In Vitro Activity of a Novel Antimycobacterial Compound, N-Octanesulfonylacetamide, and Its Effects on Lipid and Mycolic Acid Synthesis

doi:10.1128/AAC.45.4.1143-1150.2001

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Antimicrobial Agents and Chemotherapy, April 2001, p. 1143-1150, Vol. 45, No. 4
0066-4804/01/$04.00+0 DOI: 10.1128/AAC.45.4.1143-1150.2001
Copyright © 2001, American Society for Microbiology. All rights reserved.

In Vitro Activity of a Novel Antimycobacterial Compound, N-Octanesulfonylacetamide, and Its Effects on Lipid and Mycolic Acid Synthesis

Nikki M. Parrish,¹ Todd Houston,²^, Paul B. Jones,²^, Craig Townsend,² and James D. Dick¹^,³^,^*

Department of Pathology, School of Medicine,¹ Department of Molecular Microbiology and Immunology, School of Public Health,³ and Department of Chemistry, Johns Hopkins School of Arts and Sciences,² Johns Hopkins University, Baltimore, Maryland

Received 29 September 2000/Returned for modification 8 November 2000/Accepted 22 January 2001

	ABSTRACT

Top Abstract Introduction Materials and Methods Results Discussion References

$beta$ -Sulfonyl carboxamides have been proposed to serve as transition-state analogues of the $beta$ -ketoacyl synthase reaction involvedin fatty acid elongation. We tested the efficacy of N-octanesulfonylacetamide(OSA) as an inhibitor of fatty acid and mycolic acid biosynthesisin mycobacteria. Using the BACTEC radiometric growth system, weobserved that OSA inhibits the growth of several species of slow-growingmycobacteria, including Mycobacterium tuberculosis (H37Rv andclinical isolates), the Mycobacterium avium complex (MAC), Mycobacteriumbovis BCG, Mycobacterium kansasii, and others. Nearly all speciesand strains tested, including isoniazid and multidrug resistantisolates of M. tuberculosis, were susceptible to OSA, with MICsranging from 6.25 to 12.5 µg/ml. Only three clinical isolatesof M. tuberculosis (CSU93, OT2724, and 401296), MAC, and Mycobacteriumparatuberculosis required an OSA MIC higher than 25.0 µg/ml. Rapid-growingmycobacterial species, such as Mycobacterium smegmatis, Mycobacteriumfortuitum, and others, were not susceptible at concentrationsof up to 100 µg/ml. A 2-dimensional thin-layer chromatographysystem showed that OSA treatment resulted in a significant decreasein all species of mycolic acids present in BCG. In contrast, mycolicacids in M. smegmatis were relatively unaffected following exposureto OSA. Other lipids, including polar and nonpolar extractableclasses, were unchanged following exposure to OSA in both BCGand M. smegmatis. Transmission electron microscopy of OSA-treatedBCG cells revealed a disruption in cell wall synthesis and incompleteseptum formation. Our results indicate that OSA inhibits the growthof several species of mycobacteria, including both isoniazid-resistantand multidrug resistant strains of M. tuberculosis. This inhibitionmay be the result of OSA-mediated effects on mycolic acid synthesisin slow-growing mycobacteria or inhibition via an undescribedmechanism. Our results indicate that OSA may serve as a promisinglead compound for future antituberculous drugdevelopment.

	INTRODUCTION

Top Abstract Introduction Materials and Methods Results Discussion References

Tuberculosis continues to be the leading cause of death worldwide due to an infectious agent (8). Approximately 8 millionnew active cases arise each year, with about 3 million deaths(8). Of equivalent concern has been the emergence of multidrug-resistantMycobacterium tuberculosis. As a result, newly infected individualsno longer have the assurance that prophylaxis with isoniazid (INH)will eliminate infection or that active disease will be treatablewith our current arsenal of drugs. In addition, therapies forthe treatment of atypical mycobacterial infections in immunocompromisedpatients are limited (24). Thus, the development of new drugsis essential in combating both drug resistant M. tuberculosisand opportunistic infections with atypical mycobacteria, suchas the Mycobacterium avium complex(MAC).

Potential new targets for antimycobacterial drug development may exist among the synthetic enzymes needed to make the uniquelipids produced by mycobacteria, such as mycolic acids. Thesehigh-molecular-weight, $alpha$ -alkyl, $beta$ -hydroxy fatty acids comprisethe single largest component of the mycobacterial cell envelope(3, 4, 9, 10, 29, 30, 37). They are found infree lipids as trehalose mono- and dimycolate and esterified tothe arabinogalactan matrix of the mycobacterial cell wall (5,10). They are vital for the growth and survival of mycobacteria,as evidenced by the bactericidal properties of mycolic acid inhibitorydrugs, such as isoniazid and ethionamide (1, 2, 32, 33,43, 44, 47, 48, 51, 53-58).

Synthesis of mycolic acids and other mycobacterial lipids requires a variety of fatty acid synthase and elongation enzymes(7, 10, 23). Although the synthesis of fatty acids is essentiallythe same at the primary chemical level, fatty acid synthases (FAS)are organized into two types. In Type I FAS (FAS I), most oftenfound in eukaryotes, the individual enzymatic reactions are containedin one multienzyme complex. In Type II FAS (FAS II), commonlyfound in prokaryotes, the enzyme functions are carried out byseven individual proteins. Mycobacteria are known to possess bothFAS I and II (6, 7, 23). Thus, inhibition of these enzymes,especially those involved in chain elongation of unique mycobacterialfatty acids, may provide novel targets for drugdesign.

In the past, characterization of FAS has been aided through the use of two natural product inhibitors of FAS components, ceruleninand thiolactomycin (15, 16, 36, 39-42, 46). Cerulenin isa potent inhibitor of both FAS I and FAS II systems while thiolactomycininhibits only synthases of the FAS II variety. Activity of bothof these inhibitors on the mycolic acids of mycobacteria has recentlybeen described (25, 42, 50). Although cerulenin and thiolactomycinare structurally different, both compounds inhibit the two-carbonhomologation catalyzed by the $beta$ -ketoacyl synthase, the condensingenzyme required for fatty acid biosynthesis. Specifically, ceruleninirreversibly inhibits the $beta$ -ketoacyl synthase (20, 39, 40),while thiolactomycin inhibits both the $beta$ -ketoacyl-acyl carrierprotein (ACP) synthase and acetyl coenzyme A:ACP transacylase(15). $beta$ -Sulfonyl carboxamides were designed to mimic the transitionstate of the reaction catalyzed by the $beta$ -ketoacyl synthase. Inthe following study we evaluated the in vitro activity of oneof these compounds, N-octanesulfonylacetamide (OSA), on a varietyof mycobacteria and specifically evaluated its effects on lipidand mycolic acid synthesis in Mycobacterium bovis BCG and Mycobacteriumsmegmatis.

	MATERIALS AND METHODS

Top Abstract Introduction Materials and Methods Results Discussion References

Synthesis of OSA. The synthesis of alkyl sulfoxides and sulfones has been described previously (22). Briefly, OSA was synthesized in threesteps from commercially available materials. Octyl bromide andmethyl thioglycolate were reacted together to yield methyl 3-thioundecanoate.This sulfide was then oxidized to the sulfoxide by using 3-chloroperoxybenzoicacid. OSA was obtained from the ammonylysis of the methyl ester.Overall yield was 70% following crystallization of the final product(Fig. 1).

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FIG. 1. Structure of OSA.

Mycobacteria. M. tuberculosis strains H37Rv and CSU93 (52), M. bovis (ATCC 35734), M. bovis BCG (Pasteur strain, ATCC 35734), Mycobacteriumkansasii (ATCC 12478), Mycobacterium paratuberculosis (ATCC 19698),and M. smegmatis (mc² 6 1-2c) (53) were utilized as reference strains. Clinical andother isolates were speciated using standard methods (38) andincluded MAC, Mycobacterium fortuitum, Mycobacterium chelonei,Mycobacterium abscessus, and both INH- and multidrug-resistantclinical isolates of M. tuberculosis.

