From the Laboratoire Mixte de Recherche, CNRS/Institut National de la Recherche Agronomique (INRA)/Bayer CropScience (UMR 1932), Bayer CropScience, 14-20 Rue Pierre Baizet, 69263 Lyon Cedex 9, France
Received for publication, March 3, 2003 , and in revised form, April 10, 2003.
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ABSTRACT |
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INTRODUCTION |
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In plants, we have recently described the first biochemical characterization of the biotin synthase reaction (21). The bio2 gene product is a homodimer of 78 kDa presenting a high amino acid sequence similarity with the bacterial protein (4). Therefore, the CX3CX2C box is conserved and probably implied in an iron-sulfur ligation. Indeed, as its bacterial counterpart, the aerobically purified enzyme contains a [2Fe-2S]2+ center according to the UV-visible spectrum (22). Moreover, the catalytic mechanism of the reaction is AdoMet-dependent, and the synthesis of biotin is inhibited by acidomycin, a structural analogue of biotin (21). Like its bacterial counterpart, the bio2 gene product needs additional protein factors to function. Bacterial accessory proteins implied in the biotin synthase reaction efficiently complemented the plant enzyme (21). Our previous study has also shown the importance of mitochondria in the plant biotin synthesis. Therefore, we postulate that a mitochondrial physiological electron transfer system is required for plant biotin synthase reaction. It is probably similar to the system found in E. coli but implies different proteins because no flavodoxin has been documented in plants.
In the present work, we report the identification and the characterization of mitochondrial accessory proteins involved with bio2 gene product in the plant biotin synthase reaction, including a low potential electron transfer chain. Cloning, expression, and purification of each of these proteins allowed the reconstitution, for the first time, of an in vitro functional plant biotin synthase complex.
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EXPERIMENTAL PROCEDURES |
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Plant Material, Bacterial Strains, and PlasmidsPotato tubers (Solanum tuberosum L.) were obtained from a local market. The biotin auxotroph Lactobacillus plantarum (ATCC 8014) was obtained from the American Type Culture Collection (Manassas, VA). DNA manipulation was performed in E. coli DH5 cells (Invitrogen). Expression vectors pET28b(+), pET29a(+), pET21a(+), and the host strain E. coli BL21 (DE3) were from Novagen. Thermo-competent cells of this strain, prepared according to the method described in Ref. 23, were transformed with the different expression vectors used. The plasmid pBkat37 (carrying the molecular chaperones GroES and GroEL genes) (22) and the plasmid pSBET (24) (providing Arg triplets AGA and AGG frequently found in plant genes and in low abundance in E. coli) were used for optimal expression and correct folding of the recombinant proteins when indicated.
Preparation of Purified MitochondriaPotato tuber mitochondria were purified using Percoll gradients (25). Intact mitochondria were lysed in buffer A (50 mM Tris-HCl (pH 8.0), 10% (w/v) glycerol, 1 mM dithiothreitol, 150 mM KCl, 5 mM 6-aminohexanoic acid, 1 mM benzamidine HCl, and 1 mM phenylmethylsulfonyl fluoride) by sonication with a Vibra-cell disrupter (Sonics and Materials, Danbury, CT). The suspension was then centrifuged (100,000 x g, 20 min). The pellet and the supernatant comprised the mitochondrial membranes and the soluble fraction (matrix), respectively. Mitochondrial matrix (4 g of proteins) was concentrated (20 mg protein/ml) using Jumbosep-3 tubes (Filtron).
Mitochondrial Matrix FractionationMitochondrial matrix (400 mg of proteins) was loaded onto a gel filtration column (Superdex S200 Fast Flow, 2.6 cm x 60 cm, Amersham Biosciences) equilibrated with buffer A. Proteins were eluted with 320 ml of buffer A (flow rate 2 ml/min). Eighty fractions of 4 ml were collected and combined into four proteinaceous pools (pool I, fractions 140; pool II, fractions 4150; pool III, fractions 5158; pool IV, fractions 5980). Each pool was concentrated using Jumbosep-3 tubes (Filtron) and desalted on a PD10 Sephadex G-25(M) column (Amersham Biosciences). The gel filtration column chromatography was repeated 10-fold in order to fractionate 4 g of mitochondrial matrix proteins.
