Tetraethylammonium and Amantadine Identify Distinct Organic Cation Transporters in Rat Renal Cortical Proximal and Distal Tubules

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AMANTADINE

Vol. 290, Issue 1, 295-302, July 1999

Tetraethylammonium and Amantadine Identify Distinct Organic Cation Transporters in Rat Renal Cortical Proximal and Distal Tubules¹

Kerry B. Goralski² and Daniel S. Sitar

Departments of Pharmacology and Therapeutics (K.B.G., D.S.S.), Internal Medicine (D.S.S.), and Pediatrics and Child Health (D.S.S.), and Centre on Aging (D.S.S.), University of Manitoba, Winnipeg, Manitoba, Canada

	Abstract

Top Abstract Introduction Materials and Methods Results Discussion References

Tetraethylammonium (TEA) and amantadine are two organic cations that are secreted by the kidney. It appears that each cationmay characterize distinct renal tubule organic cation transportpathways. To test this hypothesis, we investigated the renal proximaland distal tubule energy-dependent transport properties of TEAand amantadine. Isolated tubules were incubated at 25°C in bicarbonatebuffer (Krebs-Henseleit solution) and nonbicarbonate buffer (Cross-Taggart)with varying concentrations of [¹⁴C]TEA or [³H]amantadine to determine initial rates of energy-dependent uptakeof TEA and amantadine, respectively. The uptake of TEA could bestbe described by two transport sites, a high-affinity site anda lower affinity site. TEA uptake was not influenced by the presenceof bicarbonate. Consistent with our previously reported data,amantadine uptake could also be described by two transport sites,a high-affinity-capacity site that is bicarbonate-dependent anda lower-affinity-capacity transport site that is bicarbonate-independent.The renal tubule uptake of amantadine into proximal and distaltubules, in Krebs-Henseleit solution or Cross-Taggart buffers,was not inhibited by 10 to 1000 µM of TEA. However, tubule accumulationof TEA could be inhibited (>90%) by amantadine in proximal anddistal tubules in Krebs-Henseleit solution and Cross-Taggart buffers.In proximal tubules, N¹-methylnicotinamide was not able to inhibit amantadine uptakebut it reduced TEA uptake by 60 to 70% at similar concentrations.These data support the existence of multiple renal tubule organiccation transporters that have different substrate affinity andcontrolling mechanisms. It is also apparent that amantadine characterizesorganic cation transporters that are distinct from those characterizedby TEA.

	Introduction

Top Abstract Introduction Materials and Methods Results Discussion References

The kidney functions as an organ of drug elimination that can remove drugs from the blood by glomerular filtration and tubularsecretion. Renal tubule organic cation secretion involves transport-mediatedpassage from the peritubular capillaries, across the basolateralmembrane, and into the tubule cell, followed by transport intothe tubule lumen, across the luminal membrane. In the kidney,numerous endogenous or exogenous organic cations can be secretedby the renal tubules (Rennick, 1981).

An abundance of information pertaining to the renal tubule organic cation transport system comes from studies with tetraethylammonium(TEA) as a prototypical organic cation substrate. Original studiesdemonstrated that TEA is secreted by the proximal tubules of thenephron (Rennick and Moe, 1960). Most subsequent studies havefocused on the proximal tubule as the only component of the nephronthat has the capacity for transport of organic cations, with littleattention given to distal tubules and their ability to transportTEA, or other organic cations. Transport of TEA across the basolateralmembrane of proximal tubules is a saturable, energy-dependent,carrier-mediated process that is driven by the inside negativemembrane potential and is independent of pH (Takano et al., 1984;Sokol and McKinney, 1990). Efflux from the tubule cell into thelumen is mediated by a saturable H⁺/organic cation exchanger that uses a proton gradient derivedfrom the Na⁺/H⁺ exchanger also located in the luminal membrane (Takano et al.,1984; Rafizadeh et al., 1987). However, the TEA model alone maynot be sufficient to account for the renal tubule secretion pathwaysof other organiccations.