Susceptibility testing. Susceptibility testing and determination of MICs for M. tuberculosis, M. bovis, M. kansasii, and M. bovis BCG were done usingthe BACTEC radiometric growth system (Becton Dickinson, Sparks,Md.) and a standardized method (42, 49). Initial stock solutions(1 mg/ml) and subsequent dilutions of OSA, cerulenin (Sigma, St.Louis, Mo.), and thiolactomycin (generously provided by T. Yoshida)were prepared in dimethyl sulfoxide (Sigma). A modification ofthis procedure adopted by The National Jewish Center for Immunologyand Respiratory Medicine was used to determine MICs for MAC (17).Susceptibility testing of M. paratuberculosis was accomplishedby varying the standard BACTEC protocol to include the additionof mycobactin J (Allied Monitor, Fayette, Mo.) to commerciallyprepared 12B media (Becton Dickinson). Initial mycobactin J solutions(2 mg/ml) were brought up in 95% ethanol and diluted in steriledistilled water to a concentration of 40 µg/ml. Mycobactin J wasthen added to each BACTEC vial (final concentration = 1.0 µg/ml)along with OSA. All primary drugs were purchased from Becton Dickinson.Susceptibilities and MIC determinations of specific inhibitorsfor M. smegmatis, M. fortuitum, M. chelonei, and M. abscessuswere established by broth dilution using Middlebrook 7H9-ADC incubatedat 37°C for 4days.

Treatment of cultures with OSA and lipid pulse labeling. BCG and MAC cells were grown in M7H9-ADC-Tween (Difco, Detroit, Mich.) to early log phase. From this, a 1.0 McFarland suspensionwas prepared and diluted to yield a final concentration of 3 ×10⁷ cells/ml in a total volume of 50 ml in M7H9-ADC-Tween. Cultureswere aerated and incubated at 37°C for 24 h (approximately 1 generationtime). Each inhibitor was added at its MIC (final concentrations:thiolactomycin, 25.0 µg/ml [BCG] and 75.0 µg/ml [M. smegmatis];OSA, 6.25 µg/ml [BCG], 25.0 µg/ml [MAC], and 100 µg/ml [M. smegmatis]),and cultures were incubated under the same conditions for approximately1 generation time (BCG and MAC, approximately 24 h; M. smegmatis,approximately 5 h). Subsequently, 1 µCi of [1,2-¹⁴C]acetic acid (Amersham, Arlington Heights, Ill.)/ml was addedand the cultures were incubated as before for an additional 24h. In order to demonstrate a concentration-dependent effect ofOSA on mycolic acid synthesis in BCG, lipid pulse labeling wasalso performed at OSA concentrations of 12.5 and 25.0 µg/ml. Aslight variation of this protocol was used for labeling in M.smegmatis cells. Since this species of mycobacteria was not susceptibleto OSA, the highest concentration tested (100 µg/ml) in this studywas used for labeling purposes. Additionally, a 0.5 McFarlandsuspension was done with an initial incubation time of 10 h priorto the addition of compound and subsequent incubations of 5 heach (based on a doubling time of 3 to 5 h) following the additionof drug and label, respectively. All assays were performed induplicate.

Preparation of extractable mycobacterial lipids. Extractions were performed as previously described (13, 34, 42). Briefly, 100 to 150 mg (wet weight) of cells was suspendedin methanolic saline (methanol-0.3% aqueous NaCl [100:10, vol/vol][2 ml]) and extracted three times with petroleum ether, yieldingnonpolar extractable lipids. The remaining cells and residualaqueous phase were boiled for 5 min, cooled for 5 min at 37°C,and extracted with monophasic chloroform-methanol-0.3% NaCl (90:100:30,vol/vol; used once) and chloroform-methanol-0.3% NaCl (50:100:40,vol/vol; used twice). All extracts were subsequently dried underN₂ at room temperature. The defatted cells containing saponifiablelipids weresaved.

Mycolic acid extraction and preparation of MAMES and FAMES. Extractions of mycobacterial mycolic acids were performed as previously described (13, 35, 42). Briefly, 50-ml culturesof M. smegmatis, BCG, or MAC cells were harvested by centrifugationat 3,000 × g for 10 min. Equal volumes of cells (100 to 150 mg[wet weight]) were extracted to remove polar and nonpolar extractablelipids (13, 42). The resulting defatted cells containing boundmycolic acids and other saponifiable lipids were subjected toalkaline hydrolysis in methanol (1 ml), 30% KOH (1 ml), and toluene(0.1 ml) at 75°C overnight and subsequently cooled to room temperature(13, 42). The mixture was then acidified to pH 1 with 3.6%HCl and extracted three times with diethyl ether. Combined extractswere dried under N₂. Mycolic acid methyl esters (MAMES) and otherlong-chain fatty acids (fatty acid methyl esters [FAMES]) wereprepared by mixing dichloromethane (1 ml), a catalyst solution(1 ml) (14), and iodomethane (25 ml) for 30 min; centrifuging;and discarding the upper phase. The lower phase was dried underN₂.

[1,2-¹⁴C]acetate incorporation into mycobacterial lipids. Incorporation of [1,2-¹⁴C]acetate into polar and nonpolar extractable and saponifiable lipid fractions was determined by scintillationcounting and expressed in counts per minute (cpm) (Beckman LS6500multi-purpose scintillationcounter).

Analysis of MAMES and FAMES. Mycobacterial saponifiable extracts containing MAMES and FAMES were dissolved in chloroform and equal counts (in counts perminute) of each sample were loaded onto thin-layer chromatography(TLC) plates (20- by 20-cm silica gel G, 250-µm-diamter analyticalplates; Analtech, Newark, Del.). Samples were subsequently subjectedto a 2-dimensional solvent system (petroleum ether [bp 60 to 80°C]-acetone[95:5, vol/vol]) in the first dimension [three times] and toluene-acetone[97:3, vol/vol] in the second dimension [one time]).

Data analysis. Mycolic acids of each species of mycobacteria were identified according to methods described by Dobson et al. (13, 42).Visualization and comparison of thin-layer chromatograms weredone using a Fuji Systems (Fujix BAS 1000) phosphorimager. Spotswere quantified using NIH Image (version 1.57; National Institutesof Health, Bethesda, Md.) software programs. Due to the nonequivalencyof the counts per minute as determined by scintillation countingand phosphor counts as determined by phosphorimaging, relativeintensities of chromatographed compounds were calculated for eachTLC plate on the basis of total number of phosphor counts perplate. Phosphor counts for MAMES and FAMES were normalized foreach TLC plate pair (control and inhibitor treated). The differencein normalized phosphor counts between each control and inhibitortreated pair represents the percentchange.

Electron microscopy. All chemicals and reagents for electron microscopy were obtained from Electron Microscopy Sciences, Ft. Washington, Pa. Cultures(50 ml) of BCG were grown to early log phase (optical densityat 600 nm, ~0.2), at which time OSA (100 µg/ml) or diluent (dimethylsulfoxide) was added to treated and control cultures, followedby additional aeration and incubation at 37°C for 24 h. Cellswere harvested by low-speed centrifugation and washed in 0.1 Mcacodylate (CACO) buffer (pH 7.3). Washed cells were then fixedin 0.1 M CACO buffer (pH 7.3) containing 2.0% glutaraldehyde-osmiumtetroxide (1:1, vol/vol) for 45 min at 4°C (11, 28, 45).Secondary fixation was done at 4°C overnight in 4.0% formaldehyde-1.0%glutaraldehyde. Samples were post-fixed at room temperature for1 h in 0.1 M CACO buffer containing 1% tannic acid and dehydratedthrough a graded ethanol series of 50, 70, 95 (twice), and 100%(three times). Subsequently, samples were infiltrated at roomtemperature with a series of Spurrs resins (Spurrs-ethanol [1:1,vol/vol; 2 h], Spurrs-ethanol [2:1, vol/vol; 2 h], and pure Spurrs[overnight]), and blocks were polymerized at 60°C for 48 h. Sectionswere cut on a Sorvall MT2B microtome, and 80-nm-thick sectionswere picked up on 200-mesh copper grids and stained with uranylacetate and lead citrate. Prepared samples were then analyzedon a Hitachi HU12A electronmicroscope.

