Succinyl-CoA:(R)-Benzylsuccinate CoA-Transferase: an Enzyme of the Anaerobic Toluene Catabolic Pathway in Denitrifying Bacteria

doi:10.1128/JB.183.14.4288-4295.2001

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Journal of Bacteriology, July 2001, p. 4288-4295, Vol. 183, No. 14
0021-9193/01/$04.00+0 DOI: 10.1128/JB.183.14.4288-4295.2001
Copyright © 2001, American Society for Microbiology. All rights reserved.

Succinyl-CoA:(R)-Benzylsuccinate CoA-Transferase: an Enzyme of the Anaerobic Toluene Catabolic Pathway in Denitrifying Bacteria

Christina Leutwein and Johann Heider^*

Mikrobiologie, Institut für Biologie II, Universität Freiburg, 79104 Freiburg, Germany

Received 18 September 2000/Accepted 30 April 2001

	ABSTRACT

Top Abstract Introduction Materials and Methods Results Discussion References

Anaerobic microbial toluene catabolism is initiated by addition of fumarate to the methyl group of toluene, yielding (R)-benzylsuccinateas first intermediate, which is further metabolized via $beta$ -oxidationto benzoyl-coenzyme A (CoA) and succinyl-CoA. A specific succinyl-CoA:(R)-benzylsuccinateCoA-transferase activating (R)-benzylsuccinate to the CoA-thioesterwas purified and characterized from Thauera aromatica. The enzymeis fully reversible and forms exclusively the 2-(R)-benzylsuccinyl-CoAisomer. Only some close chemical analogs of the substrates areaccepted by the enzyme: succinate was partially replaced by maleateor methylsuccinate, and (R)-benzylsuccinate was replaced by methylsuccinate,benzylmalonate, or phenylsuccinate. In contrast to all other knownCoA-transferases, the enzyme consists of two subunits of similaramino acid sequences and similar sizes (44 and 45 kDa) in an $alpha$ ₂ $beta$ ₂conformation. Identity of the subunits with the products of thepreviously identified toluene-induced bbsEF genes was confirmedby determination of the exact masses via electrospray-mass spectrometry.The deduced amino acid sequences resemble those of only two othercharacterized CoA-transferases, oxalyl-CoA:formate CoA-transferaseand (E)-cinnamoyl-CoA:(R)-phenyllactate CoA-transferase, whichrepresent a new family of CoA-transferases. As suggested by kineticanalysis, the reaction mechanism of enzymes of this family apparentlyinvolves formation of a ternary complex between the enzyme andthe twosubstrates.

	INTRODUCTION

Top Abstract Introduction Materials and Methods Results Discussion References

Some bacteria are known to metabolize aromatic hydrocarbons, such as toluene, in the absence of oxygen. The metabolic pathwayinvolved in the anaerobic catabolism of toluene is currently underinvestigation (for a review, see reference 19). Overall, tolueneis oxidized to benzoyl-coenzyme A (CoA), a common intermediatein the anaerobic catabolic pathways of many aromatic compounds(reviewed in reference 20). The first step is an unusual additionof the methyl group of toluene to the double bond of a fumaratecosubstrate (5, 7; Fig. 1). This reaction is catalyzed by theglycyl-radical enzyme (R)-benzylsuccinate synthase and yieldsexclusively the (R)-(+)-enantiomer of benzylsuccinate (6, 25,26). Further catabolism of (R)-benzylsuccinate to benzoyl-CoAproceeds via a specific $beta$ -oxidation pathway (26; Fig. 1). Theenzymes of this pathway are encoded by nine genes, which are arrangedin a toluene-induced operon (24). $beta$ -Oxidation of benzylsuccinateis initiated by a succinyl-CoA:(R)-benzylsuccinate CoA-transferaseproducing benzylsuccinyl-CoA (26). Analogous initial reactionsas outlined for anaerobic toluene metabolism have recently alsobeen described for anaerobic catabolism of m-xylene (23), m-cresol(28), p-cresol (29), and 2-methylnaphthalene (2), and thecorresponding benzylsuccinate analogs of these substrates havebeen identified (2, 23, 28, 29). However, the subsequentreactions of these pathways are not yet known.

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FIG. 1. Pathway of anaerobic toluene degradation. Enzymes: BSS, (R)-benzylsuccinate synthase; BSCT, succinyl-CoA:(R)-benzylsuccinate CoA-transferase; BSDH, (R)-benzylsuccinyl-CoA dehydrogenase; PIH, (E)-Phenylitaconyl-CoA hydratase; HADH, 3-hydroxyacyl-CoA dehydrogenase; BST, benzoylsuccinyl-CoA thiolase; SDH, succinate dehydrogenase. Chiral C atoms of as-yet-unknown configuration are indicated with circles.

CoA-transferases catalyze the reversible transfer of CoA between organic acids and are known from many bacterial and eukaryoticspecies. Based on their reaction mechanisms and amino acid sequences,the currently known enzymes can be grouped into three families.(i) CoA-transferases of family I, e.g., for 3-oxoacids (15,30, 35), acetate, butyrate (4, 33, 36), or glutaconate(9, 22, 27), contain two dissimilar subunits in differentaggregation states ( $alpha$ ₂ $beta$ ₂ or $alpha$ ₄ $beta$ ₄), except for mammalian succinyl-CoA:acetoacetateCoA-transferases, where the subunits are fused to a single polypeptide(15, 30). A conserved amino acid sequence motif in the $beta$ -subunit(Prosite entry PS01274) contains an active-site glutamate residue,which is involved in the reaction mechanism (27, 31); anotherconserved amino acid sequence motif is present in the $alpha$ -subunit(Prosite entry PS01273). These enzymes operate by a ping-pongmechanism: in the first half of the reaction a covalently boundglutamyl-CoA thioester intermediate of the enzyme is formed byreacting with a suitable CoA-donor compound. The enzyme-CoA intermediatethen reacts with a CoA-acceptor compound in the other half ofthe reaction (27, 31, 35). CoA-transferases of family Iare specifically inactivated by treatment with hydroxylamine orborohydride when they are preincubated with a CoA-donor compound.The former inhibitor causes formation of a hydroxamate at theCoA-activated glutamate, and the latter reduces glutamyl-CoA toglutamic alcohol (27, 31, 35). (ii) A second family of CoA-transferasesis defined by the transferase subunits of citrate and citramalatelyases. The physiological substrate transferred by these enzymesis an enzyme-associated acyl-carrier protein (ACP) subunit containinga protein-bound CoA moiety. Transfer of free CoA moieties is onlyobserved as a side reaction under in vitro conditions (10, 11,17). The catalytic mechanisms of these enzymes require ternary-complexformation of the enzyme, donor ACP-thioester (acetyl-ACP), anda thioester-acceptor compound (citrate or citramalate; 10, 11).(iii) Finally, the first members of a third family of CoA-transferaseswere recently characterized: (E)-cinnamoyl-CoA:(R)-phenyllactate CoA-transferase from Clostridium sporogenes (16) and formyl-CoA:oxalateCoA-transferase from Oxalobacter formigenes (3, 32). Theseenzymes differ in sequence from the enzymes of families I andII, and a reaction mechanism similar to that of family II enzymeshas been suggested for one member (16).

In this communication, we report on the purification and biochemical characterization of succinyl-CoA:(R)-benzylsuccinateCoA-transferase from the denitrifying bacterium Thauera aromatica,the second enzyme of anaerobic toluene metabolism. We provideevidence that this enzyme belongs to the emerging family III ofCoA-transferases.

