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Applied and Environmental Microbiology, February 2001, p. 591-597, Vol. 67, No. 2
Laboratory of Microbiology, Wageningen
University, NL-6703 CT Wageningen, The Netherlands
Received 6 September 2000/Accepted 2 November 2000
Efficient host-vector systems have been developed for the
versatile, strictly anaerobic, halo- and fumarate-respiring
gram-positive bacterium Desulfitobacterium
dehalogenans. An electroporation-based transformation
procedure resulting in approximately 103 to 104
transformants per µg of the cloning vector pIL253 was developed and validated. The broad-host-range vector pG+host9 was
shown to replicate at a permissive temperature of 30°C, whereas the
replicon was not functional at 40°C. The D. dehalogenans frdCAB operon, predicted to encode
a fumarate reductase, was cloned, characterized, and targeted for
insertional inactivation by pG+host9 carrying a
0.6-kb internal frdA fragment. Single-crossover integration
at the frdA locus occurred at a frequency of 3.3 × 10 It has been shown for a wide range
of haloorganic compounds that reductive dechlorination is the
first crucial step in the degradation of such pollutants (15,
25). Halorespiring bacteria have received increasing attention
during the past decade due to a significant contribution to reductive
dehalogenation processes occurring in anoxic polluted environments such
as soils, aquifers, and sediments (14, 24). In contrast to
the cometabolic reductive dehalogenation catalyzed by various
metal-containing tetrapyrrol cofactors in a variety of anaerobic
bacteria, this reaction is catalyzed at much higher rates by specific
enzymes in halorespiring microbes, where it is coupled to energy
conservation by electron transport-coupled phosphorylation (14,
18, 31). One of these strains is the versatile, low-G+C,
gram-positive bacterium Desulfitobacterium dehalogenans, which is able to link the oxidation of
several electron donors such as hydrogen, formate, lactate, and
pyruvate to the reduction of various organic and inorganic acceptors,
including ortho-chlorinated phenols (o-CP),
fumarate, and nitrate (37). Recently, the
o-CP-reductive dehalogenase (CPR) from D. dehalogenans has been purified and characterized at
the biochemical and genetic levels (33, 39). Comparison
with other chloroalkene- and haloaromate-reductive dehalogenases
isolated and characterized from various phylogenetically distinct
halorespiring bacteria indicated that these enzymes share significant
similarities in both structural and functional properties, suggesting
that they constitute a novel class of corrinoid-containing reductases
(for recent reviews, see references 18 and 31).
The detailed molecular analysis of the cpr gene cluster in
D. dehalogenans led to the identification
of genes encoding putative regulatory proteins and protein-folding
catalysts, the transcription of which was specifically induced under
halorespiring conditions. From these results, their potential
involvement in regulation and maturation of the reductive dehalogenase
complex has been suggested (33). Additional
genomic loci that appear essential for functional
o-CP respiration of D. dehalogenans have been identified by means of random
chromosomal integration of the conjugational transposon
Tn916 (32). Nevertheless, detailed structural
and functional analysis of these proteins has been hampered by the absence of genetic techniques for D. dehalogenans, including transformation, gene cloning,
and specific gene disruption and insertion. Moreover, the development
of such genetic modification tools would also enable the design of
strains with improved performance in the bioremediation of polluted
environments (19, 35).
Host-vector systems that allow for the genetic, metabolic, and protein
engineering of low-G+C gram-positive bacteria (LGB) have been developed
and optimized mainly for industrially applied strains of lactic acid
bacteria, for bacilli, and, to a lesser extent, for clostridia (for
reviews see references (10 to 12 and 41). It has been
shown that vectors based on the theta replicon of the broad-host-range
conjugative plasmid pAM The main objectives of this study were (i) to develop an efficient
protocol for the transformation of D. dehalogenans, (ii) to investigate the suitability of
gene transfer systems previously developed for other LGB, (iii) to
confirm temperature-sensitive replication of pG+host9 in
D. dehalogenans, and (iv) to demonstrate its
applicability for specific gene disruption using the putative fumarate
reductase-encoding frdA gene as a model target.
Materials.
