Nephrotoxicants Induce Endothelin Release and Signaling in Renal Proximal Tubules: Effect on Drug Efflux

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Vol. 59, Issue 6, 1433-1440, June 2001

Nephrotoxicants Induce Endothelin Release and Signaling in Renal Proximal Tubules: Effect on Drug Efflux

Sylvie A. Terlouw, Rosalinde Masereeuw, Frans G. M. Russel, and David S. Miller

Department of Pharmacology and Toxicology, University Medical Centre Nijmegen, Nijmegen, The Netherlands (S.A.T., R.M., F.G.M.R.); Laboratory of Pharmacology and Chemistry, National Institute of Environmental Health Sciences, National Institutes of Health, Research Triangle Park, North Carolina (D.S.M.); and Mount Desert Island Biological Laboratory, Salisbury Cove, Maine (S.A.T., D.S.M.)

	Abstract

Top Abstract Introduction Materials and Methods Results Discussion References

We previously used killifish proximal tubules, fluorescent substrates, and confocal microscopy to demonstrate that transportmediated by the multidrug resistance protein (Mrp2) and by P-glycoproteinwas reduced by nanomolar concentrations of endothelin-1 (ET),acting through a basolateral B-type ET receptor and protein kinaseC (PKC). Here we show that representatives of two classes of nephrotoxicantsdecrease transport by activating the endothelin-PKC signalingpathway. Exposing tubules to radiocontrast agents (iohexol, diatrizoate)or aminoglycoside antibiotics (gentamicin, amikacin) reduced Mrp2-mediatedfluorescein methotrexate (FL-MTX) transport from cell to tubularlumen. Pretreating the tubules with an ET_B-receptor antagonistor with PKC-selective inhibitors abolished these effects. Thenephrotoxicants activated signaling by inducing release of ETfrom the tubules, because adding of an antibody against ET tothe medium abolished the effects. Elevating medium Ca²⁺ also reduced FL-MTX transport; this reduction was abolished whentubules were pretreated with an ET antibody, an ET_B-receptor antagonist,PKC-selective inhibitors, or the Ca²⁺ channel blocker, nifedipine. None of these drugs by themselvesaffected FL-MTX transport. Importantly, nifedipine also blockedthe ET_B-receptor/PKC-dependent reduction in FL-MTX transport causedby gentamicin and diatrizoate. These results for two classes ofstructurally unrelated nephrotoxicants suggest that Ca²⁺-dependent ET release and subsequent action through an autocrinemechanism may be an early response to tubularinjury.

	Introduction

Top Abstract Introduction Materials and Methods Results Discussion References

Endothelins (ETs) are polypeptide hormones that are potent vasoconstrictors. ET isoforms (ET-1, ET-2, and ET-3) are synthesizedin many tissues and can affect the function of vascular and nonvasculartissues by interacting with two pharmacologically distinct, Gprotein-coupled receptors, ET_A and ET_B. ETs have been implicatedin diseases involving the vasculature, such as acute myocardialinfarction, atherosclerosis, congestive heart failure, and hypertension(Rubanyi and Polokoff, 1994; Hocher et al., 1997). In the kidney,ET regulates blood flow, glomerular hemodynamics, and sodium andwater homeostasis (Rubanyi and Polokoff, 1994) but also playsa role in a number of renal diseases, including acute and chronicrenal failure, renal glomerular and interstitial fibrosis, diabeticnephropathy, vascular rejection of the transplanted kidney, reperfusioninjury, and nephrotoxicity induced by a variety of chemicals (e.g.,cyclosporin A, cisplatin, and radiocontrast agents) (Clavell andBurnett, Jr. 1994; Rubanyi and Polokoff, 1994; Bruzzi et al.,1997; Hocher et al., 1997; Haug et al., 1998). Urinary ET-1 excretionincreases in chronic renal failure from a variety of causes, includingradiocontrast nephropathy and during cyclosporin and cisplatinadministration (Bruzzi et al., 1997; Hocher et al., 1997). Underpathophysiological conditions, the ET receptor density in kidneychanges dramatically, especially that of the ET_B receptor (Hocheret al., 1997). Finally, ET receptor antagonists have been usedin animal models of acute renal failure to limit the effects ofnephrotoxicants and of reperfusion injury (Bird et al., 1996;Krause et al., 1997).

Clearly, disruption of vascular function is an important element of the role of ET in renal disease. However, recent studiesprovide evidence for direct tubular effects of ET. For example,in renal proximal tubule, ET regulates Na⁺/H⁺ exchange, Na⁺-HCO₃ cotransport and fluid absorption (Garcia and Garvin, 1994; Guntupalliand DuBose, 1994). Moreover, an increase in ET production wasobserved in renal proximal tubules after exposure to cyclosporinA, mercury, high-molecular-weight proteins, and hypoxia, suggestingthat these nephrotoxicants can act through ET to alter tubularfunction (Zoja et al., 1995; Bruzzi et al., 1997; Haug et al.,1998; Yanagisawa et al., 1998).