	MATERIALS AND METHODS

Top Abstract Introduction Materials and Methods Results Discussion References

Materials and bacterial strains. Chemicals were obtained from Fluka, Merck, Sigma, or Roth; biochemicals were from Boehringer or Gerbu; and the ATP monitoringkit was from Merlin. High-performance liquid chromatography (HPLC)equipment was from Merck or Waters, and fast-performance liquidchromatography (FPLC) equipment was from Pharmacia. [2,3-¹⁴C]succinate (specific radioactivity, 2.6 GBq mmol¹) was from American Radiolabeled Compounds. The R and S enantiomersof benzylsuccinate were prepared from the racemate as describedpreviously (26); enantiomer purities were >90%. CoA-thioestersof benzylsuccinate and other dicarboxylic acids were synthesizedvia the internal anhydrides as described elsewhere (26). T.aromatica strain K172 (1) was isolated by Tschech and Fuchs(34) and has been deposited in Deutsche Sammlung von Mikroorganismen(DSMZ 6984). Azoarcus sp. strains T (DSMZ 9506; 18) and M3 (DSMZ12184; 21) were obtained from Josef Zeyer, ETH Zürich; Azoarcussp. strain B5-1 was isolated from an enrichment culture on 3-methylbenzoatein the laboratory of Georg Fuchs, University of Freiburg (unpublishedresults).

Growth of bacterial cells and preparation of cell extract. Denitrifying bacteria were grown at 30°C under denitrifying conditions in mineral salt medium, as described previously (7).Cell harvesting and storage were performed as described earlier(7). Cell extract was prepared under aerobic conditions at4°C. Frozen cells were suspended in one volume of buffer A (10mM triethanolamine hydrochloride-NaOH [pH 7.5], 10% [vol/vol]glycerol) containing 0.05 mg of DNase I (g of cells)¹. Cells were broken by passage through a French pressure cellat 137 MPa; the lysate was centrifuged at 100,000 × g for 60 min.The supernatant was used immediately or kept frozen at $-$ 70°C withoutdetectable loss of activity for up to 3months.

Enzyme assays. The forward reaction of succinyl-CoA:(R)-benzylsuccinate CoA-transferase was measured by a photometric assay coupled to thereaction of endogenous succinate dehydrogenase of T. aromaticaas described previously (26) or by analysis of benzylsuccinyl-CoAformation via HPLC (reference 26 and as described below). Thereverse reaction of the enzyme was measured by a coupled luminometricassay with the endogenous succinate-CoA ligase of T. aromaticaand luciferase as auxiliary enzymes. The enzyme was assayed in100 mM triethanolamine hydrochloride-NaOH (pH 7.5) containing2.5 mM MgCl₂, 5 mM NaH₂PO₄, 0.1 mM ADP, 1 mM succinate, 2% (vol/vol)ATP-monitoring kit, 0.1 mU of partially purified succinate-CoAligase (0.2 µg of protein), 10 µl of diluted cell extract or columnfraction, and (if necessary) 0.1 mM P₁-P₅-bis-(adenosine-5')-pentaphosphateto inhibit myokinase activity. The reaction was started by addingbenzylsuccinyl-CoA to a final concentration of 0.1 mM. The reactionwas followed continuously in a luminometer 1250 (Pharmacia-LKB)and calibrated with an ATP standard (Merlin). The auxiliary enzymesuccinate-CoA ligase was enriched by passing extracts of toluene-growncells over a DEAE-Sepharose column (Pharmacia; diameter, 2.2 cm;volume, 30 ml). The column was eluted with a linear gradient of50 to 200 mM NaCl in buffer A over 7 column volumes. Succinate-CoAligase eluted between 90 and 115 mM NaCl with a recovery of 95%and an enrichment factor of 3.8. The active fractions were pooled;they contained 7.8 mg of protein ml¹ and a specific activity of 0.5 µmol min¹ (mg of protein)¹. No succinyl-CoA:(R)-benzylsuccinate CoA-transferase activitywas detectable in these fractions. Steady-state kinetic experimentswere performed for the reverse reaction with purified enzyme,using varied concentrations of succinate and chemically synthesized(R)-benzylsuccinyl-CoA that contained both possible regioisomers(2-and 3-benzylsuccinyl-CoA; see below). Concentrations of bothsubstrates varied from 0.25 to 7 times the respective K_mvalues.

Product analysis. Routine analysis of the CoA-thioesters produced was performed by HPLC at room temperature with UV detection at 260 nm usinga C₁₈ reversed-phase column (5 µm; LiChrospher 100 RPC-18; Merck),as described previously (26). However, chemically synthesizedbenzylsuccinyl-CoA consisted of two isomeric compounds (2- and3-benzylsuccinyl-CoA), which comigrated under the standard HPLCconditions (26). Partial separation of the two compounds wasachieved by a modified HPLC protocol. The column was eluted over25 min at a flow rate of 1 ml min¹ with a gradient of 1 to 25% (vol/vol) acetonitrile in 50 mM acetatebuffer containing 50 mM phosphate (pH 4.5). Chemically synthesizedbenzylsuccinyl-CoA and enzymatically produced benzylsuccinyl-CoAwere analyzed in portions of 1 to 2 nmol per run. Because of thepoor peak resolution, comigration tests of the enzymatically producedbenzylsuccinyl-CoA regioisomer were confirmed by spiking enzymaticconversion reaction mixtures with different amounts of chemicallysynthesized benzylsuccinyl-CoA.

Enzyme purification. All purification steps were performed under aerobic conditions at 6°C with an FPLC System (Pharmacia). Extracts of T. aromaticacells grown on toluene (12.5 ml of a 100,000 × g supernatant)were applied to a DEAE-Sepharose column (Pharmacia; diameter,2.2 cm; volume, 30 ml) which had been equilibrated with bufferA. The column was washed with buffer A at a flow rate of 1 mlmin¹ for 4 column volumes. The column was eluted with steps of 100and 180 mM NaCl; each step was applied over 4 to 5 column volumes.Fractions of 5 ml were collected. Succinyl-CoA:benzylsuccinateCoA-transferase activity eluted in a volume of 60 ml when the180 mM NaCl step was applied. Two-thirds of the eluate (40 ml)were loaded on a ceramic hydroxyapatite column (Bio-Rad; diameter,1.6 cm; volume, 20 ml) equilibrated with buffer A. The columnwas washed with 60 ml of buffer A, and the CoA-transferase activitywas eluted with 22 mM sodium phosphate in buffer A over 2 to 3column volumes. The active fractions were pooled (final volume,60 ml). Half of the pool (30 ml) was applied on a Q-Sepharosecolumn (Pharmacia; diameter, 1.1 cm; volume, 10 ml) which wasequilibrated with buffer A containing 180 mM NaCl. The columnwas eluted with steps of 180 and 250 mM NaCl at a flow rate of1 ml min¹. Each step was applied over 3 to 4 column volumes. The CoA-transferaseactivity eluted in a volume of 70 ml when 250 mM NaCl was applied.The eluate was concentrated to a volume of 1.5 ml by ultrafiltrationwith an exclusion limit of 30 kDa (Amicon 8400, with a PM-30 membrane).Concentrated eluate (500 µl) was loaded on a Superdex 200 column(Pharmacia; diameter, 1.6 cm; volume, 120 ml). The column wasequilibrated and eluted with buffer A containing 100 mM NaCl ata flow rate of 0.8 ml min¹, and fractions of 1.6 ml were collected. The CoA-transferaseeluted in a volume of 8 ml. The fractions were pooled and concentrated35-fold by ultrafiltration. No loss of activity was recorded duringthe concentrationsteps.