Gel filtration pool IV (180 mg of proteins) was applied to a DEAE-Sepharose Fast-Flow column (2.6 x 12 cm, Amersham Biosciences) equilibrated with buffer B (50 mM Tris-HCl (pH 8.0), 10% (w/v) glycerol, 1 mM dithiothreitol). The column was washed with 50 ml of buffer B. Elution was then performed with a linear gradient of KCl from 0 to 0.3 M (300 ml) and 0.3 to 0.5 M (50 ml) in buffer B (flow rate 2 ml/min). One hundred fractions of 4 ml were collected. A 100-µl aliquot of each 4-ml fraction was assayed for biotin-forming activity in combination with pure Bio2 and gel filtration pool II (see "Results"). Fractions eluted with 80150 and 350450 mM KCl were required to restore biotin synthase activity. Separate pools of these fractions were concentrated using Jumbosep-3 tubes and desalted on a PD10 Sephadex G-25(M) column. The DEAE-Sepharose column 350450 mM KCl eluted pool (10 mg protein) was further fractionated on a hydroxylapatite Bio-Gel HTP column (5 x 1 cm, Bio-Rad) equilibrated previously with buffer C (50 mM potassium phosphate (pH 6.8), 1 mM dithiothreitol). Proteins were eluted with a linear gradient of phosphate buffer from 0 to 100 mM potassium phosphate (100 ml) in buffer C (flow rate 0.5 ml/min). Fifty fractions of 2 ml were collected. A 50-µl aliquot of each 2-ml fraction was assayed for biotin-forming activity in combination with pure Bio2, gel filtration pool II, and DEAE-Sepharose column 80150 mM KCl eluted pool (see "Results"). The pooled active HTP fractions (0.7 mg of protein) were concentrated using Macrosep-3 tubes, desalted, and stored at 80 °C.
Gel filtration pool II was fractionated onto a DEAE-Sepharose Fast-Flow column. The chromatographic conditions were the same as those described previously for fractionation of gel filtration pool IV. A 100-µl aliquot of each eluted fraction was assayed for biotin-forming activity in association with purified recombinant Bio2, Adx1, and AdxR proteins (see below for definitions). Active fractions were pooled, concentrated using Macrosep-10 tubes, and stored at 80 °C until use.
Engineering of Expression VectorsThe oligonucleotide primers utilized in this study (synthesized by MWG Biotech) are listed in Table I. For protein expression, adxR, adx1, adx2, and nfs1 cDNAs were cloned into pET expression vectors (Table I). Full-length cDNAs were obtained by PCR amplification of an A. thaliana (var. Columbia) cDNA library constructed in pYES (26). The PCR fragments were cloned into the cloning vector pPCR-Script (Stratagene) or pCR4Blunt-TOPO (Invitrogen) according to the manufacturer's instructions. All the cDNAs were sequenced, and the resulting sequences were submitted to the GenBankTM Data Bank. After proper restriction enzyme digestion, DNA fragments containing the coding sequences were subcloned into different pET expression vectors (Table I). The E. coli expression vector pET28b(+) was used to place a His6 tag at the NH2 terminus of the polypeptide.
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Arabidopsis bio2 cDNA cloning has been described previously (22). The NdeI-BamHI DNA fragment containing the bio2 coding sequence was subcloned into the plasmid pET28b(+) in-frame with an NH2-terminal His6 tag coding sequence, yielding the plasmid pET28-bio2.
Expression of Recombinant ProteinsFor correct Bio2 and Adx1 folding, BL21 strains containing the plasmid pET28-bio2 or pET28-adx1m were transformed with the pBkat37 vector, whereas efficient expression of Nfs1 protein was achieved with BL21 strain co-transformed with the plasmid pET21-nfs1 and pSBET. The E. coli BL21 cells transformed with the different expression vectors were grown at 37 °C in Luria-Bertani medium supplemented with the appropriate antibiotics. When A600 reached 0.6, 1 mM isopropylthio--D-galactoside was added to induce recombinant protein synthesis. The cells were further grown for 16 h at 28 °C, harvested, and centrifuged for 20 min at 4,000 x g. After resuspension in appropriate buffer, each bacterial pellet was disrupted by sonication with a Vibra-Cell disrupter (100 pulses every 3 s on power setting 5). The soluble protein extract was separated from the cell debris by centrifugation at 18,000 x g for 30 min.