Recently, Masereeuw et al. (2000) demonstrated another tubular function of ET. Using isolated killifish proximal tubules andconfocal microscopy, we found that ET acted through a basolateralET_B receptor and protein kinase C (PKC) to regulate two luminal,ATP-driven xenobiotic transporters, P-glycoprotein, and multidrugresistance protein 2 (Mrp2). We also showed that when isolatedtubules were exposed to the nephrotoxic radiocontrast agent iohexol,transport through P-glycoprotein and Mrp2 was reduced. Transportwas restored, however, when tubules were pretreated with an ET_B-receptorantagonist, suggesting that iohexol had fired the ET signalingsystem and that such signaling could be an early event in tubulartoxicity. In the present study, we use changes in Mrp2-mediateddrug secretion to establish the generality of the finding andto begin to characterize the pathophysiological mechanisms involved.We demonstrate that representatives of two classes of nephrotoxicantscaused ET release from the tubules followed by autocrine activationof ET signaling. Ca²⁺ influx seems to be one stimulus for ETrelease.

	Materials and Methods

Top Abstract Introduction Materials and Methods Results Discussion References

Chemicals. FL-MTX and phorbol 12-myristate 13-acetate (PMA) were purchased from Molecular Probes (Eugene, OR). The ET_A receptor antagonist(JKC-301) and ET_B receptor antagonist (RES-701-1) were obtainedfrom Peninsula Laboratories (Belmont, CA). Bis-indolylmaleimideI (BIM), nifedipine, diatrizoate, amikacin, gentamicin, and monoclonalanti-ET-1 IgG (mouse-derived) were purchased from Sigma ChemicalCo. (St. Louis, MO). Rabbit polyclonal antibodies directed againstMrp2 (k78 mrp2) were obtained as described previously (van Aubelet al., 1998). Fluorescein-labeled anti-rabbit IgG was purchasedfrom Kirkegaard & Perry Lab, Inc. (Gaithersburg, MD). Iohexolwas obtained from Nycomed (Oslo, Norway). All other chemicalswere obtained from commercial sources at the highest purityavailable.

Animals and Tissue Preparation. Killifish (Fundulus heteroclitus) were collected by local fishermen in the vicinity of Mount Desert Island, Maine, and maintainedat the Mount Desert Island Biological Laboratory in tanks withnatural flowing sea water. Renal tubular masses were isolatedin a marine teleost saline based on that of Forster and Taggart(1950), containing 140 mM NaCl, 2.5 mM KCl, 1.5 mM CaCl₂, 1.0mM MgCl₂ and 20 mM Tris at pH 8.0. All experiments were carriedout at 18 to 20°C. Under a dissecting microscope, each mass wasteased with fine forceps to remove adherent hematopoietic tissue.Individual killifish proximal tubules were dissected and transferredto a foil-covered Teflon chamber (Bionique, Saranac Lake, NY)containing 1.5 ml of marine teleost saline with 1 µM FL-MTX andadded effectors. The chamber floor was a 4- × 4-cm glass coverslipto which the tubules adhered lightly and through which the tissuecould be viewed by means of an inverted microscope. Tubules wereincubated at room temperature for 30 min until steady state wasreached for FL-MTX. Analysis of tubule extracts by high-performanceliquid chromatography showed no metabolic degradation of FL-MTXwhen incubated with killifish proximal tubules for periods ofat least 1 h (Schramm et al., 1995; Masereeuw et al., 1996).

Confocal Microscopy. The chamber containing renal tubules was mounted onto the stage of an Olympus FluoView inverted confocal laser scanning microscope(Olympus, Tokyo, Japan) and viewed through a 40× water immersionobjective (NA 1.15). Excitation was provided by the 488-nm lineof an argon laser. A 510-nm dichroic filter and a 515-nm long-passemission filter were used. Neutral density filters and low laserintensity were used to avoid photobleaching. With the photomultipliergain set to give an average luminal fluorescence intensity of1500 to 3000 (on a scale of 0-4096), tissue autofluorescence wasundetectable. To obtain an image, dye-loaded tubules in the chamberwere viewed under reduced, transmitted light illumination, anda single proximal tubule with well-defined lumen and undamagedepithelium was selected. The plane of focus was adjusted to cutthrough the center of the tubular lumen and an image was acquiredby averaging four scans. The confocal image was viewed on a high-resolutionmonitor and saved to an optical disk. In previous studies, ithas been shown that there is a linear relationship between fluorescenceintensity and dye concentration (Miller and Pritchard, 1991).However, because of the many uncertainties in relating cellularfluorescence to actual compound concentration in cells and tissueswith complex geometry, data are reported here as average measuredpixel intensity rather than estimated dye concentration. Fluorescenceintensities were measured from stored images using National Institutesof Health Image 1.61 software as described previously in greatdetail (Masereeuw et al., 1996; Miller et al., 1996). Briefly,two or three adjacent cellular and luminal areas were selectedfrom each tubule, and the average pixel intensity for each areawas calculated after background subtraction. The values used forthat tubule were the means of all the selected areas. For immunohistochemistrywith anti-Mrp2 antibodies and a fluorescent secondary antibody,killifish renal tubules were treated as described previously (Masereeuwet al., 2000).

