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Previous Article | Next Article 
Journal of Bacteriology, April 2000, p. 2238-2244, Vol. 182, No. 8
Division of Microbiology, GBF-National
Research Center for Biotechnology, D-38124 Braunschweig,
Germany,1 and Institut de Biologie
Structurale, IBS-LSMP, F-38027 Grenoble Cedex
1,2 and Départment de
Recherche Fondamentale sur la Matière
Condensée/SCIB/SCPM, Commissariat à l'Energie
Atomique
Received 13 October 1999/Accepted 13 January 2000
The first step in the degradation of dibenzofuran and
dibenzo-p-dioxin by Sphingomonas sp. strain RW1
is carried out by dioxin dioxygenase (DxnA1A2), a ring-dihydroxylating
enzyme. An open reading frame (fdx3) that could potentially
specify a new ferredoxin has been identified downstream of
dxnA1A2, a two-cistron gene (J. Armengaud, B. Happe, and
K. N. Timmis, J. Bacteriol. 180:3954-3966, 1998). In the present
study, we report a biochemical analysis of Fdx3 produced in
Escherichia coli. This third ferredoxin thus far identified
in Sphingomonas sp. strain RW1 contained a
putidaredoxin-type [2Fe-2S] cluster which was characterized by
UV-visible absorption spectrophotometry and electron paramagnetic
resonance spectroscopy. The midpoint redox potential of this ferredoxin
(E'0 = Sphingomonas sp. strain
RW1 was isolated from the River Elbe in Germany on the basis of its
ability to grow aerobically on dibenzofuran and
dibenzo-p-dioxin as the sole sources of carbon and energy
(35). The degradative pathways of these two compounds in RW1
have been extensively studied, resulting in the biochemical and genetic
characterization of the key enzymes. The initial reaction is an
oxygenolytic attack on the carbon atoms adjacent to the ether bridge,
and it is carried out by a three-component dioxin dioxygenase system.
Unlike the well-known class IIB and class III dioxygenases, which
involve electrons provided by a Rieske-type [2Fe-2S] ferredoxin, the
dioxin dioxygenase has been shown to be associated with a
putidaredoxin-type [2Fe-2S] ferredoxin (8). The gene of
this ferredoxin, designated fdx1, has been cloned and
characterized (4), as has the gene of its cognate reductase (5). In this type of ferredoxin, the prosthetic group is
coordinated with the polypeptide by four cysteine residues arranged in
the pattern
Cys-X5-Cys-X2-Cys-Xn-Cys and thus
differs significantly from the Rieske-type [2Fe-2S] ferredoxins
containing a [2Fe-2S] cluster bound to the polypeptide by two
cysteine and two histidine residues. The nature and the position of the
ligands influence the properties of the Fe-S cluster. The ferredoxins
containing a Rieske-type cluster exhibit a high redox potential ( In a recent report (2), we described the cloning and
characterization of the cistrons coding for the two subunits of the dioxin dioxygenase. Surprisingly, an open reading frame encoding a
putative polypeptide exhibiting similarity to Fdx1 is located 1,923 nucleotides downstream of these two cistrons (6). The product of this gene, Fdx3, is thus an alternative candidate for the
electron donor of the dioxin dioxygenase. In order to facilitate the
isolation and biochemical characterization of the fdx3
product, an expression system was designed to allow purification from
Escherichia coli of a recombinant holoferredoxin. The
biochemical, spectroscopic, and redox properties of this third
ferredoxin identified in Sphingomonas sp. strain RW1 are
presented in this study and compared with those of Fdx1.
Bacterial strains, plasmids, and reagents.
Restriction
enzymes and reagents for genetic procedures were purchased from New
England Biolabs, Boehringer Mannheim, Promega, United States
Biochemicals, and Sigma. The medium used for bacterial growth was
Luria-Bertani medium. The bacterial strains, plasmids, and
oligonucleotides used in this study are listed in Table
1 and 2.
0021-9193/00/$04.00+0
Copyright © 2000, American Society for Microbiology. All rights reserved.
A Second [2Fe-2S] Ferredoxin from Sphingomonas sp.