Analysis of substrate preference. The products of the CoA-transferase reaction were analyzed by HPLC as described previously (26). To test the substrate preferenceof succinyl-CoA:(R)-benzylsuccinate CoA-transferase, succinatewas replaced by (R,S)-methylsuccinate, maleinate, fumarate, formate,acetate, propionate, glutarate, malonate, or oxalate; benzylsuccinatewas replaced by (R,S)-methylsuccinate, (R,S)-phenylsuccinate,2- or 3-phenylpropionate, 4-phenylbutyrate, or benzylmalonate.An analogous test was performed with benzoyl-CoA as the potentialalternative CoA donor instead of succinyl-CoA and (R,S)-benzylsuccinateas acceptor. The assays (total volume, 100 µl) were performedin 100 mM Tris-HCl [pH 7.5] containing a 2.5 mM concentrationof the substrate analog to be tested and 3 µg of purified CoA-transferaseafter preparative gel filtration. The reactions were started with0.5 mM of the appropriate CoA-thioester and incubated at 30°C.After 10 min, the assay mixtures were split: one half (50 µl)of each assay mixture was retrieved and acidified to pH 3 withformic acid (10% [vol/vol] final concentration); the remaininghalf was brought to pH 9 by adding 10 µl of 0.1 M NaOH and heatingat 80°C for 15 min to hydrolyze CoA-thioesters. The alkaline-treatedsamples were then acidified to pH 3 with formic acid (10% [vol/vol]final concentration). Precipitated protein was removed by centrifugation(20,000 × g; 4°C; 10 min), and the samples were analyzed by HPLC(26). If the substrate analogs were converted to CoA-thioesters,new peaks absorbing at 260 nm were observed, which disappearedafter alkaline treatment. The correlation of these peaks withthe predicted CoA-thioesters was checked by chemical synthesisand HPLC analysis of CoA-thioesters of maleate, methylsuccinate,and phenylsuccinate. Although the chemically synthesized CoA-thioesterswere mixtures of the possible positional and conformational isomers,they all contained one compound that comigrated with the enzymaticallyformed thioester (data notshown).

Isotope exchange experiments. Assay mixtures containing 100 mM Tris-HCl (pH 7.5), 6.5 µg of purified CoA-transferase, and 125 Bq of [¹⁴C]succinate (final concentration, 0.5 µM) were prepared in a totalvolume of 100 µl. Control assay mixtures also contained 1 mM benzylsuccinate.The reactions were started by adding 1 mM succinyl-CoA and incubatingat room temperature. After 5 and 20 min, samples (50 µl) weretaken; the reaction was stopped by adding formic acid (10% [vol/vol])and reaction products were analyzed by HPLC as described before.UV absorption at 260 nm and radioactivity (Ramona detector; Raytest)of the eluate were monitoredsimultaneously.

Inactivation experiments. Two types of experiments were performed. (i) The first type was inactivation by sodium borohydride. Enriched CoA-transferaseafter the Q-Sepharose step (160 µg of protein) was added to 1ml of a 0.5 M triethanolamine hydrochloride buffer (pH 7.5), whicheither contained or lacked benzylsuccinyl-CoA (250 µM). The enzymewas treated with 10 µl of a 1 M NaBH₄ solution in 1 M NaOH, and10 µl of a 1 M HCl solution was added immediately afterwards.The mixtures were incubated for 10 min at room temperature andtested for CoA-transferase activity by the coupled luminometricassay. (ii) The second type of experiment involved inactivationby hydroxylamine. The same enzyme batch as used for the aboveexperiments (3.2 µg of protein) was added to 0.1 ml of a 0.1 MTris-HCl buffer (pH 7.5), which either contained or lacked benzylsuccinyl-CoA(250 µM). The enzyme was treated with 10 mM hydroxylamine for15 min at room temperature and assayed by the coupled luminometricassay.

Native molecular mass determination. The molecular mass of the native CoA-transferase was determined by size exclusion chromatography and by Ferguson plot analysis.Concentrated eluate of the preparative gel filtration (100 µl,1.4 mg ml¹) was applied on a Superdex 200-HR (Pharmacia; diameter, 1.1 cm;volume, 20 ml). The column was equilibrated and eluted with bufferA containing 100 mM NaCl. The following molecular mass standardproteins were used to calibrate the column: ferritin (450 kDa),catalase (240 kDa), alcohol dehydrogenase (150 kDa), bovine serumalbumin (67 kDa), and ovalbumin (45 kDa); inclusion and exclusionvolumes were determined with blue dextran and vitamin B₁₂, respectively.Additionally, the native mass of the enzyme was confirmed by Fergusonplot. Purified CoA-transferase and standard proteins were separatedon native acrylamide gels (5, 6, 6.5, and 8% polyacrylamide [wt/vol]).The following proteins were used as standards: different aggregationforms of bovine serum albumin (monomer, 67 kDa; dimer, 134 kDa;trimer, 201 kDa; tetramer; 268 kDa); ovalbumin (45 kDa); and carboanhydrase(29 kDa). The migration positions of the proteins were used tocalculate the molecular mass of the native CoA-transferase afterstaining the gels with Coomassie blue or by silver staining (12).

Other methods. Evaluation of kinetic experiments and fitting to equations describing different two-substrate mechanisms was performed bythe program Leonora (13), using the original data from duplicatedexperiments. Sodium dodecyl sulfate-polyacrylamide gel electrophoresis(SDS-PAGE) (8% [wt/vol] polyacrylamide gels) was performed asdescribed previously (12). Proteins were stained with Coomassieblue. Protein concentrations were determined according to themethod of Bradford (8) or by a modification of the Lowry method(12), using a bovine serum albumin standard which had been calibratedby its absorption at 280 nm. UV-visible spectra were recordedby a Perkin-Elmer UV/Vis spectrometer Lambda 2S. Electrospray-massspectrometry of purified protein was performed with a FinniganTSQ700 mass spectrometer with electrospray interface. The proteinwas applied on a C₄ HPLC column (0.8 by 150 mm; Vydac) directlycoupled to the mass spectrometer and eluted by a linear gradientfrom 10 to 95% acetonitrile in 0.1% trifluoroacetic acid at aflow rate of 20 µl min¹.

	RESULTS

Top Abstract Introduction Materials and Methods Results Discussion References

Enzyme assays for succinyl-CoA:(R)-benzylsuccinate CoA-transferase. Continuous enzyme assays were developed to measure the forward and reverse reactions of succinyl-CoA:(R)-benzylsuccinate CoA-transferaseof toluene-grown cells of T. aromatica. The assay for the forwardreaction coupled benzylsuccinate-dependent formation of free succinatefrom succinyl-CoA to the succinate dehydrogenase reaction. Therate (± standard deviation) measured by this assay in cell extractswas 15 ± 5 nmol min¹ (mg of protein)¹ (26). The reverse reaction, synthesis of succinyl-CoA frombenzylsuccinyl-CoA and succinate, was measured by a luminometriccoupled enzyme assay with succinate-CoA ligase and firefly luciferase.Partially purified succinate-CoA ligase from T. aromatica wasused as auxiliary enzyme. The enzyme preparation was devoid ofCoA-transferase activity and had a specific succinate-CoA ligaseactivity of 510 ± 15 nmol min¹ (mg of protein)¹. The specific activity of succinyl-CoA:(R)-benzylsuccinate CoA-transferasein cell extracts, as measured by this assay, was 25 ± 5 nmol min¹ (mg of protein)¹.

