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Applied and Environmental Microbiology, April 2003, p. 2126-2132, Vol. 69, No. 4
0099-2240/03/$08.00+0     DOI: 10.1128/AEM.69.4.2126-2132.2003
Copyright © 2003, American Society for Microbiology. All Rights Reserved.

Cloning, Expression, and Purification of Choline Dehydrogenase from the Moderate Halophile Halomonas elongata

Giovanni Gadda^1,2* and Elien Elizabeth McAllister-Wilkins¹

Department of Chemistry,¹ Department of Biology and The Center for Biotechnology and Drug Design, Georgia State University, Atlanta, Georgia 30303-3038²

Received 23 September 2002/ Accepted 7 January 2003

Top Abstract Introduction Materials and Methods Results Discussion References

 
Choline dehydrogenase (EC 1.1.99.1) catalyzes the four-electron oxidation of choline to glycine-betaine via a betaine-aldehyde intermediate. Such a reaction is of considerable interest for biotechnological applications in that transgenic plants engineered with bacterial glycine-betaine-synthesizing enzymes have been shown to have enhanced tolerance towards various environmental stresses, such as hypersalinity, freezing, and high temperatures. To date, choline dehydrogenase has been poorly characterized in its biochemical and kinetic properties, mainly because its purification has been hampered by instability of the enzyme in vitro. In the present report, we cloned and expressed in Escherichia coli the betA gene from the moderate halophile Halomonas elongata which codes for a hypothetical choline dehydrogenase. The recombinant enzyme was purified to more than 70% homogeneity as judged by sodium dodecyl sulfate-polyacrylamide gel electrophoresis and by treatment with 30 to 50% saturation of ammonium sulfate followed by column chromatography using DEAE-Sepharose. The purified enzyme showed similar substrate specificities with either choline or betaine-aldehyde as the substrate, as indicated by the apparent V/K values (where V is the maximal velocity and K is the Michaelis constant) of 0.9 and 0.6 µmol of O₂ min^-1 mg^-1 mM^-1 at pH 7 and 25°C, respectively. With 1 mM phenazine methosulfate as the primary electron acceptor, the apparent V_max values for choline and betaine-aldehyde were 10.9 and 5.7 µmol of O₂ min^-1 mg^-1, respectively. These V_max values decreased four- to sevenfold when molecular oxygen was used as the electron acceptor. Altogether, the kinetic data are consistent with the conclusion that H. elongata betA codes for a choline dehydrogenase that can also act as an oxidase when electron acceptors other than molecular oxygen are not available.

Top Abstract Introduction Materials and Methods Results Discussion References

 
Availability of water is the most important limiting factor affecting the survival and growth of both beneficial and pathogenic microorganisms. Since microorganisms lack systems for active water transport, environmental changes in osmolarity are compensated by either transport or synthesis of compatible solutes, a group of inert organic solutes that can be accumulated in the intracellular milieu to very high levels without affecting the metabolic function of the cell (for a recent review, see reference 7). Among the compatible solutes that have been identified to date, glycine-betaine is the most widely used in that it is found not only in bacteria but also in animals (29, 35, 41, 48) and plants (15, 43). Although uptake of external glycine-betaine has been described in some bacteria, such as Corynebacterium glutamicum (12, 33), Listeria monocytogenes (13, 14, 24, 30), and Bacillus subtilis (22), the preferred strategy utilized by both prokaryotic and eukaryotic cells involves the enzymatic formation of glycine-betaine from choline as a precursor (5, 8, 21, 23, 31, 36, 37, 45). Three different enzymatic systems have been described for the oxidative formation of glycine-betaine from choline. A soluble choline oxidase (EC 1.1.3.17) is found in the gram-positive soil bacteria Arthrobacter globiformis and Arthrobacter pascens (19, 37) and in the fungus Cylindrocarpon didymum (28, 47). Choline monooxygenase (EC 1.14.15.7), in combination with betaine-aldehyde dehydrogenase (EC 1.2.1.8), has been identified in a limited number of higher plants, such as spinach (36), sugar beet, and amaranth (38). A membrane-associated choline dehydrogenase (EC 1.1.99.1) coupled to betaine-aldehyde dehydrogenase has been described in marine invertebrates, such as oysters (31, 32), and in bacteria, such as Escherichia coli (27) and Pseudomonas aeruginosa (39, 45). In E. coli, the biosynthetic pathway for the production of glycine-betaine from choline has been well characterized at the genetic level, where it has been shown that four genes encoding choline dehydrogenase (betA), betaine-aldehyde dehydrogenase (betB), a putative regulator (betI), and a choline transporter (betT) are clustered in the bet operon (3). Based on nucleotide sequence alignment, similar Bet pathways have been recently proposed for Sinorhizobium meliloti (34) and the moderate halophile Halomonas elongata (9). Since H. elongata is capable of thriving in hypersaline environments with NaCl concentrations as high as 4 M (46), its Bet pathway represents an excellent model for studying the molecular basis of osmoprotection.