Data Analysis. Data are given as means ± S.E. Mean values were considered to be significantly different when P < 0.05 by use of the appropriatepaired or unpaired t test, or by a one-way ANOVA followed by Bonferroni'smultiple comparisontest.

	Results

Top Abstract Introduction Materials and Methods Results Discussion References

Nephrotoxicants and Mrp2-Mediated Transport. The present experiments were conducted using isolated renal proximal tubules from a teleost fish, the killifish. This hasproven a powerful model for the study of secretory transport inan intact proximal tubule. As discussed previously (Miller, 1987;Pritchard and Miller, 1991), renal tissue from certain marineteleosts offers several important advantages for the study ofsecretory transport in proximal tubule. Teleost kidneys containa high proportion of proximal tubules that are easily isolatedand that remain viable for long periods. When tubules are isolated,broken ends rapidly reseal to form a closed, fluid-filled, luminalcompartment that communicates only with the medium through thetubular epithelium. Thus, this tissue has the appropriate geometryfor the study of transepithelial secretion in intact tubules.Moreover, secretory transport mechanisms found in teleost tubulesseem to be identical to those found in mammalian proximal tubules(Pritchard and Miller, 1991; Masereeuw et al., 1996; Miller etal., 1996). Finally, when teleost tubules are used along withfluorescent substrates and quantitative fluorescence microscopy,the mechanisms driving both uptake by the cells and secretioninto the tubular lumen can be examined (Masereeuw et al., 1996;Miller et al., 1996).

Figure 1, A and B, show confocal images of control tubules after 30-min (steady-state) incubation in medium with 1 µM FL-MTX.The fluorescence distribution pattern is the same as shown previously(i.e., fluorescence intensity in lumen>cells>medium). We havedemonstrated that this pattern is indicative of a two-step process,involving uptake at the basolateral membrane mediated by an as-yet-uncharacterizedtransporter for large organic anions and secretion into the lumenmediated by a teleost form of Mrp2 (for data on substrate andinhibitor specificities as well as immunostaining with Mrp2 antibodies,see Masereeuw et al., 2000

). Figure 1, C-F, shows confocal imagesof tubules incubated in media with FL-MTX and representativesof two classes of nephrotoxicants: the aminoglycosides, amikacinand gentamicin, and the radiocontrast agents, diatrizoate andiohexol. All nephrotoxic agents tested reduced the luminal accumulationof FL-MTX but had minimal effects on cellular accumulation. Thisinhibition pattern is the same as that seen with specific inhibitorsof Mrp2, such as the competitor leukotriene C₄. As shown previously(Masereeuw et al., 1996

, 2000

), the absence of an increase incellular fluorescence when luminal transport was blocked indicatesthat efflux into the lumen is not an important determinant ofsteady-state cellular FL-MTX accumulation. The steady-state cellularlevels of FL-MTX seem to set independently of events at the luminalmembrane.

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Fig. 1. Confocal images of killifish proximal tubules after incubation in medium with 1 µM FL-MTX for 30 min in absence or presence of nephrotoxicants. Controls (A and B), and in presence of 50 µM amikacin (C), 10 µM gentamicin (D), 100 µM diatrizoate (E), and 300 µM iohexol (F).

To elucidate the mechanism by which these compounds reduced Mrp2-mediated transport, we measured steady-state cellular andluminal accumulation of FL-MTX (average cellular and luminal fluorescenceintensities) in tubules exposed to the nephrotoxicants withoutand with pharmacological agents that act at specific cellularsites. Initially, we determined the concentration-dependence ofinhibition of transport for each of the nephrotoxic compounds.Figure 2 shows data for the aminoglycoside antibiotic, gentamicin,which at 1 to 100 µM reduced luminal fluorescence in a concentration-dependentmanner; cellular fluorescence was not affected by gentamicin.Similar experiments were conducted with the other nephrotoxicants(not shown); for each, we selected for further study a concentrationthat caused about 50% reduction in luminal fluorescence. Table1 presents the inhibition data for each of the compounds. Aswith gentamicin (above), only luminal fluorescence was reduced,no significant reductions in cellular fluorescence were found.Thus, all of these chemicals reduced Mrp2-mediated transport ofFL-MTX.

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Fig. 2. Inhibition of FL-MTX transport by gentamicin. Tubules were incubated for 30 min in medium containing 1 µM FL-MTX and 0 to 100 µM gentamicin. Data are given as mean ± S.E. for 13 to 43 tubules from one to three fish. $black-square$ , lumen;

, cells.