Analysis of reaction products. We have previously shown that succinyl-CoA:(R)-benzylsuccinate CoA-transferase specifically forms a CoA-thioester from (R)-benzylsuccinate(26). However, the biologically relevant benzylsuccinyl-CoAisomer has not yet been fully identified, since two differentregioisomers can be formed, 2- or 3-benzylsuccinyl-CoA (Fig. 2).Chemically synthesized (racemic) benzylsuccinyl-CoA indeed consistedof 2- and 3-benzylsuccinyl-CoA in a reproducible molar ratio of2:1, respectively, as evident from the chemical shifts of thethioester-carbonyl groups detected by ¹³C-nuclear magnetic resonance (NMR) analysis (26; W. Eisenreich,A. Bacher, C. Leutwein, and J. Heider, unpublished data). Thetwo isomers of racemic or enantiomerically pure benzylsuccinyl-CoAcomigrated under standard HPLC conditions but were partially separatedby a modified HPLC procedure (Fig. 2). The molar ratio of thetwo isomers was calculated as 2:1 from the integrated peak areas,assuming similar absorption coefficients at 260 nm. Therefore,the earlier eluting peak can be assigned to 2- and the latterto 3-benzylsuccinyl-CoA (Fig. 2). Although enzymatically synthesizedbenzylsuccinyl-CoA was not obtained in sufficient amounts for¹³C-NMR analysis, it eluted as a single compound in HPLC assaysand comigrated with 2-benzylsuccinyl-CoA (Fig. 2).

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FIG. 2. HPLC analysis of the enzymatically formed benzylsuccinyl-CoA isomer. Chemically synthesized (solid line) and enzymatically synthesized (broken line) benzylsuccinyl-CoA were separated by HPLC and monitored by their absorption at 260 nm. The dotted line represents the hypothetical elution profile of 3-benzylsuccinyl-CoA; it represented 30 to 40% of the amount of chemically synthesized benzylsuccinyl-CoA. The curve was calculated by subtracting the elution profile of enzymatically synthesized benzylsuccinyl-CoA from that of the chemically synthesized isomer mixture. The structures of the benzylsuccinyl-CoA isomers were inferred from correlation with NMR data as shown.

Purification of succinyl-CoA:(R)-benzylsuccinate CoA-transferase. Succinyl-CoA:(R)-benzylsuccinate CoA-transferase was purified from toluene-grown cells of T. aromatica in four chromatographicsteps (Table 1). The enzyme was stable in air, and thereforeall purification steps were performed under aerobic conditions.In initial experiments, we observed that the enzyme was completelyinactivated during passage over DEAE-Sepharose when eluted withlinear gradients of NaCl. Therefore, all anion exchange and hydroxyapatitechromatographic steps were performed with step gradients, whichwere not detrimental for enzyme activity. Monitoring of enzymeactivity during purification was done by the luminometric assayfor the reverse reaction. Addition of the myokinase inhibitorbis-adenosine pentaphosphate was necessary for luminometric assayswith cell extracts and fractions of the first column, but notwith the active fractions of the later steps of the purification.Activity eluted from the DEAE-Sepharose column between 100 and180 mM NaCl. The larger portion of the active fractions was appliedto a hydroxyapatite column, and enzyme activity eluted in a stepbetween 0 and 22 mM sodium phosphate. The next purification stepwas chromatography on Q-Sepharose: half of the active fractionafter hydroxyapatite chromatography was applied, and the enzymeeluted in a step between 180 and 250 mM NaCl. The final step ofthe purification, gel permeation chromatography on Superdex 200HR, was only applied for small aliquots. Although this step obviouslycaused severe inactivation of the enzyme, it was necessary forpurification. Several other columns, such as Mono-Q, hydrophobiccolumns, or dye affinity columns, were tested, but they eitherinactivated the enzyme or did not yield further purification effects.An SDS-polyacrylamide gel of the active fractions during the purificationis shown in Fig. 3; the enzyme is essentially pure after the gelfiltration step. As calculated from the enrichment factor andyield, the CoA-transferase corresponds to at least 0.6% of thetotal soluble protein of toluene-grown cells of T. aromatica.

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TABLE 1. Purification of succinyl-CoA:benzylsuccinate CoA-transferase from T. aromatica^a

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FIG. 3. SDS-PAGE of active fractions during purification of succinyl-CoA:benzylsuccinate CoA-transferase. A Coomassie-stained gel is shown, in which the pooled fractions of the purification were analyzed. Low polyacrylamide concentrations (8% [wt/vol]) were used to separate the two CoA-transferase subunits. The purified enzyme was checked for the absence of contaminating proteins smaller than 30 kDa, which migrated in the front in these gels. Lanes: 1, protein standards; 2, crude extract (16 µg of protein); 3, DEAE-Sepharose fraction (12 µg of protein); 4, hydroxyapatite fraction (12 µg of protein); 5, Q-Sepharose fraction (12 µg of protein); 6, gel filtration fraction (1.5 µg of protein). The masses of standard proteins in kilodaltons are indicated on the left margin.

Molecular properties of succinyl-CoA:(R)-benzylsuccinate CoA-transferase. Purified succinyl-CoA:(R)-benzylsuccinate CoA-transferase consisted of two polypeptides migrating at apparent masses of 44and 45 kDa during SDS-PAGE (Fig. 3). Both subunits of the purifiedenzyme were blocked for N-terminal sequencing. However, exactmolecular masses of the subunits were determined by electrospray-massspectrometry (44.81 and 45.47 kDa). These masses match well withthose predicted for two recently identified toluene-induced proteins,BbsF (44.798 kDa) and BbsE (45.482 kDa). These are encoded ina common operon (bbs, for beta-oxidation of benzylsuccinate) togetherwith other enzymes involved in $beta$ -oxidation of benzylsuccinate(24). The mass of the native enzyme (mean ± standard deviation)was determined as 215 ± 15 kDa by passage over a calibrated Superdex200 HR gel filtration column and as 225 ± 26 kDa by a Fergusonplot from native gel electrophoresis. Thus, the subunit compositionof succinyl-CoA:(R)-benzylsuccinate CoA-transferase appears tobe $alpha$ ₂ $beta$ ₂. The UV-visible spectrum of purified enzyme did not exhibitunusual features. The absorption coefficient of the enzyme at280 nm was 304 mM¹ cm¹ per holoenzyme ( $alpha$ ₂ $beta$ ₂), which is in reasonable agreement withthe absorption coefficient calculated from the tryptophan andtyrosine content of BbsE and BbsF ( $varepsilon$ ₂₈₀ = 284 mM¹ cm¹).

Catalytic properties of succinyl-CoA:(R)-benzylsuccinate CoA-transferase. Purified enzyme was assayed with succinyl-CoA and (R)- or (S)-benzylsuccinate (2 mM final concentration); the products formedafter different incubation times were analyzed by HPLC. Only (R)-benzylsuccinatewas converted to 2-benzylsuccinyl-CoA at rates of 320 ± 50 nmolmin¹ (mg protein)¹, whereas no reaction was observed with the (S) enantiomer. Ratesof 2-(R)-benzylsuccinyl-CoA formation were not significantly loweredin assays containing 2 mM (R)-benzylsuccinate plus (S)-benzylsuccinatein up to fivefold excess. Enantiomer specificity of the reversereaction was tested by the luminometric assay, using chemicallyprepared (R)-, (S)-, and racemic benzylsuccinyl-CoA. All preparationswere mixtures of 2- and 3-benzylsuccinyl-CoA (molar ratio of 2:1,as analyzed by HPLC). Purified enzyme was active with (R)-benzylsuccinyl-CoA,whereas no activity was detected when (S)-benzylsuccinyl-CoA wasused as substrate. In contrast to the free acid, (S)-benzylsuccinyl-CoAinhibited CoA-transferase activity, as evident from enzyme assayscontaining (R)-benzylsuccinyl-CoA (90 µM) and increasing concentrationsof (S)-benzylsuccinyl-CoA. Activities dropped to 70% with racemicbenzylsuccinyl-CoA, to 40% with a 5-fold excess, and below thedetection limit with a 10-fold excess of (S)-benzylsuccinyl-CoA.