Amantadine, a clinically used organic cation drug, is eliminated by the kidneys, and renal tubule secretion is important inthis process (Bleidner et al., 1965; Aoki et al., 1979). Amantadinehas been used extensively in our laboratory as a prototypicalsubstrate for characterizing the mechanisms of renal tubule organiccation transport. The mechanisms controlling amantadine secretionby the kidney appear to be different than for TEA. Amantadinetransport and accumulation have been demonstrated in proximaland distal tubules of male and female rats, with transport propertiesbeing heterogeneous within tubules, between tubules, and betweensexes (Wong et al., 1991-1993; Escobar et al., 1994, 1995; Escobarand Sitar, 1995, 1996). It is believed that these findings arerepresentative of amantadine influx via an energy-dependent saturablecomponent of the basolateral membrane (Escobar and Sitar, 1995).Transport sites for amantadine in proximal and distal tubulescan be subdivided into bicarbonate-dependent (high-affinity, high-capacity)sites responsible for most of the amantadine uptake and less efficientbicarbonate-independent (lower affinity, lower capacity) sites(Escobar et al., 1994; Escobar and Sitar, 1995). Although a bicarbonate-dependentbasolateral transport component has been reported for the cationN¹-methylnicotinamide (NMN) (Ullrich et al., 1991), a similar transportphenomenon has not been demonstrated for TEA. Membrane potentialand activity of the basolateral membrane Na⁺/K⁺-ATPase are not rate limiting for the renal tubule uptake of amantadine(Escobar and Sitar, 1995, 1996). These findings suggest that mostamantadine uptake occurs as a nonelectrogenic step at the basolateralmembrane as opposed to electrogenic uptake for TEA. Consideringthe apparent differences in amantadine and TEA renal tubule transportcharacteristics, we hypothesize that amantadine and TEA are selectivefor distinct basolateral membrane organic cation transportersin the kidney. Identifying distinct renal organic cation transportersand their substrate specificity by using TEA and amantadine asorganic cation probes may allow for the prediction of potentialdrug interactions in thekidney.

	Materials and Methods

Top Abstract Introduction Materials and Methods Results Discussion References

Renal Tubule Preparation. Experimental procedures involving the use of animals have been approved by the University of Manitoba Protocol Managementand Review Committee. Separation of proximal and distal tubuleswas performed by the Percoll density-gradient centrifugation method(Vinay et al., 1981; Gesek et al., 1987) as modified by Wong etal. (1990) and current modifications to improve the tissue preparation.The modified procedures are as follows: Four male Sprague-Dawleyrats (Charles River breeding stock; University of Manitoba, Canada)weighing 250 to 300 g were anesthetized with pentobarbital sodium(50 mg/kg). Kidneys were removed, immediately decapsulated, andthen placed in ice-cold Krebs-Henseleit solution (KHS) (pH 7.4).KHS contained 118 mM NaCl, 4.7 mM KCl, 1.2 mM MgCl₂, 1.4 mM KH₂PO₄,25 mM NaHCO₃, 2.5 mM CaCl₂, and 11 mM glucose. Renal corticalsections were then dissected from the medullary tissue approximately1 mm from the corticomedullary junction and placed in ice-coldKHS buffer (20 ml). Next, the cortical sections were finely mincedwith a tissue chopper (Mickle Lab. Engineering Co. Ltd., Gomshall,Surrey, UK). Minced tissue was placed in 10 ml of cold KHS andadded to a KHS-collagenase solution containing 15 ml of KHS, 1ml of 10% BSA, and 10 mg of low trypsin collagenase A (0.23 U/mglysozyme) and oxygenated for 2 min with 95% O₂/5% CO₂.

The tissue was then incubated at 31°C with shaking (100 oscillations/min) in a Dubnoff incubator (Precision Scientific Co.,Chicago, IL). During the digestion, the tissue was gently pipettedfor 5 min with a large-bore (5-ml) pipette at 15-min intervalsto assist in breaking up the tissue. To ensure adequate digestionof the tissue, the progress of digestion was monitored at 5-minintervals (beginning 30 min after the start of incubation) bylight microscopy (100× magnification) of a small aliquot of tissuefrom the digestion mixture. The duration of the digestion wasconsistently between 35 and 45 min. The digestion procedure wasterminated by addition of 30 ml of ice-cold KHS, and the tissuewas filtered through a polyethylene mesh filter (pore size 292µm) to remove any large undigested fragments. The tissue was thenwashed three times by sequential resuspension in KHS, followedby low-speed centrifugation (4°C, 60g for 1 min). The final pelletwas resuspended in 40 ml of a 50% Percoll solution (20 ml eachof Percoll and double-strength KHS at pH 7.4) and centrifugedfor 30 min at 27,000g (4°C). Proximal and distal tubules wereremoved from the gradient (bands IV and II from the top of thecentrifuge tube, respectively) and washed three times by sequentialresuspension in KHS followed by low-speed centrifugation (4°C,60g for 1min).