Purification of Recombinant Bio2 and Adx1 ProteinsBio2 and Adx1 proteins were both purified by metal-chelate column chromatography. The cells containing the overexpressed Bio2 or Adx1 proteins were resuspended in buffer D (20 mM Tris-HCl (pH 7.9), 500 mM NaCl)) supplemented with 5 mM imidazole. The soluble protein extract was applied to a nickel-nitrilotriacetic acid-agarose column (1.6 x 4 cm, Qiagen) previously equilibrated with 30 ml of buffer D supplemented with 5 mM imidazole. The column was washed with buffer D supplemented with 50 mM imidazole. The recombinant protein was then eluted using buffer D supplemented with 250 mM imidazole. Fractions containing the recombinant protein (Bio2 or Adx1) were pooled and dialyzed against 50 mM Tris-HCl (pH 8.0), 15% (w/v) glycerol. Purified enzymes were aliquoted and stored at 80 °C until use.
Purification of Recombinant AdxR ProteinPurified Adx1 protein (20 mg) was immobilized on Affi-Gel 10 (Bio-Rad) mini-columns according to the manufacturer's instructions. The cells containing the overexpressed AdxR were resuspended in buffer B and disrupted by sonication. The soluble protein extract (400 mg proteins) was loaded onto a Green-A-matrix (1.6 x 10 cm, Sigma) column equilibrated previously with buffer B. The column was washed with 100 ml of buffer B. Elution was then performed with 50 ml of buffer B supplemented with 1.5 M of KCl (flow rate 0.5 ml/min). Fractions containing proteins were combined, concentrated with Jumbosep-10 tubes, desalted, and loaded (50 mg of proteins) onto the Affi-Gel-Adx1 (1 x 3 cm) column that had been equilibrated with buffer B. The column was washed with 50 ml of buffer B containing 50 mM of KCl. Proteins were eluted with 4 ml of buffer B supplemented with 1 M of KCl. The AdxR-containing fractions were combined, concentrated, and stored aliquoted at 80 °C.
Purification of Recombinant Nfs1 ProteinThe overexpressed Nfs1 protein was insoluble in E. coli. Inclusion bodies containing the recombinant protein were prepared and purified as described in Ref. 27. After separation on 12% SDS-PAGE, inclusion bodies proteins were stained with Coomassie Blue to locate the Nfs1 protein band. This band was then excised, placed into dialysis tubing (SnakeSkinT Dialysis Tubing 10K, Pierce), submitted to electroelution for 4 h at 50 V in 50 mM NH4HCO3, 0.1% SDS, and freeze-dried overnight. The prepared polypeptide (0.5 mg) was resuspended in phosphate-buffered saline and used to obtain rabbit antibodies.
Enzyme Activity AssaysBiotin synthase activity was measured in the presence of the bio2 gene product (10 µM monomer) and protein fractions (matrix proteins and/or purified recombinant accessory proteins), according to the radiochemical and microbiological protocols described previously (21). The standard reaction mixture, in a final volume of 100 µl, contained 50 mM Tris-HCl (pH 8.0), 2 mM dithiothreitol, 0.5 mM Fe(NH4)2(SO4)2, 1 mM NADPH, 0.2 mM AdoMet, 5 mM fructose 1,6-bisphosphate, 0.1 mM thiamine pyrophosphate, 0.15 mM DTB, and 0.5 mM L-cysteine (or 1 mM Na2S when indicated).
Cytochrome c reduction was assayed in 50 mM Tris-HCl (pH 8.0) in the presence of 50 µM cytochrome c,50 µM NADPH, 10 µM Adx1, and 60 nM AdxR. The reduction of cytochrome c was followed by the absorption increase at 550 nm.
