A Glutathione S-Transferase with Activity towards cis-1,2-Dichloroepoxyethane Is Involved in Isoprene Utilization by Rhodococcus sp. Strain AD45

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Applied and Environmental Microbiology, August 1998, p. 2800-2805, Vol. 64, No. 8
0099-2240/98/$04.00+0
Copyright © 1998, American Society for Microbiology. All rights reserved.

A Glutathione S-Transferase with Activity towards cis-1,2-Dichloroepoxyethane Is Involved in Isoprene Utilization by Rhodococcus sp. Strain AD45

Johan E. T. van Hylckama Vlieg, Jaap Kingma, Arjan J. van den Wijngaard, and Dick B. Janssen^*

Department of Biochemistry, Groningen Biomolecular Sciences and Biotechnology Institute, University of Groningen, 9747 AG Groningen, The Netherlands

Received 27 February 1998/Accepted 12 May 1998

	ABSTRACT

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Rhodococcus sp. strain AD45 was isolated from an enrichment culture on isoprene (2-methyl-1,3-butadiene). Isoprene-grown cellsof strain AD45 oxidized isoprene to 3,4-epoxy-3-methyl-1-butene,cis-1,2-dichloroethene to cis-1,2-dichloroepoxyethane, and trans-1,2-dichloroetheneto trans-1,2-dichloroepoxyethane. Isoprene-grown cells also degradedcis-1,2-dichloroepoxyethane and trans-1,2-dichloroepoxyethane.All organic chlorine was liberated as chloride during degradationof cis-1,2-dichloroepoxyethane. A glutathione (GSH)-dependentactivity towards 3,4-epoxy-3-methyl-1-butene, epoxypropane, cis-1,2-dichloroepoxyethane,and trans-1,2-dichloroepoxyethane was detected in cell extractsof cultures grown on isoprene and 3,4-epoxy-3-methyl-1-butene.The epoxide-degrading activity of strain AD45 was irreversiblylost upon incubation of cells with 1,2-epoxyhexane. A conjugateof GSH and 1,2-epoxyhexane was detected in cell extracts of cellsexposed to 1,2-epoxyhexane, indicating that GSH is the physiologicalcofactor of the epoxide-transforming activity. The results indicatethat a GSH S-transferase is involved in the metabolism of isopreneand that the enzyme can detoxify reactive epoxides produced bymonooxygenation of chlorinated ethenes.

	INTRODUCTION

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Perchloroethene and trichloroethene (TCE) have been widely used as solvents and degreasing agents, and improper disposal andspillage of these compounds have frequently resulted in contaminationof groundwater. Dechlorination reactions occurring in situ underanaerobic conditions may result in the accumulation of cis-1,2-dichloroethene(cis-1,2-DCE) and vinyl chloride at contaminated locations (34).There is great interest in biological methods for treatment ofsites that are contaminated with these compounds. Under aerobicconditions, vinyl chloride has been shown to serve as a growthsubstrate (14), whereas for TCE and dichloroethenes only cometabolicdegradation has been reported. Conversion of chlorinated etheneshas been described for organisms that produce dioxygenases ormonooxygenases with broad substrate ranges (3, 7, 12,20, 23, 36, 37).

Oxidation of chlorinated ethenes by monooxygenases results in the formation of epoxides (12, 16, 32). These electrophiliccompounds are unstable in aqueous solutions. The reactivitiesof the epoxides and their degradation products often result incovalent modification of cellular components, causing toxic effects(12, 23, 33). Consequently, the amount of chlorinated ethenethat can be converted by cells is limited, and continuous-treatmentsystems may be unstable (11, 22). Since the toxicity thatis associated with oxidative cometabolic degradation of chlorinatedethenes is the main limiting factor for the application of monooxygenase-expressingorganisms, it is desirable to find ways to biologically detoxifyreactive transformation products.

Theoretically, enzymatic conversion of TCE epoxide or dichloroethene epoxides to nonreactive products may decrease the toxiceffects, but information about the microbial conversion of thesecompounds is scarce. Degradation of vinyl chloride by Mycobacteriumaurum L1 proceeds via chloroepoxyethane, but the enzyme(s) thatconverts this epoxide has not been characterized (14). Cellsof Methylosinus trichosporium OB3b expressing soluble methanemonooxygenase converted cis-1,2-dichloroepoxyethane, but rapidinactivation occurred during this transformation, indicating thateven products that are more toxic were generated (32, 33).

Epoxides occur in the degradation pathways for many unsaturated aliphatic compounds (5, 6, 15, 38), and the epoxide-convertingenzymes in organisms utilizing these compounds as growth substratesmay also exhibit activity with chlorinated epoxyethanes. Indeed,the presence of epoxide-transforming enzymes has been proposedas an explanation for the decreased toxicity of trichloroethenefor isoprene-utilizing bacteria (8).

Isoprene is emitted by bacteria, fungi, animals, and plants in large amounts (26). Rates of isoprene synthesis increaseunder thermal stress conditions (27), when isoprene may functionas a stabilizing agent for biological membranes (26). Treesmay emit about 2% of the carbon assimilated as isoprene. The globalemission of isoprene is estimated to be about 3 × 10¹⁴ g year¹, which is roughly equal to the global methane emission (4).Isoprene is a reactive compound compared to other atmospherichydrocarbons due to the presence of two unsaturated bonds, andit plays a role in ozone formation via a series of photochemicalreactions (28). However, despite its important role in atmosphericchemistry, little is known about the microbial degradation ofthis compound (9, 31).

In this paper we report the isolation and characterization of an isoprene-utilizing organism that dechlorinates cis-1,2-dichloroepoxyethane.Furthermore, we show that a glutathione (GSH) S-transferase isinvolved in epoxide metabolism in this organism.

	MATERIALS AND METHODS

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Growth conditions. In all batch experiments MMY medium was used (30). Stock solutions of carbon sources were sterilized with a 0.2-µm-pore-sizefilter. The organic solvents that were tested as carbon sourceswere found to be sterile. Batch cultures were grown at 30°C in100-ml or 1- or 3-liter serum flasks filled to one-fourth theirvolume with medium, and the flasks were incubated with rotaryshaking (200 rpm). Growth was monitored by measuring the turbidityat 450 nm with a Hitachi model 100-60 spectrophotometer.