Strain RW1 Can Function as an Electron Donor for the Dioxin
Dioxygenase
Grenoble, 38054 Grenoble Cedex 9,3
France
ABSTRACT
Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
247 ± 10 mV versus normal hydrogen
electrode at pH 8.0) is similar to that exhibited by Fdx1 (245 mV), a
homologous ferredoxin previously characterized in
Sphingomonas sp. strain RW1. In in vitro assays, Fdx3 can
be reduced by RedA2 (a reductase similar to class I cytochrome P-450
reductases), previously isolated from Sphingomonas sp.
strain RW1. RedA2 exhibits a Km value of
3.2 ± 0.3 µM for Fdx3. In vivo coexpression of fdx3
and redA2 with dxnA1A2 confirmed that Fdx3 can
serve as an electron donor for the dioxin dioxygenase.
INTRODUCTION
Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
150
mV for ferredoxins associated with class IIB dioxygenases
[19]), whereas putidaredoxin-type [2Fe-2S]
ferredoxins exhibit lower redox potentials (4, 12, 13), and
ferredoxins containing a plant-type [2Fe-2S] cluster, also bound to
the polypeptide by four cysteines, have even lower potential (9,
14, 33).
MATERIALS AND METHODS
Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
TABLE 1.
E. coli strains and plasmids used in
this study
TABLE 2.
Oligonucleotides used in this study
Construction of the expression system pAJ147.
Standard DNA
manipulations were carried out as described by Sambrook et al.
(30). NdeI and BamHI restriction sites
were introduced by PCR amplification at the 5' and 3' ends of the
fdx3 gene, respectively. Oligonucleotides AJ286 and AJ287
were synthesized for this purpose on an Applied Biosystems DNA
synthesizer model 381A and used as primers without further
purification. The PCR was performed as previously described for the
amplification of another ferredoxin gene (3). Cosmid pAJ114
(2), isolated and purified with the Qiawell-8 kit (Qiagen),
was used as a PCR template. A fragment of the predicted size (340 bp)
was purified from a 2% agarose gel by means of a QiaexII extraction
kit (Qiagen) and cloned into pGEM-T plasmid (Promega) to produce
plasmid pAJ146. The integrity of the insert was verified by restriction
analysis with NotI-PstI double digestion,
followed by DNA sequencing. Nucleotide sequencing was performed on a
double-stranded template, prepared by means of a Qiawell-8 kit
(Qiagen). Sequencing reactions were carried out with an Applied
Biosystem DNA sequencing kit in the presence of 5% dimethyl sulfoxide,
and processed on a 373 Stretch Applied Biosystems automated sequencer.
The 326-bp fragment encompassing fdx3 was excised from
pAJ146 by restriction with NdeI and BamHI, purified, and ligated into the expression plasmid pET9a, which had been
digested with the same endonucleases. The plasmid generated, pAJ147,
contains the ferredoxin gene inserted downstream of the 
10 promoter.
Expression of fdx3 and purification of the
recombinant ferredoxin.
Plasmid pAJ147 was introduced into
E. coli BL21(DE3). The resulting strain was cultivated at
30°C in LB medium supplemented with 50 µM
Fe2(SO4)3 and 50 µg of kanamycin
per ml. Expression of fdx3 was induced with 0.5 mM IPTG
(isopropyl-
-D-thiogalactopyranoside) when cultures
reached an optical density at 600 nm of 0.8. Cells from 6 liters of
culture were harvested 3 h after induction and washed with 0.5 liters of 50 mM Tris-HCl-15 mM EDTA (pH 8.0). The cell paste obtained
after centrifugation was frozen in liquid nitrogen and kept at
70°C. Purification of the ferredoxin was carried out according to a
protocol based on that described for the purification of Fdx1
(4). Briefly, the cell pellet was thawed on ice and then
resuspended in 110 ml of 100 mM Tris-HCl-15 mM EDTA (pH 8.0),
containing 1 mM dithiothreitol. All steps were subsequently performed
at 4°C. Cells were broken by means of a French pressure cell (Aminco
Corp.) operated as recommended by the supplier at a pressure of 1,000 lb/in2. The crude extract was centrifuged at
18,000 × g for 30 min. The resulting supernatant fluid
was diluted twofold in 25 mM Tris-HCl-1 mM EDTA (pH 8.0) containing 1 mM dithiothreitol (buffer A) and loaded onto a 20-ml Fast-flow
DEAE-Sepharose mixture (Amersham Pharmacia Biotech) poured into a 2.5-cm-diameter Econo-column (Bio-Rad) previously equilibrated in
buffer A. After a 2-column-volume wash with buffer A containing 100 mM
NaCl, a reddish protein fraction was eluted with buffer A containing
500 mM NaCl. The DEAE fraction was concentrated to 3 ml by
ultrafiltration with an Amicon filtration unit, loaded onto a 120-ml
Superdex 200 gel filtration 1.6-cm-diameter column (Amersham
Pharmacia Biotech), and eluted with buffer A containing 100 mM NaCl at
a flow rate of 0.5 ml/min. The red fraction collected in a 6-ml volume
was concentrated a second time with an Amicon filtration unit and
desalted by repeated cycles of concentration and dilution. Finally, the
protein was applied to a 5-ml Mono-Q (Amersham Pharmacia Biotech) 1.0-cm-diameter Econo-column (Bio-Rad) which was developed with a
30-min linear gradient from 0 to 500 mM NaCl in buffer A by using an
Amersham Pharmacia Biotech fast protein liquid chromatography system at
a flow rate of 1 ml/min. Fdx3 eluted at approximately 250 mM NaCl and
was desalted by dialysis against buffer A. The purified protein was
concentrated on an Amicon filtration unit and stored in liquid
N2.