Electrophoresis and ImmunoblottingSDS-PAGE was performed in slab gels containing 12% (w/v) acrylamide. The conditions for gel preparation, sample solubilization, electrophoresis, and gel staining were detailed by Chua (28). Polypeptides were also transferred electrophoretically onto nitrocellulose sheets (Bio-Rad) as described by Towbin et al. (29). For Western blot detections, rabbit antiserum raised against the recombinant mitochondrial Nfs1 protein from Arabidopsis and guinea pig antiserum raised against the recombinant AdxR from Arabidopsis were prepared (Elevage Scientifique des Dombes, Romans, France). Polyclonal anti-rabbit serum (Bio-Rad) and polyclonal anti-guinea pig serum (Sigma) were used as a second antibody. The presence of immune complexes was analyzed by chemiluminescence with an ECL kit (Roche Applied Science).
Analytical MethodsProtein concentration was determined either by the Bradford method (30) using Bio-Rad protein-assay reagent, with -globulin as a standard, or for pure proteins by measuring the absorbance at 205 nm (31). UV-visible spectra were recorded using a Uvikon 860 (Kontron) spectrophotometer. DNA sequencing was performed on both strands using the Prism Kit with fluorescent dideoxynucleotides (Applied Biosystems, Genome Express, Meylan, France). Internal peptide sequencing was performed by Edman degradation after tryptic digestion of the proteins and purification of the resulting peptides by high pressure liquid chromatography (Institut Pasteur, Laboratoire de microséquençage des protéines, Paris, France). Kinetic data were fitted to the appropriate rate equations by nonlinear regression analyses using the Kaleidagraph program (Synergy Software, Reading, PA).
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RESULTS |
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Identification of the Active Proteins in Pool IVPool IV was fractionated further on a DEAE-Sepharose column. None of the individual fractions eluted from the DEAE-Sepharose column were active in the biotin synthase assay. This implied that more than one component was present in pool IV and that these components had been separated on the anion-exchange column. Indeed, under our in vitro assay conditions (see "Experimental Procedures"), both fractions eluted with 80150 and 350450 mM KCl, respectively, were required, in addition to the bio2 gene product and the gel filtration pool II (see Fig. 1), to trigger efficient biotin synthase activity.
Identification of the Active Protein in the DEAE Column 350450 mM KCl Eluted PoolThe DEAE 350450 mM KCl eluted pool was loaded onto a hydroxylapatite (HTP) column. The active component was eluted with a linear phosphate-buffered gradient. Biotin synthase activity was measured with each of these HTP fractions in association with Bio2, gel filtration pool II (see Fig. 1), and the DEAE 80150 mM KCl eluted pool. Biotin production was observed with the HTP fractions eluted with 3050 mM phosphate buffer. At this stage of the purification, a slight red coloration was associated with this mitochondrial active fraction. UV-visible absorbance spectrum showed characteristic peaks for iron-sulfur proteins containing [2Fe-2S] clusters (Fig. 2A). SDS-PAGE analysis of the concentrated active fraction revealed the presence of two major proteins, named P1 and P2, and less abundant proteins of higher molecular masses (Fig. 2B). The apparent molecular masses of the P1 and P2 proteins were 22 and 16 kDa, respectively. SDS-PAGE analysis of the individual active HTP fractions showed that only the quantitative variation of the P1 protein was perfectly correlated with the quantitative variation of the biotin synthase activity (data not shown). As a result, despite the occurrence of two major proteins, P1 protein and not P2 protein seemed to play a role in the biotin synthase reaction. To confirm this, both P1 and P2 proteins prepared from potato tuber mitochondria were digested with trypsin, and the resulting peptides were purified by high pressure liquid chromatography. Two peptides from P1 protein and one from P2 protein were sequenced, respectively (Fig. 2C). As shown in Fig. 2C, P2 protein was identified as H-protein, one of the components of the mitochondrial glycine cleavage system by a FASTA search in the Arabidopsis genome data base. Thus, as expected, this protein was unlikely to be involved in the physiological reduction system required for biotin synthase activity. On the contrary, a strong similarity was found between the two peptide sequences