Bacterial glycine-betaine-synthesizing enzymes recently have become a major target in the creation of stress-resistant transgenic plants with the goal of genetically engineering stress tolerance in crop plants of economic interest (for a recent review, see reference 40). Model studies of Synechococcus sp. PCC 7942 or Arabidopsis thaliana transformed with the gene from A. globiformis that encodes choline oxidase, codA, have demonstrated an improved tolerance to salt stress (11) or high and freezing temperatures (2, 16, 40). Enhanced tolerance to low temperatures or high-salt conditions has been also observed during germination of transgenic seeds of A. thaliana transformed with codA (1, 17). Similarly, improved resistance towards salinity and low temperature has been shown in transgenic tobacco expressing the two E. coli genes betA and betB (18), demonstrating that choline dehydrogenase and/or betaine-aldehyde dehydrogenase are also of considerable interest for practical applications. Despite these significant biotechnological advances, the biochemical and kinetic characterization of choline dehydrogenase has lagged behind and only minimal biochemical studies on choline dehydrogenase purified from rat liver mitochondria (44) and a Pseudomonas strain (39) have been reported to date.

Choline dehydrogenase catalyzes the four-electron oxidation of choline to glycine-betaine via a betaine-aldehyde intermediate (44) (Fig. 1) and shows an absolute requirement for an electron acceptor other than molecular oxygen for catalysis (39, 44). Although, based on primary sequence alignment, the enzyme has been grouped in the glucose-methanol-choline flavin-dependent oxidoreductase superfamily (10), no clear biochemical evidence has been shown indicating the presence of flavin adenine dinucleotide (FAD) as a cofactor. In contrast, pyrroloquinoline quinone (PQQ) has been proposed to be bound to Pseudomonas choline dehydrogenase (39).

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FIG. 1. Oxidation of choline to glycine-betaine catalyzed by choline dehydrogenase.

As a first step towards a biochemical and mechanistic characterization of choline dehydrogenase aimed at a better understanding of the properties of the enzyme, we cloned and expressed the betA gene from H. elongata and partially purified and characterized the resulting enzyme by using steady-state kinetics with choline or betaine-aldehyde as the substrate. The data presented in this study indicate that in H. elongata the betA gene codes for a choline dehydrogenase, which is also able to utilize molecular oxygen in catalysis in the absence of other electron acceptors.