All gases were obtained from Hoek Loos (Schiedam,
The Netherlands). When appropriate, experiments were carried out in an
anaerobic glove box (Coy Laboratory Products, Grass Lake, Mich.) under
an atmosphere of 96% N2 and 4% H2. The oxygen
concentration was kept low with the palladium catalyst RO-20, provided
by BASF (Arnhem, The Netherlands).
Bacterial strains, plasmids, and culture conditions.
D. dehalogenans strain JW/IU-DC1 (DSM 9161)
(37) was routinely grown under anaerobic conditions (gas
phase, 100% N2) at 37°C in basal mineral medium as
described by Neumann et al. (26), supplemented with 0.1%
peptone, 30 mM NaHCO3, and trace elements and vitamin
solution as recommended by the German Collection of Microorganisms
and Cell Cultures (Brunswick, Germany). An electron donor and an
electron acceptor were added to the appropriate concentrations from
sterile anaerobic stock solutions.
0099-2240/01/$04.00+0 DOI: 10.1128/AEM.67.2.591-597.2001
Copyright © 2001, American Society for Microbiology. All rights reserved.
Development of a Gene Cloning and Inactivation
System for Halorespiring Desulfitobacterium
dehalogenans
ABSTRACT
Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
4 per cell and resulted in partially impaired fumarate
reductase activity. The gene cloning and inactivation systems described here provide a solid basis for the further elucidation of the halorespiratory network in D. dehalogenans and
allow for its further exploitation as a dedicated degrader.
INTRODUCTION
Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
1 (6), among which are the
cloning vectors pIL252 and pIL253, are functional in all genera of LGB
studied, indicating their potential use for halorespiring genera of
LGB, such as Desulfitobacterium and Dehalobacter (12, 30). Similarly, vectors of the pG+host
series of thermosensitive derivatives of yet another broad-host-range plasmid, pWV01, have been proven to be instrumental for high-efficiency gene inactivation, replacement, and insertional mutagenesis, especially in poorly transformable LGB (2, 12, 22, 23).
MATERIALS AND METHODS
Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
DNA isolation and manipulation. Total DNA of D. dehalogenans was isolated as described previously (39). Plasmid DNA was isolated from E. coli by using the alkaline lysis method, and standard DNA manipulations were performed according to established procedures (28) and manufacturers' instructions. Isolation of plasmid DNA from L. lactis was performed as described previously (13). L. lactis was transformed according to the method of Wells et al. (40). Large-scale preparations of plasmid DNA (pIL253, pG+host9) were purified by CsCl density gradient centrifugation (28).
Enzymes were purchased from Life Technologies B.V. (Breda, The Netherlands), Roche Molecular Biochemicals (Mannheim, Germany), or New England Biolabs (Beverly, Mass.). Oligonucleotides were obtained from Eurogentec (Seraing, Belgium), Life Technologies Inc., and MWG Biotech (Ebersberg, Germany). PCR products were purified prior to subsequent manipulation using the QIAquick PCR purification kit (Qiagen GmbH, Hilden, Germany).Transformation procedure and competence of D. dehalogenans.
For the transformation of D. dehalogenans, the electroporation-based method
described by Wells et al. (40) was modified and optimized
for use with anaerobic bacteria. Cells of D. dehalogenans were grown in the presence of 40 mM
glycine with 20 mM lactate as the electron donor and 20 mM fumarate as
the electron acceptor. Unless otherwise indicated, all subsequent steps
were carried out in the anaerobic glove box. Exponentially growing
cells were harvested at an A600 of approximately
0.2 by centrifugation at 2,600 × g for 10 min at 4°C
and then resuspended in 0.15 volume of ice-cold anaerobic washing
buffer (0.5 M sucrose-10% glycerol). Cells were recovered by
centrifugation at 4,000 × g for 10 min at 4°C,
washed with 0.05 volume of washing buffer, recentrifuged, and finally
resuspended in 0.001 volume of washing buffer. For electroporation, DNA
was added in 0.5 to 1.0 µl of deionized water to 40 µl of
concentrated cell suspension and transferred to precooled 0.2-cm
electroporation cuvettes. A single pulse was applied outside the glove
box at different settings (field strength, 12.5 kV · cm1; capacitance, 25 µF; resistance, 200 to 800 
)
using a Gene Pulser (Bio-Rad, Hercules, Calif.). Immediately after
electroporation, cells were moved back into the anaerobic glove box,
mixed with 0.96 ml of recovery medium (growth medium containing 20 mM
lactate and fumarate and 0.5 M sucrose), and incubated at 37°C for
5 h. To determine the influence of the transformation procedure on the viability of D. dehalogenans, appropriate
dilutions were inoculated onto plates without erythromycin containing
20 mM lactate and fumarate as described previously (32).
