Aminoglycosides: Perspectives on Mechanisms of Action and Resistance and Strategies to Counter Resistance

doi:10.1128/AAC.44.12.3249-3256.2000

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Antimicrobial Agents and Chemotherapy, December 2000, p. 3249-3256, Vol. 44, No. 12
0066-4804/00/$04.00+0
Copyright © 2000, American Society for Microbiology. All rights reserved.

MINIREVIEW
Aminoglycosides: Perspectives on Mechanisms of Action and Resistance and Strategies to Counter Resistance

Lakshmi P. Kotra, Jalal Haddad, and Shahriar Mobashery^*

Department of Chemistry, Wayne State University, Detroit, Michigan 48202

	INTRODUCTION

Top Introduction Conclusion References

Aminoglycosides are among the most commonly used broad-spectrum antibiotics in the anti-infective armamentarium. The vastmajority of aminoglycosides are bactericidal, they have predictablepharmacokinetics, and they often act in synergy with other antibiotics,properties that make them valuable as anti-infectives. Furthermore,despite the potential for renal toxicity, ototoxicity, and bacterialresistance, several members of this family of antibiotics haveenjoyed clinical use for severaldecades.

Aminoglycosides are multifunctional hydrophilic sugars that possess several amino and hydroxy functionalities. The amine moietiesare mostly protonated in biological media; hence, these antibioticscan be considered polycationic species for the purpose of understandingtheir biological interactions. Since they are polycationic, theyshow a binding affinity for nucleic acids. Specifically, aminoglycosidespossess high affinities for certain portions of RNAs, especiallythe prokaryotic rRNA (12-14, 38, 39). In addition, aminoglycosidesbind to the hammerhead ribozyme (45, 49), tRNA^Phe (26), the Rev response element (RRE) transcriptional activationregion in human immunodeficiency virus (HIV) (8, 18), theribozyme from hepatitis delta virus (41), and group I self-splicingintrons (6, 51, 52).

There are only a handful of structural studies on the interactions of aminoglycoside antibiotics with specific RNA sequences.One such study aimed at understanding the molecular interactionsof paromomycin (Fig. 1) with the aminoacyl site (A-site)-decodingregion of rRNA (12-14, 39). Another dealt with the interactionsof tobramycin (Fig. 1) with an RNA aptamer (23). In 1998, Yoshizawaet al. (57) elucidated the structure of gentamicin Cla boundto an A-site RNA complex. These studies used nuclear magneticresonance techniques to elucidate the three-dimensional structuresof the complexes of RNA and aminoglycosides. In addition to thesestructural investigations, several footprinting studies and effortswith semisynthetic aminoglycosides have been reported for RNAinteractions (1, 7, 8, 30, 48). In this minireview,structural determinants that are responsible for the specificrecognition of certain RNA folds by aminoglycosides, which haveimplications for the mechanisms of action of these antibiotics,will be examined. Recent determination of the low-resolution X-raystructure of the 70S ribosome from Thermus thermophilus has shedlight on the global features of various domains in rRNAs and theirinteractions with mRNA and tRNA (5). In light of the structuralinformation presented above, mechanistic features of aminoglycosidebinding to rRNA will be discussed as well.

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FIG. 1. Structures of aminoglycosides.

The topics of the biological activities, resistance, and toxicities of aminoglycoside antibiotics have been reviewed (4,10, 31, 32, 44). The present report addresses the complementarysubjects of the molecular interactions responsible for the activitiesof this class of antibiotics, the structural factors responsiblefor the specificity, and the efforts made to design novel derivativesof aminoglycosideantibiotics.

	STRUCTURAL BASES FOR MECHANISM OF ACTION

The 16S rRNA from Escherichia coli is well studied among the rRNA subunits, and in particular, the interactions of variousaminoglycoside antibiotics with the 16S rRNA and their effectson the process of translation of mRNA into polypeptide have beenscrutinized (35). Similar rRNA structures exist in other organisms,such as yeast and Tetrahymena (33). Treatment of rRNA with anaminoglycoside protects several nucleic bases in rRNA from chemicalmodification, implying that these molecules possess high affinitiesfor certain sites in rRNA. This mode of binding was likened byNoller (35) to that of enzyme inhibitors, which usually bindto the active sites of enzymes and interfere with their activities.Different classes of aminoglycoside antibiotics bind to differentsites on the rRNA, depending on the structural complementaritybetween the two. For example, neomycin, paromomycin (Fig. 1),gentamicin, and kanamycin are believed to bind to the A-site onthe 16S rRNA in E. coli in a similar fashion and were shown toprotect bases A1408 and G1494 in chemical footprinting experiments(Fig. 2) (33). Four bases, A1408, A1492, A1493, and G1494, inthe rRNA A-site interact with tRNA, although with different affinities.The binding of the aforementioned aminoglycosides to the A-sitein the decoding region (i.e., the site of codon and anticodonrecognition) interferes with the accurate recognition of cognatetRNA by rRNA during translation (35). These interactions arealso thought to interfere with the translocation of tRNA fromthe A-site to the peptidyl-tRNA site (P-site).