Top Abstract Introduction Materials and Methods Results Discussion References

 
Materials.
Plasmid pDC4 containing the bet operon from H. elongata was a kind gift of Joaquin J. Nieto, University of Seville, Spain. Restriction endonucleases NcoI and BamHI, T4 DNA ligase, and calf intestinal alkaline phosphatase were obtained from Promega. Pfu DNA polymerase was obtained from Stratagene or from Roche Molecular Biomedicals. Luria-Bertani agar, Luria-Bertani broth, ampicillin, chloramphenicol, tetracycline, isopropyl-ß-D-thiogalactopyranoside (IPTG), FAD, PQQ, lysozyme, and phenylmethylsulfonyl fluoride (PMSF) were obtained from Sigma-Aldrich. The plasmid vector pET23d(+) was obtained from Novagen. Electrophoresis-grade agar, choline chloride, and betaine-aldehyde were purchased from ICN Biomedicals. Oligonucleotides were custom synthesized on a Beckman Oligo model 1000 M by the DNA Core Facility of the Biology Department of Georgia State University. Plasmids and primer extension reaction products were purified by using mini-kits from Qiagen. Site-directed mutagenesis was performed by using a QuikChange site-directed mutagenesis kit from Stratagene. E. coli strain OrigamiB(DE3)pLysS (Novagen) was used for protein expression, and strain XL1-Blue (Stratagene) was used during cloning procedures. E. coli strain XL1-Blue cells harboring plasmid pETCHDhe or pETCHDhe-S2A and strain OrigamiB(DE3)pLysS cells harboring plasmid pETCHDhe were stored at -80°C as 7% dimethyl sulfoxide suspensions. DNA sequencing was carried out with an Applied Biosystems Big Dye kit on an Applied Biosystems model ABI 377 DNA sequencer by the DNA Core Facility of the Biology Department of Georgia State University.

Cloning of betA into expression vector pET23d(+).
E. coli strain MKH13 harboring plasmid pDC4 was grown on Luria-Bertani agar medium containing 50 µg of chloramphenicol/ml for 16 h at 37°C. Single colonies were used to inoculate 5 ml of Luria-Bertani broth containing 50 µg of chloramphenicol/ml, and the resulting liquid cultures were grown for 16 h at 37°C. The cells were harvested by centrifugation at 14,000 x g for 10 min, and the plasmid vector was isolated by using a QIAquick Spin miniprep kit (Qiagen) according to the manufacturer's instructions. The extracted plasmid was then used for primer extension amplification of the betA gene by using oligonucleotide primers containing NcoI and BamHI restriction endonuclease sites designed to anneal to the 5' and 3' ends of the gene, respectively. The NcoI (GAACCGCCATGGCTCAAGCAACTGAG) and BamHI (CGCACTCGTGGATCCCTACGATGCCTGTTTGGC) restriction sites introduced at the 5' ends of the sense and antisense primers (underlined) allow cloning of betA into the corresponding sites of pET23d(+). Primer extension reaction was performed with an Eppendorf Mastercycler for 1 min at 95°C followed by 30 cycles of 0.5 min at 95°C, 1 min at 60°C, 3.5 min at 68°C, and a 5-min final step at 68°C in a total volume of 50 µl by using 20 ng of template DNA, 2.5 U of Pfu DNA polymerase, and the polymerase manufacturer's suggested protocol. The resulting primer extension reaction product was purified with the QIAquick kit.

The pET23d(+) vector was isolated from a 5-ml liquid culture of E. coli strain XL1-Blue grown for 16 h at 37°C in Luria-Bertani broth containing 50 µg of ampicillin/ml by using a QIAprep Spin miniprep kit from Qiagen following the manufacturer's instructions.

Both the amplified betA and pET23d(+) were digested for 2 h at 37°C with 30 U of NcoI according to the manufacturer's instructions. After the digestion was stopped by using the QIAquick kit, DNA was further digested with BamHI. To minimize self-ligation of the plasmid, pET23d(+) was incubated with 30 U of calf intestine alkaline phosphatase for 3 h at 25°C, followed by purification of the DNA with the QIAquick kit. The betA gene (100 ng) was then ligated into pET23d(+) (40 ng) by incubation with 10 U of T4 DNA ligase for 16 h at 15°C, and the ligation mixture was used directly to transform E. coli strain XL1-Blue competent cells by using the heat shock method of Inoue et al. (20). The resulting transformant colonies obtained by plating on Luria-Bertani agar plates containing 50 µg of ampicillin/ml were screened for the presence of betA by colony primer extension reaction with 2.5 U of Pfu DNA polymerase according to the procedure described above. The correct construct, pETCHDhe-S2A, was sequenced in both directions by using oligonucleotide primers designed to bind to the DNA regions of pET flanking the inserted gene.