Transformants were selected on plates containing 20 mM lactate and
fumarate and 5 µg of erythromycin/ml. Further subcultivation of
single colonies in liquid medium was performed as described previously
(32). Plasmid DNA was isolated from D. dehalogenans using a protocol modified from reference 13. Briefly, protoplasts were prepared from 12 ml of
early-stationary-phase culture in 250 µl of THMS buffer (30 mM
Tris-HCl [pH 8.0] and 3 mM MgCl2 in 25% sucrose)
containing 20 mg of lysozyme/ml (38). Subsequently,
plasmid DNA was purified by alkaline lysis and recovered by isopropanol
precipitation. Agarose gel electrophoresis and Southern blot analysis
were used to check for the presence of plasmids.
Thermosensitivity of pG+host9 in D. dehalogenans.
To determine the segregational
stability of the thermosensitive vector pG+host9 in
D. dehalogenans, an early-stationary-phase
culture of plasmid-carrying D. dehalogenans that
was grown in the presence of 40 mM pyruvate and 5 µg of
erythromycin/ml at 30°C was diluted 40-fold into medium without
antibiotics and incubated at 30°C to stationary phase (0 h). This
culture was then diluted 100-fold into fresh medium without antibiotics
and incubated at 30, 37, and 40°C. Appropriate dilutions were
inoculated onto plates with or without erythromycin (5 µg/ml) at 0.1, 16, and 40 h after dilution and were incubated at 30°C. After
40 h of growth, all cultures had reached stationary phase.
Cultures were again diluted 10-fold and kept for an additional 24 h at the respective temperatures until stationary phase was reached (68 h). Total DNA was isolated from samples taken at 0, 40, and 68 h,
digested with EcoRI, and analyzed by Southern blot analysis.
Linearized pG+host9 was used as a plasmid-specific probe
for hybridization. Hybridization with a probe specific for the D. dehalogenans frdAC genes was used as an internal
standard. This probe was a PCR product obtained with primers BG355
(positions 942 to 974 of the frd gene cluster) and IK04
[5'-(A/G)TG NGC NCC NC(G/T) NS(A/T) (C/T)TC-3'; positions 3157 to 3140 of the frd gene cluster] (see
below and Fig. 3). A Hybond-N+ nylon transfer membrane
(Amersham Life Science, Little Chalfont, United Kingdom) was used for
Southern blot analysis, and probes for hybridization experiments were
labeled by nick translation in the presence of
[
-32P]dATP (Amersham Pharmacia Biotech).
Cloning of a putative fumarate reductase-encoding operon. The degenerated primers IK01 [5'-GA(A/G) (A/G/T)(G/C)N (G/T)(G/C)N A/C)GN GGN GAN GGN GG-3'; positions 2312 to 2334] and IK04, which were designed based on an amino acid sequence alignment of known bacterial fumarate reductases, were used to PCR amplify a fragment of a putative fumarate reductase-encoding operon from the chromosomal DNA of D. dehalogenans. The resulting 0.85-kb PCR product was cloned in E. coli using XcmI-digested pMON38201, yielding pLUW902. Subsequently, Southern blot analysis of PstI-EcoRI-digestedchromosomal DNA of D. dehalogenans revealed a 3-kb fragment that strongly hybridized with the radiolabeled 0.85-kb PCR product. The 3-kb fragment was cloned in E. coli using PstI-EcoRI-digested pUC18, resulting in pLUW903. pLUW904 was obtained by inverse PCR (36) that was performed as described previously (39) with BamHI-digested and self-ligated chromosomal DNA of D. dehalogenans by using the divergent primer pair BG283 and BG284 (positions 2456 to 2477 and positions 2356 to 2335, respectively).