After the final wash, proximal and distal tubule fractions were normally resuspended in the desired volume of KHS. If thetransport assays included measurements in the absence of bicarbonate,the last wash and the final resuspension of the tubule fragmentswould be done with Cross-Taggart (CT) buffer. The CT buffer contained135 mM NaCl, 4.7 mM KCl, 1.2 mM MgCl₂, 1.4 mM KH₂PO₄, 15 mM sodiumphosphate buffer (pH 7.4), 1.0 mM CaCl₂, and 11 mM glucose, andwas pH adjusted with NaOH. Tissue protein was determined beforethe transport assays by the biuret method. At this point, theresuspension volume was adjusted to give a final protein concentrationof 6 to 8 mg/ml. The proximal and distal tubule suspensions werekept on ice until just before the start of transport assays, whenthey were warmed to room temperature by 20 min incubation in a25°C water bath. The purity of tubule fractions was assessed bymeasuring levels of enzyme markers (alkaline phosphatase for proximaland hexokinase for distal tubules) and by microscopic examinationas previously reported (Scholer and Edelman, 1979

; Vinay et al.,1981

; Wong et al., 1991

Amantadine and TEA Transport Studies. Linear rates for the energy-dependent renal tubule uptake of amantadine and TEA were determined in the presence (KHS buffer)and absence (CT buffer) of bicarbonate. For the amantadine transportassays, tubes were prepared (in triplicate) that contained a fixedamount of [³H]amantadine (1 nM) and unlabeled amantadine (final assay concentrations10-500 µM) in a volume of 150 µl of either KHS or CT buffer. Proximalor distal tubule suspensions (50 µl in the appropriate buffer)were added to each assay tube to begin the transport reaction.After addition of the tubule suspension, the assay tubes wereincubated for 30 s in a 25°C water bath with shaking (100 oscillations/min).The reactions were terminated by addition of 2 × 4 ml of ice-coldKHS, followed by rapid filtration under negative pressure, throughglass fiber filters (no. 32; Schleicher & Schuell, Inc., Keene,NH). The filters were immediately placed into scintillation vialscontaining 4 ml of Ready Safe scintillation fluid (Beckman InstrumentsInc., Fullerton, CA) and counted in a Beckman model LS5801 scintillationcounter.

The same procedure was followed for the TEA transport studies, except that each assay tube contained 10 µM [¹⁴C]TEA and unlabeled TEA (if necessary) to give final TEA concentrationsranging from 10 to 500 µM. Incubations for TEA lasted 1 min, comparedto 30 s for amantadine, to ensure the linearity of initial uptakerates. Nonspecific uptake of radioactivity to tissue and filterswas determined by measuring uptake of [³H]amantadine or [¹⁴C]TEA in the presence of a saturating amount of unlabeled amantadine(10 mM) or TEA (10 mM), respectively. Nonspecific uptake was subtractedfrom total radioactivity to determine the energy-dependent uptakeof thesecompounds.

Inhibition Studies. Inhibition of [¹⁴C]TEA (10 µM) energy-dependent uptake by unlabeled amantadine and NMN (10-1000 µM) and inhibition of [³H]amantadine uptake (10 µM) by TEA and NMN (10-1000 µM) were determinedin proximal and distal tubules in KHS and CT buffers (pH 7.4).The same procedures as described for the transport assays wereused for the inhibitorstudies.

Chemicals. [³H]Amantadine (28 Ci/mmol) was obtained from Amersham International (Buckinghamshire, UK). [¹⁴C]TEA was obtained from American Radiolabeled Chemicals, Inc.(St. Louis, MO). Collagenase was obtained from Boehringer Mannheim(Laval, Quebec, Canada). Unlabeled amantadine was obtained fromDupont Canada Inc. (Mississauga, Ontario, Canada). Unlabeled TEAand NMN were obtained from Sigma Chemical Co. All other chemicalswere of the highest grade available from commercialsuppliers.