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FIG. 2. (A) Stereo view of the partial structure of the 70S rRNA complexed with three tRNA molecules (Protein Databank code, 486D [available at http://www.rcsb.rutgers.edu]). The A-site region on the 16S rRNA is shown in white, where aminoacyl tRNA `A` (in yellow) is bound near the A-site of rRNA. Two other tRNAs, peptidyl and exit, "P" (in red) and "E" (in green), respectively, are shown as well. The backbone of the penultimate stem of the 16S rRNA molecule and the 900-loop are shown in violet. The binding site of paromomycin at the A-site is indicated by the white arrow. (B) Stereo view of the solution structure of RNA A-site template bound by paromomycin, which approximately corresponds to the A-site region on the 16S rRNA in white in panel A. The Connolly surface of the A-site RNA is rendered according to the electrostatic potential by using the MOLCAD program (Tripos, Inc., St. Louis, Mo.), and the aminoglycoside is shown in a ball-and-stick representation. The most electronegative potential is rendered in blue, and the most electropositive potential is rendered in red on the surface; all other colors show the potentials between blue and red. The arrow in white shows the kink generated by A1492, which does not have a base-pairing partner. The arrow in yellow shows the pocket generated by the A1408 · A1493 base pair and A1492. The arrow in red shows the location of the 3-amine on ring II, the site for acetylation by AAC(3).

Puglisi and coworkers (12-14, 39) recently provided structural evidence on the mode of interactions of paromomycin, a representativeaminoglycoside of the neomycin class, with a 27-nucleotide RNAtemplate that was designed to mimic the A-site region of the 16SrRNA in E. coli (Fig. 3A). The design of the RNA template wasbased on previous knowledge that paromomycin interacts with theC1407 · G1494 base pair, A1408, A1493, and U1495 and that thesebases are absolutely necessary for high-affinity binding (39)(shown in gray in Fig. 3A). Additional structural features, suchas the pocket created by the asymmetry in the internal loop regiondue to the presence of A1492 and the base pairing of C1409 · G1491at the lower stem region, are also important. These structuralcharacteristics collectively create a pocket that is optimal forthe binding of paromomycin (see below).

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FIG. 3. (A) Model of the A-site RNA template used to study the interactions of paromomycin. The box represents the portion of the rRNA that is homologous to the A-site. (B) RNA aptamer template used to study the interactions of tobramycin.

In the native A-site RNA template, the stem has base-pairing interactions at U1406 · U1495 (noncanonical) and C1407 · G1494(Fig 3A). Upon binding of paromomycin, the distinct structureformed by A1408, A1492, and A1493 is stabilized (Fig. 2B) andbases A1408 and A1493 form a noncanonical base pair (12, 39).Nucleotide A1492, which does not have any base-pairing interactions,creates a kink in the RNA structure, and the combined effectsof A1492 and the A1408 · A1493 base pair creates a bulge in theA-site where paromomycin binds and further extends the angle ofthe kink (Fig. 2B). The functional groups on paromomycin, suchas the hydroxyl and amino groups, participate in specific interactionswith the RNA molecule (seebelow).

The pocket created by A1492 and the A1408 · A1493 base pair is occupied by ring II of paromomycin, and this ring stacks abovebase G1491 (shown by a yellow arrow in Fig. 2B) (12). Ring Iof paromomycin makes specific contacts with the "universally"conserved base pairs U1406 · U1495 and C1407 · G1494 in the rRNA.It is noteworthy that ring I is absolutely necessary for specificbinding of aminoglycoside antibiotics to rRNA. Rings III and IVof paromomycin extend these interactions further into the majorgroove of rRNA. The amino and hydroxyl moieties mostly contributeto the nonspecific interactions of paromomycin with rRNA; thus,they are not sequence-dependent interactions. Another importantpoint is that the base pair C1409 · G1491 provides the seat forbinding of aminoglycoside in the pocket, and a mismatch base pairin this position results in the loss of binding (12). In general,aminoglycosides that share structural features with paromomycinbind to rRNA similarly (13). However, different aminoglycosideantibiotics appear to bind to the same binding site in more thanone conformation (28). In essence, the conformation of the aminoglycosidethat does bind to RNA must satisfy the electronic and steric constraintsof the binding site. In a different study on the complex of gentamicinCla and the A-site RNA template, rings I and II of gentamicinCla (which are similar to those of paromomycin) exhibited bindinginteractions similar to those in the complex of paromomycin andthe A-site RNA template (57). However, ring III in gentamicinCla interacts with base pairs U1406 · U1495 and G1405 · C1496in the upper stem region (Fig. 3A). From these observations, Puglisiand coworkers (57) proposed that all the aminoglycosides thattarget the A-site of the 16S rRNA bind in a common manner, similarto rings I and II in paromomycin andgentamicin.

Although the overall structure of rRNA is conserved among all species in an evolutionary sense, there are differences thatmake binding of aminoglycosides more specific $---$ by at least a 10-foldhigher affinity $---$ to the rRNA of prokaryotes than to that of eukaryotes(19, 35, 38). This is not a large difference in bindingaffinity and may in part explain the toxic effects of these antibioticsin mammalian systems. Eukaryotic rRNA contains a guanine in placeof A1408, resulting in a G1408 · A1493 base pair. In addition,the matched base pair at C1409 · G1491 does not exist in eukaryotes.These differences collectively result in lowered affinities ofaminoglycosides for the eukaryotic rRNA (12, 19, 35, 38).Having outlined these differences, binding of aminoglycosidesto the A-site of rRNA in prokaryotes alters the conformation ofthe A-site and affects the specific interactions of mRNA and tRNAat this site, resulting in erratic codon-anticodon interactions.There is a paucity of structural information on the specificsof these interactions at the ribosomal level to date (see below),but the clear and ultimate consequence is disruption of the translationprocess.