Plasmid constructions and single-crossover integration into the D. dehalogenans chromosome. A 578-bp ApaI-EcoRI internal fragment of the D. dehalogenans frdA gene was cloned in E. coli MC1061 using ApaI-EcoRI-digested pG+host9, yielding pLUW906. Subsequently, electrocompetent cells of D. dehalogenans were transformed with plasmid DNA isolated from E. coli MC1061 using a QAprep Spin Miniprep kit (Qiagen GmbH). Recovery after electroporation and cultivation on selective plates were performed at 30°C. Erythromycin-resistant colonies that appeared within 5 days were transferred to liquid selective medium containing 40 mM pyruvate and were incubated at 30°C. Cultures were diluted 20-fold in the same medium, grown at 30°C for 8 h to reach log phase, and then shifted to 40°C for 16 h (3 to 5 generations). Appropriate dilutions were incubated on plates in the presence of 20 mM pyruvate and erythromycin at 40°C in order to detect integration events and on nonselective plates at 40°C for the determination of viable cell counts. The ratio of the two counts was used to determine the frequency of integration per cell as described by Biswas et al. (2). Integrants that were isolated at 40°C were subsequently routinely maintained in selective medium containing 20 to 40 mM pyruvate. Southern blot analysis of HincII-digested chromosomal and plasmid DNA and preparation of pG+host9- and D. dehalogenans frdAC-specific probes were performed as described above.
DNA sequencing and sequence analysis. DNA sequencing was performed using a LiCor (Lincoln, Nebr.) DNA sequencer 4000L. Plasmid DNA used for sequencing reactions was purified with the QIAprep Spin Miniprep kit (Qiagen GmbH). Reactions were performed using the Thermo Sequenase fluorescent-labeled primer cycle sequencing kit (Amersham Pharmacia Biotech). Fluorescently (IRD 800) labeled universal sequencing primers were purchased from MWG Biotech. Sequence similarity searches and alignments were performed using the BLAST 2.0 program (1) (National Center for Biotechnology Information, Bethesda, Md.) and the Clustal X (34) and GeneDoc (K. B. Nicholas and H. B. J. Nicholas, GeneDoc: a tool for editing multiple sequence alignments, 1997) programs and DNAstar package (DNASTAR Inc., Madison, Wis.), respectively.
Enzyme and protein assays. Harvesting of cells and preparation of cell extracts by sonication under anoxic conditions were performed as described previously (39). Fumarate reductase activities were determined spectrophotometrically at 30°C in 1 ml of 100 mM Tris-HCl (pH 8.0) as described previously (32). One unit of enzyme activity corresponds to the amount of enzyme catalyzing the conversion of 1 µmol of substrate or 2 µmol of benzyl viologen per min. Succinate dehydrogenase activity was measured with 2,6-dichlorophenolindophenol and phenazine methosulfate as an artificial electron acceptor as described by Schirawski and Unden (29). Protein was determined according to the method of Bradford, with bovine serum albumin as the standard (5).
Nucleotide sequence accession number. The nucleotide sequence of the putative fumarate reductase-encoding operon has been deposited in GenBank under accession no. AF299117.
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RESULTS |
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Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
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|---|
Development of an electroporation-based transformation protocol for
D. dehalogenans.
To allow for the
application of plasmid vector systems for genetic manipulation of the
strict anaerobe D. dehalogenans, an electroporation-based transformation protocol for this bacterium was
designed and optimized using the promiscuous plasmid pIL253 (30). Because this cloning vector, which is a
derivative of the broad-host-range thetareplicating plasmid
pAM1, carries an erythromycin resistance marker, we checked D. dehalogenans for its sensitivity to this antibiotic.
On plates that contained 0.1 µg of erythromycin/ml, 6.5 × 106 CFU/ml was obtained, compared to 4 × 107 CFU/ml on plates without any antibiotic. At
erythromycin concentrations of 0.25 and 0.5 µg/ml, microcolonies
colonies appeared after 4 days, whereas no colonies developed at
concentrations of 
1 µg of erythromycin/ml, indicating that the
frequency of spontaneous resistance to erythromycin is below 2.5 × 107 per CFU. Subsequently, a concentration of 5 µg
of erythromycin/ml was used in solid and liquid media for the
selection of strains of D. dehalogenans carrying
the erythromycin resistance marker.