Batch enrichments were carried out at 30°C as described previously (30). Pure cultures were obtained by repeated streakingonto MMY agar plates that were incubated in a desiccator withisoprene in the gas phase. The organisms were maintained on 0.8%nutrient broth agar plates.

In continuous culture, the organisms were grown at a dilution rate of 0.026 h¹ in MMY medium to which extra (NH₄)SO₄ (0.5 g liter¹), MgSO₄ (0.2 g liter¹), and yeast extract (20 mg liter¹) were added. All components except phosphate buffer were sterilizedseparately to prevent the formation of precipitates. Cells weregrown in a continuous culture at a dilution rate of 0.026 h¹. The pH was regulated continuously by titration with 1 N NaOH.The growth substrate was added by bubbling air (flow rate, 4.1ml min¹) through a flask containing isoprene kept on ice. Other conditionswere as follows: working volume, 2.35 liters; temperature, 30°C;impeller speed, 1,175 rpm; and airflow rate, 29.2 ml min¹. This resulted in a steady state in which the cell density was2.1 mg ml¹, the growth yield was 0.54 g of cells g of isoprene¹, and the dissolved oxygen concentration was 7 to 10% of air saturation.

Identification of strain AD45. Taxonomic identification was carried out by workers at the LMG Culture Collection (University of Ghent, Ghent, Belgium), whoused fatty acid analysis and a metabolic fingerprint.

For analysis of the 16S rRNA gene, genomic DNA was isolated from a 2-ml overnight culture grown on nutrient broth. Ampicillin200 (µg ml¹) and lysozyme 100 (µg ml¹) were added, and the culture was incubated for 2 h at 30°C. Aftercentrifugation (10,000 × g, 10 min), 5 µl of 1 M Tris-chloride(pH 8.4), 1 µl of 0.5 M EDTA (pH 8.0), and 5 µl of 5 M NaCl wereadded. Lysozyme was added to a final concentration of 2 mg ml¹, and the cells were incubated at 37°C for 2 h. The cells werelysed by adding 80 µl of 10% sodium dodecyl sulfate, followedby overnight incubation at 65°C. After 60 µl of 3 M sodium acetate(pH 7.0) was added, the lysate was incubated at 65°C. After 60µl of 3 M sodium acetate (pH 7.0) was added, the lysate was incubatedat 65°C for another 2 h. The DNA was purified and isolated bystandard phenol-chloroform extraction and ethanol precipitationmethods (25). The 16S rRNA gene was analyzed by PCR amplificationof a ca. 1,320-bp fragment of the 16S rRNA gene. Amplification,sequencing, and sequence analysis were carried out as describedby Marchesi and coworkers (19) by using the data bank and analysistools of the Ribosomal Database Project (18).

Degradation experiments with cell suspensions. Experiments to examine degradation of all compounds except cis-1,2-dichloroepoxyethane were carried out with cells grown inbatch cultures on 2 mM isoprene. Cells were centrifuged and resuspendedto a density of 0.2 mg ml¹. Substrate was added, and degradation was monitored as describedpreviously (30). The kinetics of degradation of isoprene andcis-1,2-DCE were determined by headspace analysis. In the caseof cis-1,2-DCE, 1 mM sodium succinate was added as a reductant.Substrate depletion was monitored by analyzing seven headspacesamples over a period of 15 min. The kinetic parameters were estimatedby transforming the data by the method of Hanes Woolf as describedby Oldenhuis et al. (23).

For cis-1,2-dichloroepoxyethane degradation experiments, strain AD45 cells grown in continuous culture were centrifuged (10,000× g, 10 min) and resuspended to a density of 40 mg ml¹ in MMY medium. Inactivation with 1,2-epoxyhexane was carriedout by incubating cells with 1 mM 1,2-epoxyhexane for 15 min at30°C. The cells were washed twice with MMY medium to remove excess1,2-epoxyhexane. Activities were measured by monitoring substrateconcentrations by on-line gas chromatography essentially as describedby Van Hylckama Vlieg et al. (32), with some minor modifications.A 38-ml incubation vessel which contained 7 ml of a vigorouslystirred cell suspension was used. Gas was continuously withdrawnfrom the headspace, and after passage through a 35-µl sample loopit was reinjected into the headspace, since reinjection in thewater phase resulted in excessive foam formation at the high celldensities that were used. At 1-min time intervals, the contentsof the sample loop were injected into the gas chromatograph andanalyzed isothermally at 90°C. Assays were started by adding cis-1,2-dichloroepoxyethanefrom a 50 mM stock solution in 10 mM sodium phosphate buffer (pH7.0). Gas chromatography-mass spectrometry was performed as describedby Van Hylckama Vlieg et al. (32). To determine chloride levels,parallel incubations were carried out, from which 300-µl sampleswere removed at different times. The samples were rapidly chilledon ice and centrifuged (15,000 × g, 1 min) to remove the cells.Each supernatant (200 µl) was lyophilized to remove excess cis-1,2-dichloroepoxyethane.Water (200 µl) was added, and chloride levels were determinedby the method of Bergmann and Sanik (3a).

Preparation of cell extracts and enzyme assays. The cells used to prepare cell extracts were harvested from late-exponential-phase batch cultures or from continuous cultures.After centrifugation (15 min, 10,000 × g), the cells were resuspendedin 50 mM Tris-HCl buffer (pH 7.5) (Tris buffer). All subsequentsteps were carried out at 0 to 4°C. The cells were washed twicewith Tris buffer before they were resuspended in 3 volumes of10 mM Tris buffer containing 1 mM $beta$ -mercaptoethanol and 1 mM EDTA(TEM buffer). The cells were disrupted by sonication (4 ml, 250-Woutput) 10 times for 10 s with 1-min intervals to cool the suspensionon ice. A cell extract was obtained by centrifugation (60 min,40,000 × g).

GSH S-transferase activities were assayed at 30°C in 50 mM Tris-Cl buffer (pH 8.5) (assay buffer) containing substrate ata concentration of 5 mM (all substrates except cis- and trans-1,2-dichloroepoxyethanes)or 1 mM (cis- and trans-1,2-dichloroepoxyethanes) and 5 mM ofglutathione (GSH), which was added from a 0.5 M stock solutionin assay buffer. Substrate depletion was monitored by on-linegas chromatography. A dimensionless Henry coefficient for cis-1,2-dichloroepoxyethaneof 0.011 was used to calculate activities (32). The followingdimensionless Henry coefficients for the other epoxides were determinedas described previously (32): epoxypropane, 0.007; 1,2-epoxyhexane,0.02; and 3,4-epoxy-3-methyl-1-butene, 0.02. Chloride liberationin assays performed with cis-1,2-dichloroepoxyethane was monitoredby removing 300-µl samples from parallel incubation mixtures asdescribed above. Samples were quenched with 1% H₂O₂ to avoid nonenzymaticreaction of GSH with cis-1,2-dichloroepoxyethane. Activities wereexpressed in units per milligram of protein. One unit was definedas the activity that catalyzed the conversion of 1 µmol of substrateper min.