The single nucleotide substitution inserted at position 4 of betA during the cloning process was removed from pETCHDhe-S2A by primer extension reaction with the Stratagene QuikChange site-directed mutagenesis kit according to the manufacturer's protocol. The sense and antisense oligonucleotide primers used were GAGATATACCATGTCTCCAAGCAACTGAG and CTCAGTTGCTTGAGACATGGTATATCTC, respectively, with the single nucleotide substitution underlined. Primer extension reaction was carried out with an Eppendorf Mastercycler for 0.5 min at 95°C followed by 16 cycles of 0.5 min at 94°C, 1 min at 55°C, and 12 min at 72°C using 50 ng of pETCHDhe-S2A as the template. The primer extension reaction, after digestion with endonuclease DpnI, was used to directly transform E. coli strain XL1-Blue competent cells. The resulting plasmid, pETCHDhe, was sequenced in both directions by using oligonucleotide primers designed to bind to DNA regions of pET flanking the inserted gene. Competent E. coli strain OrigamiB(DE3)pLysS cells were transformed with plasmid pETCHDhe.

Expression of choline dehydrogenase in E. coli.
A single colony of E. coli strain OrigamiB(DE3)pLysS harboring plasmid pETCHDhe was used to inoculate 50 ml of Luria-Bertani broth containing 50 µg of ampicillin/ml, 34 µg of chloramphenicol/ml, and 12 µg of tetracycline/ml at 37°C. After 16 h, 18 ml of the starter culture was used to inoculate 1.5 liters of Luria-Bertani broth containing 50 µg of ampicillin/ml at 37°C. When the culture's optical density at 600 nm reached 0.8, IPTG was added to a final concentration of 0.8 mM and the temperature of the culture was lowered to 25°C. After 4 h, cells were harvested by centrifugation at 5,000 x g for 10 min at 4°C and stored at -20°C. Typically, 1.5 liters of culture yielded approximately 5 g of cell wet paste.

Purification of choline dehydrogenase.
The purification of choline dehydrogenase was carried out at 4°C as follows. The cell paste, typically 5 g, was suspended in 4 volumes of a solution containing 1 mM EDTA, 100 mM NaCl, 0.1 mM PMSF, 0.2 mg of lysozyme/ml, and 50 mM Tris-Cl (pH 8.0) and allowed to incubate with stirring for 30 min on ice. The resulting slurry was passed through an SLM Aminco French pressure cell two times at 20,000 lb/in² and then clarified by centrifugation at 5,000 x g for 20 min. The supernatant was brought to 30% ammonium sulfate saturation, incubated with stirring on ice for 30 min, and then centrifuged at 12,500 x g for 20 min. The supernatant was brought to 50% ammonium sulfate saturation and treated as described above. The resulting pellet was suspended in 5 ml of 1 mM EDTA-20 mM potassium phosphate (pH 7.0) and dialyzed against three 250-ml 1-h changes of the same buffer. After dialysis, precipitated proteins were removed by centrifugation at 12,500 x g for 20 min and the resulting supernatant was loaded onto a Hi-Prep 16/10 DEAE Fast Flow column connected to an Äktaprime Amersham Pharmacia Biotech system equilibrated with 1 mM EDTA-20 mM potassium phosphate (pH 7.0). The column was eluted with 100 ml of the same buffer followed by a linear gradient from 0 to 1 M NaCl developed over 200 ml at a flow rate of 4 ml/min. The fractions with the highest purity as judged by enzymatic activity, UV-visible absorbance, and sodium dodecyl sulfate-polyacrylamide gel electrophoresis (SDS-PAGE) were pooled together and concentrated with the addition of 50% ammonium sulfate saturation followed by centrifugation. The resulting pellet was suspended in 2 M sorbitol-20% glycerol-20 mM potassium phosphate (pH 7.0) and dialyzed overnight against three 250-ml 1-h changes of the same buffer. After removal of precipitated proteins by centrifugation, the enzyme was stored at -20°C.