Analytical methods. Protein concentration determination, sodium dodecyl sulfate-polyacrylamide gel electrophoresis (SDS-PAGE), molecular weight determination, UV-visible absorption spectrophotometry, electron paramagnetic resonance (EPR) spectroscopy, and electrospray mass spectrometric measurements were carried out as previously described (1, 3). The redox potential of the [2Fe-2S] cluster of the recombinant Fdx3 was determined spectrophotometrically with 5-deazariboflavin as a photoreductant and phenosafranin as a redox indicator. By means of the Nernst equation, the intermediate redox potentials were determined by stepwise photoreduction of Fdx3 at 25°C (pH 8.0) inside an anaerobic glove box and measurement of the extent of phenosafranin reduction, as A250, and the ratio of the oxidized and reduced forms of Fdx3, calculated from the absorption at 410 nm. Cuvettes of a 0.2-cm light path contained 8 µM 5-deazariboflavin, 16 mM sodium oxalate, 52.6 µM phenosafranin, and 100 µM Fdx3 in 25 mM potassium phosphate buffer (pH 8.0).
In vitro electron transfer assays.
Recombinant reductase
RedA2 and ferredoxin Fdx1, used as a control, were purified as
previously described (5) with E. coli BL21(DE3)(pAJ111) and E. coli BL21(DE3)(pAJ104) cells,
respectively. RedA2 activity was routinely assayed as reduction of
2,6-dichlorophenolindophenol (Cl2IND) at 25°C, monitored
at 600 nm in a UV-2401 PC Shimadzu UV-visible recording
spectrophotometer under the same conditions as previously reported
(5) and assuming a molar absorption coefficient of
600nm = 20.6 mM
1 · cm1 (10). The assay system contained 100 µM
Cl2IND, 150 µM NADH, and 6.8 nM RedA2 in 50 mM Tris-HCl
(pH 8.0). In addition, ferredoxin-dependent cytochrome c
reduction was measured by the decrease in A550
by using a molar absorption coefficient of 550nm = 20 mM1 · cm1 (10). In
this case, the reaction mixture (0.5 ml) contained 50 µM cytochrome
c, 150 µM NADH, various amounts (from 2 to 20 µM) of
ferredoxin Fdx3 (or Fdx1 as a control), and 22.7 nM RedA2 in 50 mM
Tris-HCl (pH 8.0). The reductase was shown to not directly reduce
cytochrome c under these conditions. The
Km value for Fdx3 and corresponding standard
deviation were determined from a linear regression algorithm of
Lineweaver-Burk plots made in duplicate from independent kinetic data
obtained at 25°C. RedA2 activity was measured as a function of NADH
concentration in the presence of Cl2IND as an electron
acceptor and as a function of Fdx3 concentration in the cytochrome
c-Fdx3-dependent reduction.
