Aminoglycosides: Nephrotoxicity

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Antimicrobial Agents and Chemotherapy, May 1999, p. 1003-1012, Vol. 43, No. 5
0066-4804/99/$04.00+0
Copyright © 1999, American Society for Microbiology. All rights reserved.

MINIREVIEW
Aminoglycosides: Nephrotoxicity

Marie-Paule Mingeot-Leclercq^* and Paul M. Tulkens

Unité de Pharmacologie Cellulaire et Moléculaire, Université Catholique de Louvain, Brussels, Belgium

	INTRODUCTION

Top Introduction Conclusion References

Aminoglycosides have long been one of the commonest causes of drug-induced nephrotoxicity (137). Although a clear recognitionof the patient- and treatment-related risk factors (91), combinedwith the once-a-day schedule and effective monitoring procedures(98), have definitely improved the situation over what prevailedin the early 1980s (115), we are still short of having broughtthe safety of aminoglycosides to that of the main other wide-spectrumantibiotics. Chemical research aimed at obtaining intrinsicallyless toxic compounds has met with only modest success, and fewof the other approaches proposed to reduce the toxicities of theavailable agents have reached practical clinical applications.Yet, because aminoglycosides are very effective antibiotics wellsuited to the treatment of severe infections (35), it seemsimportant to maintain and even develop efforts to improve theirtherapeutic indices. The present minireview tries to present ina prospective way the status of both the basic and the clinicalresearch on aminoglycoside nephrotoxicity in order to clarifythe main issues and to pinpoint strategies that may eventuallylead to their safer use. Ototoxicity, which is the second mainadverse effect of aminoglycosides and which, in contrast to nephrotoxicity,is irreversible, will not be considered here since it has alreadybeen reviewed in this journal (52) and elsewhere (10). A companionminireview (83) examines and discusses the recent research dealingwith the activities of aminoglycosides and bacterialresistance.

	GENERAL FEATURES OF AMINOGLYCOSIDE NEPHROTOXICITY

Nephrotoxicity induced by aminoglycosides manifests clinically as nonoliguric renal failure, with a slow rise in serum creatinineand a hypoosmolar urinary output developing after several daysof treatment. Aminoglycosides are nephrotoxic because a smallbut sizable proportion of the administered dose ( $approx$ 5%) is retainedin the epithelial cells lining the S1 and S2 segments of the proximaltubules (135) after glomerular filtration (30). Aminoglycosidesaccumulated by these cells are mainly localized with endosomaland lysosomal vacuoles (108, 112) but are also localized withthe Golgi complex (108). They elicit an array of morphologicaland functional alterations of increasing severity, which are presentedin a summary fashion in Table 1, with their ultrastructural appearanceschematically depicted in Fig. 1. We have distinguished betweenlow and high dose effects since there is probably more than aquantitative difference between the changes seen under these twoconditions (130).

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TABLE 1. Main alterations elicited by aminoglycosides in kidney cortex

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FIG. 1. Ultrastructural alterations induced in proximal tubular cells during aminoglycoside treatment. (A) Control. Changes detected early on and at low doses (B) consist mainly of the enlargement of lysosomes, which most likely occurs by fusion of preexisting structures and which is caused by the progressive deposition of polar lipids which adopt a concentric lamellar disposition (myelin-like structures, most commonly referred to as myeloid bodies); the other subcellular structures are usually well preserved. Later changes or changes observed with high doses (C) include the apparent rupture of lysosomes (with the release of myeloid bodies in the cytosol), extensive mitochondrial swelling and damage, dilatation of the endoplasmic reticulum cisternae, shedding of the apical brush-border villi, pericellular membrane discontinuities, and the occurrence of apoptotic nuclei. These alterations do not necessarily coexist in all cells. The figure is adapted from reference 76 and is based on the typical descriptions given in references 38, 40, 71, 76, 77, 127, and 138.