Another structural study was performed on binding of tobramycin (Fig. 1) to an RNA aptamer (23). The RNA aptamer that wasused in this study was a 26-nucleotide stem-loop RNA (Fig. 3B).There are four mismatch pairs, U7 · G20, G8 · U19, G9 · A18, andU11 · U16, in this RNA aptamer that are part of the zippered hairpinloop. Tobramycin binds in this groove partially encapsulated bythe surface of the deep groove and the guanine base of the residueG15 (Fig. 4). In this complex, ring I of tobramycin sits on thefloor of the deep groove. One of the amino groups on ring II oftobramycin interacts with the phosphate backbone in the deep groove,and the other amino group is exposed to the solvent. Ring IIIis positioned in the center of the deep groove, with hydroxylgroups directed toward the floor of the groove. The conformationof the RNA aptamer described above was suggested to be similarto those of the hairpin loops in tRNA and rRNA (23).

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FIG. 4. Stereo view of the complex of tobramycin bound to the RNA aptamer. The green Connolly surface represents a portion of the aminoglycoside binding site.

The 7.5-Å-resolution X-ray structure of the functional complex of T. thermophilus 70S rRNA containing tRNA and mRNA is helpfulto put the above discussion in perspective (5). From this structure,one could envision how well the model studies with smaller RNAtemplates such as the tobramycin-RNA aptamer and the A-site-RNAwith paromomycin (see above) would fit into the complete structureof rRNA. The A-site in the 16S rRNA subunit of the 70S rRNA isseen near the interface of tRNA and the 50S rRNA subunit, in theproximity of the codon-anticodon pair (Fig. 2A). Upon comparisonof the solution structure of the A-site RNA template to the A-sitein the X-ray structure of 70S rRNA, the X-ray structure appearedto be closely related to the paromomycin-bound RNA template butnot to the native solution structure of the A-site RNA template(5). This is intriguing and suggests that perhaps in the functionalform the bulge or kink near bases A1492 and A1493 always existsin the 70S rRNA. If this were true, it implies that the bindingpocket for paromomycin is already in existence when the 70S rRNAbecomes functional; hence, it is predisposed for inhibition byparomomycin. This contradicts the assertion that binding of paromomycinincreases the kink angle at the binding site. Evidence in supportof this idea comes from a recent study that suggested that theaffinities of different aminoglycosides for the A-site RNA templateare different, and the ability of these antibiotics to inhibitprotein synthesis in vitro varies as well (15). Gentamicin andseveral other related antibiotics interact with the A-site RNAwith dissociation constants (K_d) in the micromolar range, butthey inhibited an in vitro translation process, with 50% inhibitoryconcentrations in the nanomolar range (15). The latter findingwas inferred as the result of aminoglycoside binding to the intactrRNA in the decoding region (A-site), and the difference in bindingto intact rRNA versus that to the A-site template RNA may be dueto the differences in the conformations of these two RNAs, asdiscussedabove.

The A-site makes weak contacts with the mRNA and tRNA, implying that this region plays a role in recognition of appropriatetRNA via subtle changes in the free energy (5). The bindingof aminoglycoside near this site may affect the delicate processof interactions between codon and anticodon. It was also proposedthat the presence of an aminoglycoside stabilizes the complexof mRNA and tRNA at the A-site, which in turn affects the processof translation (5). It is difficult to surmise all the effectsof aminoglycosides on the rRNA structure, and further structuralstudies with the aminoglycosides bound to the complexes, suchas the 70S rRNA, will be helpful in elucidating and understandingthe subtle changes that lead to the antibiotic actions ofaminoglycosides.

A number of investigations have used synthetic probes to understand the interactions between RNA templates and aminoglycosides.It has been suggested that aminoglycosides bind to more than onetarget site in the ribozyme (6, 30). Recently, several aminoglycosideantibiotics such as neomycin B, tobramycin, and kanamycin A havebeen dimerized either symmetrically or asymmetrically by usinga "tether," and their binding affinities were compared to thoseof the monomeric parent aminoglycosides (30). It was suggestedthat if there were multiple binding sites on the RNA, the dimerizedaminoglycosides should bind with a higher affinity than the parentantibiotic, provided that multiple binding sites are accessible.It was indeed observed that the dimerized aminoglycosides bindto the Tetrahymena ribozyme 20- to 1,200-fold better than theparent aminoglycosides. One explanation for the higher bindingaffinity could be the increased number of positively charged aminogroups on the dimerized aminoglycoside, but this effect seemsto be synergistic with the entropic advantage gained by dimerization(30). It also indicated the presence of multiple high-affinitybinding sites for aminoglycoside antibiotics in an RNA molecule.Another study attempted to exploit the RNA binding propertiesof paromomycin and the intercalating behaviors of certain compoundssuch as pyrene and thiazole orange (48). This strategy envisionedaminoglycosides as a means for the delivery of intercalating agentsto the RNA. The conjugate of paromomycin with thiazole orangeor pyrene showed better binding properties to the 27-nucleotideA-site RNA template. In fact, the dissociation constant for theparomomycin-thiazole orange conjugate was measured at 46 nM, whichwas reported as the highest affinity that the rRNA A-site hasshown for anyligand.