Detection of GSH-epoxide conjugates in deproteinized cell extracts. An isoprene-grown cell suspension (18 mg ml¹) harvested from a continuous culture was divided into two equal portions. Oneportion was incubated with 1 mM 1,2-epoxyhexane at room temperaturefor 15 min, and the other was used as a control. All subsequentsteps were carried out at 0 to 4°C. The cells were centrifugedand washed twice before they were resuspended in 6 ml of 10 mMpotassium phosphate buffer (pH 7.0). Lysozyme and EDTA were addedto final concentrations of 0.17 mg ml¹ and 1 mM, respectively, and after 1 h the cells were disruptedby sonication. Deproteination of cell extracts was carried outessentially as described by Fahey et al. (10). The extractswere lyophilized and resuspended in 200 ml of water. Proteinswere precipitated by adding HCl to a final concentration of 0.1N, and after vortexing the precipitates were removed by centrifugationat 15,000 × g for 10 min. The supernatants were mixed with anequal volume of 4 M sodium methanesulfonate, and the mixtureswere frozen in liquid nitrogen. After warming, the insoluble portionswere removed by centrifugation at 15,000 × g.

The GSH-epoxyhexane conjugate that was used as a reference was synthesized with partially purified enzyme in a standard enzymeassay by using 5 mM 1,2-epoxyhexane and 10 mM GSH. After 90% ofthe 1,2-epoxyhexane was converted, the sample was lyophilizedto remove the remaining epoxide.

The GSH-epoxide conjugates present in the supernatants were analyzed by reversed-phase high-performance liquid chromatography(HPLC) with a Merck Hitachi model L-6200A system equipped witha Lichrosorb 5C18 column (20 by 4.6 mm) and a Merck Hitachi modelL4000 UV detector. For data acquisition a Merck Hitachi modelD-2500 Chromato-Integrator was used. The buffer system consistedof 0.1% trifluoroacetic acid in water (buffer A) and 0.1% trifluoroaceticacid in acetonitrile (buffer B). The following elution protocolwas used: 0 to 5 min, 0% isocratic buffer B; 5 to 75 min, 0 to67% buffer B linear gradient; 75 to 80 min, 67 to 100% bufferB linear gradient (column regeneration). The elution profile wasobtained by measuring the absorbance at 214 nm.

Chemicals. Both cis-1,2-dichloroepoxyethane and trans-1,2-dichloroepoxyethane were synthesized with M. trichosporium OB3b as describedpreviously (32). The concentrations in the stock solutions thatwere obtained were determined by overnight hydrolysis in 50 mMKOH at 80°C and subsequent determination of chloride levels. Otherchemicals were obtained from AGA Gas B.V. (Amsterdam, The Netherlands),Acros Organics ('s-Hertogenbosch, The Netherlands), or Aldrich(Milwaukee, Wis.).

	RESULTS

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Degradation of halogenated ethenes by isoprene-utilizing cultures. Four different pure cultures capable of growing with isoprene as the sole source of carbon and energy were isolated from freshwatersediment. The doubling times in liquid media containing isopreneas a growth substrate ranged from 3.5 to 16 h. All strains weregram positive and nonfermentative and differed in colony morphologyand color during growth on nutrient broth agar plates. Suspensionsof washed cells (0.2 mg ml¹) prepared from batch cultures grown on isoprene were tested forthe ability to degrade TCE and trans-1,2-DCE. The culture withthe highest growth rate on isoprene, designated strain AD45, showedthe highest activity with chlorinated ethenes, as judged by gaschromatography and the amount of chloride released.

We also tested whether enrichment with other compounds having isoprene-like structures would result in the isolation of newcultures that are capable of cometabolic degradation of chlorinatedethenes. Four mixed cultures were isolated with 3-methyl-3-butene-1-ol,2-methyl-3-butene-2-ol, 2-methyl-2-butene, and 2-methyl-2-penteneand were grown for 10 days on one of these substrates in the presenceof 200 µM TCE or 200 µM trans-1,2-DCE. None of the cultures degradedTCE or trans-1,2-DCE, and no chloride release was detected.

All subsequent experiments were carried with strain AD45, since this culture showed the highest activity with halogenatedethenes. Strain AD45 was tentatively identified as a Rhodococcussp. based on fatty acid analysis and a metabolic fingerprint.Analysis of the 16S rRNA gene sequence revealed that the closestorganisms as determined by similarity rank (S_ab, 0.850 to 0.942)were all Rhodococcus spp., and the highest score was obtainedwith Rhodococcus globerulus (18).

In batch cultures strain AD45 grew on isoprene, 3,4-epoxy-3-methyl-1-butene, phenol, 3-methyl-3-butene-1-ol, 3-methyl-1-butanol,glycerol, 1,2-propanediol, ethanol, and glucose. This organismdid not grow on 2,3-dimethyl-2-butene, 3,3-dimethyl-1-butene,2-methyl-2-pentene, 2-methyl-2-butene, benzene, toluene, 3-methyl-2-butene-1-ol,2-methyl-3-butene-1-ol, 1-pentene, 1-hexene, epoxypropane, 1,2-epoxybutane,glycolate, glyoxylate, citrate, allylalcohol, or methanol.