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TABLE 1
Effect of various nephrotoxic agents on the transport of 1 µM FL-MTX from cell to tubular lumen in killifish proximal tubules
Luminal and cellular fluorescence intensities of control tubules and tubules exposed to various nephrotoxicants. All four nephrotoxic chemicals significantly reduced luminal FL-MTX accumulation (P < 0.01), whereas cellular accumulation was not affected. Values are expressed as mean ± S.E., N = 24 to 45 from two to three fish.

ET Signaling. Previous experiments showed that the reduction of Mrp2-mediated transport caused by iohexol could be prevented by pretreatingtubules with 100 nM concentrations of the ET_B receptor antagonist,RES-701-1. The ET_A receptor antagonist, JKC-301 was without effectand neither receptor antagonist by itself altered transport (Masereeuwet al., 2000). Figure 3A shows that 100 nM RES-701-1 was alsoprotective when tubules were exposed to gentamicin. As with iohexol,JKC-301 had no such protective effect. In contrast, when Mrp2-mediatedFL-MTX transport was reduced by leukotriene C₄, RES-701-1 waswithout effect, indicating that the receptor antagonist did notinteract with the transporter (Fig. 3B). Results of experimentswith all four nephrotoxic compounds are summarized in Table 2.In each case, pretreating the tubules with 100 nM RES-701-1 preventedthe nephrotoxicant-induced decrease in luminal fluorescence. Althoughthe reversal of RES-701-1 on the iohexol-treated tubules seemsto be incomplete, the reversal was comparable with the controltubules and significantly higher than the iohexol treatment alone.

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Fig. 3. Effect of the ET_B receptor antagonist, RES-701-1 (100 nM) on the gentamicin-induced (A) and leukotriene C₄-induced (B) reduction in FL-MTX transport. C, effect of 1 µM BIM (PKC inhibitor) on FL-MTX transport in gentamicin-treated tubules. Tubules were incubated for 30 min in medium containing 1 µM FL-MTX without (control) or with the indicated additions. Data are given as mean ± S.E. for 10 to 18 tubules from a single fish. **, Significantly lower than controls, P < 0.01. $black-square$ , lumen;

, cells.

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TABLE 2
Reversal of the effect of various nephrotoxic agents on the transport of 1 µM FL-MTX from cell to tubular lumen in killifish proximal tubules
Data are expressed as percentage of FL-MTX transported compared with control tubules. The PKC-selective inhibitor BIM (1 µM), the ET_B receptor antagonist RES-701-1 (100 nM), and the Ca²⁺ channel blocker nifedipine (10 µM) significantly reduced the inhibition mediated by the various nephrotoxicants (P < .01). Data are given as mean ± S.E., N = 10 to 45 from one to three fish.

In killifish proximal tubules, ET acting through the ET_B receptor signals a decrease in Mrp2-mediated transport by activatingPKC (Masereeuw et al., 2000

). If the nephrotoxicants activatedthis signaling pathway, their effects should be abolished whenPKC activation is prevented. To establish whether PKC activationis an intermediate step in the action of the nephrotoxic agents,we used a PKC-selective inhibitor, BIM. Although BIM by itselfdid not affect FL-MTX transport, for every nephrotoxicant, itdid prevent the decrease in Mrp2-mediated FL-MTX transport (Fig.3C and Table 2).

Together, these findings indicate that the four nephrotoxic compounds trigger a signaling pathway that involves the ET_B receptorand PKC activation. Because these compounds are so structurallydiverse and so different from the natural ligands for the ET_Breceptor, it is unlikely that the compounds themselves are receptoragonists. Rather, the data imply that nephrotoxicant exposurecauses ET release from the tubules and that ET acts by an autocrinemechanism to fire the signaling pathway that ultimately reducesMrp2-mediated transport. To test this directly, we pretreatedtubules for 30 min with an excess of a monoclonal antibody againstET-1 (cross-reacts with ET-2 and ET-3) and then exposed tubulesto gentamicin. Figure 4A shows that exposing tubules to the antibodyalone did not affect FL-MTX transport, but that pretreating tubuleswith an ET antibody prevented the decrease in transport inducedby gentamicin. In contrast, pretreatment with a different, nonspecific,monoclonal antibody (a donkey-derived $alpha$ -rabbit-HRP IgG), did notprevent the decrease in FL-MTX transport caused by gentamicin(Fig. 4B).

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Fig. 4. Effect of 10 µM gentamicin (B) on FL-MTX transport and reversal by 1% (v/v) antibody against ET-1 (A), but not by a monoclonal antibody not specific for ET (B). Tubules were pretreated without (control) or with the antibody for 30 min and were subsequently incubated for 30 min in medium containing 1 µM FL-MTX without (control) or with 10 µM gentamicin or gentamicin plus the antibody. Data are given as mean ± S.E. for 14 to 15 tubules from a single fish. **Significantly lower than controls, P < 0.01. $black-square$ , lumen;

, cells.