	RESULTS

Top Abstract Introduction Materials and Methods Results Discussion References

In vitro susceptibilities. Tables 1 and 2 show the susceptibility of various mycobacterial species and strains to OSA using the BACTEC radiometricgrowth system. Nearly all strains of M. tuberculosis and otherslow-growing mycobacterial species, such as M. bovis, M. bovisBCG, and M. kansasii, were susceptible to OSA, with MICs rangingfrom 6.25 to 12.5 µg/ml. Only three clinical isolates of M. tuberculosis(CSU 93, 42-1C9383, and 10129-3), the MAC, and M. paratuberculosisrequired a higher OSA MIC of 25 µg/ml. None of the rapid-growingmycobacterial species tested, M. smegmatis, M. fortuitum, M. chelonei,and M. abscessus, were susceptible to OSA at concentrations upto 100 µg/ml. Resistance to known antimycobacterial agents didnot give cross-resistance to OSA. Three clinical isolates of M.tuberculosis, resistant to either INH alone or INH plus rifampin,ethambutol, streptomycin, and pyrazinamide (19), were foundto be susceptible to OSA, with MICs of 12.5 and 6.25 µg/ml, respectively.Similar results were obtained for cerulenin as previously reported(42). BCG and M. smegmatis were susceptible to thiolactomycinat a MIC of 25 and 75 µg/ml, respectively.

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TABLE 1. Susceptibility of different species of mycobacteria to OSA

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TABLE 2. Activities of OSA and first-line antimycobacterial drugs against various strains of M. tuberculosis^a

Overall effects of OSA on mycobacterial lipids. Labeling assays were conducted at the calculated MIC (6.25 µg/ml) of OSA for BCG and at the highest concentration of compoundtested for M. smegmatis. This particular concentration of OSAis not equivalent to the lethal concentration of compound in mycobacteria,as evidenced by continued ¹⁴CO₂ production in the radiometric susceptibility test system,which indicated continued metabolism, albeit at a reduced levelrelative to those of controls. OSA had no significant effect on[¹⁴C]acetate incorporation into nonpolar extractable or polar extractablelipids at a concentration of 6.25 µg/ml, the calculated MIC forM. bovis BCG, or 100 µg/ml for M. smegmatis (Fig. 2). A moderatedecrease in the incorporation of label was observed in saponifiablelipids in OSA-treated BCG. However, this change was not statisticallysignificant. Label incorporation into the same lipid fractionin M. smegmatis was unaltered by exposure to OSA (Fig. 2). Inorder to demonstrate a concentration-dependent effect of OSA onlipid metabolism, studies were run at 12.5 µg/ml (two times theMIC) and 25.0 µg/ml (four times the MIC). At these higher concentrations,there was a dose-dependent decrease of label incorporation inthe saponifiable lipid fraction with a concomitant increase oflabel in the nonpolar extractable fraction (data not shown).

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FIG. 2. Effects of OSA on the synthesis of various lipid fractions in M. bovis BCG and M. smegmatis. Incorporation of [1,2-¹⁴C]acetate into extractable polar, nonpolar, and saponifiable lipids in the presence and absence of OSA. Abbreviations: NPF, nonpolar extractable lipids; PLF, polar extractable lipids; SF, saponifiable lipids, including mycolic acids. Concentrations of OSA used: for M. smegmatis, 100 µg/ml; for M. bovis BCG, 12.5 µg/ml. Differences were not statistically significant.

Effect of OSA on mycolic acid synthesis as compared with thiolactomycin. Qualitative and quantitative analysis of mycobacterial saponifiable lipids containing MAMES was performed using [¹⁴C]acetate pulse-labeling with 2-dimensional TLC and phosphorimaging.Differences in the effects of OSA and thiolactomycin were foundbetween BCG and M. smegmatis. OSA treatment in BCG resulted ininhibition of all mycolic acids commonly found in this mycobacterialspecies (Fig. 3; Table 3). This decrease or percent change inboth $alpha$ - and keto-mycolates reached greater than 90% with an OSAconcentration of four times the MIC. Similar results were demonstratedfor MAC (data not shown). However, in M. smegmatis, individualmycolate classes were only slightly inhibited following exposureto OSA (Fig. 4; Table 3). Other lipids present in the saponifiablefraction included FAMES. No appreciable change was observed inthis lipid class following OSA treatment in either of the twomycobacterial species characterized in this study (Fig. 3 and4; Table 3).

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FIG. 3. Two-dimensional TLC showing the comparative effects of OSA and thiolactomycin on the mycolic acids of M. bovis BCG. First dimension, petroleum ether (bp 60 to 80°C)-acetone (95:5, vol/vol; three times); second dimension, toluene-acetone (97:3, vol/vol; one time). Abbreviations: ori, origin; $alpha$ , $alpha$ -mycolate; k, keto-mycolate. Equivalent counts per minute of the saponifiable lipid fraction were spotted at each origin.

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TABLE 3. Effects of OSA and thiolactomycin on the mycolic acids of M. bovis BCG and M. smegmatis

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FIG. 4. Two-dimensional TLC showing the comparative effects of OSA and thiolactomycin on the mycolic acids of M. smegmatis. First dimension, petroleum ether (bp 60 to 80°C)-acetone (95:5, vol/vol; three times); second dimension, toluene-acetone (97:3, vol/vol; one time). Abbreviations: ori, origin; $alpha$ , $alpha$ -mycolate; $alpha$ ', $alpha$ '-mycolate; e, epoxymycolate. Equivalent counts per minute of the saponifiable lipid fraction were spotted at each origin.

Thiolactomycin caused a decrease in all mycolate species in BCG (Fig. 3; Table 3) and M. smegmatis. However, while thiolactomycinuniformly inhibited all mycolate species in BCG, in M. smegmatis,a differential effect was observed between individual mycolicacid classes. Both $alpha$ -mycolates and epoxymycolates were nearlycompletely diminished (95 and 87%, respectively), whereas $alpha$ '-mycolateswere less affected (57%) (Fig. 4; Table 3). In contrast to OSA,FAMES accumulated in both BCG and M. smegmatis following treatmentwiththiolactomycin.

Transmission electron microscopy of OSA-treated BCG. Inhibition of mycolic acid synthesis is known to disrupt the mycobacterial cell wall. Figure 5 shows transmission electronmicrographs of OSA-treated BCG cells during cell division. Controlorganisms exhibited an intact cell wall and clearly defined septum,whereas in the presence of OSA, cell wall synthesis was disruptedwith incomplete septum formation. In addition, outer-wall-associatedlipids appeared to be dispersed from the electron transparentzone of the mycolic acids.

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FIG. 5. Transmission electron microscopy of OSA-treated M. bovis BCG (6.25 µg/ml). (Top) Intact cell wall ultrastructure (left) (magnification, ×117,000) and completed septum (right) (magnification, ×108,000). (Bottom) Disrupted cell wall ultrastructure (left) (magnification, ×130,000) and incomplete septum formation (right) (magnification, ×78,000).