of the P1 protein and two adrenodoxin-like proteins of Arabidopsis, annotated as putative mitochondrial ferredoxins (Fig. 2C). Adrenodoxins are small iron-sulfur proteins with electron transfer properties that belong to the large family of the [2Fe-2S]-type ferredoxins ubiquitously found in plants, animals, and bacteria. These properties of Adx made P1 protein a good candidate for being the HTP 3050 mM phosphate eluted pool component involved in the biotin synthase reaction. It is also responsible for the reddish coloration of this HTP active fraction (Fig. 2A). We have isolated and sequenced full-length cDNAs from Arabidopsis that we named adx1 and adx2, corresponding to these putative mitochondrial ferredoxins, as described under "Experimental Procedures." Both Adx1 and Adx2 deduced amino acid sequences consist of 197 residues yielding proteins of 22 kDa. The alignment of Adx sequences from very distant species like Arabidopsis, Bos taurus, and Rickettsia prowazekii shows high overall similarity (about 50%) and high conservation in several protein domains (Fig. 3A). Moreover, we evidenced 90% of similarity between both Arabidopsis Adx-like protein sequences (Fig. 3A). As a result, we realized all subsequent experiments with only one Arabidopsis Adx-like protein, the Adx1 protein. The coding sequence for the putative Adx1 mature protein (amino acid 44197) was cloned into the E. coli expression vector pET28 in-frame with an NH2-terminal His6 tag coding sequence. Efficient expression of the recombinant protein was achieved in E. coli BL21 (DE3) strain, which contains the T7 polymerase system. Then the Adx1 protein was purified by standard nickel-affinity chromatography. On SDS-PAGE, the purified Adx1 protein showed a single band with a molecular mass of 22 kDa (Fig. 4A, lane 1). The pure native protein has a reddish coloration and contains a [2Fe-2S] center according to the UV-visible spectrum (Fig. 4B). Moreover, the potato HTP biotin synthase activating fraction, resulting from the DEAE 350450 mM KCl eluted pool fractionation, could be efficiently replaced by this purified recombinant Adx1 protein for in vitro biotin synthase reaction (in an assay mixture also comprising Bio2, gel filtration pool II, and the DEAE 80150 mM KCl eluted pool). All these results indicate that the Adx1 protein is one of the elements involved in the physiological reduction system required for plant biotin synthase activity.
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Identification of the Active Protein in the DEAE Column 80150 mM KCl Eluted PoolThe primary function of Adx in mammals is to supply electrons from an NADPH-dependent adrenodoxin reductase to different electron acceptors. Thus, we speculated that, by inference, an AdxR-like protein was the active component present in the DEAE 80150 mM KCl eluted pool. Interestingly, a BLAST search in the Arabidopsis data base allowed us to identify a protein presenting high overall similarity with the well characterized bovine AdxR (Munich Information Center for Protein Sequences (MIP) accession number At4g32360, annotated ferredoxin-NADP+ reductase like-protein) (Fig. 3B). The full-length cDNA from Arabidopsis encoding this putative AdxR was isolated and cloned into the E. coli expression vector pET29. The deduced amino acid sequence consists of 483 residues yielding a protein of 53 kDa. A two-step protocol was devised to purify to near homogeneity the putative AdxR from Arabidopsis overexpressed in E. coli cells, including an affinity chromatography onto an Affi-Gel-Adx1 column (for details, see "Experimental Procedures"; Fig. 4A, lane 2). The pure protein has a yellow coloration, and its UV-visible absorbance spectrum shows characteristic peaks for FAD-containing flavoproteins (Fig. 4C). Antibodies raised against this purified Arabidopsis putative AdxR were prepared and used for Western blot analysis. As shown in Fig. 5, antibodies raised against the recombinant protein from Arabidopsis reacted with a single 50-kDa polypeptide, exclusively in pool IV from the gel filtration chromatography and in the 80150 mM KCl eluted pool from the DEAE column. More importantly, the substitution of this last fraction by the purified putative AdxR from Arabidopsis was efficient for the biotin synthase assay. These results confirm the presence of an AdxR-like protein in the DEAE 80150 mM KCl eluted pool and strongly suggest that AdxR is associated with Adx1 to form the physiological reduction system required for plant biotin synthase reaction.