To study the mechanism by which the function of Mrp2 is regulated by ET, killifish tubules were preincubated for 30 min inthe presence or absence of 10 nM ET-1 and were subsequently immunostainedusing antibodies to Mrp2. The control tubules showed a very brightluminal staining. However, the tubules treated with ET-1 showedthe same pattern (Fig. 5). There was no difference in averagefluorescence intensity or band thickness, suggesting that if ETsignaled internalization of Mrp2, it was not detectable usingconfocal microscopy.

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Fig. 5. Confocal micrographs of killifish tubules immunostained with anti-Mrp2 antibodies and a fluorescent secondary antibody in the absence (A) and presence of 10 nM ET-1 for 30 min (B).

Involvement of Ca²⁺. In the vascular endothelium, ET-1 release is signaled by an increase in intracellular Ca²⁺ (Tasaka and Kitazumi, 1994; Carlini et al., 1995; Marsen et al.,1996). Moreover, elevated intracellular Ca²⁺ is known to be one response of renal proximal tubule cells toacute injury (Humes, 1986; Smith et al., 1992; Rose et al., 1994).The Ca²⁺ concentration in the normal medium used for the present experimentswas 1.5 mM. Increasing medium Ca²⁺ to 3 mM reduced secretion of FL-MTX by 60% (Fig. 6, A and B).Pretreating tubules with BIM or RES-701-1 abolished this reduction,indicating that the increase in medium Ca²⁺ affected a process that was upstream of both PKC and the ET_Breceptor. To test whether increased medium Ca²⁺ induced ET release, tubules were pretreated with the monoclonalantibody against ET-1 (above) and then exposed to 3 mM Ca²⁺. Figure 6C shows that exposure to the antibody prevented theCa²⁺-induced decrease in FL-MTX secretion.

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Fig. 6. Protection against Ca²⁺-induced reduction in FL-MTX transport by the ET_B receptor antagonist RES-701-1 (A), by 1 µM BIM (B), and by 1% (v/v) antibody against ET-1 (C). Tubules were pretreated for 30 min with normal medium (control, 1.5 mM Ca²⁺) or medium with 3 mM Ca²⁺ (in the presence or absence of the antibody, C). Proximal tubules were subsequently incubated for 30 min in medium containing 1 µM FL-MTX without (control) or with the indicated additions. Data are given as mean ± S.E. for 11 to 15 tubules from a single fish. **, Significantly lower than controls, P < 0.01. $black-square$ , lumen;

, cells.

The obvious experiment at this point was to determine whether nephrotoxin effects on FL-MTX transport could be seen when tubuleswere maintained in Ca²⁺-free medium. Our attempts to do this were unsuccessful, becausein the absence of nephrotoxicants, luminal accumulation of FL-MTXwas nearly abolished when Ca²⁺ was removed from the medium. We suspect that, as suggested previously(Kottra and Fromter, 1983

), Ca²⁺ depletion opened the tight junctions, resulting in increasedleakiness of the tubule and run down of lumen-to-bath concentrationgradients.

From these results, it was not clear how the increase in medium Ca²⁺ was causing ET release from the tubules. One possibility wasthat raising extracellular Ca²⁺ increased influx, which in turn increased intracellular freeCa²⁺. We attempted to reduce Ca²⁺ influx using nifedipine, a drug that blocks Ca²⁺ channels (Matsunaga et al., 1994

). By itself, 10 µM nifedipinedid not significantly affect FL-MTX transport (Table 2). However,pretreating tubules with nifedipine did prevent the decrease inFL-MTX secretion caused by increased medium Ca²⁺ (Fig. 7A and Table 2). To determine whether the inhibition ofFL-MTX secretion by the various nephrotoxic agents was causedby a Ca²⁺-dependent mechanism, tubules were exposed to gentamicin or diatrizoatein presence or absence of nifedipine. Again, the nephrotoxicant-inducedreduction in luminal FL-MTX accumulation was abolished by nifedipine(Fig. 7B; Table 2).

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Fig. 7. Protection against Ca²⁺-induced (A) and gentamicin-induced (B) reduction in FL-MTX transport by 10 µM nifedipine. A, tubules were pretreated for 30 min with normal medium (control with 1.5 mM Ca²⁺) or medium with 3 mM Ca²⁺. Tubules were subsequently incubated for 30 min in medium containing 1 µM FL-MTX without (control) or with the indicated additions. B, tubules were incubated for 30 min without (control) or with 10 µM gentamicin or gentamicin plus 10 µM nifedipine. Data are given as mean ± S.E. for 14 to 17 tubules from a single fish. **, Significantly lower than controls, P < 0.01. $black-square$ , lumen;

, cells.