Identification of the primary oxidation products of isoprene, cis-1,2-DCE, and trans-1,2-DCE. A concentrated cell suspension (7.5 mg ml¹) harvested from a continuous culture was used to identify the primary oxidationproduct of isoprene. When a pulse of isoprene was added, whichresulted in a concentration of isoprene in the liquid phase of3 mM, accumulation of a product was observed. The retention timeof this product during gas chromatography was identical to theretention time of 3,4-epoxy-3-methyl-1-butene. This compound waswell separated from 3,4-epoxy-2-methyl-1-butene, which is theother epoxide that can be generated by the oxidation of isoprene.A mass spectrometry analysis of the primary oxidation productand commercially available 3,4-epoxy-3-methyl-1-butene revealedthe presence of ions with m/z (relative intensity of the primaryoxidation product, relative intensity of standard 3,4-epoxy-3-methyl-1-butene)39 (100, 100), 55 (74, 74), 29 (68, 41), 43 (63, 74), 53 (50,56), 41 (44, 29), 27 (40, 36), 56 (31, 17), 83 (23, 23), 54 (22,30), 69 (22, 22), 50 (18, 18), 51 (15, 18), 26 (12, 9), 84 (molecularion) (6, 6), and 38 (5, 8). Thus, the compound was identifiedas 3,4-epoxy-3-methyl-1-butene.

In analogous experiments with cis-1,2-DCE and trans-1,2-DCE products accumulated that were identified as the correspondingepoxides as described previously (32).

Kinetics of biodegradation. The kinetics of degradation of isoprene and cis-1,2-DCE by cell suspensions of Rhodococcus sp. strain AD45 were determined.The K_m for isoprene conversion was 0.8 µM, and the V_max was 76nmol min¹ mg of cells¹. The K_m for cis-1,2-DCE was 63 µM, and the V_max was 8 nmol min¹ mg of cells¹.

The cells also degraded toluene, styrene, and propylene. The rate of toluene oxidation was 10 nmol min¹ mg of cells¹ at a concentration of 73 µM in the medium. Propylene was convertedto epoxypropane. Degradation of toluene and cis-1,2-DCE was inhibitedby isoprene, indicating that these compounds compete for the sameactive site.

Conversion of cis-1,2-dichloroepoxyethane by cell suspensions. Cell suspensions harvested from a continuous culture were used to test whether Rhodococcus sp. strain AD45 can degrade cis-1,2-dichloroepoxyethane.All organic chlorine was liberated as chloride during degradationof cis-DCE epoxide (Fig. 1). The following two different stagesof epoxide degradation were distinguished: a first stage (fromzero time to 2 min), during which approximately 0.3 to 0.32 mMepoxide was rapidly degraded; and a second stage (after 2 min),during which degradation proceeded at a lower rate, 0.12 nmolmin¹ mg of cells¹.

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FIG. 1. Conversion of cis-1,2-dichloroepoxyethane by cell suspensions of Rhodococcus sp. strain AD45 (40 mg [dry weight] ml¹). The depletion of cis-1,2-DCE (solid symbols) and the generation of chloride (open symbols) were monitored with time. Incubations were carried out with active cells (circles), 1,2-epoxyhexane-inactivated cells (squares), and heat-killed cells (triangles).

No degradation of cis-1,2-dichloroepoxyethane was observed with heat-killed cells. Cells that were treated with 1,2-epoxyhexanealmost completely lost cis-1,2-dichloroepoxyethane-degrading activity.

Epoxide-degrading activity in cell extracts. We prepared cell extracts to determine which type of enzymes was involved in epoxide conversion. A GSH-dependent specificactivity of 5.4 U mg of protein¹ towards 3,4-epoxy-3-methyl-1-butene was observed in extractsof isoprene-grown cultures. GSH could not be replaced by otherthiols, such as cysteine, lipoic acid, or coenzyme A. No activitywas detected in assays for epoxide dehydrogenase (6), epoxideisomerase (15), or epoxide hydrolase (24). In the presenceof GSH, other epoxides were also converted by the cell extracts.The specific activities were 2.5 U mg¹ with epoxypropane, 0.3 U mg¹ with cis-1,2-dichloroepoxyethane, and 0.5 U mg¹ with trans-1,2-dichloroepoxyethane.

The GSH-dependent activities in cell extracts of cultures grown on other carbon sources were also determined. A specific activityof 2.1 U mg¹ with 3,4-epoxy-3-methyl-1-butene was detected in an extract ofa culture grown on 3,4-epoxy-3-methyl-1-butene. In an extractof glucose-grown cells the activities were 0.1 U mg¹ with 3,4-epoxy-3-methyl-1-butene, 0.1 U mg¹ with epoxypropane, and less than 0.05 U mg¹ with cis-1,2-dichloroepoxyethane. With ethanol-grown cells thespecific activities were 0.3 U mg¹ with 3,4-epoxy-3-methyl-1-butene, 0.2 U mg¹ with epoxypropane, and less than 0.05 U mg¹ with cis-1,2-dichloroepoxyethane. No activity was detected withextracts from cells grown on 3-methyl-3-butene-1-ol or 2-methyl-butanol.The results indicated that an inducible GSH S-transferase is involvedin epoxide conversion.

A sample of partially purified enzyme (33a) was used to study the conversion of cis-1,2-dichloroepoxyethane. All organicchlorine was released as chloride. This activity was absent withheat-killed enzyme (Fig. 2).

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FIG. 2. Conversion of cis-1,2-dichloroepoxyethane by partially purified GSH S-transferase from Rhodococcus sp. strain AD45. Depletion of cis-1,2-DCE (solid symbols) and generation of chloride (open symbols) were determined in incubations with active enzyme (0.08 mg ml¹) (circles) or heat-inactivated enzyme (squares).

Accumulation of GSH-1,2-epoxyhexane conjugate in 1,2-epoxyhexane-inactivated cells. Epoxide degradation by cell extracts of Rhodococcus sp. strain AD45 was dependent on the addition of GSH. However, we couldnot exclude the possibility that in vivo another thiol may actas a cofactor, as has been observed with other epoxide-degradingorganisms. For instance, GSH was not the physiological cofactorin the metabolism of epoxypropane by Xanthobacter sp. strain Py2despite that fact that after GSH was added, activity could bedetected (39). We also observed that addition of low concentrationsof 1,2-epoxybutane and 1,2-epoxyhexane strongly inhibited growthon isoprene but not growth on ethanol (Fig. 3) and irreversiblyinhibited the epoxide-degrading activity of cell suspensions (Fig.1). Since the epoxide-transforming GSH-dependent enzyme exhibitedactivity with various epoxides, the inhibition observed may havebeen caused by the accumulation of nonmetabolizable conjugatesof thiol and 1,2-epoxyhexane. Therefore, we analyzed cell extractsprepared from 1,2-epoxyhexane-inactivated cells for the presenceof such conjugates. In HPLC traces obtained with deproteinizedextracts of inactivated cells, a compound eluting at 26 min wasdetected which was absent in traces of extracts of active cells(Fig. 4). The retention time of this compound was identical tothat of the GSH-1,2-epoxyhexane conjugate that was synthesizedwith partially purified GSH S-transferase. Analysis by HPLC-massspectrometry showed that the two peaks represented a compoundwith a molecular mass (m/z) of 408, which is consistent with thetheoretical value for the protonated molecular ion. Analysis ofthe sample prepared with partially purified enzyme also revealedthe presence of a compound eluting at 13 min with m/z 613, whichis in agreement with the theoretical value for the protonatedmolecular ion oxidized GSH (GSSG). This compound may be generatedby autooxidation from excess GSH during sample preparation (1).From Fig. 4, traces A and C, we calculated that approximately3 nmol of GSH was present per mg (dry weight) of cells, assumingthat all intracellular GSH was converted to the conjugate.