Assays.
The concentration of choline dehydrogenase was determined by the method of Bradford (6) by using the Bio-Rad protein assay kit with bovine serum albumin as the standard. The oxidase activity of the enzyme was measured with 10 mM choline as the substrate in air-saturated 50 mM potassium phosphate, pH 7.0, by monitoring the rate of oxygen consumption with a computer-interfaced Oxy 32 oxygen-monitoring system (Hansatech Instrument Ltd.) thermostated at 25°C. The dehydrogenase activity of the enzyme was measured with 1 mM phenazine methosulfate as the primary electron acceptor and under the conditions described above using a coupled assay in which the enzymatically reduced phenazine methosulfate is spontaneously reoxidized by molecular oxygen. One unit of enzymatic activity corresponds to the conversion of a micromole of oxygen per minute. For determination of the steady-state kinetic parameters of choline dehydrogenase with choline or betaine-aldehyde as the substrate, the concentration of substrate was varied between 1 and 50 mM. SDS-PAGE was carried out in 10% slab gels by the method of Laemmli (26). Proteins were visualized by staining with Coomassie brilliant blue G-250.

Data analysis.
Steady-state kinetic data were analyzed with Kaleidagraph software (Adalbeck Software, Reading, Pa.) by fitting initial reaction rates at different substrate concentrations to the Michaelis-Menten equation for one substrate, v = VA/(K + A), where V is the maximal velocity, K is the Michaelis constant, and A is the concentration of the substrate.

Top Abstract Introduction Materials and Methods Results Discussion References

 
Cloning of betA from H. elongata.
The bet operon of H. elongata containing the genes for choline uptake (betI) and glycine-betaine biosynthesis (betBA) was recently cloned in plasmid pDC4 by Canovas et al. (9). Plasmid pDC4 was used to amplify betA by primer extension reaction with Pfu DNA polymerase. Directional cloning of betA into plasmid pET23d(+) was accomplished by engineering NcoI and BamHI endonuclease sites at the 5' and 3' ends of betA, respectively. The resulting construct, pETCHDhe-S2A, was then used to transform E. coli strain XL1-Blue competent cells by using the heat shock method of Inoue et al. (20). Of the 125 transformant colonies obtained by plating on Luria-Bertani agar plates containing 50 µg of ampicillin/ml, 12 were screened for the presence of betA by colony primer extension reaction with Pfu DNA polymerase. One-third of the screened colonies were found to contain betA, as shown by the presence of an 1,700-bp band when the primer extension reaction mixture was analyzed by agarose gel electrophoresis. Successful construction of plasmid pETCHDhe-S2A was confirmed by nucleotide sequence analysis.

In the cloning procedure, a single nucleotide substitution (T G) was introduced at position 4 of betA as a result of the use of an NcoI endonuclease restriction site at the 5' end of the gene. The choice of an NcoI site was dictated by the observation that this site contains an ATG start codon and is not present at any internal portion of the gene. The single nucleotide substitution was removed from pETCHDhe-S2A by using the method of Kunkel (25), and the sequence of the resulting plasmid pETCHDhe was found to be correct.