The structural requirements for RNA binding by aminoglycosides indicated that a bulge in the RNA sequence is necessary toallow binding of aminoglycosides (7). By using a specific stem-loopderivative of the RNA aptamer, a series of chemical interference,chemical modification, and mutation studies was performed to understandthe structural requirements for binding of tobramycin to the RNAaptamer. This aminoglycoside appeared to interact mainly withthe nucleic bases in the RNA aptamer but not with the phosphatebackbone. The presence of a bulge, however, was proposed to beimportant for the high-affinity binding of tobramycin in a stoichiometricratio, and it was concluded that a bulge creates a cavity forinteractions of the aminoglycoside and the nucleic base (7).This analogy can be applied to other RNA sites such as the hammerheadregion and the A-site, where a cavity is present due to the noncanonicalbase-pairing or loops or bulges that create a suitable site forthe aminoglycosides to interact with the anionic phosphate groupsand the nucleic bases. Along these lines, Westhoff and colleagues(49) put forward a proposal that the interaction of aminoglycosideswith RNA is likely to be shape specific rather than sequencespecific.

Consistent with this concept, the electrostatic fields in the RNA folds were deemed as the guiding force for binding (seebelow). Hermann and Westhoff (20) were able to identify thedocking confirmations of several aminoglycoside antibiotics invarious RNA templates, such as tobramycin-RNA aptamers and theA-site region in the 16S RNA, for which structural informationwas available. On the basis of those observations, the bindingmode of aminoglycosides to the trans-activating response elementregion in HIV was predicted (20). In another study on RRE inHIV, the binding region for the Rev protein, Cho and Rando (8)investigated the role of a single-base bulge and a cavity forbinding of aminoglycosides. Consistent with previous hypotheses,it was deduced that grooves in the nonduplex regions of RNA areimportant for high-affinity binding of aminoglycosides to RNA.In this case, the single-base bulge did not affect binding, butthe cavity, a G-rich region consisting of two noncanonical basepairs and one single bulged U, has a high affinity for aminoglycosides.Tampering with the cavity decreased the affinity of the RRE RNAfor aminoglycosides, thus indicating that the noncanonical basepair-containing bulges are the primary aminoglycoside-bindingsites in this RNA template (8).

	RESISTANCE TO AMINOGLYCOSIDES AND STRATEGIES TO COUNTER IT

Even though the binding site for aminoglycosides is in rRNA, resistance to aminoglycosides is not manifested by alterationof this target in general. This is in part due to the fact thatthe function of the rRNA is central in the protein biosyntheticprocess and that this function is so well preserved across generathat it cannot be impaired by the possibility of such structuralalteration. In addition, all organisms have multiple copies ofthe genes that encode rRNA. In order to generate an rRNA resistantto a certain antibiotic that binds to it, all these genes willhave to be mutated, and the probability of the occurrence of suchan event is virtually nonexistent. Moreover, it is easier foran organism either to modify the rRNA target posttranslationallyor to produce resistance enzymes (see below). On the other hand,there are some reports of mutations in the ribosomal proteinsthat confer resistance to certain antibiotics. For example, mutationsin the ribosomal protein L10e lead to resistance to sordarin,a tetracyclic diterpene glycoside antifungal agent that selectivelyinhibits fungal protein biosynthesis (24). Mutations in anotherribosomal protein, L22, confer resistance to erythromycin, andrecently, the X-ray crystal structure of this protein from T.thermophilus was determined (50). Mutations that confer resistanceto erythromycin are on a beta-hairpin loop on L22, and it waspostulated that this region may be in proximity to the erythromycin-bindingsite near the peptidyl transfer center (50). However, thesetypes of mechanisms for resistance are not seen for aminoglycosides.It is also observed that certain mutations in the highly conserved530 stem-loop region in rRNA result in "streptomycin dependence,"perturbing (actually reducing) the translational error frequency(22, 37). However, there is no three-dimensional structuralinformation on this observation for us to be able to comment onit further. Resistance to aminoglycosides is widely reported,but the preponderance of the cases of resistance to these agentshas not been as overwhelming as that of the cases of resistanceto $beta$ -lactam antibiotics. This may be due in part to the more frequentuse of $beta$ -lactams in the clinic, but it may also be due to thedifferences in the mechanisms of dissemination of the resistancedeterminants (34, 55). Whereas methylation of 16S rRNA inaminoglycoside-producing organisms gives high-level resistanceto the actions of these antibiotics (3, 46), the most commonmechanism for clinical resistance to aminoglycosides is theirstructural modification by specific enzymes expressed in resistantorganisms. The sites of modifications in kanamycin B by variousenzymes are shown schematically in Fig. 5. The binding of themodified aminoglycoside antibiotics to their target sites is compromised.There are three classes of these enzymes: aminoglycoside phosphotransferases(APHs), aminoglycoside nucleotidyltransferases (ANTs), and aminoglycosideacetyltransferases (AACs). Within each class, there are enzymeswith different regiospecificities for aminoglycoside modifications:there are four nucleotidyltransferases [ANT(6), ANT(4'), ANT(3"),and ANT(2")], seven phosphotransferases [APH(3'), APH(2"), APH(3"),APH(6), APH(9), APH(4), and APH(7")], and four acetyltransferases[AAC(2'), AAC(6'), AAC(1), and AAC(3)]. There also exists a bifunctionalenzyme, AAC(6')-APH(2"), that can acetylate and phosphorylateits substrates sequentially (2, 9). The issue of the originsof these resistance enzymes has been discussed in recent reviewsand will not be repeated here in the interest of brevity (32,55).

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FIG. 5. Sites of modification on kanamycin B by various aminoglycoside-modifying enzymes. The arrows point to the sites of modification by the specific enzymes, namely, acetyltransferases, phosphotransferases, and nucleotidyltransferases.