	DISCUSSION

Top Abstract Introduction Materials and Methods Results Discussion References

In this study, we demonstrate that OSA, a compound designed to inhibit fatty acid synthesis by mimicking the transition stateof the $beta$ -ketoacyl synthase, is inhibitory for a broad range ofslow-growing mycobacterial species, including multidrug-resistantM. tuberculosis. OSA treatment reduced mycolic acid accumulationin BCG and MAC cells, presumably by its effect on FAS systemsin these mycobacteria. Cross-resistance was not observed for isolatesresistant to isoniazid, rifampin, ethambutol, streptomycin, andpyrazinamide. A comparison of isoniazid, a known inhibitor ofmycolic acid synthesis, and OSA revealed pertinent information.Isoniazid has been shown to inhibit both InhA, an enoyl-ACP reductaseinvolved in fatty acid elongation, and KasA, a $beta$ -ketoacyl-ACPsynthase (2, 12, 28, 31, 32). INH resistance has beenassociated with mutations in both of these genes, as well as theKatG gene, which encodes the mycobacterial catalase-peroxidase(54, 55, 57, 58). In this study, the mechanism of INHresistance for the M. tuberculosis isolates used was not determined.Of relevance is the finding that OSA inhibited the growth of INH-resistantM. tuberculosis (>0.04 µg/ml) as well as MAC, typically resistantto INH (>2.5 µg/ml) (19). This observation suggests that theinhibition of mycolic acid synthesis by OSA may be due to interactionwith an enzymatic target different from that of INH, indicatinga novel and possibly unexploited mechanism of action of OSA inM. tuberculosis.

Although OSA was designed to inhibit $beta$ -ketoacyl synthases, it has not been tested as an inhibitor of isolated FAS. In an earlier,related study conducted in our laboratory, structurally relatedsulfones and sulfoxides were found to inhibit FAS I isolated fromM. smegmatis (41). Several of these compounds were both FASI inhibitors and active against M. tuberculosis H37Rv in the radiometricgrowth assay. However, the correlation was not exact and issuesof cell wall permeability and solubility prevented direct comparisonof the data. OSA was selected for further study based on its solubilityand its performance in whole-cellassays.

The differential susceptibility to OSA observed between slow- and rapid-growing mycobacterial species argues for the presenceof unique targets in BCG and MAC. M. smegmatis may contain thesame OSA target as BCG and MAC but possesses alternate cell wallcompounds that permit survival in spite of OSA inhibition. Anotherpotential possibility is the requirement for alteration, i.e.,activation, of OSA prior to its interaction with the target protein(s)which may occur in slow-growing mycobacteria but not in rapid-growingspecies. However, the most probable interpretation is that differencesin the mycolic acid biosynthetic pathway may exist between mycobacterialspecies. This possibility is further strengthened when the workof other investigators is considered in conjunction with our own.For example, InhA, a long chain, enoyl-ACP-dependent reductaseinvolved in fatty acid elongation, is present in both M. smegmatisand M. tuberculosis (31). Several studies have revealed compellingevidence that InhA is the target for KatG-activated INH in M.smegmatis (12, 44). However, additional investigations suggestthat this particular enzyme is not the principal target for KatG-activatedINH in M. tuberculosis (31, 32). This discrepancy may reflectinherent differences in mycolate biosynthesis between the twoorganisms (31, 32, 42). Additionally, previous studies inour laboratory examining the effect of cerulenin on mycolate synthesisin M. smegmatis and BCG revealed clear differences in mycolicacid profiles between these two mycobacterial species followinginhibitor exposure. Not only did the changes in mycolate synthesisdiffer between BCG and M. smegmatis, they were in direct opposition.For instance, completed mycolates decreased in BCG following exposureto cerulenin, whereas in M. smegmatis, all mycolate species increased,again suggesting that inherent differences in the mycolate biosyntheticpathway between the two species are responsible for these disparateresponses (42).

This possibility is further strengthened by the differential effect of thiolactomycin on individual mycolic acid classes inM. smegmatis. In both the present study and that of other investigators(50), exposure to thiolactomycin resulted in substantially decreasedamounts of $alpha$ -mycolates and epoxymycolates, with a minor decreasein $alpha$ '-mycolates (49). The authors of the previous study suggestedthat potential targets for thiolactomycin in this mycobacterialspecies include an elongation enzyme leading from either the C_24:1 $Delta$ 5intermediate or from the shorter-chain $alpha$ '-mycolates to the longer $alpha$ -mycolates and oxygenated mycolates (50). In view of the currentexperimental evidence, the latter seems to be the more likelypossibility. It should be noted that $alpha$ '-mycolates, commonly foundin rapid-growing mycobacteria, are not present in BCG and otherslow-growing mycobacteria characterized in this study (18).Thus, while thiolactomycin treatment of BCG and M. smegmatis resultedin inhibition of both $alpha$ -mycolates and oxygenated mycolates, thepresence of $alpha$ '-mycolic acids in the latter case may partiallyexplain the differences observed in MICs between the two mycobacterialspecies (for BCG, 25.0 µg/ml; for M. smegmatis, 75 µg/ml) andindicate that disparities in mycolate biosynthesis may exist betweenBCG and M. smegmatis. One could speculate that such differencesmay extend to other slow- versus rapid-growing mycobacterialspecies.

Differences in mycolic acid profiles following OSA treatment in BCG and M. smegmatis were also noted. In the present study,all mycolic acids were significantly and uniformly inhibited inOSA-treated BCG ( $alpha$ - and keto-mycolates). This inhibition increasedwith an increasing concentration of OSA. In contrast, the effectof OSA on the mycolates of M. smegmatis ( $alpha$ ', $alpha$ , and epoxy) wasnegligible and not inhibitory to growth. Previous studies havesuggested the existence of multiple ACP-dependent FAS II systemsin mycobacteria, responsible for not only fatty acid biosynthesisbut also mycolic acid biosynthesis (2, 32, 42, 44). Suchsystems could be envisioned to interact with separate and distinct $beta$ -ketoacyl-ACP synthases as well as other enzymes involved inbiosynthetic reactions of this type, including $beta$ -ketoacyl-ACPreductases, $beta$ -hydroxyacyl-ACP dehydratases, and $beta$ -enoyl-ACP reductases.A biological precedent for the existence of such enzymes has beendescribed for Esherichia coli, in which multiple $beta$ -ketoacyl-ACPsynthases have been found (21, 26, 27). Although thiolactomycinwas originally thought to inhibit all three $beta$ -ketoacyl-ACP synthasesin E. coli, recent evidence suggests that the principal targetof thiolactomycin in this particular organism may be only $beta$ -ketoacyl-ACPI (25). Since OSA was designed to inhibit the $beta$ -ketoacyl synthaseby mimicking the transition state of the reaction catalyzed bythis enzyme, this compound could in theory inhibit both the multifunctionalFAS I and monofunctional FAS II mycobacterial systems, as in thecase of cerulenin. However, in this study, additional assays wereperformed which were designed to indirectly determine FAS I activityin the presence of each inhibitor by measuring phospholipid production.Only cerulenin, known to inhibit both FAS I and FAS II systems,interfered with phospholipid synthesis in either BCG or M. smegmatis(42). Neither thiolactomycin, active only against FAS II systems,nor OSA inhibited phospholipid synthesis in either of the twomycobacterial species tested (data not shown), suggesting thatthe principal target of OSA may lie in an ACP-dependent FAS IIsystem. In addition, previous work in our laboratory and othershas demonstrated that cerulenin and thiolactomycin strongly inhibited[¹⁴C]acetate incorporation into other extractable mycobacterial lipids,a finding consistent with the known mechanism of action of bothinhibitors. In contrast, OSA inhibited only mycolic acids, withno appreciable change in label incorporation in any of the othermycobacterial lipid classes tested. This distinction suggeststhe presence of a unique and highly specific target for this compoundin slow-growing mycobacteria. Such a target may involve an as-yet-unidentifiedenzyme or enzyme system present in slow-growing mycobacteria whichis not present or inactive in rapid-growingspecies.