A recent report suggests that, in addition to blocking Ca²⁺ entry, nifedipine can also inhibit PKC (Hempel et al., 1999

). Ifsuch inhibition occurred in our renal tubules, it would have acteddownstream to block the effects of elevated medium Ca²⁺ and the nephrotoxicants. This is not the case. We previouslydemonstrated that activation of PKC with phorbol ester reducesFL-MTX secretion in killifish tubules (Masereeuw et al., 2000

).Our additional experiments show that exposing tubules to 10 µMnifedipine did not alter the effects of 10 to 100 nM PMA on FL-MTXtransport. For example, in one experiment with 14 tubules pertreatment, fluorescence intensities in lumens and cells of controltubules averaged 2700 ± 190 and 740 ± 40 U, respectively; correspondingvalues for tubules exposed to 10 nM PMA were 1000 ± 130 and 600± 50 U; corresponding values for tubules exposed to 10 nM PMAplus 10 µM nifedipine were 870 ± 130 and 640 ± 30 U. Thus, inthe experiments presented here, nifedipine did not inhibit PKC.

Cellular Energy Metabolism. It is clear from the above that short exposures to nephrotoxic compounds as well as increased medium Ca²⁺ results in a reduction in transport mediated by Mrp2. It is notclear from these experiments whether those reductions result fromspecific regulation of transporter function or from toxicity (e.g.,reduced ATP levels). Previous experiments with killifish proximaltubules showed that Mrp2 was not the only transporter under PKCcontrol. Activation of PKC also reduced transport by P-glycoproteinat the luminal membrane (Miller et al., 1998) and by an organicanion transporter at the basolateral membrane (Miller, 1998).The latter transporter is part of the classic Na⁺-dependent and ouabain-sensitive organic anion system that handlessmall organic anions [e.g., p-aminohippurate and fluorescein (Pritchardand Miller, 1993)]. FL secretion mediated by this transporteris particularly sensitive to changes in cellular metabolism andion gradients (Miller and Pritchard, 1991; Miller et al., 1993).However, unlike FL-MTX transport (Masereeuw et al., 2000), FLtransport was not affected by 0.5 to 1 nM ET-1 (Fig. 8A). Ourunpublished data indicate that this transporter is regulated byparathyroid hormone rather than ET. Thus, FL transport providesa sensitive but ET-independent tool to monitor toxic effects.Figure 8B shows that at concentrations that substantially reducedFL-MTX secretion, neither gentamicin nor diatrizoate reduced transportof 1 µM FL. In contrast, when nephrotoxicant concentrations wereraised 5 to 10 fold, all of the treatments did reduce FL secretion(data not shown), suggesting toxicity with acute exposure to higherlevels. These data indicate that the lower concentrations of nephrotoxicantsused in FL-MTX experiments did not disrupt cellular energy metabolism.Thus, the observed nephrotoxicant-induced reductions in FL-MTXtransport resulted from altered transporter function.

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Fig. 8. Lack of effect of ET-1 (A) or the nephrotoxic agents gentamicin (10 µM) and diatrizoate (100 µM) on FL transport. Proximal tubules were incubated for 30 min in medium containing 1 µM FL without (control) or with the indicated additions. Data are given as mean ± S.E. for 11 to 33 tubules from one to three fish. $black-square$ , lumen;

, cells.

	Discussion

Top Abstract Introduction Materials and Methods Results Discussion References

The renal proximal tubule is both the segment of the nephron responsible for the active excretion of toxic chemicals, andan important target tissue for many of those same chemicals. Thus,it should not be surprising to find a convergence of these aspectsof proximal tubule function and dysfunction. Using a comparativemodel and confocal microscopy, we recently demonstrated that twoATP-driven xenobiotic efflux pumps on the luminal membrane ofproximal tubule epithelial cells, P-glycoprotein and Mrp2, wereunder the short-term control of ET acting through a basolateralET_B receptor and PKC (Masereeuw et al., 2000). Moreover, we alsofound that the nephrotoxic radiocontrast agent, iohexol, decreasedtransport mediated by Mrp2 and P-glycoprotein by firing this signalingsystem. This observation provided a pathophysiological contextin which to view regulation of drug export ATPases by ET, a hormonethat has been implicated in a number ofnephropathies.

In the present study, we found that representatives of two classes of nephrotoxic compounds decreased Mrp2-mediated transportby activating ET_B receptor/PKC signaling. That is, each of thefour nephrotoxicants tested reduced Mrp2-mediated FL-MTX secretioninto the tubular lumen and this reduction in transport was abolishedwhen an ET_B receptor-specific antagonist or a PKC-selective inhibitorblocked signaling. Figure 9 gives an overview of this sequenceof events. Note that nephrotoxicant-induced signaling alteredtransporter function rather than energy supply to the transporter.Neither gentamicin nor diatrizoate affected secretion of FL atconcentrations that clearly reduced FL-MTX transport. FL secretionis mediated by the classic, Na⁺-dependent organic anion system, which is particularly sensitiveto changes in cellular energy metabolism (Miller and Pritchard,1991; Miller et al., 1993).

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Fig. 9. Scheme illustrating the mechanism of nephrotoxicant-induced inhibition of transport by Mrp2. Various nephrotoxic agents cause an opening of Ca²⁺ channels. The resulting increase in intracellular Ca²⁺ concentration stimulates the release of ET, which subsequently activates the basolateral ET_B receptor. This leads to a reduction in Mrp2 transport activity through stimulation of PKC.