	EFFECTS OF CLINICAL DOSES IN ANIMALS AND HUMANS

After only a few days of administration of clinical doses to humans or of low multiples of the human therapeutic dose to animals(typically 10 to 20 mg/kg of body weight for a laboratory rat),aminoglycosides induce conspicuous and characteristic changesin lysosomes of proximal tubular cells consistent with the accumulationof polar lipids (myeloid bodies) (10, 22, 71, 138). Thesechanges are preceded and accompanied by signs of tubular dysfunctionsor alterations (release of brush-border and lysosomal enzymes;decreased reabsorption of filtered proteins; wasting of K⁺, Mg²⁺, Ca²⁺, and glucose; phospholipiduria; and cast excretion [for a review,see reference 35]). In humans, the occurrence of these signsmay be followed by the development of overt renal failure characterizedmainly by a nonoliguric and even often polyuric hypoosmotic fallin creatinine clearance (35). Progression to oliguric or anuricrenal failure is infrequent, and recovery upon drug discontinuationis most often observed. Occasionally, a Fanconi's syndrome (18)or a Bartter's-like syndrome (74) has been observed. A correlationbetween the development of these clinical signs and the severityor rate of progression of the subclinical alterations remainsdifficult to establish mainly because of large interpatient variations.Consequently, the usefulness of monitoring the subclinical changesto detect individuals at risk has remained questionable. In animals,tubular alterations have clearly been associated with the developmentof focal necroses and apoptoses in the tubular epithelium, togetherwith an extensive tubular and peritubular cell proliferation (77,127), without an apparent change in kidneyfunction.

	EFFECTS OF HIGH DOSE IN ANIMALS

High doses (40 mg/kg or more for gentamicin) are necessary in animals to rapidly induce extended cortical necrosis and overtrenal dysfunction (71, 95). At this stage, a large numberof structural, metabolic, and functional alterations are observedin tubular cells (Table 1), and several of these alterationshave been claimed to be responsible for cell death or dysfunction.Many of the changes observed at the level of the apical membrane(25, 45, 46, 113, 116) could, however, be merely mediatedby a direct effect of the drug on this structure during its initialstages of uptake in proximal tubular cells. Conversely, othereffects, such as inhibition of protein synthesis and modulationof gene expression, mitochondrial alterations, or inhibition ofenzymes located on the cytosolic side of the pericellular membrane,must involve uptake and intracellular distribution of the drugto the correspondingtargets.

	ORIGIN OF TOXICITY

A major difficulty and a point of many controversies has been and still is ascertainment of which changes, among the numerousones described above, are truly responsible for toxicity. It ispartly the lack of unambiguous knowledge in this area which hasprevented the launching of large-scale programs aimed at designingor screening new aminoglycosides on a rational basis after thetrial-and-error approaches followed during the period from 1970to 1980 had proven to be poorly successful (97).

	TUBULAR NECROSIS

Histopathological studies strongly support the concept that tubular necrosis (and related phenomena) is the primary causeof functional toxicity. Frustratingly enough, however, the mechanismof this necrosis remains unsettled and cannot be unambiguouslytraced to a single, well-determined cause. It is, moreover, perfectlypossible that no single change or alteration is important perse but that tubular cells eventually die because of the simultaneousoccurrence of multiple changes (56). Three plausible lines ofhypotheses have, however, beenpresented.