1, a capacitance of 25 µF, and a resistance of 200 to
800 . After a subsequent incubation of 5 h in the presence of
0.5 M sucrose, cells were inoculated onto plates with or without 5 µg
of erythromycin/ml. After 3 days of incubation at 37°C, colonies were
counted to determine survival and transformation efficiency. The pulse
resulted in a 40 to 65% decrease in CFU on nonselective plates with
decreasing resistance compared to the survival of an aliquot of
concentrated cells that was kept inside the anaerobic chamber and was
not subjected to a pulse (Fig. 1). The
highest numbers of transformants were obtained at a resistance of 400 , resulting in a pulse time constant of approximately 7.5 ms. Both
shorter and longer pulse times (200 , 4.7 ms; 600 , 12.8 ms; 800 , 16.4 ms) resulted in significantly lower numbers of transformants
(Fig. 1). Routinely, 3,000 ± 1,900 transformants (maximal value,
6.6 × 103) were obtained per µg of CsCl-purified
pIL253, independent of the amount of plasmid DNA (ranging from 50 to
800 ng) used in the electrotransformation. In order to check the
transformants for the presence and concentration of plasmid,
erythromycin-resistant colonies were transferred to liquid selective
medium containing 20 mM lactate and fumarate, and plasmid DNA was
isolated from early-stationary-phase cultures
(A600 = 0.25). Plasmid DNA was detectable
by agarose gel electrophoresis, and quantification indicated a
concentration of 5 ng of pIL253/ml of culture, corresponding to
approximately 10 copies per cell (data not shown).
|
Segregational stability and thermosensitivity of
pG+host9 in D. dehalogenans.
The thermosensitive broad-host-range pG+host vector family
has been shown to be instrumental for high-efficiency gene inactivation and replacement in gram-positive bacteria (2). In order to study the applicability of this system in the halorespiring
bacterium D. dehalogenans,
electrocompetent cells were transformed with CsCl-purified
pG+host9. To ensure functional replication,
posttransformation incubation and cultivation on selective media were
performed at 30°C. Transformation yielded, on average, 600 transformants per µg of plasmid DNA. Colonies that appeared on
selective plates were transferred to liquid medium. Plasmid DNA was
isolated from early-stationary-phase cultures and could be detected by
agarose gel electrophoresis (data not shown). In order to determine the
permissive and nonpermissive temperatures for the replication of
pG+host9 in D. dehalogenans, the
segregational stability of the plasmid at nonselective concentrations
of erythromycin was analyzed at different temperatures. A culture of
D. dehalogenans containing the plasmid was
diluted into fresh medium without any antibiotic and incubated at 30, 37, and 40°C. The ratio of the CFU on selective plates to the CFU on
nonselective plates at 30°C was determined at 0, 16, and 40 h
after dilution. Whereas this ratio decreased only 50% for the culture
that was incubated at 30°C (0.51 at 0 h and 0.26 at 40 h), it
dropped 72- and 48,000-fold at 37 and 40°C, respectively, within 7 generations (Fig. 2A). No influence of
the incubation temperature on segregational stability was observed in
the case of the nonthermosensitive plasmid pIL253 (data not shown). Similar results were obtained by Southern blot analysis of total DNA that was isolated before and 7 (40 h) and 10 generations (68 h) after the shift to nonselective conditions,
respectively (Fig. 2B). The amount of plasmid-derived sequences
detected following growth for 10 generations at 37 or 40°C was found
to be more than 1,000-fold lower than that detected in cells grown at
30°C.
|
Cloning and sequence analysis of a putative fumarate
reductase-encoding frdBAC gene cluster.