Construction of a redA2/fdx3 expression vector and resting cell assays. A 1,289-bp fragment containing the redA2 gene and 23 upstream nucleotides, which includes the putative ribosome binding site of redA2, was PCR amplified from cosmid pAJ108 with the oligonucleotides AJ317 and AJ316, which introduced EcoRI and NotI restriction sites at the 5' and 3' ends of this fragment, respectively. A fragment of the predicted size was purified from a 1% agarose gel and cloned into the pGEM-T plasmid to generate plasmid pAJ128. A 555-bp fragment containing the fdx3 gene was also PCR amplified from cosmid pAJ114 by means of oligonucleotides AJ320 and AJ321, which introduced NotI and BamHI sites at the 5' and 3' ends of the fragment, respectively. A fragment of the predicted size was purified from a 1% agarose gel and cloned into pGEM-T plasmid to generate plasmid pAJ148. The integrity of the two PCR-amplified fragments was checked by sequencing both strands. Plasmids pAJ128 and pAJ148 were digested with NotI and EcoRI and with NotI and BamHI, respectively, and the resulting 1,262- and 541-bp fragments were purified and ligated to EcoRI- and BamHI-cleaved plasmid pBluescript II KS to produce plasmid pAJ149 carrying the redA2 and fdx3 genes expressed from the Plac promoter.
Dioxin dioxygenase activity in resting cells of E. coli DH5
(pAJ127)(pAJ149), with E. coli DH5(pAJ127)(pAJ130)
as a control, cultured in LB medium containing 30 µg of kanamycin per
ml and 100 µg of ampicillin per ml was measured under conditions
identical to those previously described (2). Relative
activities correspond to the average of activities measured in
duplicate assays after 1, 2, and 3 h of incubation.
Secondary structural element prediction and three-dimensional structure modeling. Prediction of secondary structural elements of Fdx1 and Fdx3 was carried out by using the Jpred2 resources (a consensus method for protein secondary structure prediction) of the EMBL-European BioInformatics Institute (http://jura.ebi.ac.uk:8888/). A three-dimensional structural model was calculated according to the method of Lund et al. (20) by using the CPHmodels resources from the Center for Biological Sequence analysis (http://genome.cbs.dtu.dk/services/CPHmodels) from the amino acid sequences of Fdx1 and Fdx3 with the putidaredoxin three-dimensional structure (28) as a template. The three-dimensional structures were viewed with WebLab ViewerPro 3.0 software (Molecular Simulations, Inc.).
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RESULTS |
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Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
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Expression of the fdx3 gene and purification of the
product.
Cells of E. coli strain BL21(DE3) carrying
plasmid pAJ147, which contains the fdx3 gene downstream of a
T7 expression system and optimized translational signals, were induced
with IPTG for 3 h. Analysis of cell extracts by SDS-PAGE revealed
the accumulation of a polypeptide with an apparent molecular mass lower
than 14 kDa (Fig. 1, lane 1). The
recombinant ferredoxin was also seen as a brown band migrating close to
the buffer front in a 10% native polyacrylamide gel (Fig. 1, lane 4),
which suggested that this protein was produced in a holoform.
Recombinant Fdx3 was purified by a simple three-step purification
protocol, previously used for Fdx1, a protein exhibiting a similar
theoretical isoelectric point and molecular weight (4), and
consisting of DEAE-Sepharose chromatography followed by gel filtration
on a Superdex 200 Prep Grade column and Mono-Q chromatography. One
major contaminant protein, 18 kDa in size, was still present at this
stage (Fig. 1, lane 3) and could not be removed without a dramatic
decrease in the holo-Fdx3/apo-Fdx3 ratio. The purification yielded
approximately 2.3 mg of recombinant Fdx3 per liter of culture.
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Biochemical and spectroscopic characterization of recombinant Fdx3. (i) Biochemical properties. The purified recombinant Fdx3 was subjected to electrospray mass spectrometry in the positive mode. The average mass of the apoferredoxin (11,259 ± 3 Da) determined by electrospray ionization mass spectrometry matches within 3 Da the expected mass calculated from the nucleotide-derived amino acid sequence with the initial methionine removed (11,262 Da). The removal of the initial methionine was expected (the second amino acid residue in the polypeptide chain is a proline, a small-side-chain-length residue [10]), despite the high levels of expression, because efficient processing of the N-terminal amino acid has been previously observed in E. coli in such cases (32). The molecular mass of the purified Fdx3 was determined to be 13 ± 2 kDa by gel filtration on a calibrated Superdex 200 Prep Grade chromatography column. Therefore, this ferredoxin behaves as a monomeric protein under the conditions employed. The recombinant Fdx3 exhibits behavior similar to that of Fdx1 (Fig. 1, lanes 5 and 6) during electrophoresis on a 10% polyacrylamide gel, under nondenaturing conditions. In that case, both proteins (which have close molecular masses), present very theoretical acidic isoelectric points (3.9 to 4.0) and migrate close to the buffer front. They thus have similar physicochemical properties.