Kinetic parameters of succinyl-CoA:(R)-benzylsuccinate CoA-transferase were only recorded for the reverse reaction becausethe assays for the forward direction were not sensitive enoughto obtain reliable initial activity values at low substrate concentrations.The assays were performed with chemically synthesized (R)-benzylsuccinyl-CoA(2- and 3-benzylsuccinyl-CoA in 2:1 ratio). The indicated concentrationsof (R)-benzylsuccinyl-CoA relate to the isomer mixture as appliedin the experiments; concentrations of the relevant regioisomercorrespond to 67% of these values. The kinetic data were evaluatedby curve fitting of the data to the Michaelis-Menten equationand statistical evaluation (13). They were consistent with anassumed ternary-complex mechanism but significantly differentfrom those expected from ping-pong kinetics. This is also evidentfrom double-reciprocal plots of activity versus benzylsuccinyl-CoAor succinate concentrations, which yielded intersecting lines(Fig. 4). K_m values of 40 ± 8 µM for 2- plus 3-(R)-benzylsuccinyl-CoAand 160 ± 30 µM for succinate were calculated from the best-fittingternary complex equation (13, 14).

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FIG. 4. Double-reciprocal plot of succinyl-CoA:benzylsuccinate CoA-transferase activity versus succinate concentration. The assays were performed by the standard luminometric assay in the presence of 5 (a), 15 (b), 30 (c), 60 (d), or 120 (e) µM concentrations of a chemically synthesized regioisomer mixture of 2- and 3-(R)-benzylsuccinyl-CoA (molar ratio, 2:1). Reactions were started with the indicated concentrations of succinate. The symbols represent mean values of two measurements.

The substrate preference of succinyl-CoA:(R)-benzylsuccinate CoA-transferase was tested by HPLC analysis of the CoA-thioestersformed in enzyme assays with chemical analogs of benzylsuccinateand succinate, respectively. Benzylsuccinate analogs were testedwith succinyl-CoA, and succinate analogs were tested with (racemic)benzylsuccinyl-CoA as CoA donor (Table 2). From these tests,it became evident that the enzyme is quite specific for the twonatural substrates. Detectable CoA-thioester formation was observedwith (R, S)-phenylsuccinate and benzylmalonate in lieu of benzylsuccinate,and with maleinate replacing succinate. (R, S)-Methylsuccinatewas the only substrate tested that replaced either succinate orbenzylsuccinate as a CoA-acceptor compound (Table 2). The CoA-transferasereaction was also analyzed for isotope exchange activity betweenunlabeled succinyl-CoA and [2,3-¹⁴C]succinate. About 50% of ¹⁴C-labeled succinate was converted to [¹⁴C]succinyl-CoA after 20 min in the absence of benzylsuccinate,suggesting that the enzyme indeed catalyzes CoA transfer betweensuccinyl-CoA and succinate. However, no isotope exchange between[¹⁴C]succinate and [¹⁴C]succinyl-CoA occurred under the same conditions in the presenceof 1 mM benzylsuccinate. Finally, succinyl-CoA could not be replacedas CoA donor for benzylsuccinate by benzoyl-CoA, the second productof $beta$ -oxidation of benzylsuccinyl-CoA besides succinyl-CoA (7).

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TABLE 2. Substrate analogs of succinyl-CoA:benzylsuccinate CoA-transferase

Inactivation assays of succinyl-CoA:(R)-benzylsuccinate CoA-transferase. CoA-transferases of family I are specifically inactivated by incubation with NaBH₄ or hydroxylamine in the presence of CoA-thioesters(27, 31). Therefore, we tested the effect of these compoundson succinyl-CoA:(R)-benzylsuccinate CoA-transferase. Enzyme wasincubated in the absence of CoA-thioesters or in the presenceof 0.25 mM benzylsuccinyl-CoA for 10 min with 0.1 to 10 mM NaBH₄and with 10 mM hydroxylamine, respectively, and then assayed bythe coupled luminometric test. No inactivation by hydroxylaminewas recorded in the tests with and without benzylsuccinyl-CoA,suggesting that no reactive enzyme-CoA intermediate was present.However, the inactivation data with borohydride were somewhatambiguous. No inactivation was detected with 0.1 mM NaBH₄, buta decrease of activity in the presence of benzylsuccinyl-CoA to25% and further to 3.5% was observed at NaBH₄ concentrations of1 and 10 mM, respectively. The same treatments did not affectthe enzyme in the absence of benzylsuccinyl-CoA. The reason forthis partial inactivation is notknown.

Succinyl-CoA:benzylsuccinate CoA-transferase activity in other denitrifying bacteria. General occurrence of the benzylsuccinate-activating enzyme was tested by determining succinyl-CoA:benzylsuccinate CoA-transferaseactivity by the luminometric test in other alkylbenzene-metabolizingdenitrifying bacteria; the toluene-degrading Azoarcus sp. strainB5-1 and the Azoarcus sp. strains T and M3, which degrade tolueneor m-xylene (18, 21), were chosen for these tests. Enzymeactivity was detected in extracts of toluene-grown cells of allthese strains, whereas extracts of control cells grown on benzoatedid not show detectable activity (Table 3). The observed specificenzyme activities were close to the calculated minimum valueswhich are needed to explain the observed growth rates of cellsgrown on toluene. Surprisingly, m-xylene-grown cells of Azoarcussp. strains T and M3 also contained specifically induced CoA-transferaseactivity for the "wrong" substrate, benzylsuccinyl-CoA, whichwas more than two times higher than the activity in toluene-growncells of the same strains (Table 3).

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TABLE 3. Succinyl-CoA:benzylsuccinate CoA-transferase activities in toluene- and m-xylene-degrading denitrifying bacteria^a

	DISCUSSION

Top Abstract Introduction Materials and Methods Results Discussion References

Succinyl-CoA:benzylsuccinate CoA-transferase of T. aromatica is a strictly toluene-induced enzyme that catalyzes the reversibleregio- and enantio-selective synthesis of 2-(R)-benzylsuccinyl-CoA.The detected specific activity in cell extracts is in accordancewith the calculated rate of toluene degradation. The enzyme isthe first described CoA-transferase consisting of two subunitsof very similar amino acid sequences. The subunits were identifiedas the gene products of the toluene-induced bbsE and bbsF genes.The two subunits of succinyl-CoA:benzylsuccinate CoA-transferaseare similar to the sequences of known and putative CoA-transferasesof family III, e.g., oxalyl-CoA:formate CoA-transferase from O.formigenes (32), (E)-cinnamoyl-CoA:(R)-phenyllactate CoA-transferasefrom C. sporogenes, and a probable homologue of the latter derivedfrom the Clastridium difficile genome (16). No sequence similaritywas detected with CoA-transferases of families I and II. CoA-transferaseactivities acting on benzylsuccinate were found in different strainsof toluene- or m-xylene-degrading denitrifying bacteria. Theseand previously reported data (5, 26) suggest that activationof benzylsuccinate [and probably also that of (3-methylbenzyl)-succinategenerated from m-xylene] occurs by a CoA-transferase rather thanan ATP-dependent CoA-ligase reaction in all knownstrains.

Succinyl-CoA:(R)-benzylsuccinate CoA-transferase shows a rather strong preference for its natural substrates, succinate and(R)-benzylsuccinate, respectively, and the corresponding CoA-thioesters,and it does not react with the (S)-enantiomer of benzylsuccinate.Surprisingly, the enzyme is inhibited by high concentrations of(S)-benzylsuccinyl-CoA, while it is apparently not affected byfree (S)-benzylsuccinate. It may be speculated that the attachedCoA moiety affords better binding of the wrong enantiomer to theenzyme. However, since no defined 2-or 3-(S)-benzylsuccinyl-CoAisomers are available, we have not further investigated the mechanismof this inhibition so far. The enzyme is partially active whensuccinate is replaced by maleate and is inactive with fumarate,suggesting that the two carboxyl groups of succinate bind to theenzyme in syn conformation. The distance of the carboxyl groupsof succinate seems to be another important factor, since neithermalonate nor glutarate were accepted as substrate analogs. Alternativesubstrates partially replacing (R)-benzylsuccinate were benzylmalonateand phenylsuccinate, but the enzyme did not accept analogs withonly one carboxy group, such as 3-phenylpropionate and 4-phenylbutyrate.Thus, recognition of (R)-benzylsuccinate probably requires bothcarboxyl groups. The isotope exchange experiment between succinateand succinyl-CoA and the relatively high conversion rates of succinyl-CoAwith methylsuccinate indicate that the benzylsuccinate-bindingsite may also accept small nonaromatic dicarboxylicacids.