The first hypothesis assumes that aminoglycosides exert their toxicity in direct relation to their local concentration. Thiswould therefore designate lysosomes as a key site and lysosomalalterations as a main cause of toxicity, since this is where thebulk of the tissue-bound drug is primarily stored. So far, however,the molecular and cytological links between the lysosomal alterationsand cell necrosis have not been uncovered. A second hypothesisis that aminoglycosides become toxic once they are released fromlysosomes. This release would take place when, and probably because,a critical threshold in lysosomal alterations and/or drug accumulationhas been reached. Almost all the alterations listed in Table 1are consistent with this hypothesis. If triggered abruptly, therelease of large quantities of aminoglycosides from lysosomescould indeed cause the simultaneous development of a number ofotherwise unrelated metabolic changes, many of which are capableof causing cell death. The question, then, is to distinguish betweenreal toxic events from trivial or secondary effects, as well asfrom artifacts. A typical example is the inhibition of mitochondrialrespiration and Ca²⁺ transport or lipid peroxidation, both of which were claimed tobe causes of irreversible cell damage but which detailed studieseventually showed occur after cell death (31, 140). Aminoglycosidesreleased from lysosomes could, however, act indirectly as nephrotoxins.In this connection, gentamicin was shown to chelate mitochondrialiron, forming a very oxidant Fe(II)-gentamicin complex capableof causing hair cell death (100). Finally, a third hypothesisis that the drug stored in lysosomes is intrinsically nontoxicbut that, in parallel to endocytic uptake, a small amount of aminoglycosidereaches a critical, nonlysosomal target and causes toxicity (bythis hypothesis, lysosomal storage could even protect the cellby retaining or diverting aminoglycosides from reaching thesemore crucial targets). Apical and basolateral membranes appearto be the best candidates because they are readily accessiblein intact cells (from the extracellular fluids) and because changesat their levels may result in many potentially lethal effects.For instance, the changes in renal brush-border Na⁺ and P_i cotransport and Na⁺ and H⁺ exchange have been ascribed to an increase in membrane fluiditycaused by a direct effect of gentamicin (79). Along the samelines, gentamicin was shown to cause the simultaneous inhibitionof very different membrane protein species including Na⁺/K⁺ ATPase and a release of lactate dehydrogenase, resulting in anapparently multifactorial cell death process. Yet, many "membraneeffects" actually require more than a simple contact of the drugwith the outer part of the pericellular membrane (inhibition ofNa⁺/K⁺ ATPase, for instance, occurs only if the aminoglycoside has accessto the cytoplasm [34]). This clearly raises the question ofa primary access of the drug to intracellular, nonlysosomal sites.Cell fractionation techniques applied to the kidney cortexes ofrats treated with low doses detect aminoglycosides only in endocyticvacuoles and lysosomes (40). Yet, an autoradiographic studyhas suggested an early, transient occurrence of gentamicin inthe cytosol of proximal tubular cells (139). In contrast, cellculture studies have always found the drug to be vacuolarly distributed,with a main localization in lysosomes, even though a recent studyby confocal microscopy has shown that some of these vacuoles belongto the Golgi complex (108). The link between nonlysosomal localizationsof aminoglycosides and the onset of early toxicity therefore remainsan area for moreinvestigations.

	RENAL FAILURE

While the determinants of cell damage still remain undefined, more knowledge concerning the mechanisms causing the impairmentof the renal function is available. Activation of the renin-angiotensinsystem and the ensuing local vasoconstriction appear to be primarilyresponsible for the decrease in glomerular filtration (45).This explains very well the aggravating effect of nonsteroidalanti-inflammatory drugs on aminoglycoside nephrotoxicity, sincethese drugs inhibit the production of the vasodilatatory prostaglandinPGE₂ (4). An increase in proximal intratubular free-flow pressureof single nephrons, most likely related to necrotic obstruction,has also been observed (5), suggesting that the decline ofglomerular filtration has a multifactorial origin and involvesa combination of tubular and nontubular mechanisms. The hypoosmoticpolyuria, characteristic of the aminoglycoside toxicity, has beenshown to result from the decreased fluid reabsorption by proximaltubules, secondary to an impaired solute reabsorption (64, 105),evidenced by the ion-wasting phenomena describedabove.

	EARLY COMPENSATION, REPAIR OF KIDNEY TISSUE AND POSTTOXIC ADAPTATION

The kidney has a large capacity to compensate for tubular insults so that an ongoing cell death process may long remain undetectedby functional explorations. The demonstration that tubular cellsundergo a marked proliferative response, even after low-dose treatmentswith aminoglycosides, has shed a new light on the significanceof the so-called nontoxic alterations seen under these conditions(127). It may be speculated that one of the reasons why patientsappear to be more sensitive to gentamicin than healthy animals(or young human volunteers) is their decreased ability to effectivelyregenerate and to sufficiently compensate for the spotty necroticinsults (131). The importance of regeneration for protectionagainst renal dysfunction is clearly demonstrated by the factthat laboratory rats survive the repeated administration of relativelyhigh daily doses of aminoglycosides (typically, 40 mg for gentamicinper kg per day for at least 42 days). After a first episode ofacute tubular necrosis that occurs within 8 to 10 days and thatis associated with a marked azotemia, renal function returns almostto normal, as if the kidney had become refractive (27, 28).This stage is actually related to the simultaneous occurrenceof necrosis and regeneration of tubules in an asynchronous fashion(49). Regenerating cells are also less differentiated (127)and apparently less susceptible to aminoglycosides (accumulationof gentamicin is actually reduced in the cortex of animals treatedfor long periods of time by a mechanism that involves not a decreasein its binding but probably altered intracellular trafficking[119]).

	DETERMINANTS OF THE AMINOGLYCOSIDE EARLY INSULT TO PROXIMAL TUBULES

While the molecular mechanisms of toxicity themselves are still unclear, it remains that the drugs must somehow physicallyinteract with one or several cellular constituents to initiatethe cascade of events leading to toxicity. Approaches aimed atreducing aminoglycoside toxicity should therefore preferably betargeted at preventing or modulating these early interactions.To us, two phenomena appear to be essential in this context, namely,the uptake of aminoglycosides into proximal tubular cells andtheir interactions with phospholipids in cells (130).