(ii) Spectroscopic properties. The UV-visible absorption spectrum of recombinant Fdx3 in the oxidized state shows the general features of a ferredoxin containing a [2Fe-2S] cluster. In the native state, broad charge transfer bands centered around 314, 412, and 460 nm were evident. These maxima are typical of ferredoxins containing a putidaredoxin-type [2Fe-2S] cluster and differ slightly from those of ferredoxins containing a plant-type [2Fe-2S] cluster characterized by a maximum at 420 nm rather than 414 nm. They strongly differ from those of ferredoxins containing a Rieske-type [2Fe-2S] cluster, which exhibit maxima at 325 and 460 nm with a broad shoulder around 575 nm (11, 31), or containing a [3Fe-4S] or [4Fe-4S] cluster, which are both characterized by broad charge transfer bands around 390 to 410 and 280 to 300 nm (15, 16). Upon reduction with excess dithionite, the recombinant ferredoxin changes color, and the UV-visible absorption spectrum shows only one maximum, centered at 538 nm, as is the case with other reduced ferredoxins containing a [2Fe-2S] cluster (3).
The [2Fe-2S] cluster in Fdx3 was further characterized by EPR spectroscopy. In the native state, the recombinant ferredoxin is EPR silent, whereas in the dithionite-reduced state, a nearly axial signal with apparent g values at 1.92, 1.94, and 2.02 was evident (Fig. 2). This EPR signal is typical of a ferredoxin containing a putidaredoxin-type [2Fe-2S] cluster. A comparison of the EPR spectra of reduced Fdx1 and Fdx3 shows a very minor difference at high field strength, the Fdx1 signal being slightly more axial, suggesting that the geometries of their Fe-S clusters are highly similar. This indicates that the environments of the Fe-S cluster are probably nearly the same in both proteins.
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Electron transfer properties of recombinant Fdx3. (i) Determination
of the midpoint redox potential.
The redox potential of the
[2Fe-2S] cluster of the recombinant Fdx3 was determined
spectrophotometrically as described in Materials and Methods. The
midpoint redox potential obtained was E0' = 247 (± 10) mV
versus that of the normal hydrogen electrode. This potential is in the
range of values reported for homologous ferredoxins (4, 12,
13), except for the hydrogenosomal [2Fe-2S] ferredoxin from the
protozoan Trichomonas vaginalis, which exhibits an atypical
redox potential of 347 mV (34).
Cytochrome c-mediated reduction.
Purified
recombinant RedA2 flavoprotein exhibited a specific activity of 95 µmol · min1 · mg1 in the
Cl2IND reduction assay and 0.54 µmol · min1 · mg1 in the Fdx3-dependent
cytochrome c reduction assay. The specific activity of RedA2
in the same assay carried out with Fdx1 is similar (0.55 µmol
· min1 · mg1). The
Km value for Fdx3 was determined to be 3.2 ± 0.3 µM, slightly lower than that recorded for Fdx1, 3.7 ± 0.4 µM, but statistically, the measured values were not significantly different.
The recombinant Fdx3 is able in vivo to transfer electrons to the
dioxin dioxygenase.
The dioxin dioxygenase DxnA1A2 has been
previously shown to function efficiently with Fdx1 and RedA2, when
expressed from a two-plasmid expression system in E. coli
DH5 cells (2). We designed a new two-expression system by
using the pAJ127 plasmid containing the cistrons of the and subunits and the pAJ149 plasmid containing the genes of the Fdx3
ferredoxin and the RedA2 reductase from Sphingomonas sp.
strain RW1. These two plasmids are derivatives of pBBR1-MCS2 and
pBluescript, respectively, and are therefore compatible with one
another. The levels of expression of dxnA1, like those of
dxnA2, in both strains were estimated to be similar. Dioxin
dioxygenase activity in the Fdx3 strain E. coli
DH5(pAJ127)(pAJ149) and in the Fdx1 strain E. coli
DH5(pAJ127)(pAJ130) was measured as conversion of dibenzofuran and
dibenzo-p-dioxin to 2,2',3-trihydroxybiphenyl (2,2',3-THB)
and 2,2',3-trihydroxydiphenyl-ether (2,2',3-THD-ether), respectively.