Given the wide range of chemical structures involved, it is unlikely that the four nephrotoxic compounds interacted directlywith the ET_B receptor. Rather, they seemed to induce ET releasefrom the tubules, with the hormone subsequently acting by an autocrinemechanism to trigger the pathway. In support of this supposition,the ability of the aminoglycoside antibiotic, gentamicin, to reduceMrp2-mediated transport was abolished when tubules were pretreatedwith an antibody against ET. Another monoclonal antibody, whichdoes not bind ET, had no such effect. Thus, the tubules releasedET in response to gentamicin. Because an activation of the ET_Breceptor was shown for the other three nephrotoxic agents as well,we speculate that this activation is a result of a release ofET by the tubules. Experiments in the presence of an antibodyagainst ET should resolve thisissue.

Released ET seems to have acted locally. In the experiments, each chamber contained micrograms of tubules in 1.5 ml of medium.The threshold for ET-1 action on FL-MTX transport in these tubulesis about 500 pM (Masereeuw et al., 2000). Because the amount ofhormone released from the tubules would be small and the overalldilution factor great, the average concentration of hormone inthe bulk solution must have been well below this threshold. However,after ET release, concentrations in the vicinity of the tubulescould have easily exceeded the threshold and provided sufficienthormone at the basolateral membrane to activate signaling throughthereceptor.

An ET-signaled reduction in Mrp2-mediated transport could be the result of internalization of the transporter or a reducedintrinsic activity of Mrp2 caused by phosphorylation. A decreasein the luminal amount of Mrp2 could not be detected using confocalmicroscopy. However, the resolution of the confocal microscope(about 0.25 µm) could be insufficient to measure redistributionof the transporter, leaving the question of the regulatory mechanismunanswered. Evidently, more research on this subject isneeded.

As in endothelial cells (Tasaka and Kitazumi, 1994; Carlini et al., 1995; Marsen et al., 1996), ET release from proximal tubulesseemed to be Ca²⁺-dependent. Increasing medium Ca²⁺ decreased FL-MTX secretion and this decrease was abolished whentubules were pretreated with a PKC-selective inhibitor, an ET_Breceptor antagonist, or the anti-ET IgG (present study). Thus,ET release and activation through its receptor and PKC was triggeredby elevated extracellular Ca²⁺. Consistent with increased Ca²⁺ influx being one stimulus for ET release, the L-type Ca²⁺ channel blocker, nifedipine, abolished the reduction in FL-MTXtransport seen in response to elevated Ca²⁺ and to gentamicin and diatrizoate. Influx of Ca²⁺ by other channels than the L-type cannot be excluded, becauserelatively high concentrations of nifedipine were used. Moreover,the exact localization of the Ca²⁺ channel is still controversial (Zhang and O'Neil, 1996); however,O'Neil et al. (1997) showed the expression of high-affinity dihydropyridinereceptors at the apical as well as the basolateral membrane. Thesebinding sites seem to be part of distinct Ca²⁺ channels, indicating that it is reasonable to assume that a nifedipine-sensitiveCa²⁺ channel is present at the basolateral membrane of proximal tubulecells. Experiments are currently in progress to determine theextent to which elevated extracellular Ca²⁺ and nephrotoxicants alter intracellular Ca²⁺ within the tubularepithelium.

When we first reported that the radiocontrast agent, iohexol, reduced transport mediated by Mrp2 and P-glycoprotein by activatingthe ET_B receptor/PKC signaling pathway, we questioned whetherthis phenomenon represented a protective mechanism (an attemptto conserve ATP, perhaps to maintain low intracellular Ca²⁺) or an early event in nephrotoxicity (Masereeuw et al., 2000).With regard to the latter possibility, recent evidence suggestsa role for P-glycoprotein in modulating cell death (reviewed inJohnstone et al., 2000). Multidrug resistant tumor cells overexpressingP-glycoprotein were protected from multiple forms of caspase-dependentapoptosis. However, protection was not extended to caspase-independentforms of cell lysis. Inhibition of P-glycoprotein, whether byan antibody or the drug verapamil, reduced resistance to apoptosis,indicating that overexpression of the transporter was not sufficientto protect; rather, the transporter had to be functional. Furtherevidence for a protective role of P-glycoprotein in renal cellscomes from a recent study using a renal cell line where Thévenodet al. (1999) found that up-regulation of P-glycoprotein protectedcells from cadmium- and reactive oxygen species-induced apoptosis.Given these recent findings for P-glycoprotein, our previous resultsfor P-glycoprotein and Mrp2 (Masereeuw et al., 2000), and ourpresent results for Mrp2, it is tempting to speculate that 1)both multidrug resistance transporters serve protective functions,and 2) a reduction in rate of Mrp2 transport could make proximaltubule cells more susceptible to damage by nephrotoxic compoundsthrough an early loss of this protectivemechanism.