Crystal structures for four aminoglycoside-modifying enzymes have been reported (21, 36, 42, 53, 56). These arefor ANT(4'), AAC(3), AAC(6'), and APH(3') type IIIa [APH(3')-IIIa].It is interesting that the same forces that drove the evolutionof aminoglycoside biosynthesis for binding to the ribosomal sitesalso would appear to have driven evolution of the resistance enzymes.Namely, electrostatic interactions appear to be quite significant.It was noted that the positively charged aminoglycoside is attractedto APH(3')-IIIa, since the active site of the enzyme providesfavorable interactions due to the excessive negative charge distributionin this region of the surface (21, 55). Once the complex formsbetween the two (i.e., the substrate and the enzyme), this electrostaticattraction on the substrate is complemented by specific electrostaticinteractions between the active site and the aminoglycoside inAPH(3')-Ia, -IIa, and -IIIa, as documented by studies of specificdeaminated aminoglycosides (29, 40). In the same sense thatthe amines in the structures of aminoglycosides are importantfor binding to rRNA, they would appear to be significant $---$ perhapsindispensable $---$ for recognition of the drugs by the resistanceenzymes.

The structural modifications of aminoglycosides result in a severe reduction of the ability of the modified antibiotic tobind to the target RNA due to unfavorable steric and/or electrostaticinteractions. For example, acetylation of the amine group at position3 on paromomycin (Fig. 1) results in unfavorable steric clashesin the A-site RNA, as can be surmised from the structure of thecomplex between paromomycin and A-site RNA (shown by a red arrowin Fig. 2B). In addition, acetylation in this case would interferewith the necessary electrostatic attraction between the RNA andthe aminoglycoside as well. Another example is phosphorylationof aminoglycoside at the 3' position (corresponding to the 3'site in ring II of paromomycin [Fig. 1]) due to the action ofAPH(3'). Considering that kanamycin A [a substrate for APH(3')enzymes] binds in a fashion similar to that for paromomycin atthe A-site of rRNA, ring II should fit into the pocket createdby A1492. However, the phosphate group at the 3' position wouldinterfere with this binding due to the repulsive electrostaticand steric interactions between the 3' phosphate and the phosphatebackbone of the rRNA, resulting in poor binding of the 3'-phosphorylatedaminoglycosides at the A-site ofrRNA.

Gentamicin C is susceptible to at least five or six modifying enzymes, and the same pattern can be seen for the semisyntheticantibiotic tobramycin. A major breakthrough was the preparationof amikacin (Fig. 1), a kanamycin A derivative with the aminogroup at position 1 acylated by 4-amino-2-hydroxybutyrate. Thepresence of the aminohydroxybutyryl group in general preventsthe enzymatic modification of amikacin at multiple positions.This antibiotic undergoes acetylation by different types of AAC(6'),as well as by a few other aminoglycoside-modifying enzymes suchas AAC(2'), APH(2"), and ANT(2"). The activity of the parent antibioticis not compromised by this synthetic alteration because the aminohydroxybutyrylgroup does not interfere with binding to the A-site of rRNA. Theaminohydroxybutyryl functionality at position 1 of amikacin appearsto fit well into the extended cleft, as seen in the model generatedfrom the nuclear magnetic resonance structure of the A-site RNA;the amino group in this moiety may also enhance binding of amikacinto RNA through electrostatic interactions (unpublished resultsfrom our group). Consequently, greater than 80% of the gentamicin-resistantmembers of Enterobacteriaceae and 25 to 85% of Pseudomonas aeruginosa-resistantstrains are sensitive to amikacin (25, 27). A recent surveillancestudy conducted in North America indicated that amikacin is stillan active antimicrobial agent against P. aeruginosa (11). Similarstudies in Europe showed that amikacin exhibited activity againstgram-negative bacilli superior to those of gentamicin and tobramycin(43).

To date, all attempts to make semisynthetic aminoglycosides have focused on the synthesis of derivatives that circumvent resistanceenzymes. Examples of such antibiotics are dibekacin and tobramycin,which lack the 3'-hydroxyl group and are therefore not substratesfor APH(3') compounds. Other examples are isepamycin and amikacin,both of which have an acylated N-1 group, which makes them poorersubstrates for a number of the modifying enzymes. Recently, 3'-oxo-kanamycinA (Fig. 1) was designed and prepared (16). This prototypic aminoglycosideserves as a good substrate for the common APH(3'). However, theproduct of phosphorylation is inherently unstable, and it releasesthe phosphoryl group to the solution as inorganic phosphate, regeneratingthe original antibiotic. Such an antibiotic renders these bacterialresistance enzymes obsolete for the resistant bacterium (16).Further applications such as this await futureexperimentation.

As described earlier, recent investigations have revealed that rings I and II of the neomycin class of aminoglycosides areessential for RNA binding and that they are sufficient to directthe binding of aminoglycosides to the unique binding pocket inthe RNA A-site (1, 12, 13, 17, 41). Wong and coworkers(1, 17) suggested that the 1,3-hydroxylamine moiety presentin almost all aminoglycoside antibiotics may be an important recognitionmotif for RNA binding. They investigated small molecules thatrecognize RNA with the 1,3-hydroxylamine motif as a core (1,17). To test this idea, a series of aminoglycoside derivativesbearing either one or two of these recognition motifs for RNAinteraction was synthesized (1, 15). Some of these new compoundsshowed antibiotic activities, and a few were found to be effectivein binding to the rRNA A-site sequence (1, 15, 54). Althoughthese derivatives (such as structures 5 and 6 in Fig. 1) bindto the truncated model of the rRNA A-site in the submicromolarrange, there is only a weak correlation between RNA binding affinityand antibacterial activity. For instance, despite stronger bindingaffinities than neamine, some of these compounds were weaker antibiotics.On the contrary, compounds such as gentamicin and ribostamycin,even though they contain a neamine-like core moiety, exhibit goodantibiotic activity but are poor A-site binders (54). A possibleexplanation is that in vitro binding to this RNA construct doesnot precisely mimic the in vivo binding event in the ribosomein everyrespect.