Data Analysis. For individual experiments, each data point for the transport and inhibition studies was performed in triplicate. Data areexpressed as means ± S.E. of at least four experiments. Transportrates are reported as specific uptake (nonspecific uptake subtracted)of amantadine or TEA by the tubules in nanomoles per milligramof protein per minute. Apparent K_m and V_max values were determinedby nonlinear regression fit to the Michaelis-Menten equation witha nonlinear regression program (WinNonlin version 1.1; PharsightCorp., Palo Alto, CA). IC₅₀ values were determined from the amantadineinhibition profiles by regressive probit analysis of increasinginhibitor concentrations (Cheng and Prusoff, 1973). Dixon (1953)and Cornish-Bowden (1974) analyses were used to determine thenature of inhibition. K_m and V_max data from these experimentswere analyzed by a two-way ANOVA model with the factors buffer(bicarbonate versus nonbicarbonate) and tubule (proximal versusdistal). Observed transport rates for inhibition data were comparedwithin tubule group with the repeated measures ANOVA model. Multiplecomparisons of the significant ANOVA were performed by Tukey'shonestly significant difference (HSD) test. Differences betweenmeans with p $<=$ .05 were considered significant. All statisticalanalyses were performed with Systat for Windows 6.0.1 (SPSS Inc.,Chicago,IL).

	Results

Top Abstract Introduction Materials and Methods Results Discussion References

Amantadine and TEA Transport Studies. Data characterizing the degree of separation of proximal and distal tubules with our methodology have been previously reportedin detail by our laboratory (Wong et al., 1991, 1993; Escobaret al., 1994; Escobar and Sitar, 1995, 1996). Visual enumerationof the tubules in either fraction by hemocytometry indicates purityof $>=$ 80%. Enzyme assays demonstrate that alkaline phosphatase activityis dominant in proximal tubules, whereas hexokinase activity isdominant in distal tubules, which is consistent with their reporteddistribution in the nephron (Scholer and Edelman, 1979; Vinayet al., 1981; Gesek et al., 1987). TEA uptake was linear for atleast 60 s (r² for linear regression ranged from 0.89 to 0.98) in proximal tubulesand distal tubules in the presence and absence of bicarbonate,as shown in Fig. 1. Amantadine uptake into proximal and distaltubules was linear for at least 30 s (data not shown), as previouslyreported by our laboratory (Wong et al., 1990). Both proximaland distal tubule segments accumulated [¹⁴C]TEA and [³H]amantadine in a saturable manner (data not shown). Eadie-Hofsteeplots for energy-dependent TEA uptake versus concentration areshown in Fig. 2. The biphasic nature of the plots reveals thatTEA uptake into proximal and distal tubules may be characterizedby two transport sites, a high-affinity transport site and a loweraffinity transport site. TEA concentrations of 10 to 60 µM wereused to characterize the high-affinity TEA transport site, andconcentrations of 100 to 500 µM were used to characterize thelower affinity transport site. Figure 3 shows K_mTEA1 and V_maxTEA1(K_m and V_max for TEA uptake at the high-affinity site). K_mTEA1and V_maxTEA1 were similar in CT and KHS buffers in both proximaland distal tubules. The lack of a difference in kinetic parametersbetween buffer groups allowed us to combine the data from eachbuffer group such that we could increase the power (n = 16, comparedto 8) of detecting a difference in K_m or V_max between proximaland distal tubules. Comparing proximal and distal tubules whendata from both buffer groups were combined indicated that K_mTEA1was less (higher affinity) in proximal (33.4 ± 4.8 µM) than indistal (49.4 ± 4.8 µM) tubules (p < .05). The difference in V_maxTEA1in proximal tubules (0.295 ± 0.034 nmol · mg¹ · min¹) compared with distal tubules (0.209 ± 0.034 nmol · mg¹ · min¹) approached significance (p < .08). For the observed differencebetween mean proximal and distal tubule V_maxTEA1, a power calculationwith grouped standard deviation (0.133 nmol · mg¹ · min¹) indicated that at least 37 replicates would be required to detecta significant difference when symbol 97 = 0.05 and symbol 98 =0.20 and thus was not pursued. For the lower-affinity site, K_mTEA2and V_maxTEA2 were similar between tubule fragments and were notdependent on the presence of bicarbonate in the medium (Fig. 4).K_m and V_max for the lower affinity TEA uptake sites were 5- to10-fold and 3- to 4-fold greater, respectively, than for the high-affinitysites.