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Characterization of the Arabidopsis Adx-AdxR Reaction The efficiency of the electron transfer between recombinant AdxR and recombinant Adx1 from Arabidopsis was tested by measuring the cytochrome c reduction at 550 nm. This reduction was only observed in the presence of purified AdxR, purified Adx1, and NADPH. It was completely abolished if one of these three components was absent (data not shown). Consequently, NADPH, AdxR, and Adx1 form an active electron transfer chain allowing the cytochrome c reduction. We determined the Michaelis constant of AdxR with NADPH and NADH using the same cytochrome c reduction test. The Km values for NADPH and NADH were 2.4 and 1000 µM, respectively. Moreover, the concentration dependence of Adx1 was explored using NADPH as an electron source. The half-maximal velocity of the reaction was observed with 0.5 µM Adx1. These values are similar to those reported for mammalian proteins (3234). As a result, the Arabidopsis AdxR, like the mammalian proteins, primarily transfers electrons from NADPH. On the contrary, the yeast AdxR equivalent (Arh1p) could receive electrons from either NADPH or NADH because the apparent Km value is roughly the same for both substrates in vitro (35).
Identification of Pool II Component from the Gel Filtration Chromatography Required for the Plant Biotin Synthase ReactionAs described above, AdxR and Adx1 from Arabidopsis formed a functional electron transfer chain. However, when biotin synthase activity driven by Bio2 was measured in the presence of these two purified recombinant proteins, biotin production during the reaction was low. Addition of the gel filtration pool II strongly enhanced the biotin production level (Fig. 6A). In order to identify the component responsible for this positive effect, gel filtration pool II was fractionated further on a DEAE-Sepharose column. Each of the eluted fractions was tested in the biotin synthase assay (including purified recombinant Bio2, Adx1, and AdxR proteins). Enhanced biotin production was only observed with the DEAE fractions eluted with 220280 mM KCl. Interestingly, this protein fraction and cysteine could efficiently be replaced by Na2S (Fig. 6A). As a result, we supposed that the DEAE column 220280 mM KCl eluted pool probably metabolized the cysteine present in the assay medium for sulfide production. Such proteins, which are able to pull out a sulfur atom from cysteine, have already been described and named cysteine desulfurase. We have cloned a cDNA from Arabidopsis encoding a cysteine desulfurase-like protein (Nfs1) (21). The deduced amino acid sequence consists of 453 residues yielding a protein of 50 kDa. Moreover, transient expression of green fluorescent protein fusion protein into Arabidopsis cells demonstrated a mitochondrial location for this protein (36). The resulting protein was overexpressed in E. coli cells. Unfortunately, the plant recombinant protein was exclusively insoluble in E. coli under all the culture conditions tested and was recovered in the inclusion body fraction. Expression of the mature protein devoid of the transit peptide did not improve solubility (data not shown). Nevertheless, the inclusion bodies were purified, and rabbit antibodies raised against this protein were prepared. Then potato mitochondrial matrix, gel filtration pool II, and DEAE column 220280 mM KCl eluted pool were subjected to Western blot analysis (Fig. 6B). Antibodies raised against Nfs1 from Arabidopsis reacted with a single polypeptide of 47 kDa in each of these fractions. Moreover, a significant enrichment of the Nfs1-like protein was observed in the DEAE column 220280 mM KCl eluted pool. In addition, this protein enrichment was perfectly correlated with the biotin synthase stimulating activity. Although no pure soluble recombinant cysteine desulfurase could be tested for biotin synthase stimulating activity in this study, all together our results suggest an essential role of this protein in the biotin synthase reaction.
