the urate transporter in rat renal brush-border membranes. J Pharmacol Exp Ther 276: 125-129[Abstract/Free Full Text].
Johnston CI (1995) Angiotensin receptor antagonists: Focus on losartan. Lancet 346: 1403-1407[Medline].
MacFadyen RJ and Reid JL (1994) Angiotensin receptor antagonists as a treatment for hypertension. J Hypertens 12: 1333-1338[Medline].
Moller JV and Sheikh I (1983) Renal organic anion transport system: Pharmacological, physiological and biochemical aspects. Pharmacol Rev 34: 315-358[Medline].
Nakashima M, Uematsu T, Kosuge K and Kanamura M (1992) Pilot study of the uricosuric effect of DuP 753, a new angiotensin II receptor antagonist, in healthy subjects. Eur J Clin Pharmacol 42: 333-335[Medline].
Pritchard JB (1988) Coupled transport of p-aminohippurate by rat kidney basolateral membrane vesicles. Am J Physiol 255: F597-F604[Abstract/Free Full Text].
Pritchard JB (1990) Rat renal cortical slices demonstrate p-aminohippurate/glutarate exchange and sodium/glutarate coupled p-aminohippurate transport. J Pharmacol Exp Ther 255: 969-975[Abstract/Free Full Text].
Roch-Ramel F, Guisan B and Diezi J (1997) Effects of uricosuric and antiuricosuric agents on urate transport in human brush-border membrane vesicles. J Pharmacol Exp Ther 280: 839-845[Abstract/Free Full Text].
Shimada H, Moewes B and Burckhardt G (1987) Indirect coupling to Na⁺ of p-aminohippuric acid uptake into rat renal basolateral membrane vesicles. Am J Physiol 253: F795-F801[Abstract/Free Full Text].
Shimomura A, Chonko AM and Grantham JJ (1981) Basis for heterogeneity of para-aminohippurate secretion in rabbit proximal tubules. Am J Physiol 240: F430-F436.
Shpun S, Evans KK and Dantzler WH (1995) Interaction of $alpha$ -KG with basolateral organic anion transporter in isolated rabbit renal S3 proximal tubules. Am J Physiol 268: F1109-F1116[Abstract/Free Full Text].
Tsunoda K, Abe K, Hagino T, Omata K, Misawa S, Imai Y and Yoshinaga K (1993) Hypotensive effect of losartan, a nonpeptide angiotensin II receptor antagonist, in essential hypertension. Am J Hypertens 6: 28-32[Medline].
Welborn JR, Shpun S, Dantzler WH and Wright SH (1998) Effect of $alpha$ -ketoglutarate on organic anion transport in single rabbit renal proximal tubules. Am J Physiol 274: F165-F174[Abstract/Free Full Text].
Werner D and Roch-Ramel F (1991) Indirect Na⁺ dependency of urate and p-aminohippurate transport in pig basolateral membrane vesicles. Am J Physiol 261: F265-F272[Abstract/Free Full Text].

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