Characterization of choline dehydrogenase expressed in E. coli.
Recombinant choline dehydrogenase was produced in large quantities, greater than 5% of the total cell proteins, by using E. coli strain OrigamiB(DE3)pLysS cells, which provide an oxidizing environment in the cytosol. The choice of such a host cell strain was suggested by preliminary experiments on the expression of recombinant choline dehydrogenase from Sinorhizobium meliloti (Bethany Russell and Giovanni Gadda, unpublished results). Soluble and active enzyme was obtained by incubating the cell cultures in the presence of 0.8 mM IPTG at 25°C for 4 h after the optical density at 600 nm reached 0.8 (Fig. 2). Cell extracts of host cells which did not harbor the pETCHDhe plasmid did not show any protein band with the mass expected for choline dehydrogenase (Fig. 2) and were devoid of enzymatic activity, indicating that no choline-oxidizing activities other than the overexpressed enzyme were present in the cell extracts. Initial attempts to purify the enzyme expressed in E. coli by using octyl-, phenyl-, carboxymethyl-, or Q-Sepharose columns were unsuccessful as a result of the significant instability of the enzyme in the presence of high salt concentrations and the fact that choline dehydrogenase did not bind to these matrixes (data not shown). Also, initial attempts to use streptomycin sulfate to precipitate nucleic acids from the cell extract led to the observation that a substantial fraction of the enzymatic activity partitioned in the insoluble fraction (data not shown) and could not be rescued in solution. In contrast, most of the contaminant proteins could be removed from the cell extract by binding to a Hi-Prep 16/10 DEAE Fast Flow column after treatment of the cell extract with 30 to 50% saturation of ammonium sulfate and dialysis (Table 1). The resulting partially purified enzyme could then be stabilized in solution in the presence of 2 M sorbitol and 20% glycerol, at pH 7.0, and was found to be more than 70% homogeneous by SDS-PAGE (Fig. 2). The UV-visible absorbance spectrum of the purified active enzyme did not show significant absorbance above 300 nm; in contrast, a peak centered at 256 nm was observed in the UV region of the spectrum, suggesting that nucleic acids might copurify with the enzyme (data not shown).

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FIG. 2. Purification of recombinant choline dehydrogenase from H. elongata. Lanes: 1, marker proteins (E. coli ß-galactosidase [116 kDa], rabbit muscle phosphorylase b [97 kDa], rabbit muscle fructose-6-phosphate kinase [84 kDa], bovine serum albumin [66 kDa], bovine liver glutamic dehydrogenase [55 kDa], chicken egg ovalbumin [45 kDa], rabbit muscle glyceraldehydes-3-phosphate dehydrogenase [36 kDa], bovine erythrocytes carbonic anhydrase [29 kDa], bovine pancreas trypsinogen [24 kDa], and soybean trypsin inhibitor [20 kDa]); 2, cell extract of E. coli strain OrigamiB(DE3)pLysS; 3, cell extract of E. coli strain OrigamiB(DE3)pLysS harboring plasmid pETCHDhe induced with 0.8 mM IPTG; 4, partially purified choline dehydrogenase.

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TABLE 1. Purification of recombinant H. elongata choline dehydrogenase

Based on the deduced amino acid sequence of betA and in vivo experiments with [methyl-¹⁴C]choline on E. coli-harboring plasmids containing an E. coli choline transporter and betA from H. elongata, it has been previously proposed that betA from H. elongata encodes choline dehydrogenase (9). Since choline dehydrogenase is capable of using either choline or betaine-aldehyde as a substrate (27, 44), we determined the apparent steady-state kinetic parameters for the partially purified enzyme with these substrates in air-saturated 50 mM potassium phosphate (pH 7.0 and 25°C). Initial rates of reaction were measured by monitoring the rate of oxygen consumption in the presence of 1 mM phenazine methosulfate as the primary electron acceptor with various concentrations of choline or betaine-aldehyde as the substrate for the recombinant enzyme. As shown in Fig. 3, the enzyme was active on both substrates. During the course of this study, it was noticed that when phenazine methosulfate was not added in the assay reaction mixture the enzyme was still able to oxidize choline (Fig. 4). Consequently, the apparent steady-state kinetic parameters for either choline or betaine-aldehyde were also determined with molecular oxygen as the primary electron acceptor. As shown in Fig. 3, the apparent V_max values for choline and betaine-aldehyde in the absence of phenazine methosulfate decreased seven- and fourfold, respectively. In contrast, no significant changes were seen in the V/K values. The values of the kinetic parameters determined in this study are summarized in Table 2.

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FIG. 3. Steady-state kinetic parameters of choline dehydrogenase with choline (A) or betaine-aldehyde (B) as the substrate. Initial rates of reaction were determined with choline or betaine-aldehyde as the substrate in the presence (•) or absence () of 1 mM phenazine methosulfate in air-saturated 50 mM potassium phosphate (pH 7.0 and 25°C).