The kinetic investigations on succinyl-CoA:(R)-benzylsuccinate CoA-transferase indicate that catalysis proceeds via a ternarycomplex of enzyme and the two substrates without an enzyme-boundintermediate. In addition to these data, several other observationsare consistent with an assumed ternary-complex mechanism of theenzyme. (i) The recently characterized similar family III enzyme(E)-cinnamoyl-CoA:(R)-phenyllactate CoA-transferase was also shownto operate by a ternary-complex mechanism by kinetic analysis(16). (ii) Succinyl-CoA:(R)-benzylsuccinate CoA-transferasepreincubated with benzylsuccinyl-CoA was insensitive against hydroxylaminetreatment, which would inactivate CoA-transferases of family I.(iii) The observed inhibition of isotope exchange between succinyl-CoAand succinate by added benzylsuccinate may be explained by outcompetingsuccinate for binding to the benzylsuccinate site, if a ternary-complexmechanism is assumed. The only observation not consistent withthis assumption is the inactivation of the enzyme by high concentrationsof NaBH₄, but the same behavior was also reported for the relatedenzyme (E)-cinnamoyl-CoA:(R)-phenyllactate CoA-transferase (16).Therefore, we suggest a CoA transfer mechanism between succinyl-CoAand (R)-benzylsuccinate without an enzyme-bound CoA intermediate,similar to the proposed mechanism of (E)-cinnamoyl-CoA:(R)-phenyllactateCoA-transferase (16). It remains to be proven whether this isa general property of CoA-transferases of family III. A ternary-complexmechanism is also used by CoA-transferases of family II; the majordifference between the enzymes of families II and III seems toreside in the activated substrates used, as the natural substratesof family II enzymes are thioesters of small enzyme-associatedACPs (10, 11, 17), whereas all known family III enzymesemploy diffusible thioesters ofCoA.

Apart from their similar amino acid sequences and enzyme kinetics, family III CoA-transferases seem to be surprisingly different.This relates to the relatively strong substrate preference ofthe respective enzymes, and especially to their subunit compositions.All three characterized enzymes exhibit different oligomeric states:formyl-CoA:oxalate CoA-transferase is monomeric (3); succinyl-CoA:(R)-benzylsuccinateCoA-transferase is an $alpha$ ₂ $beta$ ₂ heterotetramer of two very similarsubunits; and the subunit of (E)-cinnamoyl-CoA:(R)-phenyllactateCoA-transferase is part of a larger phenyllactate dehydrataseenzyme complex which also contains the subsequent enzyme of themetabolic pathway, (R)-phenyllactyl-CoA dehydratase (16).

	ACKNOWLEDGMENTS

We thank G. Fuchs (Mikrobiologie, Universität Freiburg) for his support and many helpful discussions during this work. P.Gräber and A. Labahn (Physikalische Chemie, Universität Freiburg)are thanked for help in the development of the luminometric assayand for making their luminometer available. W. Eisenreich (OrganischeChemie, Technische Universität München) is acknowledged forrecording NMR spectra, and P. Hoerth and W. Haehnel (Biochemieder Pflanzen, Universität Freiburg) are acknowledged for electrospray-massspectrometryanalysis.

This work was supported by grants from the DeutscheForschungsgemeinschaft.

	FOOTNOTES

^* Corresponding author. Mailing address: Mikrobiologie, Institut für Biologie II, Universität Freiburg, Schänzlestr. 1, 79104Freiburg, Germany. Phone: 49-761-203-2774. Fax: 49-761-203-2626.E-mail: heiderj{at}uni-freiburg.de.

Dedicated to W. Buckel on the occasion of his 60thbirthday.

REFERENCES

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References

1. Anders, A., A. Kaetzke, P. Kämpfer, W. Ludwig, and G. Fuchs. 1995. Taxonomic position of aromatic degrading denitrifying pseudomonad strains K172 and KB740 and their description as new members of the genera Thauera, T. aromatica sp. nov., and Azoarcus, A. evansii sp. nov., respectively, members of the beta subclass of Proteobacteria. Int. J. Syst. Bacteriol. 45:327-333[Abstract/Free Full Text].

2. Annweiler, E., A. Materna, M. Safinowski, A. Kappler, H. H. Richnow, W. Michaelis, and R. U. Meckenstock. 2000. Anaerobic degradation of 2-methylnaphthalene by a sulfate-reducing enrichment culture. Appl. Environ. Microbiol. 66:5329-5333[Abstract/Free Full Text].

3. Baetz, A. L., and M. J. Allison. 1990. Purification and characterization of formyl-coenzyme A transferase from Oxalobacter formigenes. J. Bacteriol. 172:3537-3540[Abstract/Free Full Text].

4. Barker, H. A., I. M. Jeng, N. Neff, J. M. Robertson, F. K. Tam, and S. Hosaka. 1978. Butyryl-CoA:acetoacetate CoA-transferase from a lysine-fermenting Clostridium. J. Biol. Chem. 253:1219-1225[Free Full Text].

5. Beller, H. R., and A. M. Spormann. 1997. Anaerobic activation of toluene and o-xylene by addition to fumarate in denitrifying strain T. J. Bacteriol. 179:670-676[Abstract/Free Full Text].

6. Beller, H. R., and A. M. Spormann. 1998. Analysis of the novel benzylsuccinate synthase reaction for anaerobic toluene activation based on structural studies of the product. J. Bacteriol. 180:5454-5457[Abstract/Free Full Text].

7. Biegert, T., G. Fuchs, and J. Heider. 1996. Evidence that oxidation of toluene in the denitrifying bacterium Thauera aromatica is initiated by formation of benzylsuccinate from toluene and fumarate. Eur. J. Biochem. 238:661-668[Medline].

8. Bradford, M. M. 1976. A rapid and sensitive method for the quantitation of microgram quantities of protein utilizing the principle of protein-dye binding. Anal. Biochem. 72:248-254[CrossRef][Medline].

9. Buckel, W., U. Dorn, and R. Semmler. 1981. Glutaconate CoA-transferase from Acidaminococcus fermentans. Eur. J. Biochem. 118:315-321[Medline].

10. Buckel, W., V. Buschmeier, and H. Eggerer. 1971. The action mechanism of citrate lyase from Klebsiella aerogenes. Hoppe-Seyler's Z. Physiol. Chem. 352:1195-1205[Medline].

11. Buckel, W., and A. Bobi. 1975. The enzyme complex citramalate lyase from Clostridium tetanomorphum. Eur. J. Biochem. 64:255-262[CrossRef][Medline].

12. Coligan, J. E., B. M. Dunn, H. L. Ploegh, D. W. Speicher, and P. T. Wingfield. 1995. Current protocols in protein science. John Wiley & Sons Inc., New York, N.Y.

13. Cornish-Bowden, A. 1995. Analysis of enzyme kinetic data. Oxford University Press, Oxford, United Kingdom.

14. Cornish-Bowden, A. 1995. Fundamentals of enzyme kinetics. Oxford University Press, Oxford, United Kingdom.

15. Corthésy-Theulaz, I. E., G. E. Bergonzelli, H. Henry, D. Bachmann, D. F. Schorderet, A. L. Blum, and N. Ornston. 1997. Cloning and characterization of Helicobacter pylori succinyl-CoA:acetoacetate CoA-transferase, a novel prokaryotic member of the CoA-transferase family. J. Biol. Chem. 272:25659-25667[Abstract/Free Full Text].