	UPTAKE OF AMINOGLYCOSIDES IN TUBULAR CELLS

Aminoglycosides bind to the brush-border membrane in their cationic form (19). The initial points of attachment are probablythe acidic phospholipids (and mainly phosphatidylserine, an abundantacidic phospholipid of brush borders), since modulation of themembrane content in these phospholipids results in commensuratechanges in uptake (90). Quickly thereafter, aminoglycosidesare transferred to the transmembrane protein megalin, with whichthey become internalized in endosomes (89). Megalin binds tomany polybasic drugs and peptides and is expressed in the renaltubule epithelium and a few other specialized epithelial celltypes including retinal and inner ear epithelia (143). It isprobably responsible for the selective uptake and toxicity ofaminoglycosides by these cells (109, 121) (the toxicity of intravitrealgentamicin toward retinal pigmented epithelium is a little-knownbut well-established fact [15]). N-Acetylneuraminic acid, thecortical content of which is increased in the kidneys during gentamicintreatment (60), could also be involved. Perhaps the most interestingaspect of this uptake process, from a toxicological point of view,is its saturable character at concentrations which are clinicallyrelevant (apparent K_m in rats, $approx$ 15 µg/ml [39]).

	INTERACTION OF AMINOGLYCOSIDES WITH PHOSPHOLIPIDS

Once transferred from endosomes to lysosomes through the physiological process of endosome-lysosome fusion, aminoglycosideswill be exposed to a fairly acidic pH ( $approx$ 5), at which they willbe fully protonated and therefore expected to bind tightly tonegatively charged structures. Among those, cellular membranes,which autophagy and heterophagy bring continuously to lysosomes,are probably a main target since they contain an average of 5to 20% acidic phospholipids. In vitro studies show that aminoglycosidesbind tightly to acidic phospholipids, primarily by electrostaticforces (20), and cause a marked decrease in the mobility ofthe phosphate heads in membrane bilayers (86). As shown in Fig.2, gentamicin bound to phosphatidylinositol lies close to theinterface, being inserted in the monolayer at the level of thephospho group and extending toward the hydrophobic phase up tothe level of the ester linkage of the fatty acids (101, 133).The binding of aminoglycosides to lipid bilayers causes theiraggregation (134) as well as the inhibition of the activitiesof phospholipases (48, 75). The latter is due to the neutralizationof the surface negative charge which these enzymes require tofully express their activity (84, 96), as well as, perhaps,to the lesser accessibility of the substrate to the enzyme catalyticsite (17). Enzyme inhibition and membrane aggregation most likelyaccount for the conspicuous accumulation of myeloid bodies observedin lysosomes in vivo (myeloid bodies isolated from the renal cortexessentially contain phospholipids and proteins [the latter probablyentrapped in the bilayers] but little cholesterol [3]). Themain critical drug-related parameters involved in phospholipaseinhibition appear to be (i) the energy of interaction betweenthe drug and the surrounding negatively charged phospholipids,(ii) the drug orientation at the lipid-water interface, and (iii)the drug accessibility to the aqueous phase (85, 87). Althoughneither the phospholipid accumulation nor the inhibition of phospholipaseactivity by itself explains cell death, the extent of phospholipidosisinduced by most aminoglycosides correlates rather nicely withtheir nephrotoxic potential (131). Moreover, as we shall seelater, impairment of the binding of aminoglycosides to phospholipidsor displacement of them from phospholipid layers protects againstthe development of both phospholipidosis and renal toxicity.