The versatile
gram-positive anaerobe D. dehalogenans has the
ability to utilize fumarate as the terminal electron acceptor for
anaerobic respiration with H2, formate, lactate, or
pyruvate as the electron donor. High fumarate reductase activity is
readily detectable in cell extracts of D. dehalogenans grown in the presence of fumarate or
yeast extract (32, 37). In order to provide an
easy-to-screen target gene for the development of genetic modification approaches, we amplified a 0.85-kb fragment from the chromosome of
D. dehalogenans using degenerated primers that
were designed based on a primary sequence alignment of known
succinate:quinone oxidoreductases (17). Sequence analysis
indicated significant similarity with the flavoproteins of fumarate
reductases and succinate dehydrogenases present in the databases. The
subsequent isolation and analysis of a 5.3-kb
PstI-BamHI chromosomal fragment from D. dehalogenans revealed the presence of three
closely linked genes, frdCAB, and a fourth open
reading frame, aabH, potentially encoding a polypeptide with
significant similarity to ATP-binding cassette transporter binding
proteins. The three genes frdC, frdA, and frdB
potentially code for polypeptides of 208, 578, and 251 amino acids with
calculated molecular masses of 23,728, 64,441, and 28,043 Da,
respectively (Fig. 3A). The predicted
gene products exhibit significant similarities with the type B membrane
anchor, flavoprotein, and iron-sulfur-protein subunits of known
succinate:quinone oxidoreductases, respectively (17). The
highest similarities were found with the succinate dehydrogenases of
Bacillus subtilis and Paenibacillus macerans
(identities on the amino acid level, 72 and 74% for FrdA, 58 and 59%
for FrdB, and 42 and 29% for FrdC, respectively). Upstream of each of
the genes, potential Shine Dalgarno sequences that are complementary to
the 3' end of the D. dehalogenans 16S rRNA
(33) could be identified (data not shown).
|
Gene-specific single-crossover integration in the D. dehalogenans chromosome.
An internal 0.6-kb
fragment of the D. dehalogenans frdA gene was
cloned into pG+host9 in E. coli MC1061.
The resulting plasmid, pLUW906 (Fig. 3B), was introduced by
transformation into D. dehalogenans, where it
was stably maintained at 30°C. Subsequently, cultures of D. dehalogenans containing either pLUW906 or pG+host9
were shifted to 40°C to induce single-crossover or spontaneous chromosomal integration, respectively. Single-crossover integration at
the frdA locus would result in the generation of two,
chromosomal copies of the frdA gene, truncated at either the
3' or the 5' end, and interrupted by the vector (Fig. 3C). Integrants
were selected as erythromycin-resistant colonies appearing at 40°C, and integration of pLUW906 occurred at a frequency of 3.3 × 104 ± 6.6 × 105 per cell
compared to 4.8 × 106 ± 6.9 × 106 per cell, for pG+host9.
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DISCUSSION |
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Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
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The recent detailed molecular analysis of the halorespiratory system in the o-CP-respiring gram-positive bacterium D. dehalogenans has brought us to a deeper understanding of structure, function, and control of this novel respiratory pathway (32, 33, 39). Previously, we described the development of an efficient plating, delivery, and screening system that has been useful for the isolation of halorespiration-deficient mutants following the chromosomal integration of the conjugative transposon Tn916 (32). These mutants have been instrumental in the identification of genes potentially encoding polypeptides which might be involved as structural components of the halorespiratory network or might play a role in their control and functional assembly. However, the instability of some of these mutants and the occurrence of preferential integration has to some extent hampered their further physiological and biochemical characterization. Here we report on the development and validation of host-vector systems for the genetic modification of the environmentally important, strictly anaerobic, low-G+C, gram-positive bacterium D. dehalogenans.
An efficient electroporation-based transformation procedure was
designed using a protocol that had previously been optimized for
the high-frequency electrotransformation of L. lactis (40). Routinely, we obtained 1.0 × 103 to 6.6 × 103 erythromycin-resistant
transformants per µg of plasmid DNA from the 4.8-kb theta-replicating
pAM1 derivative pIL253. These values observed for D. dehalogenans are in the same range as or higher than
transformation frequencies obtained for several other LGB, such as
Clostridium spp., but are lower than those obtained in genetic model strains of L. lactis (7, 9, 21,
41). Although pIL253 was maintained in D. dehalogenans at only moderate copy numbers of
approximately 10 copies per cell, compared with 45 to 85 copies for
L. lactis (12, 30), the stable replication of
the vector indicates its potential use as a cloning vector in D. dehalogenans.
Plasmids based on the thermosensitive replicon pG+host were
previously shown to conditionally replicate in various LGB as well as
in E. coli (22, 23). One of these, the 3.8-kb
rolling-circle-replicating, thermosensitive pWV01 derivative
pG+host9, was used for the development of a system for
specific gene disruption in D. dehalogenans.