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Fig. 1. Representative plots of a single experiment showing TEA (10 µM) uptake versus time into isolated renal cortical proximal (top) and distal (bottom) tubules in the presence (KHS) and absence (CT) of bicarbonate at pH 7.4. Total TEA uptake is expressed as nanomoles per milligram of protein.

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Fig. 2. Eadie-Hofstee plots for rate of TEA uptake into isolated renal cortical proximal (top) and distal (bottom) tubules. v, rate of TEA uptake (nmol · mg¹ protein · min¹); [s], concentration of TEA (µM). Each data point represents the mean ± S.E. of six to eight separate determinations.

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Fig. 3. Calculated apparent K_m (top) and V_max (bottom) values for [¹⁴C]TEA uptake by high-affinity transport site in proximal and distal tubules in the presence (KHS) and absence (CT) of bicarbonate at pH 7.4. TEA concentrations used in each experiment were 10, 20, 35, and 60 µM. Values are means ± S.E. from eight separate determinations. Treatment groups were compared by two-way ANOVA, with tubule and buffer as the grouping variables. *p < .05, $dagger$ p < .08, proximal tubules versus distal tubules when data from KHS and CT groups are combined.

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Fig. 4. Calculated apparent K_m (top) and V_max (bottom) values for [¹⁴C]TEA uptake by lower affinity transport site in proximal and distal tubules in the presence (KHS) and absence (CT) of bicarbonate at pH 7.4. TEA concentrations used in each experiment were 100, 200, 300, and 500 µM. Values are means ± S.E. of four to six separate determinations. Treatment groups were compared by two-way ANOVA, with tubule and buffer as the grouping variables. K_m and V_max for the proposed low-affinity site were not dependent on tubule type, buffer, or tubule-buffer interactions. p > .1.

Kinetic parameters for amantadine uptake are shown in Fig. 5. K_mA (K_m for amantadine uptake) was similar in both proximaland distal tubules and was increased when CT was substituted forKHS buffer (p < .001). V_maxA (V_max for amantadine uptake) wasgreater in proximal tubules than in distal tubules in both buffers(p < .001). In both tubule fragments, V_max was reduced in CT buffercompared with KHS buffer (p < .001). Unlike for TEA, Eadie-Hofsteeanalysis for amantadine uptake in either KHS or CT reveals onlya single transport component (data not shown).

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Fig. 5. Measured apparent K_m (top) and V_max (bottom) values for [³H]amantadine uptake by isolated renal proximal and distal tubules in the presence (KHS) and absence (CT) of bicarbonate at pH 7.4. Amantadine concentrations used in each experiment were 10, 20, 50, 100, 300, and 500 µM. Values are means ± S.E. of four separate determinations. Treatment groups were compared by two-way ANOVA, with tubule and buffer as the grouping variables. ***p < .001 versus KHS within tubule group. $ddager$ p < .001, proximal versus distal tubule within same buffer group.

Inhibition Studies. We first evaluated the ability of TEA to inhibit the energy-dependent renal tubule uptake of amantadine (Fig. 6). TEA concentrationsranging from 10 to 1000 µM were unable to impede the uptake ofamantadine into isolated renal proximal and distal tubules inbicarbonate or phosphate buffer at pH 7.4. Conversely, amantadinewas able to inhibit TEA uptake into proximal and distal tubules(p < .05) compared with the respective control (Fig. 7). The inhibitionprofiles were similar in bicarbonate and phosphate buffers.

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Fig. 6. TEA inhibition of 10 µM amantadine uptake into isolated renal cortical proximal and distal tubules in the presence (KHS) and absence (CT) of bicarbonate at pH 7.4. Values are means ± S.E. of four separate determinations.

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Fig. 7. Amantadine inhibition of 10 µM TEA uptake into isolated renal cortical proximal (top) and distal (bottom) tubules in the presence (KHS) and absence (CT) of bicarbonate at pH 7.4. Values are means ± S.E. of five to seven separate determinations. *p < .05, **p < .01, ***p < .001, versus control (no amantadine present); repeated measures ANOVA followed by Tukey's HSD test.