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FIG. 2. Skeleton views of the mode of assembly of gentamicin C_1a and isepamicin (in green) with phosphatidylinositol (hydrocarbon is in grey and oxygen and phosphorus atoms are in red to clearly indicate the polar domain). The two isolated drug molecules, with the same orientation, are shown on the right for ease of identification of their various parts (carbons are in grey, oxygens are in red, and nitrogens are in blue; see Fig. 1 of the companion minireview [83] for the chemical structures of isepamicin and gentamicin C_1a). The molecular modeling approach suggests that the orientations and the positions of the two drugs inserted in the phosphatidylinositol monolayer are entirely different. First, the N-6' amino groups are oriented in opposite directions (toward the lipophilic phase in the case of gentamicin and toward the water phase for isepamicin. Second, gentamicin lies above the plane of the inositol moieties and far away from the water phase (bottom), whereas isepamicin is readily accessible and is probably therefore more easily displaceable. Similar differences have been noted between kanamycin A and amikacin (133). Since both isepamicin and amikacin are characterized by a side chain at position N-1, these differences have been ascribed to the presence of this side chain (note that the orientation and position of gentamicin C_1a are very akin to those of gentamicin B, the parent, unsubstituted compound of isepamicin, and kanamycins). Such changes in position and orientation are thought to explain the lower inhibitory potential of amikacin and isepamicin toward the activities of phospholipases (for discussions, see references 16, 110, and 131). As outlined in this minireview and elsewhere (130, 133), inhibition of phospholipases is probably an important, early event in aminoglycoside nephrotoxicity. The figure was adapted from reference 133, with permission.

	REDUCING OR PROTECTING AGAINST AMINOGLYCOSIDE NEPHROTOXICITY

The goal of reducing or protecting against aminoglycoside nephrotoxicity has attracted much effort and attention over thelast decade. Based on the considerations discussed so far, theseefforts can be subdivided into several types of approaches, asillustrated in Table 2.

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TABLE 2. Main approaches toward reduction of aminoglycoside nephrotoxicity^a

Decreasing or preventing aminoglycoside accumulation by kidneys. Decreasing or preventing aminoglycoside accumulation by the kidneys would represent one of the most simple and radical approachesto reduce aminoglycoside nephrotoxicity, since it should leadto success whatever the targets of aminoglycosides are in thekidney. Aminoglycoside accumulation could be reduced either byimpairing their uptake or by enhancing their release. Reductionof uptake has been obtained by two strategies. The first one isaimed at complexing the aminoglycosides extracellularly, and thesecond one is aimed at competing with or decreasing drug bindingto the brush-border membrane. Table 2 illustrates the compoundsused in this context. Unfortunately, these approaches could notbe translated into clinical applications because of a lack ofefficacy and/or because of intrinsic toxicity (21, 81). Yet,the strategy based on competition for binding eventually led tothe recognition that aminoglycosides could be their own competitors.Early studies with animals (103) indeed revealed that administrationof the daily dose of gentamicin as a single dose (thus creatingone high daily peak level) was considerably less toxic than administrationof the same daily dose divided into three doses per day or bycontinuous infusion (38). An explanation for this unexpectedbehavior came from the finding that aminoglycoside uptake by kidneytubular cells is saturable (39), so that much of the drug thatpasses in the lumen will not be reabsorbed if the drug is tooconcentrated. Because saturation was shown to occur at a clinicallymeaningful range of concentrations, this observation triggereda large number of studies comparing the toxicities of variousdrug administration schedules. Almost at the same time, animaland clinical studies demonstrated that a high, transient peaklevel in serum was also a critical determinant of aminoglycosideefficacy (see reference 35 for a review). The once-daily dosingmode of administration of aminoglycosides was therefore clinicallytested in the late 1980s in a limited series of clinical trialsthat were at first cautious (118, 123, 132), but thereafter,it was tested with almost all indications for aminoglycosides(see reference 35 for a review and references 2, 6, 7,13, and 43 for meta-analyses plus the large number of referencescited therein). The once-daily regimen is now widely accepted(36), and it is in the official package insert recommendationsfor netilmicin and amikacin in several countries in Europe andelsewhere, even though discordant voices are still heard (12).Beyond its potential impact on the toxicity and activity of aminoglycosides,the once-daily dosing regimen also offers interesting pharmacoeconomicand practical advantages (93) and makes drug monitoring easier(98). A further development could be the implementation of once-dailyadministration at a specific hour of the day since there mightbe important circadian variations in the glomerular filtrationrate and, hence, the availability of the aminoglycoside to thekidney (a recent clinical study has indicated that the administrationof gentamicin during the midnight to 7 a.m. period was probablymore likely to cause toxicity than administration during otherperiods of the day [8, 99]).

Preventing or decreasing the lysosomal phospholipidosis induced by the cell-associated aminoglycosides. A reduction in lysosomal phospholipidosis could be achieved either by use of an aminoglycoside modified to bind less tightlyto phospholipids at an acidic pH (Fig. 3) or by the administrationof an agent that would prevent the binding of the antibiotic tophospholipids. Both strategies have been followed.