Transformation efficiencies for pG+host9 were on average 1 order of magnitude lower (6 × 102) than those for
pIL253. These differences in frequency of transformation might be due
to the difference in the mode of replication, as was previously
reported for various other strains of LGB, but could also be caused by
differences in marker gene expression (12, 20, 27). We
were able to confirm thermosensitive replication, which was
essentially absent at 40°C in D. dehalogenans.
Although moderate segregational instability was also observed at
the permissive temperature of 30°C, the relative number of viable
cells able to grow on selective plates was reduced to 2 × 105 at 40°C within 7 generations. The nonpermissive
temperature that we found for D. dehalogenans is somewhat higher than that reported for
L. lactis (22). However, as D. dehalogenans is still growing at almost maximum growth
rates at 40°C, this does not affect the applicability of the
pG+host system (37).
In order to provide a model target to test the thermosensitive vector pG+host9 for its applicability for specific gene disruption, we cloned and sequenced the putative fumarate reductase-encoding frdCAB operon from D. dehalogenans. A pG+host9 derivative containing a 0.6-kb internal frdA fragment was successfully introduced and maintained in D. dehalogenans under permissive conditions. Chromosomal integration at nonpermissive temperatures was significantly more efficient in the case of pLUW906 compared to the empty vector, and the observed integration frequencies were similar to those found for L. lactis (2). However, although stable site-specific chromosomal integration of pLUW906 into the frdA gene could be unambiguously demonstrated by Southern blot analysis and PCR analysis, the fumarate reductase activity was only partly reduced and no changes in growth with fumarate were observed compared to the growth of D. dehalogenans containing pG+host9. One possible explanation could be that at least one of the truncated frdA genes present in the pLUW906 integrant is still coding for a (partially) active fumarate reductase enzyme due to a polar effect from the inserted vector sequences. This, however, is rather unlikely, since both the 3'- and 5'-truncated frdA copies lack several conserved residues that are probably essential for fumarate reductase activity (4, 17). Another possibility could be that the frdCAB operon actually encodes a succinate dehydrogenase. Nevertheless, no significant succinate dehydrogenase activity could be detected in cell extracts of D. dehalogenans. Northern analysis of total RNA isolated from cultures of D. dehalogenans grown with different electron donors and 3-chloro-4-hydroxy-phenylacetic acid, nitrate, or fumarate as the electron acceptor indicated that transcription of the frdCAB operon is constitutive rather than being induced in the presence of fumarate. This, however, is not in agreement with the highly induced fumarate reductase activity that has been measured in fumarate-grown cells of D. dehalogenans (H. Smidt et al., unpublished data). This suggests that the frdCAB operon only partially codes for the fumarate reductase activity, which is measured with benzyl viologen as an artificial electron donor. If so, this strongly supports the presence of at least one additional fumarate reductase-encoding gene cluster.
The development of the various gene transfer systems reported here is the first example of a genetic system for a halorespiring microbe. It has significantly improved our possibilities for studying the function and regulation of chromosomal genes in D. dehalogenans, including those relevant for the novel halorespiratory pathway this organism possesses. Moreover, the present set of genetic tools will enable the further exploitation of D. dehalogenans and related strains as dedicated degraders of recalcitrant environmental pollutants.
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ACKNOWLEDGMENTS |
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We thank Richard van Kranenburg and Emmanuelle Maguin for providing plasmids pIL253 and pG+host9.
This work was partly supported by a grant from the Studienstiftung des Deutschen Volkes and contract BIO4-98-0303 of the European Union.
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FOOTNOTES |
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* Corresponding author. Mailing address: Laboratory of Microbiology, Wageningen University, Hesselink van Suchtelenweg 4, NL-6703 CT Wageningen, The Netherlands. Phone: 31-317-483118. Fax: 31-317-483829. E-mail: hauke.smidt{at}algemeen.micr.wag-ur.nl.
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REFERENCES |
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Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
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Altschul, S. F.,
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). Efficiency of transformation of D. dehalogenans was determined on plates containing 5 µg of erythromycin/ml and calculated as CFU per microgram of
CsCl-purified pIL253 (
).
). (A) Ratio of CFU on selective and nonselective plates.
(B) Normalized ratio of hybridization signal intensities obtained with
probes specific for pG+host9 and frdAC.