16. Dickert, S., A. J. Pierik, D. Linder, and W. Buckel. 2000. The involvement of coenzyme A esters in the dehydration of (R)-phenyllactate to (E)-cinnamate by Clostridium sporogenes. Eur. J. Biochem. 267:3874-3884[Medline].

17. Dimroth, P., and H. Eggerer. 1975. Isolation of subunits of citrate lyase and characterization of their function in the enzyme complex. Proc. Natl. Acad. Sci. USA 72:3458-3462[Abstract/Free Full Text].

18. Dolfing, J., J. Zeyer, P. Binder-Eicher, and R. P. Schwarzenbach. 1990. Isolation and characterization of a bacterium that mineralizes toluene in the absence of molecular oxygen. Arch. Microbiol. 154:336-341[Medline].

19. Heider, J., A. M. Spormann, H. R. Beller, and F. Widdel. 1999. Anaerobic bacterial metabolism of hydrocarbons. FEMS Microbiol. Rev. 22:459-473[CrossRef].

20. Heider, J., and G. Fuchs. 1997. Microbial anaerobic aromatic metabolism. Anaerobe 3:1-22.

21. Hess, A., B. Zarda, D. Hahn, A. Häner, D. Stax, P. Höhener, and J. Zeyer. 1997. In situ analysis of denitrifying toluene- and m-xylene-degrading bacteria in a diesel fuel-contaminated laboratory aquifer column. Appl. Environ. Microbiol. 63:2136-2141[Abstract].

22. Jacob, U., M. Mack, T. Clausen, R. Huber, W. Buckel, and A. Messerschmidt. 1997. Glutaconate CoA-transferase from Acidaminococcus fermentans: the crystal structure reveals homology with other CoA-transferases. Structure 5:415-426[Medline].

23. Krieger, C. J., H. R. Beller, M. Reinhard, and A. M. Spormann. 1999. Initial reactions in anaerobic oxidation of m-xylene by the denitrifying bacterium Azoarcus sp. strain T. J. Bacteriol. 181:6403-6410[Abstract/Free Full Text].

24. Leuthner, B., and J. Heider. 2000. Anaerobic toluene catabolism of Thauera aromatica: the bbs operon codes for the enzymes of $beta$ -oxidation of the intermediate benzylsuccinate. J. Bacteriol. 182:272-277[Abstract/Free Full Text].

25. Leuthner, B., C. Leutwein, H. Schulz, P. Hörth, W. Haehnel, E. Schiltz, H. Schägger, and J. Heider. 1998. Biochemical and genetic characterization of benzylsuccinate synthase from Thauera aromatica: a new glycyl radical enzyme catalyzing the first step in anaerobic toluene metabolism. Mol. Microbiol. 28:615-628[CrossRef][Medline].

26. Leutwein, C., and J. Heider. 1999. Anaerobic toluene catabolic pathway in denitrifying Thauera aromatica: activation and $beta$ -oxidation of the first intermediate, (R)-(+)-benzylsuccinate. Microbiology 145:3265-3271[Abstract/Free Full Text].

27. Mack, M., and W. Buckel. 1995. Identification of glutamate beta 54 as the covalent-catalytic residue in the active site of glutaconate CoA-transferase from Acidaminococcus fermentans. FEBS Lett. 357:145-148[CrossRef][Medline].

28. Müller, J. A., A. S. Galushko, A. Kappler, and B. Schink. 1999. Anaerobic degradation of m-cresol by Desulfobacterium cetonicum is initiated by formation of 3-hydroxybenzylsuccinate. Arch. Microbiol. 172:287-294[CrossRef][Medline].

29. Müller, J. A., A. S. Galushko, A. Kappler, and B. Schink. 2001. Initiation of anaerobic degradation of p-cresol by formation of 4-hydroxybenzylsuccinate in Desulfobacterium cetonicum. J. Bacteriol. 183:752-757[Abstract/Free Full Text].

30. Parales, R. E., and C. S. Harwood. 1992. Characterization of the genes encoding $beta$ -ketoadipate succinyl-coenzyme A transferase in Pseudomonas putida. J. Bacteriol. 174:4657-4666[Abstract/Free Full Text].

31. Selmer, T., and W. Buckel. 1999. Oxygen exchange between acetate and the catalytic glutamate residue in glutaconate CoA-transferase from Acidaminococcus fermentans: implications for the mechanism of CoA-ester hydrolysis. J. Biol. Chem. 274:20772-20778[Abstract/Free Full Text].

32. Sidhu, H., S. D. Ogden, H.-Y. Lung, B. G. Luttge, A. L. Baetz, and A. B. Peck. 1997. DNA sequencing and expression of the formyl-coenzyme A transferase gene, frc, from Oxalobacter formigenes. J. Bacteriol. 179:3378-3381[Abstract/Free Full Text].

33. Sramek, S. J., and F. E. Frerman. 1975. Purification and properties of Escherichia coli coenzyme A-transferase. Arch. Biochem. Biophys. 171:14-26[CrossRef][Medline].

34. Tschech, A., and G. Fuchs. 1987. Anaerobic degradation of phenol by pure cultures of newly isolated denitrifying pseudomonads. Arch. Microbiol. 148:213-217[CrossRef][Medline].

35. White, H., and W. P. Jencks. 1976. Properties of succinyl-CoA:3-ketoacid coenzyme A transferase. J. Biol. Chem. 251:1708-1711[Abstract/Free Full Text].

36. Wiesenborn, D. P., F. B. Rudolph, and E. T. Papoutsakis. 1989. Coenzyme A-transferase from Clostridium acetobutylicum ATCC 824 and its role in the uptake of acids. Appl. Environ. Microbiol. 55:317-322[Abstract/Free Full Text].