Finally, taken together, the present data provide evidence for a new common mechanism by which nephrotoxic chemicals can disruptproximal tubule function. Given the high incidence of nephrotoxicityassociated with use of radiocontrast agents and aminoglycosideantibiotics, our results for a comparative model suggest thatblockade of tubular ET_B receptors could be of value in the clinic.More research is evidentlyneeded.

	Footnotes

Received September 14, 2000; Accepted February 13, 2001

This work was supported by a travel grant from the Netherlands Organization for Scientific Research (S.A.T.).

This work was presented in part at Experimental Biology '00 and published as a preliminary abstract: Terlouw SA, MasereeuwR, Russel FGM and Miller DS (2000) Bull Mt Desert Island BiolLab 39:84-85.

Send reprint requests to: Rosalinde Masereeuw, Ph.D., Dept. of Pharmacology/Toxicology 233, University Medical Center Nijmegen, P.O. Box 9101, 6500 HB Nijmegen, The Netherlands. E-mail: r.masereeuw{at}farm.kun.nl.

	Abbreviations

ET, endothelin; Mrp2, multidrug resistance protein 2; PKC, protein kinase C; FL, fluorescein; MTX, methotrexate; PMA, phorbol 12-myristate 13-acetate; BIM, bis-indolylmaleimide I.

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				D. S. Miller, J. R. Shaw, C. R. Stanton, R. Barnaby, K. H. Karlson, J. W. Hamilton, and B. A. Stanton MRP2 and Acquired Tolerance to Inorganic Arsenic in the Kidney of Killifish (Fundulus heteroclitus) Toxicol. Sci., May 1, 2007; 97(1): 103 - 110. [Abstract] [Full Text] [PDF]

				K. E. Wever, R. Masereeuw, D. S. Miller, X. M. Hang, and G. Flik Endothelin and calciotropic hormones share regulatory pathways in multidrug resistance protein 2-mediated transport Am J Physiol Renal Physiol, January 1, 2007; 292(1): F38 - F46. [Abstract] [Full Text] [PDF]

				S. Notenboom, A. C. Wouterse, B. Peters, L. H. Kuik, S. Heemskerk, F. G. M. Russel, and R. Masereeuw Increased Apical Insertion of the Multidrug Resistance Protein 2 (MRP2/ABCC2) in Renal Proximal Tubules following Gentamicin Exposure J. Pharmacol. Exp. Ther., September 1, 2006; 318(3): 1194 - 1202. [Abstract] [Full Text] [PDF]

				S. Notenboom, D. S. Miller, L. H. Kuik, P. Smits, F. G. M. Russel, and R. Masereeuw Short-Term Exposure of Renal Proximal Tubules to Gentamicin Increases Long-Term Multidrug Resistance Protein 2 (Abcc2) Transport Function and Reduces Nephrotoxicant Sensitivity J. Pharmacol. Exp. Ther., November 1, 2005; 315(2): 912 - 920. [Abstract] [Full Text] [PDF]

				B. Bauer, A. M. S. Hartz, G. Fricker, and D. S. Miller Modulation of p-Glycoprotein Transport Function at the Blood-Brain Barrier Experimental Biology and Medicine, February 1, 2005; 230(2): 118 - 127. [Abstract] [Full Text] [PDF]

				A. M. S. Hartz, B. Bauer, G. Fricker, and D. S. Miller Rapid Regulation of P-Glycoprotein at the Blood-Brain Barrier by Endothelin-1 Mol. Pharmacol., September 1, 2004; 66(3): 387 - 394. [Abstract] [Full Text] [PDF]

				S. H. Wright and W. H. Dantzler Molecular and Cellular Physiology of Renal Organic Cation and Anion Transport Physiol Rev, July 1, 2004; 84(3): 987 - 1049. [Abstract] [Full Text] [PDF]

				S. Notenboom, D. S. Miller, P. Smits, F. G. M. Russel, and R. Masereeuw Involvement of guanylyl cyclase and cGMP in the regulation of Mrp2-mediated transport in the proximal tubule Am J Physiol Renal Physiol, July 1, 2004; 287(1): F33 - F38. [Abstract] [Full Text] [PDF]

				S. A. Terlouw, C. Graeff, P. H. E. Smeets, G. Fricker, F. G. M. Russel, R. Masereeuw, and D. S. Miller Short- and Long-Term Influences of Heavy Metals on Anionic Drug Efflux from Renal Proximal Tubule J. Pharmacol. Exp. Ther., May 1, 2002; 301(2): 578 - 585. [Abstract] [Full Text] [PDF]

				D. S. Miller, R. Masereeuw, and K. J. Karnaky Jr. Regulation of MRP2-mediated transport in shark rectal salt gland tubules Am J Physiol Regulatory Integrative Comp Physiol, March 1, 2002; 282(3): R774 - R781. [Abstract] [Full Text] [PDF]