Both bacteria exhibited similar activities toward both substrates (for
the Fdx3 strain, 17 ± 4 nmol of 2,2',3-THB/min/mg of protein
formed from dibenzofuran and 16 ± 4 nmol of
2,2',3-THD-ether/min/mg of protein formed from dibenzo-p-dioxin). In all cases, only one product was formed
by the dioxygenase from each substrate tested: namely 2,2',3-THB from
dibenzofuran, with UV-visible maxima at 206, 244, and 283 nm; and
2,2',3-THD-ether from dibenzo-p-dioxin, with maxima at 202 and 275 nm, both of which are produced via an angular attack at carbons
involved in the bridges of the multi-ring aromatic molecules.
Predicted secondary structural elements and three-dimensional
structure modeling.
At present some experimental three-dimensional
data for [2Fe-2S] putidaredoxin-type ferredoxins are available: two
models for the solution structure of putidaredoxin (27) and
terpredoxin (21) were obtained from nuclear magnetic
resonance data, and the structure of a truncated version of bovine
adrenodoxin (Adx4-108) was obtained after crystallization and X-ray
diffraction analysis (22). A multiple alignment of sequences
homologous to Fdx1 and Fdx3 and a prediction of the secondary structure
of these ferredoxins were obtained by a consensus method
(http://jura.ebi.ac.uk:8888/). The predicted presence of three
-helices and several -sheets in these two metalloproteins is in
agreement with the secondary structural elements observed in
putidaredoxin and adrenodoxin structures (23). This
indicates that the global folds among all the putidaredoxin-type
ferredoxins should be close, the [2Fe-2S] cluster environment being
the most similar. In order to spatially locate the 25 amino acids
differing in these two ferredoxins, three-dimensional structural models
of Fdx1 and Fdx3 were designed by comparative modeling with
putidaredoxin structure coordinates as a template, using a fully
automated structure prediction web server (20). Fourteen out
of these 25 residues are conservatively replaced and can be considered
to not drastically modify the structure and therefore the function of
the protein. The 11 nonconserved residues are indicated in the
Fdx1/Fdx3 model (Fig. 3). The major differences between Fdx1 and Fdx3 are located on the molecular surface
formed by juxtaposition of an N-terminal loop with the C terminus of
the molecule, the position of which is probably influenced by the
residue at position 102 (a proline in Fdx1 replaced by a serine in
Fdx3). The global charge distributions in this region are similar in
both proteins in accordance with the electric dipole vector
configuration detected in [2Fe-2S] ferredoxins (23). However, local changes should modify the contact sites with possible interacting partners. (Two negatively charged residues, one positively charged residue, and one neutral residue in Fdx1 are modified for one
negatively charged residue and three neutral residues in Fdx3.) The
second molecular surface containing four nonconserved residues
(residues 59, 63, 65, and 67) is located opposite the former, the
accessible surface being less polar in Fdx1 than in Fdx3 (Fig. 3).
These differences, except G59S, do not affect the two short -helices
(the bottom of the model presented in Fig. 3) known to be implemented
in the interaction between putidaredoxin and putidaredoxin reductase
(28). These differences should reflect the functional
importance of these molecular surfaces. This structural model indicates
that the two ferredoxins should function with very similar mechanisms,
but may differ in at least one of their physiological partners.
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DISCUSSION |
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Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
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The initial step in dibenzo-p-dioxin and dibenzofuran degradation by Sphingomonas sp. strain RW1 is carried out by a class IIA dioxygenase system. This is a multicomponent enzyme that functions with a reductase and a ferredoxin. From RW1 bacteria grown on salicylate, a monocyclic intermediate compound in the dibenzofuran degradation pathway, Bünz and Cook (8) have previously purified a ferredoxin (Fdx1) able to transfer electrons to the dioxin dioxygenase DxnA1A2 and two reductases (RedA1 and RedA2) which can transfer electrons from NADH to this ferredoxin. A new ferredoxin gene (fdx3) was recently identified downstream of the dxnA1A2 genes encoding the dioxygenase (6). The expression system based on the T7 promoter we developed and the three-step purification procedure described in this report allowed us to obtain milligram quantities of recombinant Fdx3 holoferredoxin. EPR analysis showed it to contain a putidaredoxin-type [2Fe-2S] cluster. Analysis of the redox properties of this new ferredoxin confirmed the strong similarity of Fdx3 and Fdx1 in the [2Fe-2S] cluster environment, even though their polypeptide chains differ in 25 of their 105 amino acids. A detailed comparison of Fdx1 and Fdx3 by using a three-dimensional model based on putidaredoxin structure confirms this point and pinpoints the major differences at two molecular surfaces on the proteins. This indicates that the two ferredoxins may differ in at least one of their physiological partners.