In parallel to these investigations, Tok and Rando (47) described simple 1,3(2)-aminoalcohol-containing molecules with potenciessimilar to or greater than that of paromomycin. The structuralsimplicity of these 1,2- and 1,3-aminoalcohols and their potentialas effective substituents for structurally complicated aminoglycosideantibiotics could stimulate further interest in the design andrapid syntheses of a series of new and potent antibacterialagents.

	CONCLUSIONS

Top Introduction Conclusion References

The discovery of the first aminoglycoside in 1944 stimulated considerable interest in these antibiotics. A number of subclassesof these antibiotics have been identified, and the structuresof the parent drugs have been further elaborated by chemists togenerate potent derivatives with expanded spectra of antibacterialactivity. Several of these semisynthetic aminoglycosides havealso been less prone to structural alterations by the resistanceenzymes. The current knowledge of the activities of these antibiotics,their pharmacokinetics, their structural diversity, and chemistryfor their preparation is considerable indeed. There has been aperception that investigations of aminoglycosides have reachedmaturity and that the prospects for novel insights are perhapsremote. However, structural and mechanistic information on thetarget(s) of these antibiotics and their respective resistanceenzymes has only begun to emerge in the past few years. This informationshould stimulate novel developments in the de novo design of moleculesthat bind to the ribosomal target site or molecules that wouldserve as inhibitors for the resistance enzymes in the near future.The structural and mechanistic investigations reviewed here representthe starting point for future developments in this importantarea.

	ACKNOWLEDGMENT

We are indebted to Philip Cunningham for insightful critique of themanuscript.

	FOOTNOTES

^* Corresponding author. Mailing address: Department of Chemistry, Wayne State University, Detroit, MI 48202. Phone: (313) 577-3924.Fax: (313) 577-8822. E-mail: som{at}chem.wayne.edu.

REFERENCES

Top
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6. Cech, T. R. 1990. Self-splicing of group I introns. Annu. Rev. Biochem. 59:543-568[CrossRef][Medline].

7. Cho, J., K. Hamasaki, and R. R. Rando. 1998. The binding site of a specific aminoglycoside binding RNA molecule. Biochemistry 37:4985-4992[CrossRef][Medline].

8. Cho, J., and R. R. Rando. 1999. Specificity in the binding of aminoglycosides to HIV-RRE RNA. Biochemistry 38:8548-8554[CrossRef][Medline].

9. Daigle, D. M., D. W. Hughes, and G. D. Wright. 1999. Prodigious substrate specificity of AAC(6')-APH(2"), an aminoglycoside antibiotic resistance determinant in enterococci and staphylococci. Chem. Biol. 6:99-110[CrossRef][Medline].

10. Davis, B. D. 1987. Mechanism of bactericidal action of aminoglycosides. Microbiol. Rev. 51:341-350[Free Full Text].

11. Doern, G. V., R. N. Jones, M. A. Pfaller, K. C. Kugler, and M. L. Beach. 1999. Bacterial pathogens isolated from patients with skin and soft tissue infections: frequency of occurrence and antimicrobial susceptibility patterns from the SENTRY Antimicrobial Surveillance Program (United States and Canada, 1997). SENTRY Study Group (North America). Diagn. Microbiol. Infect. Dis. 34:65-72[CrossRef][Medline].

12. Fourmy, D., M. I. Recht, S. C. Blanchard, and J. D. Puglisi. 1996. Structure of the A-site of Escherichia coli 16S ribosomal RNA complexed with an aminoglycoside antibiotic. Science 274:1367-1371[Abstract/Free Full Text].

13. Fourmy, D., M. I. Recht, and J. D. Puglisi. 1998. Binding of neomycin-class aminoglycoside antibiotics to the A-site of 16 S rRNA. J. Mol. Biol. 277:347-362[CrossRef][Medline].

14. Fourmy, D., S. Yoshizawa, and J. D. Puglisi. 1998. Paromomycin binding induces a local conformational change in the A-site of 16 S rRNA. J. Mol. Biol. 277:333-345[CrossRef][Medline].

15. Greenberg, W. A., E. S. Priestley, P. S. Sears, P. B. Alper, C. Rosenbohm, M. Hendrix, S.-C. Hung, and C.-H. Wong. 1999. Design and synthesis of new aminoglycoside antibiotics containing neamine as an optimal core structure: correlation of antibiotic activity with in vitro inhibition of translation. J. Am. Chem. Soc. 121:6527-6541[CrossRef].

16. Haddad, J., S. Vakulenko, and S. Mobashery. 1999. An antibiotic clocked by its own resistance enzyme. J. Am. Chem. Soc. 121:11922-11923[CrossRef].

17. Hendrix, M., B. P. Alper, E. S. Priestly, and C.-H. Wong. 1997. Hydroxyamines as a new motif for the molecular recognition of phosphodiesters: implications for aminoglycoside-RNA interactions. Angew. Chem. Int. Ed. Engl. 36:95-98.

18. Hendrix, M., E. S. Priestley, G. F. Joyce, and C.-H. Wong. 1997b. Direct observation of aminoglycoside-RNA interactions by surface plasmon resonance. J. Am. Chem. Soc. 119:3641-3648[CrossRef][Medline].