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FIG. 3. Toxicity of 1,2-epoxybutane and 1,2-epoxyhexane for Rhodococcus sp. strain AD45 growing on 0.9 mM isoprene (A) or 4 mM ethanol (B). Symbols: $bullet$ , no epoxide added; $black-triangle$ , 0.1 mM 1,2-epoxybutane added;

, 0.1 mM 1,2-epoxyhexane added; $open circle$ , no growth substrate. OD450, optical density at 450 nm.

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FIG. 4. Formation of the conjugate of GSH and 1,2-epoxyhexane in cell suspensions of strain AD45. (A and B) HPLC profiles recorded by measuring the absorbance at 214 nm of a deproteinized cell extract prepared from a cell suspension that was inactivated with 1,2-epoxyhexane (A) or from a suspension that was not inactivated (B). (C) Control (GSH-1,2-epoxyhexane conjugate synthesized with partially purified GSH S-transferase). The m/z values (408 and 613 Da) are in agreement with the theoretical values for the protonated molecular ions of the conjugate of GSH and 1,2-epoxyhexane and for oxidized GSH (GSSG), respectively.

	DISCUSSION

Top Abstract Introduction Materials & Methods Results Discussion References

We isolated a Rhodococcus sp. that utilizes the important environmental hydrocarbon isoprene as a sole source of carbon andenergy. Previously, Van Ginkel et al. (30) reported the isolationof several isoprene-utilizing strains that were tentatively identifiedas Nocardia sp. strains. Suspensions of these organisms that wereinactivated with 1,2-epoxybutane accumulated both 3,4-epoxy-3-methyl-1-buteneand the diepoxide (1,2-3,4-diepoxy-butane). However, Rhodococcussp. strain AD45 accumulated mainly 3,4-epoxy-3-methyl-1-butene,indicating that these strains have different metabolic features.

The results show that in strain AD45 isoprene degradation starts with the oxidation of the sterically most hindered doublebond, resulting in the formation of 3,4-epoxy-3-methyl-1-butene.The metabolism of isoprene in strain AD45 is similar to the metabolismof isoprene in mammals. In liver microsomes of various rodentspecies, for instance, the methyl-substituted double bond ratherthan the unsubstituted bond is oxidized by cytochrome P-450 (13).

An inducible GSH-dependent activity towards 3,4-epoxy-3-methyl-1-butene was detected in cell extracts of Rhodococcus sp. strainAD45, suggesting that a GSH S-transferase is involved in the metabolismof isoprene. This activity was also detected with cis- and trans-1,2-dichloroepoxyethanesand epoxypropane. The accumulation of a GSH-epoxyhexane conjugatein cells poisoned with 1,2-epoxyhexane indicates that GSH is thephysiological cofactor for the epoxide-transforming enzyme. Thelevel of conjugate accumulation corresponds to a GSH concentrationof approximately 3 nmol mg (dry weight) of cells¹ or a concentration of 2 mM in the cytoplasm. This concentrationis very high for nocardioform actinomycetes, whereas similar valueshave been reported for Streptococcus, Enterococcus, and variousgram-negative species (21). Previously, Ewers and Knackmuss(9) described a GSH-dependent activity towards 3,4-epoxy-3-methyl-1-butenein cell extracts of an isoprene-utilizing Rhodococcus sp., butthe enzyme responsible for this activity has not been furthercharacterized.

The monooxygenase involved in isoprene metabolism in strain AD45 also exhibits activity with chlorinated ethenes and toluene.Oxidation of cis-1,2-DCE and trans-1,2-DCE resulted in the formationof the corresponding epoxides, as has been found with other organismsthat express monooxygenases (3, 7, 12, 20, 23, 36,37). These epoxides were also converted by cell suspensionsof strain AD45, but the transformation rates for cis-1,2-dichloroepoxyethanewere approximately 70-fold lower than the transformation ratesfor cis-1,2-DCE. Both 1,2-dichloroepoxyethanes are substratesfor the GSH S-transferase. Reaction of cis-1,2-dichloroepoxyethanewith GSH resulted in complete liberation of organic chlorine aschloride, indicating that no toxic halogenated metabolites weregenerated. This suggests that there is a pathway in which, afternucleophilic attack of GSH, an unstable product is formed thatnonbiologically decomposes to glyoxal (Fig. 5). Analysis of glyoxalby osazone formation with 2,4-dinitrophenylhydrazine failed dueto the presence of GSH. HPLC analysis also did not reveal thegeneration of a stable GSH conjugate. The dechlorination in reactionstep 4 (Fig. 5) is analogous to the dechlorination by nonenzymichydrolysis of S-chloromethyl GSH. The latter compound is the productof nucleophilic displacement with dichloromethane, a reactionthat is catalyzed by dichloromethane dehalogenases (17). Inaqueous solution, 2-oxoaldehydes occur in nonhydrated, monohydrated,and even dihydrated forms (29). Nonhydrated 2-oxoaldehydes rapidlyreact with GSH to form a hemithioacetal. The best-studied compoundin this respect is methylglyoxal, which is generated in vivo fromglyceraldehyde 3-phosphate and dihydroxyacetone phosphate by phosphateelimination. Under physiological conditions in erythrocytes, forinstance, only 0.04% of the methylglyoxal exists as the 2-oxoaldehydeand 41% exists as the hemithioacetal, whereas the rest is presentin hydrated form. The two-stage degradation of cis-1,2-dichloroepoxyethane(Fig. 1) may be caused by decreased free GSH concentrations dueto accumulation of the hemithioacetal of glyoxal.