Subsequently, we analyzed the ability of another prototypical organic cation substrate (NMN) to inhibit amantadine and TEAuptake (Fig. 8). In proximal tubules, NMN was not able to inhibitamantadine uptake, but at higher concentrations, it reduced TEAuptake by 60 to 70% (p < .05). A similar NMN inhibition profilefor TEA was observed in distal tubules, where NMN had no effecton amantadine uptake in CT buffer but inhibited amantadine uptakeby 30 to 40% in KHS buffer (p < .05).

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Fig. 8. NMN inhibition of amantadine (squares) and TEA (circles) uptake into proximal (top) and distal (bottom) tubules. Assays were performed in KHS (solid symbols) and CT buffers (open symbols) buffers at pH 7.4. Values are means ± S.E. of four separate determinations. *p < .05, **p < .01, ***p < .001, versus respective amantadine or TEA control; repeated measures ANOVA followed by Tukey's HSD test.

Table 1 shows IC₅₀ and inhibitor dissociation constant (K_i) values for amantadine inhibition of TEA uptake. IC₅₀ values weredetermined from the amantadine inhibition profiles by regressiveprobit analysis. Dixon and Cornish-Bowden analyses confirmed thatamantadine inhibition of TEA uptake was consistent with that ofcompetitive inhibition (data not shown), justifying the determinationof K_i from IC₅₀ values by the Cheng-Prusoff (1973

) competitionmethod. K_i values were similar in proximal and distal tubulesand did not differ between KHS and CT buffers. The ratios of K_mfor amantadine uptake versus K_i for amantadine inhibition of TEAuptake were calculated (Table 1). In both proximal and distaltubules, the K_mA/K_i ratios were >1. The K_mA/K_i ratio was greaterin CT buffer than in KHS buffer.

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TABLE 1
Derived IC₅₀ and K_i values for amantadine inhibition of energy-dependent uptake of TEA by isolated rat renal cortical proximal and distal tubules compared to apparent K_m values calculated for amantadine transport under the same conditions
Concentrations are expressed in µM ± S.E.M. of four to seven experiments.

	Discussion

Top Abstract Introduction Materials and Methods Results Discussion References

Amantadine uptake into proximal and distal tubules from the rat could be described by a high-affinity-capacity, bicarbonate-dependenttransport site and a lower affinity-capacity, bicarbonate-independenttransport site and is concordant with previous studies (Escobaret al., 1994; Escobar and Sitar, 1995). The K_mA and V_maxA valuesreported herein were somewhat higher than those reported by Escobaret al. (1994). However, the same qualitative effects on amantadinetransport were maintained, namely, a decrease in V_max and an increasein K_m in the absence ofbicarbonate.

The uptake of TEA into isolated proximal and distal tubules was best characterized by a high-affinity, low-capacity componentand a lower affinity, higher-capacity component. To the best ofour knowledge, this is the first report to describe energy-dependentdistal tubule transport of TEA. Unlike amantadine, the uptakeof TEA at these two sites was similar in the presence and absenceof bicarbonate. Most other studies have described only a singletransport site for TEA, with widely varying affinity (Schali etal., 1983; Takano et al., 1984; Wright and Wunz, 1987; McKinneyet al., 1990; Ullrich et al., 1991; Takami et al., 1998). Theone exception (Grundemann et al., 1997) demonstrated a high-affinitycomponent (20 µM) and a low-affinity component (620 µM) for TEAuptake by the OCT2p transporter transfected into human 293 cells.We believe that the failure of others to detect two transportsites for TEA relates to the selection of TEA concentrations usedin attempts to characterize its transport properties. The differencein K_mTEA1 and possibly V_maxTEA1 between proximal and distal tubulessuggests that the composition of transporters involved in uptakeof TEA is different between the tubule segments, with a higheraffinity-capacity component existing in the proximal tubules.The observed differences in the bicarbonate effect on amantadineversus TEA transport further support the division of basolateralmembrane organic cation transporters into those that are bicarbonatedependent and those that are independent (Escobar et al., 1994).

The inhibition studies showed that TEA could not inhibit amantadine uptake. The highest concentration of TEA (1000 µM) wasgreater than the high- and lower-affinity K_m values for TEA uptakein proximal and distal tubules. This saturating concentrationof TEA would be expected to inhibit amantadine uptake if the twocompounds entered the tubules via identical transporters. Conversely,amantadine can block TEA uptake completely. The fact that amantadineinhibited TEA uptake but TEA did not inhibit amantadine uptakesuggests that 1) TEA is not transported and does not interactwith the bicarbonate-dependent and bicarbonate-independent amantadinetransporters; 2) amantadine interacts with the TEA transportersbut is not transported; or 3) TEA transporters also transportamantadine, but the proportion of uptake at this site is so smallthat any inhibition of amantadine uptake by TEA is masked by thelarger bicarbonate-dependent amantadine transportcomponent.