19. Hermann, T., and E. Westhoff. 1998. Saccharide-RNA recognition. Biopolymers 48:155-165[CrossRef][Medline].

20. Hermann, T., and E. Westhoff. 1999. Docking of cationic antibiotics to negatively charged pockets in RNA folds. J. Med. Chem. 42:1250-1261[CrossRef][Medline].

21. Hon, W. C., G. A. McKay, P. R. Thompson, R. M. Sweet, D. S. Yang, G. D. Wright, and A. M. Berghuis. 1997. Structure of an enzyme required for aminoglycoside antibiotic resistance reveals homology to eukaryotic protein kinases. Cell 89:887-895[CrossRef][Medline].

22. Honore, N., G. Marchal, and S. T. Cole. 1995. Novel mutation in 16S rRNA associated with streptomycin dependence in Mycobacterium tuberculosis. Antimicrob. Agents Chemother. 39:769-770[Abstract].

23. Jiang, L., and D. J. Patel. 1998. Solution structure of the tobramycin-RNA aptamer complex. Nat. Struct. Biol. 5:769-774[CrossRef][Medline].

24. Justice, M. C., T. Ku, M. J. Hsu, K. Carniol, D. Schmatz, and J. Nielsen. 1999. Mutations in ribosomal protein L10e confer resistance to the fungal-specific eukaryotic elongation factor 2 inhibitor sordarin. J. Biol. Chem. 274:4869-4875[Abstract/Free Full Text].

25. King, J. W., M. C. White, J. R. Todd, and S. A. Conrad. 1992. Alterations in the microbial flora and in the incidence of bacteremia at a university hospital after adoption of amikacin as the sole formulary aminoglycoside. Clin. Infect. Dis. 14:908-915[Medline].

26. Kirk, S. R., and Y. Tor. 1999. tRNA^Phe binds aminoglycoside antibiotics. Bioorg. Med. Chem. 7:1979-1991[CrossRef][Medline].

27. Kucers, A., and N. M. Bennett. 1987. Gentamicin, tobramycin, amikacin, sisomicin and netilmicin, p. 619. In A. Kucers, and N. M. Bennett (ed.), The use of antibiotics. William Heinemann Medical Books, London, United Kingdom.

28. Llano-Sotelo, B., and C. S. Chow. 1999. RNA-aminoglycoside antibiotic interactions: fluorescence detection of binding and conformational change. Bioorg. Med. Chem. Lett. 9:213-216[CrossRef][Medline].

29. McKay, G. A., J. Roestamadji, S. Mobashery, and G. D. Wright. 1996. Recognition of aminoglycoside antibiotics by the enterococcal/staphylococcal aminoglycoside 3'-phosphotransferase type IIIa: role of substrate amino groups. Antimicrob. Agents Chemother. 40:2648-2650[Abstract].

30. Michael, K., H. Wang, and Y. Tor. 1999. Enhanced RNA binding of dimerized aminoglycosides. Bioorg. Med. Chem. 7:1361-1371[CrossRef][Medline].

31. Mingeot-Leclercq, M.-P., and P. M. Tulkens. 1999. Aminoglycosides: nephrotoxicity. Antimicrob. Agents Chemother. 43:1003-1012[Free Full Text].

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J. Clin. Microbiol.	ALL ASM JOURNALS