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FIG. 4. Dehydrogenase and oxidase catalytic activity of choline dehydrogenase. Shown is the time course of oxygen consumption during catalysis of choline dehydrogenase with 10 mM choline as the substrate in air-saturated 50 mM potassium phosphate (pH 7.0 and 25°C) and with 1 mM phenazine methosulfate (solid line) or 0.28 mM molecular oxygen (dashed line) as the final electron acceptor.

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TABLE 2. Apparent steady-state kinetic parameters for choline dehydrogenase from H. elongataa

The effect of exogenous FAD or PQQ on the activity of purified choline dehydrogenase was determined by measuring the initial rates of reaction with choline as the substrate and 1 mM phenazine methosulfate as the primary electron acceptor in the presence or absence of 1 mM FAD or PQQ in the assay reaction mixture. With 10 mM choline, the specific activity of the enzyme was 11.8 µmol of O₂ min^-1 mg^-1 in the absence of exogenous cofactors, 12.2 µmol of O₂ min^-1 mg^-1 in the presence of PQQ, and 11.5 µmol of O₂ min^-1 mg^-1 in the presence of FAD. When the concentration of choline was lowered to 5 mM, the specific activity was 8 µmol of O₂ min^-1 mg^-1 in the absence of exogenous cofactors, 7.4 µmol of O₂ min^-1 mg^-1 in the presence of PQQ, and 7.9 µmol of O₂ min^-1 mg^-1 in the presence of FAD.

Top Abstract Introduction Materials and Methods Results Discussion References

 
Based on nucleotide sequence analysis, it was previously proposed that in the moderate halophilic bacterium H. elongata the betA gene codes for choline dehydrogenase (9). As a first step towards the biochemical and mechanistic characterization of choline dehydrogenase, we cloned and expressed the H. elongata betA gene in E. coli cells under the control of the T7 promoter, partially purified the resulting protein, and carried out a preliminary kinetic characterization of the solubilized enzyme. Our initial attempts to purify recombinant choline dehydrogenase expressed in E. coli cells by using a number of different matrixes for column chromatography were not successful as a result of the instability of the enzyme in high salt and the fact that the enzyme did not bind to the matrixes used. Previous attempts to purify choline dehydrogenase from other cellular sources, such as Pseudomonas (39) or rat liver mitochondria (44), also have been hampered by the difficulty of keeping the enzyme stable and active after extraction from its cellular source. In the present study, partial purification of stable and active H. elongata choline dehydrogenase was achieved by using column chromatography with a DEAE-Sepharose matrix after treating the cell extract with 30 to 50% saturation of ammonium sulfate.

The purified enzyme expressed from betA is a choline dehydrogenase. Clear evidence supporting such a conclusion comes from steady-state kinetic studies showing that the enzyme is capable of using either choline or betaine-aldehyde as a substrate in the presence of phenazine methosulfate as the primary electron acceptor (Fig. 3). These results are consistent with previously reported data showing that the product of the enzymatic oxidation of choline, glycine-betaine, can be formed in vivo when E. coli cells containing a choline transporter and betA from H. elongata are incubated with [methyl-¹⁴C]choline (9). The ability of the enzyme to catalyze both oxidative steps in the conversion of choline to glycine-betaine has previously been observed in choline dehydrogenase from E. coli (42) and rat liver mitochondria (44) and in choline oxidase from Arthrobacter globiformis (19).

In the absence of other primary electron acceptors, choline dehydrogenase can utilize molecular oxygen for catalysis (Fig. 4), indicating that the enzyme is also able to act as an oxidase. However, when oxygen is the electron acceptor, the V_max values with betaine-aldehyde or choline as the substrate decrease four- to sevenfold with respect to the values seen with phenazine methosulfate, indicating that an electron acceptor other than oxygen is preferred by the enzyme. Previous studies on the enzyme from rat liver mitochondria suggested that coenzyme Q might be the primary electron acceptor for the enzyme in vivo (44). The observation that the enzyme from H. elongata can act either as a dehydrogenase or an oxidase depending on the availability of electron acceptors makes this enzyme different from choline dehydrogenase from rat liver mitochondria, E. coli, or Pseudomonas, for which an absolute requirement for an electron acceptor other than molecular oxygen has been shown (27, 39, 44).