Additional information was obtained by careful analysis of FAMES in OSA-treated BCG and M. smegmatis. Other investigatorshave determined that these lipids most likely represent saturatedalkyl intermediate(s) in mycolic acid synthesis (31). While2-dimensional TLC of OSA-treated BCG revealed that mycolic acidsynthesis was inhibited, no apparent effect was seen in the FAMESpresent in this fraction when the compound was used at the MIC(6.25 µg/ml). A similar observation was noted in OSA-treated M.smegmatis. However, at four times the MIC, OSA treatment of BCGresulted in an increase in label incorporation into extractablenonpolar lipids. This may suggest that a noncovalently bound,extractable intermediate in mycolate synthesis accumulates followingOSA treatment, an effect intensified with higher concentrations(four times the MIC) of compound. In contrast, FAMES increasedin thiolactomycin-treated BCG, while mycolic acids decreased,a finding consistent with that of earlier studies using cerulenin(42). Thus, in BCG, while completed mycolates decreased withOSA, thiolactomycin, and cerulenin (42), the changes in FAMESwere clearly not the same, suggesting that inhibition of mycolicacid synthesis in BCG may occur prior to synthesis of the saturatedalkyl intermediate with OSA, but between this intermediate andcompleted mycolates with cerulenin and thiolactomycin. Alternatively,OSA-mediated inhibition of mycolate synthesis in BCG and MAC mayinvolve an as-yet-unidentified enzyme or enzyme system. In summary,the effects of OSA, cerulenin, and thiolactomycin are mycobacterialspecies specific and compound specific and inherent differencesin the mycolic acid biosynthetic pathway may exist between rapid-and slow-growingmycobacteria.

	ACKNOWLEDGMENTS

We thank Janet Folmer for performance of electron microscopy and William Bishai for providing equipment and laboratory spacefor some portions of thisstudy.

This study was financially supported in part by NIH grant AI43846, the Raynam Research Fund, and the Becton Dickinson CentennialFellowship in Clinical Microbiology (N.M.P.).

	FOOTNOTES

^* Corresponding author. Mailing address: Johns Hopkins Medical Institutions, Department of Pathology/Division of Medical Microbiology,600 N. Wolfe St., Baltimore, MD 21287. Phone: (410) 955-5077.Fax: (410) 614-8087. E-mail: jdick{at}jhmi.edu.

Present address: Department of Chemistry, Virginia Commonwealth University, Richmond,Va.

Present address: Department of Chemistry, Wake Forest University, Winston-Salem, N.C.

REFERENCES

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References

1. Altamirano, M., J. Marostenmaki, A. Wong, M. Fitzgerald, W. Black, and J. Smith. 1994. Mutations in the catalase-peroxidase gene from isoniazid-resistant Mycobacterium tuberculosis isolates. J. Infect. Dis. 169:1162-1165[Medline].

2. Bannerjee, A., E. Dubnau, A. Quemard, V. Balasubramanian, K. S. Um, T. Wilson, D. Collins, G. DeLisle, and W. R. Jacobs, Jr. 1994. inhA, a gene encoding a target for isoniazid and ethionamide in Mycobacterium tuberculosis. Science 263:227-230[Abstract/Free Full Text].

3. Barry, C., III, and K. Mdluli. 1996. Drug sensitivity and environmental adaptation of mycobacterial cell wall components. Trends Microbiol. 4:275-281[CrossRef][Medline].

4. Besra, G., and D. Chatterjee. 1994. Lipids and carbohydrates of Mycobacterium tuberculosis, p. 285-306. In B. Bloom (ed.), Tuberculosis: pathogenesis, protection, and control. ASM Press, Washington, D.C.

5. Besra, G., K. Khoo, M. McNeil, A. Dell, H. Morris, and P. Brennan. 1995. A new interpretation of the structure of the mycolyl-arabinogalactan complex of Mycobacterium tuberculosis as revealed through the characterization of oligoglycosyl alditol fragments by fast-atom bombardment mass spectrometry and ¹H-nuclear magnetic resonance spectroscopy. Biochemistry 24:84-90.

6. Bloch, K. 1975. Fatty acid synthases from Mycobacterium phlei. Methods Enzymol. 35:84-90[Medline].

7. Bloch, K. 1977. Control mechanisms for fatty acid synthesis in Mycobacterium smegmatis, p. 1-84. In A. Meister (ed.), Advances in enzymology. John Wiley and Sons, New York, N.Y.

8. Bloom, B., and C. Murray. 1992. Tuberculosis: commentary on a reemergent killer. Science 257:1055-1064[Abstract/Free Full Text].

9. Brennan, P., and P. Draper. 1994. Ultrastructure of Mycobacterium tuberculosis, p. 271-284. In B. Bloom (ed.), Tuberculosis: pathogenesis, protection, and control. ASM Press, Washington, D.C.

10. Brennan, P., and H. Nikaido. 1995. The envelope of mycobacteria. Annu. Rev. Biochem. 64:29-63[CrossRef][Medline].

11. Cunningham, A., and C. Spreadbury. 1998. Mycobacterial stationary phase induced by low oxygen tension: cell wall thickening and localization of the 16-kilodalton $alpha$ -crystallin homolog. J. Bacteriol. 180:801-808[Abstract/Free Full Text].

12. Dessen, A., A. Quemard, J. S. Blanchard, W. R. Jacobs, Jr., and J. C. Sachettini. 1995. Crystal structure and function of the isoniazid target of Mycobacterium tuberculosis. Science 267:1638-1641[Abstract/Free Full Text].

13. Dobson, G., D. Minnikin, S. Minnikin, J. Parlett, and M. Goodfellow. 1985. Systematic analysis of complex mycobacterial lipids, p. 237-265. In M. Goodfellow, and D. Minnikin (ed.), Chemical methods in bacterial systematics. Academic Press, London, United Kingdom.

14. Gyllenhaal, O., and H. Ehrsson. 1975. Determination of sulphonamides by electron-capture gas chromatography. Preparation and properties of perfluoroacyl and pentaflurobenzyl derivatives. Chromatography 107:327-333.

15. Hayashi, T., O. Yamamoto, H. Sasaki, H. Kawaguchi, and H. Okazaki. 1983. Mechanism of action of the antibiotic thiolactomycin: inhibition of fatty acid synthesis in Escherichia coli. Biochim. Biophys. Res. Commun. 115:1108-1113[CrossRef][Medline].

16. Hayashi, T., O. Yamamoto, H. Sasaki, and H. Okazaki. 1984. Inhibition of fatty acid synthesis by the antibiotic thiolactomycin. J. Antibiot. 37:1456-1461[Medline].

17. Heifets, H., P. Lindholm-Levy, J. Libonati, et al. 1993. Radiometric broth macrodilution method for determination of minimal inhibitory concentrations (MIC's) with Mycobacterium avium complex isolates. National Jewish Center for Immunology and Respiratory Medicine, Denver, Colo.

18. Hinrikson, H. P., and G. E. Pfyffer. 1994. Mycobacterial mycolic acids. Med. Microbiol. Lett. 3:49-57.

19. Inderlied, C., and M. Salfinger. 1995. Antimicrobial agents and susceptibility tests: mycobacteria, p. 1385-1404. In P. Murray (ed.), Manual of clinical microbiology. ASM Press, Washington, D.C.

20. Inokoshi, J., H. Tomoda, H. Hashimoto, A. Watanabe, H. Takeshima, and S. Omura. 1994. Cerulenin-resistant mutants of Saccharomyces cerevesiae with an altered fatty acid synthase gene. Mol. Gen. Genet. 244:90-96[CrossRef][Medline].

21. Jackowski, S., J. E. Cronan, Jr., and C. O. Rock. 1991. Lipid metabolism in prokaryotes, p. 43-85. In D. E. Vance, and J. Vance (ed.), Biochemistry of lipids, lipoproteins, and membranes. Elsevier Publishers B. V., Amsterdam, The Netherlands.

22. Jones, P. B., N. M. Parrish, T. A. Houston, A. S. Stapon, N. P. Bansal, J. D. Dick, and C. A. Townsend. 2000. A new class of anti-tuberculosis agents. J. Med. Chem. 43:3304-3314[CrossRef][Medline].

23. Kolattukudy, P., N. Fernandes, A. Azad, A. Fitzmaurice, and T. Sirakova. 1997. Biochemistry and molecular genetics of cell wall lipid biosynthesis in mycobacteria. Mol. Microbiol. 24:263-270[CrossRef][Medline].

24. Korvick, J., and C. Benson. 1996. Advances in the treatment and prophylaxis of Mycobacterium avium complex in individuals infected with human immunodeficiency virus, p. 241-262. In J. Korvick, and C. Benson (ed.), Mycobacterium avium complex infection: progress in research and treatment, vol. 87. Lung biology in Health and Disease. Marcel Dekker, Incorporated, New York, N.Y.