1.	Alper, P. B., M. Hendrix, P. Sears, and C.-H. Wong. 1998. Probing the specificity of aminoglycoside-ribosomal RNA interactions with designed synthetic analogs. J. Am. Chem. Soc. 120:1965-1978[CrossRef].
2.	Azucena, E., I. Grapsas, and S. Mobashery. 1997. Properties of a bifunctional bacterial antibiotic resistance enzyme that catalyzes ATP-dependent 2"-phosphorylation and acetyl-CoA-dependent 6'-acetylation of aminoglycosides. J. Am. Chem. Soc. 119:2317-2318[CrossRef].
3.	Beauclerk, A. A., and E. Cundliffe. 1987. Sites of action of two ribosomal RNA methylases responsible for resistance to aminoglycosides. J. Mol. Biol. 193:661-671[CrossRef][Medline].
4.	Brummett, R., and K. Fox. 1989. Aminoglycoside-induced hearing loss in humans. Antimicrob. Agents Chemother. 33:797-800[Free Full Text].
5.	Cate, J. H., M. M. Yusupov, G. Z. Yusupova, T. E. Earnest, and H. F. Noller. 1999. X-ray crystal structure of 70S ribosome functional complexes. Science 285:2095-2104[Abstract/Free Full Text].
6.	Cech, T. R. 1990. Self-splicing of group I introns. Annu. Rev. Biochem. 59:543-568[CrossRef][Medline].
7.	Cho, J., K. Hamasaki, and R. R. Rando. 1998. The binding site of a specific aminoglycoside binding RNA molecule. Biochemistry 37:4985-4992[CrossRef][Medline].
8.	Cho, J., and R. R. Rando. 1999. Specificity in the binding of aminoglycosides to HIV-RRE RNA. Biochemistry 38:8548-8554[CrossRef][Medline].
9.	Daigle, D. M., D. W. Hughes, and G. D. Wright. 1999. Prodigious substrate specificity of AAC(6')-APH(2"), an aminoglycoside antibiotic resistance determinant in enterococci and staphylococci. Chem. Biol. 6:99-110[CrossRef][Medline].
10.	Davis, B. D. 1987. Mechanism of bactericidal action of aminoglycosides. Microbiol. Rev. 51:341-350[Free Full Text].
11.	Doern, G. V., R. N. Jones, M. A. Pfaller, K. C. Kugler, and M. L. Beach. 1999. Bacterial pathogens isolated from patients with skin and soft tissue infections: frequency of occurrence and antimicrobial susceptibility patterns from the SENTRY Antimicrobial Surveillance Program (United States and Canada, 1997). SENTRY Study Group (North America). Diagn. Microbiol. Infect. Dis. 34:65-72[CrossRef][Medline].
12.	Fourmy, D., M. I. Recht, S. C. Blanchard, and J. D. Puglisi. 1996. Structure of the A-site of Escherichia coli 16S ribosomal RNA complexed with an aminoglycoside antibiotic. Science 274:1367-1371[Abstract/Free Full Text].
13.	Fourmy, D., M. I. Recht, and J. D. Puglisi. 1998. Binding of neomycin-class aminoglycoside antibiotics to the A-site of 16 S rRNA. J. Mol. Biol. 277:347-362[CrossRef][Medline].
14.	Fourmy, D., S. Yoshizawa, and J. D. Puglisi. 1998. Paromomycin binding induces a local conformational change in the A-site of 16 S rRNA. J. Mol. Biol. 277:333-345[CrossRef][Medline].
15.	Greenberg, W. A., E. S. Priestley, P. S. Sears, P. B. Alper, C. Rosenbohm, M. Hendrix, S.-C. Hung, and C.-H. Wong. 1999. Design and synthesis of new aminoglycoside antibiotics containing neamine as an optimal core structure: correlation of antibiotic activity with in vitro inhibition of translation. J. Am. Chem. Soc. 121:6527-6541[CrossRef].
16.	Haddad, J., S. Vakulenko, and S. Mobashery. 1999. An antibiotic clocked by its own resistance enzyme. J. Am. Chem. Soc. 121:11922-11923[CrossRef].
17.	Hendrix, M., B. P. Alper, E. S. Priestly, and C.-H. Wong. 1997. Hydroxyamines as a new motif for the molecular recognition of phosphodiesters: implications for aminoglycoside-RNA interactions. Angew. Chem. Int. Ed. Engl. 36:95-98.
18.	Hendrix, M., E. S. Priestley, G. F. Joyce, and C.-H. Wong. 1997b. Direct observation of aminoglycoside-RNA interactions by surface plasmon resonance. J. Am. Chem. Soc. 119:3641-3648[CrossRef][Medline].
19.	Hermann, T., and E. Westhoff. 1998. Saccharide-RNA recognition. Biopolymers 48:155-165[CrossRef][Medline].
20.	Hermann, T., and E. Westhoff. 1999. Docking of cationic antibiotics to negatively charged pockets in RNA folds. J. Med. Chem. 42:1250-1261[CrossRef][Medline].
21.	Hon, W. C., G. A. McKay, P. R. Thompson, R. M. Sweet, D. S. Yang, G. D. Wright, and A. M. Berghuis. 1997. Structure of an enzyme required for aminoglycoside antibiotic resistance reveals homology to eukaryotic protein kinases. Cell 89:887-895[CrossRef][Medline].
22.	Honore, N., G. Marchal, and S. T. Cole. 1995. Novel mutation in 16S rRNA associated with streptomycin dependence in Mycobacterium tuberculosis. Antimicrob. Agents Chemother. 39:769-770[Abstract].
23.	Jiang, L., and D. J. Patel. 1998. Solution structure of the tobramycin-RNA aptamer complex. Nat. Struct. Biol. 5:769-774[CrossRef][Medline].
24.	Justice, M. C., T. Ku, M. J. Hsu, K. Carniol, D. Schmatz, and J. Nielsen. 1999. Mutations in ribosomal protein L10e confer resistance to the fungal-specific eukaryotic elongation factor 2 inhibitor sordarin. J. Biol. Chem. 274:4869-4875[Abstract/Free Full Text].
25.	King, J. W., M. C. White, J. R. Todd, and S. A. Conrad. 1992. Alterations in the microbial flora and in the incidence of bacteremia at a university hospital after adoption of amikacin as the sole formulary aminoglycoside. Clin. Infect. Dis. 14:908-915[Medline].
26.	Kirk, S. R., and Y. Tor. 1999. tRNA^Phe binds aminoglycoside antibiotics. Bioorg. Med. Chem. 7:1979-1991[CrossRef][Medline].
27.	Kucers, A., and N. M. Bennett. 1987. Gentamicin, tobramycin, amikacin, sisomicin and netilmicin, p. 619. In A. Kucers, and N. M. Bennett (ed.), The use of antibiotics. William Heinemann Medical Books, London, United Kingdom.
28.	Llano-Sotelo, B., and C. S. Chow. 1999. RNA-aminoglycoside antibiotic interactions: fluorescence detection of binding and conformational change. Bioorg. Med. Chem. Lett. 9:213-216[CrossRef][Medline].
29.	McKay, G. A., J. Roestamadji, S. Mobashery, and G. D. Wright. 1996. Recognition of aminoglycoside antibiotics by the enterococcal/staphylococcal aminoglycoside 3'-phosphotransferase type IIIa: role of substrate amino groups. Antimicrob. Agents Chemother. 40:2648-2650[Abstract].
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MINIREVIEW Aminoglycosides: Perspectives on Mechanisms of Action and Resistance and Strategies to Counter Resistance

MINIREVIEW
Aminoglycosides: Perspectives on Mechanisms of Action and Resistance and Strategies to Counter Resistance