The substrate specificity of choline oxidase is not affected to a great extent upon substitution of an alcohol for an aldehyde substrate, as indicated by the apparent V/K values for choline and betaine-aldehyde (Table 2). Since aldehydes are partly hydrated in aqueous solution to yield a gem-diol of the formula R-CH-(OH)₂ (4), it is likely that the hydrated form of betaine-aldehyde is the actual substrate for choline dehydrogenase. If this is the case, one would not expect significant differences in the enzyme specificity upon substituting an alcohol-containing substrate, such as choline, for a gem-diol-containing substrate, such as betaine-aldehyde. The alternative explanation that the hydroxyl group of choline and the carbonyl group of betaine-aldehyde play only a minor role in defining the substrate specificity of the enzyme appears less likely in that both these groups are intimately involved in catalysis.

As pointed out by Landfald and Strøm, a glycine box of the type G-X-G-X-X-G is found in the N-terminal region of choline dehydrogenase from E. coli (27), suggesting that the enzyme might use FAD as a cofactor for catalysis. Such a sequence is also present in the enzyme from H. elongata, which shares 74% identity with the E. coli enzyme in the deduced amino acid sequence (9). However, no direct biochemical evidence has been previously reported indicating that a flavin cofactor is actually bound or required for catalysis with these enzymes. The active choline dehydrogenase purified in our study does not show any significant absorbance in the 300- to 500-nm region of the UV-visible spectrum, which would be expected for a flavin-containing enzyme with the cofactor bound in the oxidized state. Furthermore, as in the case of choline dehydrogenase from rat liver and E. coli (27, 44), addition of exogenous FAD to the assay reaction mixture did not yield an increase in the enzymatic activity of H. elongata choline dehydrogenase, indicating no requirement for soluble FAD for catalysis. Although the data presented in this study do not rule out with absolute certainty an involvement of FAD in catalysis, it is possible that a different and as-yet-unidentified cofactor is required by H. elongata choline dehydrogenase. In this respect, it has previously been shown that the enzyme from a Pseudomonas strain, which also contains a G-X-G-X-X-G putative FAD-binding site, does not contain or require FAD for catalysis (39). In that case, a positive result was obtained when the enzyme was analyzed for the presence of PQQ. However, the activity of the choline dehydrogenase purified in our study did not change when exogenous PQQ was added to the assay reaction mixture, indicating that soluble PQQ is also not required for catalysis by the enzyme.

In conclusion, the data reported in the present study are consistent with the enzyme encoded by betA in H. elongata being a choline dehydrogenase that can also act, although with a lower catalytic efficiency, as an oxidase. To our knowledge, this study represents the first instance in which a choline dehydrogenase from a bacterial source has been cloned, expressed in soluble form, and partially purified. The availability of recombinant enzyme will prove to be a useful tool for the study of the biochemical and kinetic properties of choline dehydrogenase that is aimed at achieving a better understanding of the molecular basis of osmoprotection in bacteria. This, in turn, has great potential for biotechnological applications aimed at genetically engineering stress tolerance in crop plants of economic interest.

 
This work was supported in part by grant PRF #37351-G4 from the American Chemical Society and a Research Initiation Grant from Georgia State University.

We thank Joaquin J. Nieto, University of Seville, Spain, for the kind gift of the plasmid pDC4 containing the bet operon from H. elongata. We are also indebted to Malcolm Zellars, Georgia State University, for critically reading the manuscript.

 
* Corresponding author. Mailing address: Department of Chemistry, Georgia State University, Atlanta, GA 30303-3038. Phone: (404) 651-4737. Fax: (404) 651-2751. E-mail: ggadda{at}gsu.edu.

Top Abstract Introduction Materials and Methods Results Discussion References

 

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Applied and Environmental Microbiology, April 2003, p. 2126-2132, Vol. 69, No. 4
0099-2240/03/$08.00+0     DOI: 10.1128/AEM.69.4.2126-2132.2003
Copyright © 2003, American Society for Microbiology. All Rights Reserved.

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