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FIG. 3. Structural modifications made in kanamycin A (R = OH) or kanamycin B (R = NH₂) (these aminoglycosides are the most frequently used for chemical modifications) to obtain a modulation of the potential of the drug to cause lysosomal phospholipidosis in comparison with the structure of the corresponding parent compound. The figure is from references 65, 72, 88, 111, 122, 128, and 129.

(i) Aminoglycoside modifications. As explained in the companion minireview (83), a series of 1-N-substituted derivatives of gentamicins and kanamycins weresynthesized in the late 1970s to obtain molecules resistant tothe bacterial enzymes that inactivate the parent compounds. Retrospectively,it was found that all derivatives in which the N-1 atom has beenmade nonionizable (i.e., by substitution of the amino functionwith an acyl side chain such as in amikacin) show reduced levelsof binding to acidic phospholipids together with a lesser inhibitorypotency toward lysosomal phospholipases (16). Among them, amikacin,isepamicin, and arbekacin have been successfully developed andhave been proved to cause less intense renal changes in animalsas well as in humans when they are tested under strictly comparableconditions with other currently used aminoglycosides (14, 22,70, 75, 82). For amikacin and isepamicin, this effect hasbeen ascribed to a lesser degree of interaction of the amino functionsof these drugs with the phospho group of negatively charged phospholipid(17, 110) and to changes in the orientation of the drug boundto the lipid layer (133) (see the illustration of isepamicinin Fig. 2; these models, however, have recently been challenged[17]). Efforts have therefore been made accordingly to rationallydesign new aminoglycosides with similar and, it is hoped, evenmore favorable properties. This led to the synthesis of derivativesof kanamycin B substituted at position C-6" with halogen atoms,a pseudo-halogen group (azido), or increasingly bulkier alkylchains via an intermediate N, S, or O atom, yielding the corresponding6"-amino, -amido, -thioalkyl, or -alkoxy derivatives (88), aswell as to derivatives of netilmicin and kanamycin A substitutedat positions N-1 and N-6' with amino acids (72), but with onlymodest success. In a similar context, the disaccharidic aminoglycosidesastromicin (fortimicin A) and dactimicin (2-N"-formimidoyl-astromicin)have been shown to bind less tightly to phospholipid bilayersand to be weaker inhibitors of lysosomal phospholipases (73).Their lesser nephrotoxicities observed in animals could, however,mainly be due to their lower levels of accumulation in the renalcortex (53).

Of greater interest are probably the derivatives of tobramycin, dibekacin, arbekacin, or kanamycin with a fluorine atom atposition 5, 3', or 3"' (65, 111, 122, 128, 129). These wereoriginally made to confer resistance to aminoglycoside-inactivatingenzymes, but for these derivatives chemical and biophysical considerationssuggest a reduced level of binding to phospholipids because ofa decreased basicity of the vicinal amino group through an inductiveeffect. These compounds showed increased 50% lethal doses, butexperimental data on their binding to phospholipids are notavailable.

(ii) Prevention of aminoglycoside binding to phospholipids. Polyaspartic acid has emerged as a very successful protectant against aminoglycoside-induced nephrotoxicity from the screeningof various polymers that are likely to impair the binding of aminoglycosidesto kidney membrane vesicles (142). In experimental studies withanimals, the coadministration of polyaspartic acid with gentamicinor amikacin was shown to protect against the development of phospholipidosisand phospholipiduria (61), as well against all early and latesigns of aminoglycoside nephrotoxicity (26, 37). Actually,both polyaspartic acid and the aminoglycoside reach the lysosomesby endocytosis (55) and form ion-pair complexes within theseorganelles due to the acidic pH prevailing therein. In vitro studiesdemonstrated that polyaspartic acid prevents aminoglycoside bindingto negatively charged phospholipids bilayers and thereby makesthe drug unable to inhibit the activities of lysosomal phospholipases(62). Further studies showed that polyaspartic acid also protectsagainst gentamicin-induced alterations of phospholipid metabolismin cultured cells (102) and of electrophysiological alterationsin cultured human proximal tubular cells (125). Polyasparticacid also prevents impairment by gentamicin of homotypic fusionof renal cell endosomes (42) and blocks the process of aminoglycoside-inducedaggregation of negatively charged liposomes (134), all eventswhich had been directly related to the binding of gentamicin tophospholipids. In vivo studies have now defined the limits andthe duration of the protection afforded by polyaspartic acid (120).Moreover, pharmacokinetic evaluations have shown that polyasparticacid increases the penetration of gentamicin in the so-calleddeep peripheral compartment (which most likely represents theintracellular drug-polyaspartic acid complex [141] and whichsuggests that the antibiotic is stored in a nontoxic form). Aprotective effect of polyaspartic acid against ototoxicity hasalso been demonstrated (50). A movement toward large-scale toxicologicalstudies and clinical applications of polyaspartic acid thereforeappears to be warranted but is still hindered by the lack of aclear definition of the precise type of polymer which needs tobe used. It must indeed, at the same time, be filtratable throughthe glomerulus, bind effectively to gentamicin (66), remainsufficiently stable in the kidney to afford significant protection(61), and not causing renal toxicity per se, as was shown forpolymers that are too stable (63).