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FIG. 5. Proposed pathway for the degradation of cis-1,2-DCE in Rhodococcus sp. strain AD45. Reactions 3 to 5 are nonbiological reactions postulated on the basis of the observation that all organic chlorine was liberated as chloride during degradation of cis-1,2-dichloroepoxyethane and on the basis of previously published data. The dechlorination in reaction 4 is analogous to the nonbiological dechlorination of S-chloromethyl GSH during dichloromethane degradation (17). In aqueous solutions, 2-oxoaldehydes, such as glyoxal, also occur in hydrated form. Nonhydrated glyoxal is chemically in equilibrium with GSH (29).

Bacterial conversion of epoxides is a topic that has drawn interest from people working on biocatalysis and biodegradationof organic compounds. A wide range of enzymes are involved inmicrobial metabolism of epoxides; these enzymes include epoxideisomerases, carboxylases, dehydrogenases, hydrolases, reductases,and lyases (5, 6, 15, 24, 38, 39). However, activitywith chloroepoxyethanes has not been reported for any of theseenzymes.

Apart from the GSH-dependent activity described here, the only bacterial activity with 1,2-dichloroepoxyethane that has beenreported is the activity of M. trichosporium OB3b. The solublemethane monooxygenase of this organism has activity with cis-1,2-dichloroepoxyethanebut not with trans-1,2-dichloroepoxyethane. However, this activityresults in extreme toxicity since monooxygenase activity and theviability of cells were significantly inhibited (31, 32).

Data on bacterial GSH S-transferases have been reviewed recently (35). Some of these enzymes are associated with the metabolismof aromatic compounds. Other GSH S-transferases are involved inthe reductive cleavage of ether bonds in lignin or in reductiveor hydrolytic dehalogenation reactions. An enzyme homologous toextradiol dioxygenases catalyzing ring opening in epoxides byGSH is involved in resistance to the antibiotic fosfomycin. Divalentcations are needed for optimal activity of this enzyme (2),unlike the enzyme of strain AD45. Thus, in view of its substraterange, the GSH S-transferase of strain AD45 may be a novel typeof GSH S-transferase. The biochemistry and genetics of isoprenedegradation are currently being studied.

	ACKNOWLEDGMENTS

The work of J.E.T.v.H.V. was financed by grant IOP91204 from the Dutch IOP Environmental Biotechnology Program.

Julian R. Marchesi (School of Pure and Applied Biology, University of Wales, Cardiff, United Kingdom) is acknowledged forperforming the 16S rRNA gene sequence analysis, and Piet Wietzesis acknowledged for technical support. C. Margot Jeronimus-Stratinghand Andries P. Bruins (Department of Pharmacy, University of Groningen,Groningen, The Netherlands) are acknowledged for performing themass spectrometry analysis.

	FOOTNOTES

^* Corresponding author. Mailing address: Department of Biochemistry, Groningen Biomolecular Sciences and Biotechnology Institute,University of Groningen, Nijenborgh 4, 9747 AG Groningen, TheNetherlands. Phone: 31-50-3634209. Fax: 31-50-3634165. E-mail:d.b.janssen{at}chem.rug.nl.

Present address: TNO Industrial Microbiology, 3700 AJ Zeist, The Netherlands.

REFERENCES

Top
Abstract
Introduction
Materials & Methods
Results
Discussion
References

1. Akerboom, T. P. M., and H. Sies. 1981. Assay for glutathione, glutathione disulfide, and glutathione mixed disulfides in biological samples. Methods Enzymol. 77:373-382[Medline].

2. Arca, P., C. Hardisson, and J. E. Suarez. 1990. Purification of a glutathione S-transferase that mediates fosfomycin resistance in bacteria. Antimicrob. Agents Chemother. 34:844-848[Abstract/Free Full Text].

3. Arciero, D., T. Vanelli, T. M. Logan, and A. B. Hooper. 1989. Degradation of trichloroethylene by the ammonia oxidizing bacterium Nitrosomonas europaea. Biochem. Biophys. Res. Commun. 159:640-643[Medline].

3a. Bergmann, J. G., and J. Saniko. 1957. Determination of trace amounts of chloride in naphtha. Anal. Chem. 29:241-243.

4. Brasseur, G. P., and R. B. Chatfield. 1991. The fate of biogenic trace gasses in the atmosphere, p. 1-27. In T. D. Sharkey, E. A. Holland, and H. A. Mooney (ed.), Trace gas emission from plants. Academic Press, San Diego, Calif.

5. Chion, C. K., and D. J. Leak. 1996. Purification and characterization of two components of an epoxypropane isomerase/carboxylase of Xanthobacter Py2. Biochem. J. 319:299-406.

6. De Bont, J. A. M., and W. Harder. 1980. Metabolism of ethylene by Mycobacterium E20. FEMS Microbiol. Lett. 3:89-93.

7. Ensign, S. A., M. R. Hyman, and D. A. Arp. 1992. Cometabolic degradation of chlorinated alkanes by alkene monooxygenase in a propylene-grown Xanthobacter strain. Appl. Environ. Microbiol. 58:3038-3046[Abstract/Free Full Text].

8. Ewers, J. W. C., D. Freier-Schröder, and H. J. Knackmuss. 1990. Selection of trichloroethylene (TCE) degrading bacteria that resist inactivation by TCE. Arch. Microbiol. 154:410-413[Medline].

9. Ewers, J. W. C., and H.-J. Knackmuss. 1991. Biodegradation of chloroethenes using isoprene as a co-substrate, p. 77-83. In H. Verachtert, and W. Verstraete (ed.), Proceedings of the International Symposium on Environmental Biotechnology Oostende. Royal Flemish Society of Engineers, Oostende, Belgium.

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11. Fitch, M. W., D. Weisman, P. Phelps, G. Georgiou, and G. E. Speitel, Jr. 1996. Trichloroethylene degradation by Methylosinus trichosporium OB3b mutants in a sequencing biofilm reactor. Water Res. 11:2655-2664.

12. Fox, B. G., J. G. Borneman, L. P. Wackett, and J. D. Lipscomb. 1990. Haloalkene oxidation by the soluble methane monooxygenase from Methylosinus trichosporium OB3b: mechanistic and environmental implications. Biochemistry 29:6419-6427[Medline].