25. Kremer, L., J. D. Douglas, A. R. Baulard, C. Morehouse, M. R. Guy, D. Alland, L. G. Dover, H. Lakey, W. R. Jacobs, P. J. Brennan, D. E. Minnikin, and G. S. Besra. 2000. Thiolactomycin and related-analogues as novel anti-mycobacterial agents targeting KasA and KasB condensing enzymes in Mycobacterium tuberculosis. J. Biol. Chem. 275:16857-16864[Abstract/Free Full Text].

26. Lowe, P. N., and S. Rhodes. 1988. Purification and characterization of [acyl-carrier-protein]acetyltransferase from Escherichia coli. Biochem. J. 250:789-796[Medline].

27. Magnuson, K. S., S. Jackowski, C. O. Rock, and J. E. Cronan, Jr. 1993. Regulation of fatty acid biosynthesis in Escherichia coli. Microbiol. Rev. 57:522-542[Abstract/Free Full Text].

28. McDonough, K., V. Kress, and B. Bloom. 1993. Pathogenesis of tuberculosis: interaction of Mycobacterium tuberculosis with macrophages. Infect. Immun. 61:2763-2773[Abstract/Free Full Text].

29. McNeil, M., and P. Brennan. 1991. Structure, function, and biogenesis of the cell envelope of mycobacteria in relation to bacterial physiology, pathogenesis and drug resistance; some thoughts and possibilities arising from recent structural information. Res. Microbiol. 142:451-463[Medline].

30. McNeil, M., M. Daffe, and P. Brennan. 1991. Location of the mycolyl ester substituents in the cell walls of mycobacteria. J. Biol. Chem. 266:6934-6943.

31. Mdluli, K., D. R. Sherman, M. J. Hickey, B. N. Kreiswirth, S. Morris, C. K. Stover, and C. E. Barry, III. 1996. Biochemical and genetic data suggest that InhA is not the primary target for activated isoniazid in Mycobacterium tuberculosis. J. Infect. Dis. 174:1085-1090[Medline].

32. Mdluli, K., R. Slayden, Y. Zhu, S. Ramaswamy, X. Pan, D. Mead, D. Crane, J. Musser, and C. Barry, III. 1998. Inhibition of Mycobacterium tuberculosis $beta$ -ketoacyl ACP synthase by isoniazid. Science 280:1607-1610[Abstract/Free Full Text].

33. Middlebrook, G. 1954. Isoniazid-resistance and catalase activity of tubercle bacilli. Am. Rev. Tuberc. 69:471-472[Medline].

34. Minnikin, D., A. O'Donnell, M. Goodfellow, G. Alderson, M. Athalye, A. Schaal, et al. 1984. An integrated procedure for the extraction of bacterial isoprenoid quinones and polar lipids. J. Microbiol. Methods 2:233-241[CrossRef].

35. Minnikin, D., S. Minnikin, A. O'Donnell, and M. Goodfellow. 1984. Extraction of mycobacterial mycolic acids and other long-chain compounds by an alkaline methanolysis procedure. J. Microbiol. Methods 2:243-249.

36. Morisaki, N., H. Funabashi, R. Shimazawa, J. Furukawa, A. Kawaguchi, S. Okuda, and S. Iwasaki. 1993. Effect of side-chain structure on inhibition of yeast fatty-acid synthase by cerulenin analogues. Eur. J. Biochem. 211:111-115[Medline].

37. Nikaido, H., S. Kim, and E. Rosenberg. 1993. Physical organization of lipids in the cell wall of Mycobacterium chelonae. Mol. Microbiol. 8:1025-1030[Medline].

38. Nolte, F., and B. Metchock. 1995. Mycobacterium, p. 400-437. In P. Murray, E. Baron, M. Pfaller, F. Tenover, and R. Yolken (ed.), Manual of clinical microbiology. American Society for Microbiology, Washington, D.C.

39. Omura, S. 1976. The antibiotic cerulenin, a novel tool for biochemistry as an inhibitor of fatty acid synthesis. Bacteriol. Rev. 40:681-697[Free Full Text].

40. Omura, S. 1981. Cerulenin. Methods Enzymol. 72:520-535[Medline].

41. Parrish, N. 1999. Ph.D. thesis. Johns Hopkins University, Baltimore, Md.

42. Parrish, N., F. Kuhajda, H. Heine, W. Bishai, and J. Dick. 1999. Antimycobacterial activity of cerulenin and its effects on lipid synthesis. J. Antimicrob. Chemother. 43:219-226[Abstract/Free Full Text].

43. Quemard, A., C. Lacave, and G. Laneelle. 1991. Isoniazid inhibition of mycolic acid synthesis by cell extracts of sensitive and resistant strains of Mycobacterium aurum. Antimicrob. Agents Chemother. 35:1035-1039[Abstract/Free Full Text].

44. Quemard, A., J. C. Sacchettini, A. Dessen, C. Vilcheze, R. Bittman, W. R. Jacobs, Jr., and J. S. Blanchard. 1995. Enzymatic characterization of the target for isoniazid in Mycobacterium tuberculosis. Biochemistry 34:8235-8241[CrossRef][Medline].

45. Rastogi, N., C. Frehel, and H. David. 1986. Triple-layered structure of the mycobacterial cell wall: evidence of a polysaccharide-rich outer layer in 18 mycobacterial species. Curr. Microbiol. 13:237-242.

46. Sasaki, H., H. Oishi, T. Hayashi, I. Matsura, K. Ando, and M. Sawada. 1982. Thiolactomycin, a new antibiotic: structure elucidation. J. Antibiot. 35:396-400[Medline].

47. Shoeb, H., B. Bowman, A. Ottolenghi, and A. Merola. 1985. Evidence for the generation of active oxygen by isoniazid treatment of extracts of Mycobacterium tuberculosis H37Ra. Antimicrob. Agents Chemother. 27:404-407[Abstract/Free Full Text].

48. Shoeb, H., B. Bowman, A. Ottolenghi, and A. Merola. 1985. Peroxidase-mediated oxidation of isoniazid. Antimicrob. Agents Chemother. 27:399-403[Abstract/Free Full Text].

49. Siddiqi, S. 1992. Radiometric (BACTEC) tests for slowly growing mycobacteria, p. 5.14.1-5.14.25. In H. Isenberg (ed.), Clinical microbiology procedures handbook, vol. 1. American Society for Microbiology, Washington, D.C.

50. Slayden, R., A., R. E. Lee, J. W. Armour, A. M. Cooper, I. M. Orme, P. J. Brennan, and G. S. Besra. 1996. Antimycobacterial activity of thiolactomycin: an inhibitor of fatty acid and mycolic acid synthesis. Antimicrob. Agents Chemother. 40:2813-2819[Abstract].

51. Takayama, K., H. K. Schnoes, E. L. Armstrong, and R. W. Boyle. 1975. Site of inhibitory action of isoniazid in the synthesis of mycolic acids in Mycobacterium tuberculosis. J. Lipid Res. 16:308-317[Abstract].

52. Valway, S., M. Sanchez, T. Shinnick, I. Orme, T. Agerton, D. Hoy, J. Jones, H. Westmoreland, and I. Onorato. 1998. An outbreak involving extensive transmission of a virulent strain of Mycobacterium tuberculosis. N. Engl. J. Med. 338:633-639[Abstract/Free Full Text].

53. Youtt, J. 1969. A review of the action of isoniazid. Am. Rev. Respir. Dis. 99:729-749[Medline].

54. Zhang, Y., T. Garbe, and D. Young. 1993. Transformation with katG restores isoniazid-sensitivity in Mycobacterium tuberculosis isolates resistant to a range of drug concentrations. Mol. Microbiol. 8:521-524[Medline].

55. Zhang, Y., B. Heym, B. Allen, D. Young, and S. Cole. 1992. The catalase-peroxidase gene and isoniazid resistance of Mycobacterium tuberculosis. Nature 358:591-593[CrossRef][Medline].