Daptomycin (LY 146032), which contains three Asp residues, also colocalizes in the lysosomes of the renal cortex with gentamicinand protects against lysosomal alterations in vivo (124). Invitro, it increases the negative charge density of membranes,while at the same time affecting the lipid packing (41), twoeffects which counteract those of gentamicin and facilitate theaccess of the catalytic site of the phospholipases to their lipidicsubstrate. Torbafylline (HWA-448), an analog of the vasculoactiveagent pentoxifylline, also protects against gentamicin-inducedphospholipidosis, but its mode of action is unknown (32).

Other means of protection. Among the other main approaches used so far to reduce or to protect against aminoglycoside nephrotoxicity (Table 2), themost consistent effects have been observed with the use of antioxidantsand especially deferroxamine. On the basis of the finding thatgentamicin forms complexes with mitochondrial Fe²⁺ to catalyze the formation of free oxygen radicals (see above),iron chelators were tested and were proven to be effective inthe prevention of aminoglycoside-induced ototoxicity (109, 117).Extension of this finding to nephrotoxicity appears to be possible(136), but biophysical and biochemical considerations (100)suggest that the protective effect of deferroxamine may be criticallydependent on the dosage of gentamicin. Other compounds were alsoused on account of their antioxidant effects (Table 2), but themechanisms have not always been unambiguously established. Meansof protection based on a correction of the functional abnormalitiesor on an increase in cell regeneration capabilities have alsobeen attempted, but no clinical application has so far beenmade.

	CONCLUSIONS

Top Introduction Conclusion References

The study of aminoglycoside nephrotoxicity has clearly identified several critical mechanisms, the knowledge of which mayallow for the safer use of these drugs. Among the various approachesapplicable to the presently available aminoglycosides, only once-a-daydosing has already been brought successfully to the clinic. Otherprotective approaches such as the coadministration of polyasparticacid or deferroxamine deserve preclinical and clinical development,and many more could certainly be explored. Our progress in molecularmodeling and an improved knowledge of the meaningful differencesin structure-activity and structure-toxicity relationships foraminoglycosides (see the companion minireview [83]) could alsobring us, before too long new, intrinsically less toxicaminoglycosides.

	ACKNOWLEDGMENTS

M.-P.M.-L. is Chercheur Qualifié of the Belgian Fonds National de la Recherche Scientifique. Support was received from theBelgian Fonds de la Recherche Scientifique Médicale (grants 3.4589.96,3.4516.94, and 9.4514.92), the Fonds National de la RechercheScientifique (grant 9.4546.94), the Actions de Recherches Concertées94/99-172 of the Direction Générale de la Recherche Scientifique-CommunautéFrançaise de Belgique of Belgium, and the French nonprofit organization(Association-loi 1901) Vaincre les MaladiesLysosomales.

We thank R. Brasseur (Centre de Biophysique Moléculaire Numérique, Faculté des Sciences Agronomiques de Gembloux, Gembloux,Belgium) for performing computer-aided conformational analysisof aminoglycoside-phosphatidylinositolinteractions.

	FOOTNOTES

^* Corresponding author. Mailing address: Unité de Pharmacologie Cellulaire et Moléculaire, Université Catholique de Louvain,UCL 7370 avenue E. Mounier 73, B-1200 Bruxelles, Belgium. Phone:32-2-764.73.74. Fax: 32-2-764.73.73. E-mail: mingeot{at}facm.ucl.ac.be.

REFERENCES

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MINIREVIEW Aminoglycosides: Nephrotoxicity

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Aminoglycosides: Nephrotoxicity