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16. Janssen, D. B., G. Grobben, R. Hoekstra, R. Oldenhuis, and B. Witholt. 1988. Degradation of trans-1,2-dichloroethene by mixed cultures of methanotrophic bacteria. Appl. Environ. Biotechnol. 29:392-399.

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19. Marchesi, J. R., T. Sago, A. J. Weightman, T. A. Martin, J. C. Fry, S. J. Hiom, and W. G. Wade. 1998. Design and evaluation of useful bacterium-specific primers that amplify genes coding for bacterial 16S rRNA. Appl. Environ. Microbiol. 64:795-799[Abstract/Free Full Text].

20. Nelson, M. J. K., S. O. Montgomery, W. R. Mahaffery, and P. H. Pritchard. 1987. Biodegradation of trichloroethylene and involvement of an aromatic pathway. Appl. Environ. Microbiol. 53:949-954[Abstract/Free Full Text].

21. Newton, G. L., K. Arnold, M. S. Price, C. Sherill, S. B. Delcadayre, Y. Aharonowitz, G. Cohen, J. Davies, R. Fahey, and C. Davis. 1995. Distribution of thiols in microorganisms: mycothiol is a major thiol in most actinomycetes. J. Bacteriol. 178:1990-1995[Abstract/Free Full Text].

22. Oldenhuis, R., and D. B. Janssen. 1993. Degradation of trichloroethylene by methanotrophic bacteria, p. 121-133. In J. C. Murrell, and D. P. Kelly (ed.), Microbial growth on C₁ compounds. Intercept Ltd., Andover, United Kingdom.

23. Oldenhuis, R., J. Y. Oedzes, J. J. van der Waarde, and D. B. Janssen. 1991. Kinetics of chlorinated hydrocarbon degradation by Methylosinus trichosporium OB3b and toxicity of trichloroethylene. Appl. Environ. Microbiol. 57:7-14[Abstract/Free Full Text].

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27. Sharkey, T. D., and E. L. Singsaas. 1995. Why plants emit isoprene. Nature 374:769.

28. Thompson, A. M. 1992. The oxidizing capacity of the earth's atmosphere; probable past and future changes. Science 256:1157-1165[Abstract/Free Full Text].

29. Thornally, P. J. 1990. The glyoxalase system: new developments towards functional characterization of a metabolic pathway fundamental to biological life. Biochem. J. 269:1-11[Medline].

30. Van den Wijngaard, A. J., J. Prins, A. J. A. C. Smal, and D. B. Janssen. 1993. Degradation of 2-chloroethylvinylether by Ancylobacter aquaticus AD25 and AD27. Appl. Environ. Microbiol. 59:2777-2783[Abstract/Free Full Text].

31. Van Ginkel, C. G., E. De Jong, J. W. R. Tilanus, and J. A. M. De Bont. 1987. Microbial oxidation of isoprene, a biogenic foliage volatile, and of 1,3-butadiene, an anthropogenic gas. FEMS Microbiol. Ecol. 45:275-279.

32. Van Hylckama Vlieg, J. E. T., W. de Koning, and D. B. Janssen. 1996. Transformation kinetics of chlorinated ethenes by Methylosinus trichosporium OB3b and detection of unstable epoxides by on-line gas chromatography. Appl. Environ. Microbiol. 62:3304-3312[Abstract].

33. Van Hylckama Vlieg, J. E. T., W. de Koning, and D. B. Janssen. 1997. Effect of chlorinated ethene conversion on viability and activity of Methylosinus trichosporium OB3b. Appl. Environ. Microbiol. 63:4961-4964[Abstract].

33a. Van Hylckama Vlieg, J. E. T., and D. B. Janssen. Unpublished data.

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37. Wackett, L. P., and D. T. Gibson. 1988. Degradation of trichloroethylene by toluene dioxygenase in whole-cell studies with Pseudomonas putida F1. Appl. Environ. Microbiol. 54:1703-1708[Abstract/Free Full Text].