The Fdx1 ferredoxin was shown to represent up to 5% of total protein
in exponentially growing bacteria, and Fdx1 was thus concluded to be
the electron donor of the dioxin dioxygenase (8). However,
we show here that Fdx3 has biochemical, spectroscopic, and redox
properties strikingly similar to those of Fdx1. The two isoferredoxins
are able to convey electrons from the reductase RedA2 to the
dioxygenase DxnA1A2, but the exact nature of the partners of the two
ferredoxins in Sphingomonas sp. strain RW1 remains to be
clarified. The Fdx3 ferredoxin from Sphingomonas sp. strain
RW1 shares 35 to 45% identity with a ferredoxin from Rhodococcus sp. strain NI86/21 (24), the
putidaredoxin from Pseudomonas putida (17, 25),
and the terpredoxin from a Pseudomonas strain
(26). These three ferredoxins are involved in electron transfer to monooxygenases involved in the degradation of
S-ethyl-dipropyl-carbamothioate, camphor, and -terpineol,
respectively. In these cases, the ferredoxin genes are located just
upstream (rhodocoxin) or downstream (putidaredoxin and terpredoxin) of
the gene of the cognate reductase and are probably cotranscribed.
Tentative identification of the physiological partner of the reductase
or the ferredoxin is therefore straightforward. In
Sphingomonas sp. strain RW1, however, the genes encoding
Fdx3 and Fdx1 are not located in the neighborhood of a reductase or oxidoreductase, and hence genetic evidence for partnership is lacking.
The generation of knockout mutants will probably not clarify this
point, since both the two ferredoxins and the two reductases have
similar properties and thus constitute genetic redundancy. The
existence in some bacteria of a multiple catabolic enzyme system, such
as ring-cleavage dioxygenasesthree in the polychlorobiphenyl-degrading bacterium Rhodococcus
globerulus P6 (7) and up to seven in Rhodococcus
erythropolis TA421 (18) and of several
ring-hydroxylating dioxygenasesat least four in Sphingomonas sp. strain RW1 (2) and five in
Sphingomonas aromaticivorans strain F199 (29)is
now well established. Such a diversity of isoenzymes in the same
organism is often interpreted to reflect a broader spectrum of
substrates that the microorganism can handle under disparate
environmental conditions than could be metabolized by a pathway
containing unique enzymes. However, the presence in
Sphingomonas sp. strain RW1 of two complete electron
transport chains composed of two isoferredoxins (Fdx1 and Fdx3) and two isoreductases (RedA1 and RedA2) seems to be redundant, because they
appear to be biochemically equivalent, at least as far as electron
transfer to the dioxin dioxygenase is concerned. Whether or not these
two systems are truly redundant, or each serves one function but lacks
a distinct metabolic role, should be resolved by estimation of in vivo
concentrations of Fdx1 and Fdx3 in Sphingomonas sp. strain
RW1 and analysis of the regulation of their expression.
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ACKNOWLEDGMENTS |
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We gratefully acknowledge Y. Jouanneau (CEA-Grenoble, Grenoble, France) for welcoming us to his team and allowing us to use his facilities for redox potential measurements.
This research was funded in part by the German Ministry for Education and Research (BMBF grant no. 0318896C). K. N. Timmis gratefully acknowledges the generous support of the Fonds der Chemischen Industrie.
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FOOTNOTES |
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* Corresponding author. Mailing address: Institut de Biologie Structurale, IBS-LSMP, 41 Rue Jules Horowitz, F-38027 Grenoble Cedex 1, France. Phone: (33) 4 76 88 30 37. Fax: (33) 4 76 88 54 94. E-mail: jean.armengaud{at}ibs.fr.
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REFERENCES |
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Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
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