In addition to TEA, NMN has been used to characterize organic cation transport in the kidney (Kinsella et al., 1979; Holohanand Ross, 1980). NMN has been demonstrated to inhibit renal tubuletransport of TEA (Montrose-Rafizadeh et al., 1989; Ullrich etal., 1991), but interactions with amantadine uptake have not beenreported. The fact that NMN does not inhibit amantadine uptakein proximal tubules at concentrations that inhibit TEA uptakestrengthens the argument that TEA and amantadine may characterizedifferent transportsites.

The distinctness of the organic cation transport sites for TEA and amantadine are further supported by the difference in K_mfor amantadine uptake versus the K_i for amantadine inhibitionof TEA transport. Theoretically, the K_m/K_i ratio should be near1 when TEA transport sites are the same as those previously identifiedfor amantadine and competitive inhibition is assumed. The observedK_m/K_i ratio is substantially greater than 1 for both proximaland distal tubules and is greater in CT than in KHS buffer. Thus,the bicarbonate-dependent and bicarbonate-independent amantadinetransport sites may be different from those described by TEA.

Our previous model to explain organic cation transport by renal proximal tubules (Escobar and Sitar, 1995) has been revisedto reflect the findings of this study (Fig. 9). Transport site1 in Fig. 9 represents the high-affinity-capacity, bicarbonate-dependentamantadine transporter responsible for approximately 80% of basolateralamantadine uptake into the tubule cell. Transport site 2 representsa lower affinity-capacity, bicarbonate-independent amantadinetransporter responsible for about 20% of amantadine uptake. Ourdata show that TEA is not a substrate for transport site 1 or2. Basolateral uptake of TEA may be best characterized by twoadditional bicarbonate-independent transport sites $---$ a high-affinity,low-capacity site (site 3) and a lower affinity, higher-capacitysite (site 4). Sites 3 and 4 may also represent higher-affinity,lower capacity transport sites for amantadine, as identified byamantadine inhibition of TEA uptake. In proximal tubules, NMNappears to interact with the TEA transport sites but not the amantadinetransport sites. On the luminal membrane, exit of TEA is mediatedby an H⁺/organic cation exchanger (transport site 5) that uses the H⁺ gradient (out $right-arrow$ in) created by the Na⁺/H⁺ exchanger (Takano et al., 1984; Rafizadeh et al., 1987). Transportof certain organic cations (not including TEA) across the luminalmembrane may also be mediated by the ATP-dependent P-glycoprotein(transport site 7) (Dutt et al., 1994). Further studies are necessaryto evaluate whether the mechanisms of luminal transport of amantadineare similar to those of TEA and whether amantadine is a substratefor P-glycoprotein. Our data suggest that similar organic cationtransport mechanisms for amantadine and TEA exist in the distaltubule. However, for both amantadine and TEA, existing in vivoevidence is insufficient to determine the relative contributionof the proximal and distal tubules to total renal secretion ofthese compounds.

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Fig. 9. Revised model for organic cation transport by rat renal proximal tubules when amantadine and TEA are used as prototypical substrates to characterize this system. Site 1, high-affinity-capacity, bicarbonate-dependent amantadine transporter. Site 2, low-affinity-capacity, bicarbonate-independent amantadine transporter. Site 3, high-affinity, low-capacity TEA transporter (inhibited by amantadine). Site 4, low-affinity, high-capacity TEA transporter (possibly inhibited by amantadine). Site 5, luminal membrane Na⁺/H⁺ exchanger. Site 6, H⁺/organic cation exchanger. Site 7, P-glycoprotein. A⁺, amantadine; OC⁺, organic cation; (+), activation; ( $-$ ), inhibition.