56. Zhang, Y., R. Lathigra, T. Garbe, D. Catty, and D. Young. 1991. Genetic analysis of superoxide dismutase, the 23 kilodalton antigen of Mycobacterium tuberculosis. Mol. Microbiol. 5:381-391[Medline].

57. Zhang, Y., and D. Young. 1993. Molecular mechanisms of isoniazid: a drug at the frontline of tuberculosis control. Trends Microbiol. 1:109-113[CrossRef][Medline].

58. Zhang, Y., and D. Young. 1994. Strain variation of the katG region of Mycobacterium tuberculosis. Mol. Microbiol. 14:301-308[CrossRef][Medline].

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Clin. Vaccine Immunol.	Clin. Microbiol. Rev.
J. Clin. Microbiol.	ALL ASM JOURNALS

1.	Altamirano, M., J. Marostenmaki, A. Wong, M. Fitzgerald, W. Black, and J. Smith. 1994. Mutations in the catalase-peroxidase gene from isoniazid-resistant Mycobacterium tuberculosis isolates. J. Infect. Dis. 169:1162-1165[Medline].
2.	Bannerjee, A., E. Dubnau, A. Quemard, V. Balasubramanian, K. S. Um, T. Wilson, D. Collins, G. DeLisle, and W. R. Jacobs, Jr. 1994. inhA, a gene encoding a target for isoniazid and ethionamide in Mycobacterium tuberculosis. Science 263:227-230[Abstract/Free Full Text].
3.	Barry, C., III, and K. Mdluli. 1996. Drug sensitivity and environmental adaptation of mycobacterial cell wall components. Trends Microbiol. 4:275-281[CrossRef][Medline].
4.	Besra, G., and D. Chatterjee. 1994. Lipids and carbohydrates of Mycobacterium tuberculosis, p. 285-306. In B. Bloom (ed.), Tuberculosis: pathogenesis, protection, and control. ASM Press, Washington, D.C.
5.	Besra, G., K. Khoo, M. McNeil, A. Dell, H. Morris, and P. Brennan. 1995. A new interpretation of the structure of the mycolyl-arabinogalactan complex of Mycobacterium tuberculosis as revealed through the characterization of oligoglycosyl alditol fragments by fast-atom bombardment mass spectrometry and ¹H-nuclear magnetic resonance spectroscopy. Biochemistry 24:84-90.
6.	Bloch, K. 1975. Fatty acid synthases from Mycobacterium phlei. Methods Enzymol. 35:84-90[Medline].
7.	Bloch, K. 1977. Control mechanisms for fatty acid synthesis in Mycobacterium smegmatis, p. 1-84. In A. Meister (ed.), Advances in enzymology. John Wiley and Sons, New York, N.Y.
8.	Bloom, B., and C. Murray. 1992. Tuberculosis: commentary on a reemergent killer. Science 257:1055-1064[Abstract/Free Full Text].
9.	Brennan, P., and P. Draper. 1994. Ultrastructure of Mycobacterium tuberculosis, p. 271-284. In B. Bloom (ed.), Tuberculosis: pathogenesis, protection, and control. ASM Press, Washington, D.C.
10.	Brennan, P., and H. Nikaido. 1995. The envelope of mycobacteria. Annu. Rev. Biochem. 64:29-63[CrossRef][Medline].
11.	Cunningham, A., and C. Spreadbury. 1998. Mycobacterial stationary phase induced by low oxygen tension: cell wall thickening and localization of the 16-kilodalton $alpha$ -crystallin homolog. J. Bacteriol. 180:801-808[Abstract/Free Full Text].
12.	Dessen, A., A. Quemard, J. S. Blanchard, W. R. Jacobs, Jr., and J. C. Sachettini. 1995. Crystal structure and function of the isoniazid target of Mycobacterium tuberculosis. Science 267:1638-1641[Abstract/Free Full Text].
13.	Dobson, G., D. Minnikin, S. Minnikin, J. Parlett, and M. Goodfellow. 1985. Systematic analysis of complex mycobacterial lipids, p. 237-265. In M. Goodfellow, and D. Minnikin (ed.), Chemical methods in bacterial systematics. Academic Press, London, United Kingdom.
14.	Gyllenhaal, O., and H. Ehrsson. 1975. Determination of sulphonamides by electron-capture gas chromatography. Preparation and properties of perfluoroacyl and pentaflurobenzyl derivatives. Chromatography 107:327-333.
15.	Hayashi, T., O. Yamamoto, H. Sasaki, H. Kawaguchi, and H. Okazaki. 1983. Mechanism of action of the antibiotic thiolactomycin: inhibition of fatty acid synthesis in Escherichia coli. Biochim. Biophys. Res. Commun. 115:1108-1113[CrossRef][Medline].
16.	Hayashi, T., O. Yamamoto, H. Sasaki, and H. Okazaki. 1984. Inhibition of fatty acid synthesis by the antibiotic thiolactomycin. J. Antibiot. 37:1456-1461[Medline].
17.	Heifets, H., P. Lindholm-Levy, J. Libonati, et al. 1993. Radiometric broth macrodilution method for determination of minimal inhibitory concentrations (MIC's) with Mycobacterium avium complex isolates. National Jewish Center for Immunology and Respiratory Medicine, Denver, Colo.
18.	Hinrikson, H. P., and G. E. Pfyffer. 1994. Mycobacterial mycolic acids. Med. Microbiol. Lett. 3:49-57.
19.	Inderlied, C., and M. Salfinger. 1995. Antimicrobial agents and susceptibility tests: mycobacteria, p. 1385-1404. In P. Murray (ed.), Manual of clinical microbiology. ASM Press, Washington, D.C.
20.	Inokoshi, J., H. Tomoda, H. Hashimoto, A. Watanabe, H. Takeshima, and S. Omura. 1994. Cerulenin-resistant mutants of Saccharomyces cerevesiae with an altered fatty acid synthase gene. Mol. Gen. Genet. 244:90-96[CrossRef][Medline].
21.	Jackowski, S., J. E. Cronan, Jr., and C. O. Rock. 1991. Lipid metabolism in prokaryotes, p. 43-85. In D. E. Vance, and J. Vance (ed.), Biochemistry of lipids, lipoproteins, and membranes. Elsevier Publishers B. V., Amsterdam, The Netherlands.
22.	Jones, P. B., N. M. Parrish, T. A. Houston, A. S. Stapon, N. P. Bansal, J. D. Dick, and C. A. Townsend. 2000. A new class of anti-tuberculosis agents. J. Med. Chem. 43:3304-3314[CrossRef][Medline].
23.	Kolattukudy, P., N. Fernandes, A. Azad, A. Fitzmaurice, and T. Sirakova. 1997. Biochemistry and molecular genetics of cell wall lipid biosynthesis in mycobacteria. Mol. Microbiol. 24:263-270[CrossRef][Medline].
24.	Korvick, J., and C. Benson. 1996. Advances in the treatment and prophylaxis of Mycobacterium avium complex in individuals infected with human immunodeficiency virus, p. 241-262. In J. Korvick, and C. Benson (ed.), Mycobacterium avium complex infection: progress in research and treatment, vol. 87. Lung biology in Health and Disease. Marcel Dekker, Incorporated, New York, N.Y.
25.	Kremer, L., J. D. Douglas, A. R. Baulard, C. Morehouse, M. R. Guy, D. Alland, L. G. Dover, H. Lakey, W. R. Jacobs, P. J. Brennan, D. E. Minnikin, and G. S. Besra. 2000. Thiolactomycin and related-analogues as novel anti-mycobacterial agents targeting KasA and KasB condensing enzymes in Mycobacterium tuberculosis. J. Biol. Chem. 275:16857-16864[Abstract/Free Full Text].
26.	Lowe, P. N., and S. Rhodes. 1988. Purification and characterization of [acyl-carrier-protein]acetyltransferase from Escherichia coli. Biochem. J. 250:789-796[Medline].