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1.	Akerboom, T. P. M., and H. Sies. 1981. Assay for glutathione, glutathione disulfide, and glutathione mixed disulfides in biological samples. Methods Enzymol. 77:373-382[Medline].
2.	Arca, P., C. Hardisson, and J. E. Suarez. 1990. Purification of a glutathione S-transferase that mediates fosfomycin resistance in bacteria. Antimicrob. Agents Chemother. 34:844-848[Abstract/Free Full Text].
3.	Arciero, D., T. Vanelli, T. M. Logan, and A. B. Hooper. 1989. Degradation of trichloroethylene by the ammonia oxidizing bacterium Nitrosomonas europaea. Biochem. Biophys. Res. Commun. 159:640-643[Medline].
3a.	Bergmann, J. G., and J. Saniko. 1957. Determination of trace amounts of chloride in naphtha. Anal. Chem. 29:241-243.
4.	Brasseur, G. P., and R. B. Chatfield. 1991. The fate of biogenic trace gasses in the atmosphere, p. 1-27. In T. D. Sharkey, E. A. Holland, and H. A. Mooney (ed.), Trace gas emission from plants. Academic Press, San Diego, Calif.
5.	Chion, C. K., and D. J. Leak. 1996. Purification and characterization of two components of an epoxypropane isomerase/carboxylase of Xanthobacter Py2. Biochem. J. 319:299-406.
6.	De Bont, J. A. M., and W. Harder. 1980. Metabolism of ethylene by Mycobacterium E20. FEMS Microbiol. Lett. 3:89-93.
7.	Ensign, S. A., M. R. Hyman, and D. A. Arp. 1992. Cometabolic degradation of chlorinated alkanes by alkene monooxygenase in a propylene-grown Xanthobacter strain. Appl. Environ. Microbiol. 58:3038-3046[Abstract/Free Full Text].
8.	Ewers, J. W. C., D. Freier-Schröder, and H. J. Knackmuss. 1990. Selection of trichloroethylene (TCE) degrading bacteria that resist inactivation by TCE. Arch. Microbiol. 154:410-413[Medline].
9.	Ewers, J. W. C., and H.-J. Knackmuss. 1991. Biodegradation of chloroethenes using isoprene as a co-substrate, p. 77-83. In H. Verachtert, and W. Verstraete (ed.), Proceedings of the International Symposium on Environmental Biotechnology Oostende. Royal Flemish Society of Engineers, Oostende, Belgium.
10.	Fahey, R. C., G. L. Newton, R. Dorian, and E. M. Kosower. 1981. Analysis of biological thiols at the picomole level based upon derivatization with monobromobimames and separation by cation-exchange chromatography. Anal. Biochem. 111:357-365[Medline].
11.	Fitch, M. W., D. Weisman, P. Phelps, G. Georgiou, and G. E. Speitel, Jr. 1996. Trichloroethylene degradation by Methylosinus trichosporium OB3b mutants in a sequencing biofilm reactor. Water Res. 11:2655-2664.
12.	Fox, B. G., J. G. Borneman, L. P. Wackett, and J. D. Lipscomb. 1990. Haloalkene oxidation by the soluble methane monooxygenase from Methylosinus trichosporium OB3b: mechanistic and environmental implications. Biochemistry 29:6419-6427[Medline].
13.	Gervasi, P. G., and V. Longo. 1990. Metabolism and mutagenicity of isoprene. Environ. Health Perspect. 86:85-87[Medline].
14.	Hartmans, S., and J. A. M. de Bont. 1992. Aerobic vinyl chloride metabolism in Mycobacterium L1. Appl. Environ. Microbiol. 58:1220-1226[Abstract/Free Full Text].
15.	Hartmans, S., J. P. Smits, M. J. van der Werf, F. Volkering, and J. A. M. De Bont. 1989. Metabolism of styrene oxide and 2-phenylethanol in the styrene-degrading Xanthobacter 124X. Appl. Environ. Microbiol. 55:2850-2855[Abstract/Free Full Text].
16.	Janssen, D. B., G. Grobben, R. Hoekstra, R. Oldenhuis, and B. Witholt. 1988. Degradation of trans-1,2-dichloroethene by mixed cultures of methanotrophic bacteria. Appl. Environ. Biotechnol. 29:392-399.
17.	Leisinger, T., R. Bader, R. Hermann, M. Schmid-Appert, and S. Vuilleumier. 1994. Microbes, enzymes and genes involved in dichloromethane utilization. Biodegradation 5:237-248[Medline].
18.	Maidak, B. L., G. J. Olsen, N. Larsen, R. Overbeek, M. J. McCaughey, and C. R. Woese. 1997. The RDP (Ribosomal Database Project). Nucleic Acids Res. 25:109-110[Abstract/Free Full Text].
19.	Marchesi, J. R., T. Sago, A. J. Weightman, T. A. Martin, J. C. Fry, S. J. Hiom, and W. G. Wade. 1998. Design and evaluation of useful bacterium-specific primers that amplify genes coding for bacterial 16S rRNA. Appl. Environ. Microbiol. 64:795-799[Abstract/Free Full Text].
20.	Nelson, M. J. K., S. O. Montgomery, W. R. Mahaffery, and P. H. Pritchard. 1987. Biodegradation of trichloroethylene and involvement of an aromatic pathway. Appl. Environ. Microbiol. 53:949-954[Abstract/Free Full Text].
21.	Newton, G. L., K. Arnold, M. S. Price, C. Sherill, S. B. Delcadayre, Y. Aharonowitz, G. Cohen, J. Davies, R. Fahey, and C. Davis. 1995. Distribution of thiols in microorganisms: mycothiol is a major thiol in most actinomycetes. J. Bacteriol. 178:1990-1995[Abstract/Free Full Text].
22.	Oldenhuis, R., and D. B. Janssen. 1993. Degradation of trichloroethylene by methanotrophic bacteria, p. 121-133. In J. C. Murrell, and D. P. Kelly (ed.), Microbial growth on C₁ compounds. Intercept Ltd., Andover, United Kingdom.
23.	Oldenhuis, R., J. Y. Oedzes, J. J. van der Waarde, and D. B. Janssen. 1991. Kinetics of chlorinated hydrocarbon degradation by Methylosinus trichosporium OB3b and toxicity of trichloroethylene. Appl. Environ. Microbiol. 57:7-14[Abstract/Free Full Text].
24.	Rink, R., M. Fennema, M. Smids, U. Dehmel, and D. B. Janssen. 1997. Primary structure and catalytic mechanism of the epoxide hydrolase from Agrobacterium radiobacter AD1. J. Biol. Chem. 272:14650-14657[Abstract/Free Full Text].
25.	Sambrook, J., E. F. Fritsch, and T. Maniatis. 1989. Molecular cloning: a laboratory manual, 2nd ed. Cold Spring Harbor Laboratory, Cold Spring Harbor, N.Y.
26.	Sharkey, T. D. 1996. Isoprene synthesis by plants and animals. Endeavour (Cambridge) 20:74-78.
27.	Sharkey, T. D., and E. L. Singsaas. 1995. Why plants emit isoprene. Nature 374:769.
28.	Thompson, A. M. 1992. The oxidizing capacity of the earth's atmosphere; probable past and future changes. Science 256:1157-1165[Abstract/Free Full Text].
29.	Thornally, P. J. 1990. The glyoxalase system: new developments towards functional characterization of a metabolic pathway fundamental to biological life. Biochem. J. 269:1-11[Medline].
30.	Van den Wijngaard, A. J., J. Prins, A. J. A. C. Smal, and D. B. Janssen. 1993. Degradation of 2-chloroethylvinylether by Ancylobacter aquaticus AD25 and AD27. Appl. Environ. Microbiol. 59:2777-2783[Abstract/Free Full Text].
31.	Van Ginkel, C. G., E. De Jong, J. W. R. Tilanus, and J. A. M. De Bont. 1987. Microbial oxidation of isoprene, a biogenic foliage volatile, and of 1,3-butadiene, an anthropogenic gas. FEMS Microbiol. Ecol. 45:275-279.
32.	Van Hylckama Vlieg, J. E. T., W. de Koning, and D. B. Janssen. 1996. Transformation kinetics of chlorinated ethenes by Methylosinus trichosporium OB3b and detection of unstable epoxides by on-line gas chromatography. Appl. Environ. Microbiol. 62:3304-3312[Abstract].
33.	Van Hylckama Vlieg, J. E. T., W. de Koning, and D. B. Janssen. 1997. Effect of chlorinated ethene conversion on viability and activity of Methylosinus trichosporium OB3b. Appl. Environ. Microbiol. 63:4961-4964[Abstract].
33a.	Van Hylckama Vlieg, J. E. T., and D. B. Janssen. Unpublished data.
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