rOCT1, rOCT1a, rOCT2, and rOCT3 are members of the organic cation transporter family that are expressed in the rat kidneyand have been demonstrated to transport TEA (Grundemann et al.,1994; Okuda et al., 1996; Zhang et al., 1997; Kekuda et al., 1998).Of the cloned rat organic cation transporters, rOCT1 is thoughtto be localized in basolateral membranes of S1 rat proximal tubulesegments (Koepsell, 1998). rOCT2 is located in the basolateralmembranes of S2 and S3 rat proximal tubule segments and possiblydistal tubules (Koepsell, 1998). Our data probably reflect TEAuptake by at least two of these transporters. For the proposedhigh-affinity TEA transport site, our K_mTEA1 values (33 µM forproximal tubules and 49 µM for distal tubules) closely correspondto those estimated for rOCT1a (42 µM) expressed in Xenopus oocytes(Zhang et al., 1997) and rOCT1 (38 µM) and rOCT2 (42 µM) expressedin MDCK dog kidney distal tubule cell lines (Urakami et al., 1998).For the proposed lower affinity TEA transport site, our K_mTEA2values (246-331 µM) were intermediate between those reported forTEA uptake by rOCT1 (K_m = 95 µM) and rOCT2 (K_m = 500 µM) (Grundemannet al., 1994; Koepsell, 1998). The estimated K_m for TEA uptakeby rOCT3 was 2.5 mM by tracer uptake studies (Kekuda et al., 1998).Thus, rOCT3 should not be a major contributor to TEA uptake inour preparation. Our K_mTEA1 and K_mTEA2 values are similar to thosereported for rOCT1, rOCT1a and rOCT2 and suggest that basolateralTEA uptake into isolated renal tubules may be mediated by somecombination of uptake by these transporters. The fact that expressionof rOCT1 and rOCT2 in Xenopus oocytes (Grundemann et al., 1994;Koepsell, 1998) and MDCK cells (Urakami et al., 1998) gives differentestimates of K_m suggests the cell expression system used may influencekinetic determinations. It is not known which expression systemcompares best to that of normal renal tubule cells. Therefore,our ability to identify the two TEA transporters detected in thisstudy is limited. Because TEA does not inhibit amantadine uptake,rOCT1, rOCT1a, and rOCT2 may be excluded as the bicarbonate-dependentamantadine transporters. This hypothesis remains to be testedby evaluating the ability of specific inhibitors of rOCT1 andrOCT2 to block amantadine and TEA uptake into the renal tubulepreparations.

NKT, NLT, and RST are kidney-expressed proteins that are highly homologous to the OCT family and have been speculated to transportorganic cations (Simonson et al., 1994; Mori et al., 1997; Lopez-Nietoet al., 1997). These proteins may contribute to amantadine transportin thekidney.

In summary, it has been proposed that the basolateral uptake of type 1 (small, more hydrophilic) organic cations in the proximaltubule is mediated by a single, multispecific, saturable componentof the membrane, namely, OCT1 (Koepsell, 1998). Use of differentprototypical type 1 organic cation substrates (amantadine versusTEA) gives a vastly different depiction of organic cation transportin the kidney. This discrepancy suggests that multiple transporterswith dissimilar controlling mechanisms may mediate the renal tubulebasolateral transport of type 1 organic cations in proximal anddistal tubules. Considering the observed differences in amantadineand TEA renal tubule transport, we conclude that amantadine andTEA identify distinct organic cation transport sites in the kidney.Identification of substrate specificity for the different renalorganic cation transporters may enable the prediction of potentialdrug interactions in thekidney.

	Footnotes

Accepted for publication March 17, 1999.

Received for publication December 4, 1998.

¹ This study was funded by Grants MA-11664 and MT-14710 from the Medical Research Council ofCanada.

² Recipient of a Manitoba Health Research CouncilStudentship.

Send reprint requests to: Daniel S. Sitar, Ph.D., Clinical Pharmacology Section, University of Manitoba, A206-770 Bannatyne Ave., Winnipeg, Manitoba, Canada R3E 0W3. E-mail: sitar{at}ms.umanitoba.ca

	Abbreviations

CT, Cross-Taggart; KHS, Krebs-Henseleit solution; TEA, tetraethylammonium; rOCT, rat organic cation transporter; NMN, N¹-methylnicotinamide.

	References

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AMANTADINE

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Tetraethylammonium and Amantadine Identify Distinct Organic Cation Transporters in Rat Renal Cortical Proximal and Distal Tubules1

Tetraethylammonium and Amantadine Identify Distinct Organic Cation Transporters in Rat Renal Cortical Proximal and Distal Tubules¹