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	ALL ASM JOURNALS

1.	Anders, A., A. Kaetzke, P. Kämpfer, W. Ludwig, and G. Fuchs. 1995. Taxonomic position of aromatic degrading denitrifying pseudomonad strains K172 and KB740 and their description as new members of the genera Thauera, T. aromatica sp. nov., and Azoarcus, A. evansii sp. nov., respectively, members of the beta subclass of Proteobacteria. Int. J. Syst. Bacteriol. 45:327-333[Abstract/Free Full Text].
2.	Annweiler, E., A. Materna, M. Safinowski, A. Kappler, H. H. Richnow, W. Michaelis, and R. U. Meckenstock. 2000. Anaerobic degradation of 2-methylnaphthalene by a sulfate-reducing enrichment culture. Appl. Environ. Microbiol. 66:5329-5333[Abstract/Free Full Text].
3.	Baetz, A. L., and M. J. Allison. 1990. Purification and characterization of formyl-coenzyme A transferase from Oxalobacter formigenes. J. Bacteriol. 172:3537-3540[Abstract/Free Full Text].
4.	Barker, H. A., I. M. Jeng, N. Neff, J. M. Robertson, F. K. Tam, and S. Hosaka. 1978. Butyryl-CoA:acetoacetate CoA-transferase from a lysine-fermenting Clostridium. J. Biol. Chem. 253:1219-1225[Free Full Text].
5.	Beller, H. R., and A. M. Spormann. 1997. Anaerobic activation of toluene and o-xylene by addition to fumarate in denitrifying strain T. J. Bacteriol. 179:670-676[Abstract/Free Full Text].
6.	Beller, H. R., and A. M. Spormann. 1998. Analysis of the novel benzylsuccinate synthase reaction for anaerobic toluene activation based on structural studies of the product. J. Bacteriol. 180:5454-5457[Abstract/Free Full Text].
7.	Biegert, T., G. Fuchs, and J. Heider. 1996. Evidence that oxidation of toluene in the denitrifying bacterium Thauera aromatica is initiated by formation of benzylsuccinate from toluene and fumarate. Eur. J. Biochem. 238:661-668[Medline].
8.	Bradford, M. M. 1976. A rapid and sensitive method for the quantitation of microgram quantities of protein utilizing the principle of protein-dye binding. Anal. Biochem. 72:248-254[CrossRef][Medline].
9.	Buckel, W., U. Dorn, and R. Semmler. 1981. Glutaconate CoA-transferase from Acidaminococcus fermentans. Eur. J. Biochem. 118:315-321[Medline].
10.	Buckel, W., V. Buschmeier, and H. Eggerer. 1971. The action mechanism of citrate lyase from Klebsiella aerogenes. Hoppe-Seyler's Z. Physiol. Chem. 352:1195-1205[Medline].
11.	Buckel, W., and A. Bobi. 1975. The enzyme complex citramalate lyase from Clostridium tetanomorphum. Eur. J. Biochem. 64:255-262[CrossRef][Medline].
12.	Coligan, J. E., B. M. Dunn, H. L. Ploegh, D. W. Speicher, and P. T. Wingfield. 1995. Current protocols in protein science. John Wiley & Sons Inc., New York, N.Y.
13.	Cornish-Bowden, A. 1995. Analysis of enzyme kinetic data. Oxford University Press, Oxford, United Kingdom.
14.	Cornish-Bowden, A. 1995. Fundamentals of enzyme kinetics. Oxford University Press, Oxford, United Kingdom.
15.	Corthésy-Theulaz, I. E., G. E. Bergonzelli, H. Henry, D. Bachmann, D. F. Schorderet, A. L. Blum, and N. Ornston. 1997. Cloning and characterization of Helicobacter pylori succinyl-CoA:acetoacetate CoA-transferase, a novel prokaryotic member of the CoA-transferase family. J. Biol. Chem. 272:25659-25667[Abstract/Free Full Text].
16.	Dickert, S., A. J. Pierik, D. Linder, and W. Buckel. 2000. The involvement of coenzyme A esters in the dehydration of (R)-phenyllactate to (E)-cinnamate by Clostridium sporogenes. Eur. J. Biochem. 267:3874-3884[Medline].
17.	Dimroth, P., and H. Eggerer. 1975. Isolation of subunits of citrate lyase and characterization of their function in the enzyme complex. Proc. Natl. Acad. Sci. USA 72:3458-3462[Abstract/Free Full Text].
18.	Dolfing, J., J. Zeyer, P. Binder-Eicher, and R. P. Schwarzenbach. 1990. Isolation and characterization of a bacterium that mineralizes toluene in the absence of molecular oxygen. Arch. Microbiol. 154:336-341[Medline].
19.	Heider, J., A. M. Spormann, H. R. Beller, and F. Widdel. 1999. Anaerobic bacterial metabolism of hydrocarbons. FEMS Microbiol. Rev. 22:459-473[CrossRef].
20.	Heider, J., and G. Fuchs. 1997. Microbial anaerobic aromatic metabolism. Anaerobe 3:1-22.
21.	Hess, A., B. Zarda, D. Hahn, A. Häner, D. Stax, P. Höhener, and J. Zeyer. 1997. In situ analysis of denitrifying toluene- and m-xylene-degrading bacteria in a diesel fuel-contaminated laboratory aquifer column. Appl. Environ. Microbiol. 63:2136-2141[Abstract].
22.	Jacob, U., M. Mack, T. Clausen, R. Huber, W. Buckel, and A. Messerschmidt. 1997. Glutaconate CoA-transferase from Acidaminococcus fermentans: the crystal structure reveals homology with other CoA-transferases. Structure 5:415-426[Medline].
23.	Krieger, C. J., H. R. Beller, M. Reinhard, and A. M. Spormann. 1999. Initial reactions in anaerobic oxidation of m-xylene by the denitrifying bacterium Azoarcus sp. strain T. J. Bacteriol. 181:6403-6410[Abstract/Free Full Text].
24.	Leuthner, B., and J. Heider. 2000. Anaerobic toluene catabolism of Thauera aromatica: the bbs operon codes for the enzymes of $beta$ -oxidation of the intermediate benzylsuccinate. J. Bacteriol. 182:272-277[Abstract/Free Full Text].
25.	Leuthner, B., C. Leutwein, H. Schulz, P. Hörth, W. Haehnel, E. Schiltz, H. Schägger, and J. Heider. 1998. Biochemical and genetic characterization of benzylsuccinate synthase from Thauera aromatica: a new glycyl radical enzyme catalyzing the first step in anaerobic toluene metabolism. Mol. Microbiol. 28:615-628[CrossRef][Medline].
26.	Leutwein, C., and J. Heider. 1999. Anaerobic toluene catabolic pathway in denitrifying Thauera aromatica: activation and $beta$ -oxidation of the first intermediate, (R)-(+)-benzylsuccinate. Microbiology 145:3265-3271[Abstract/Free Full Text].
27.	Mack, M., and W. Buckel. 1995. Identification of glutamate beta 54 as the covalent-catalytic residue in the active site of glutaconate CoA-transferase from Acidaminococcus fermentans. FEBS Lett. 357:145-148[CrossRef][Medline].
28.	Müller, J. A., A. S. Galushko, A. Kappler, and B. Schink. 1999. Anaerobic degradation of m-cresol by Desulfobacterium cetonicum is initiated by formation of 3-hydroxybenzylsuccinate. Arch. Microbiol. 172:287-294[CrossRef][Medline].
29.	Müller, J. A., A. S. Galushko, A. Kappler, and B. Schink. 2001. Initiation of anaerobic degradation of p-cresol by formation of 4-hydroxybenzylsuccinate in Desulfobacterium cetonicum. J. Bacteriol. 183:752-757[Abstract/Free Full Text].
30.	Parales, R. E., and C. S. Harwood. 1992. Characterization of the genes encoding $beta$ -ketoadipate succinyl-coenzyme A transferase in Pseudomonas putida. J. Bacteriol. 174:4657-4666[Abstract/Free Full Text].
31.	Selmer, T., and W. Buckel. 1999. Oxygen exchange between acetate and the catalytic glutamate residue in glutaconate CoA-transferase from Acidaminococcus fermentans: implications for the mechanism of CoA-ester hydrolysis. J. Biol. Chem. 274:20772-20778[Abstract/Free Full Text].
32.	Sidhu, H., S. D. Ogden, H.-Y. Lung, B. G. Luttge, A. L. Baetz, and A. B. Peck. 1997. DNA sequencing and expression of the formyl-coenzyme A transferase gene, frc, from Oxalobacter formigenes. J. Bacteriol. 179:3378-3381[Abstract/Free Full Text].
33.	Sramek, S. J., and F. E. Frerman. 1975. Purification and properties of Escherichia coli coenzyme A-transferase. Arch. Biochem. Biophys. 171:14-26[CrossRef][Medline].
34.	Tschech, A., and G. Fuchs. 1987. Anaerobic degradation of phenol by pure cultures of newly isolated denitrifying pseudomonads. Arch. Microbiol. 148:213-217[CrossRef][Medline].
35.	White, H., and W. P. Jencks. 1976. Properties of succinyl-CoA:3-ketoacid coenzyme A transferase. J. Biol. Chem. 251:1708-1711[Abstract/Free Full Text].
36.	Wiesenborn, D. P., F. B. Rudolph, and E. T. Papoutsakis. 1989. Coenzyme A-transferase from Clostridium acetobutylicum ATCC 824 and its role in the uptake of acids. Appl. Environ. Microbiol. 55:317-322[Abstract/Free Full Text].