27.	Magnuson, K. S., S. Jackowski, C. O. Rock, and J. E. Cronan, Jr. 1993. Regulation of fatty acid biosynthesis in Escherichia coli. Microbiol. Rev. 57:522-542[Abstract/Free Full Text].
28.	McDonough, K., V. Kress, and B. Bloom. 1993. Pathogenesis of tuberculosis: interaction of Mycobacterium tuberculosis with macrophages. Infect. Immun. 61:2763-2773[Abstract/Free Full Text].
29.	McNeil, M., and P. Brennan. 1991. Structure, function, and biogenesis of the cell envelope of mycobacteria in relation to bacterial physiology, pathogenesis and drug resistance; some thoughts and possibilities arising from recent structural information. Res. Microbiol. 142:451-463[Medline].
30.	McNeil, M., M. Daffe, and P. Brennan. 1991. Location of the mycolyl ester substituents in the cell walls of mycobacteria. J. Biol. Chem. 266:6934-6943.
31.	Mdluli, K., D. R. Sherman, M. J. Hickey, B. N. Kreiswirth, S. Morris, C. K. Stover, and C. E. Barry, III. 1996. Biochemical and genetic data suggest that InhA is not the primary target for activated isoniazid in Mycobacterium tuberculosis. J. Infect. Dis. 174:1085-1090[Medline].
32.	Mdluli, K., R. Slayden, Y. Zhu, S. Ramaswamy, X. Pan, D. Mead, D. Crane, J. Musser, and C. Barry, III. 1998. Inhibition of Mycobacterium tuberculosis $beta$ -ketoacyl ACP synthase by isoniazid. Science 280:1607-1610[Abstract/Free Full Text].
33.	Middlebrook, G. 1954. Isoniazid-resistance and catalase activity of tubercle bacilli. Am. Rev. Tuberc. 69:471-472[Medline].
34.	Minnikin, D., A. O'Donnell, M. Goodfellow, G. Alderson, M. Athalye, A. Schaal, et al. 1984. An integrated procedure for the extraction of bacterial isoprenoid quinones and polar lipids. J. Microbiol. Methods 2:233-241[CrossRef].
35.	Minnikin, D., S. Minnikin, A. O'Donnell, and M. Goodfellow. 1984. Extraction of mycobacterial mycolic acids and other long-chain compounds by an alkaline methanolysis procedure. J. Microbiol. Methods 2:243-249.
36.	Morisaki, N., H. Funabashi, R. Shimazawa, J. Furukawa, A. Kawaguchi, S. Okuda, and S. Iwasaki. 1993. Effect of side-chain structure on inhibition of yeast fatty-acid synthase by cerulenin analogues. Eur. J. Biochem. 211:111-115[Medline].
37.	Nikaido, H., S. Kim, and E. Rosenberg. 1993. Physical organization of lipids in the cell wall of Mycobacterium chelonae. Mol. Microbiol. 8:1025-1030[Medline].
38.	Nolte, F., and B. Metchock. 1995. Mycobacterium, p. 400-437. In P. Murray, E. Baron, M. Pfaller, F. Tenover, and R. Yolken (ed.), Manual of clinical microbiology. American Society for Microbiology, Washington, D.C.
39.	Omura, S. 1976. The antibiotic cerulenin, a novel tool for biochemistry as an inhibitor of fatty acid synthesis. Bacteriol. Rev. 40:681-697[Free Full Text].
40.	Omura, S. 1981. Cerulenin. Methods Enzymol. 72:520-535[Medline].
41.	Parrish, N. 1999. Ph.D. thesis. Johns Hopkins University, Baltimore, Md.
42.	Parrish, N., F. Kuhajda, H. Heine, W. Bishai, and J. Dick. 1999. Antimycobacterial activity of cerulenin and its effects on lipid synthesis. J. Antimicrob. Chemother. 43:219-226[Abstract/Free Full Text].
43.	Quemard, A., C. Lacave, and G. Laneelle. 1991. Isoniazid inhibition of mycolic acid synthesis by cell extracts of sensitive and resistant strains of Mycobacterium aurum. Antimicrob. Agents Chemother. 35:1035-1039[Abstract/Free Full Text].
44.	Quemard, A., J. C. Sacchettini, A. Dessen, C. Vilcheze, R. Bittman, W. R. Jacobs, Jr., and J. S. Blanchard. 1995. Enzymatic characterization of the target for isoniazid in Mycobacterium tuberculosis. Biochemistry 34:8235-8241[CrossRef][Medline].
45.	Rastogi, N., C. Frehel, and H. David. 1986. Triple-layered structure of the mycobacterial cell wall: evidence of a polysaccharide-rich outer layer in 18 mycobacterial species. Curr. Microbiol. 13:237-242.
46.	Sasaki, H., H. Oishi, T. Hayashi, I. Matsura, K. Ando, and M. Sawada. 1982. Thiolactomycin, a new antibiotic: structure elucidation. J. Antibiot. 35:396-400[Medline].
47.	Shoeb, H., B. Bowman, A. Ottolenghi, and A. Merola. 1985. Evidence for the generation of active oxygen by isoniazid treatment of extracts of Mycobacterium tuberculosis H37Ra. Antimicrob. Agents Chemother. 27:404-407[Abstract/Free Full Text].
48.	Shoeb, H., B. Bowman, A. Ottolenghi, and A. Merola. 1985. Peroxidase-mediated oxidation of isoniazid. Antimicrob. Agents Chemother. 27:399-403[Abstract/Free Full Text].
49.	Siddiqi, S. 1992. Radiometric (BACTEC) tests for slowly growing mycobacteria, p. 5.14.1-5.14.25. In H. Isenberg (ed.), Clinical microbiology procedures handbook, vol. 1. American Society for Microbiology, Washington, D.C.
50.	Slayden, R., A., R. E. Lee, J. W. Armour, A. M. Cooper, I. M. Orme, P. J. Brennan, and G. S. Besra. 1996. Antimycobacterial activity of thiolactomycin: an inhibitor of fatty acid and mycolic acid synthesis. Antimicrob. Agents Chemother. 40:2813-2819[Abstract].
51.	Takayama, K., H. K. Schnoes, E. L. Armstrong, and R. W. Boyle. 1975. Site of inhibitory action of isoniazid in the synthesis of mycolic acids in Mycobacterium tuberculosis. J. Lipid Res. 16:308-317[Abstract].
52.	Valway, S., M. Sanchez, T. Shinnick, I. Orme, T. Agerton, D. Hoy, J. Jones, H. Westmoreland, and I. Onorato. 1998. An outbreak involving extensive transmission of a virulent strain of Mycobacterium tuberculosis. N. Engl. J. Med. 338:633-639[Abstract/Free Full Text].
53.	Youtt, J. 1969. A review of the action of isoniazid. Am. Rev. Respir. Dis. 99:729-749[Medline].
54.	Zhang, Y., T. Garbe, and D. Young. 1993. Transformation with katG restores isoniazid-sensitivity in Mycobacterium tuberculosis isolates resistant to a range of drug concentrations. Mol. Microbiol. 8:521-524[Medline].
55.	Zhang, Y., B. Heym, B. Allen, D. Young, and S. Cole. 1992. The catalase-peroxidase gene and isoniazid resistance of Mycobacterium tuberculosis. Nature 358:591-593[CrossRef][Medline].
56.	Zhang, Y., R. Lathigra, T. Garbe, D. Catty, and D. Young. 1991. Genetic analysis of superoxide dismutase, the 23 kilodalton antigen of Mycobacterium tuberculosis. Mol. Microbiol. 5:381-391[Medline].
57.	Zhang, Y., and D. Young. 1993. Molecular mechanisms of isoniazid: a drug at the frontline of tuberculosis control. Trends Microbiol. 1:109-113[CrossRef][Medline].
58.	Zhang, Y., and D. Young. 1994. Strain variation of the katG region of Mycobacterium tuberculosis. Mol. Microbiol. 14:301-308[CrossRef][Medline].