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Reconstitution of Arabidopsis Biotin Synthase System in VitroOn the basis of the data presented above, we have reconstituted a functional Arabidopsis biotin synthase complex in vitro and defined new optimal assay conditions with each of the purified accessory proteins identified here. As noted previously, recombinant Nfs1 protein was insoluble in E. coli cells. Because Na2S replaced efficiently the Nfs1-enriched fraction plus cysteine, as a result, Na2S was subsequently used for all optimization experiments. The concentration dependence of Adx1 and AdxR was first explored. In the presence of 2.5 µM AdxR, biotin production evolves with an increasing concentration of Adx1 and finally saturates at about 5 µM (Fig. 7A). In the presence of saturating Adx1, about 1 µM AdxR was required for biotin production (Fig. 7B). These values are of the same order of magnitude as those reported for flavodoxin and flavodoxin reductase, which are components of electron transfer chain involved in the E. coli biotin synthase reaction (18). Assay conditions were also optimized with respect to small factors. Notably, fructose 1,6-bisphosphate and thiamine pyrophosphate, which stimulated biotin synthase activity in a system comprising purified Arabidopsis Bio2 protein in combination with unfractionated mitochondrial proteins (21), had no effect on the well defined plant system and thus were subsequently omitted. The reconstitution of an active Arabidopsis biotin synthase complex was also checked using the radiochemical method with [3H-DTB] as the source of radioactive label (21). This test has the advantage of making visible the product of the Arabidopsis biotin synthase reaction. Data shown in Fig. 8 confirmed that neither recombinant Arabidopsis Adx1 nor AdxR alone could support the conversion of DTB to biotin by biotin synthase. However, when AdxR and Adx1 were added to the assay mixture together at optimized concentrations, biotin synthesis was efficiently restored, as shown by the apparition of a product supporting the same migration properties as a purified standard biotin (Fig. 8).
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DISCUSSION |
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Is that the only function of Adx and AdxR in plant mitochondria? Very little is known about these proteins in plants, and the main knowledge comes from studies realized in animals, yeast, and bacteria. In mammals, they are involved in the cytochrome P450 reduction, enabling steroid hormone biosynthesis (38). In yeast, they have an important role in the heme A synthesis, the prosthetic group confined exclusively to mitochondrial and some bacterial cytochrome oxidases (39). Another function of two members of the Adx subfamily, Fdx in E. coli and Yah1p in yeast mitochondria, has attracted much attention in recent years. The fdx gene, located in the isc (iron-sulfur cluster) operon together with iscS, iscU, iscA, hscB, and hscA, is crucial for the efficient biosynthesis of Fe-S clusters in E. coli (4042). A similar machinery has been identified in yeast mitochondria (43). The YAH1 gene is essential for viability of yeast cells, and depletion of Yah1p causes a marked decrease in the activities of mitochondrial and cytosolic Fe-S proteins (44, 45). In plants, it is unlikely that Adx and AdxR, both localized in mitochondria, reduce cytochrome P450. Indeed, despite a large number of cytochrome P450 genes in Arabidopsis genome (46), none of these have been characterized in mitochondria (37). On the opposite, we cannot exclude the involvement of this redox chain in the plant Fe/S cluster biosynthesis. Indeed, some proteins showing a high overall similarity with yeast proteins involved in this process were found in the Arabidopsis data base and predicted to be mitochondrial (36). Therefore, Adx and AdxR could have a dual function with respect to the bio2 gene product, a specific function in the biotin synthase reaction and a more general role in its Fe/S cluster biosynthesis (47). Finally, recent studies (48, 49) support the conclusion that both biotin synthase and lipoate synthase are strongly mechanistically related proteins. Consequently, the implication of Adx and AdxR in the mitochondrial lipoate synthase reaction that catalyzes the formation of two C-S bonds from octanoic acid could also be suggested.
The proteins involved in the physiological reduction system for plant biotin synthase reaction identified in this report are different from those described for bacterial systems. Indeed, in E. coli this system is composed of flavodoxin and flavodoxin (ferredoxin)-NADP+ reductase (14, 1719). In a previous study, we showed that heterologous interaction between Arabidopsis Bio2 protein and bacterial proteins yielded a functional biotin synthase complex (21). Flavodoxin and ferredoxin (flavodoxin)-NADP+ reductase were supposed to be these bacterial components. However, the Adx-type ferredoxin from E. coli (Fdx) was recently described as the kinetically and thermodynamically preferred partner for ferredoxin (flavodoxin)-NADP+ reductase (50). Consequently, the involvement of this ferredoxin in the E. coli biotin synthase reaction is not excluded. Whatever the proteins involved in the electron transfer to Bio2, protein-protein interactions are essential for the formation of an active biotin synthase complex. Further studies, which are in progress in our laboratory, will enable us to elucidate the nature of these interactions. Studies of the mechanism by which these proteins are recruited for biotin synthesis could provide essential information about biotin synthesis regulation in the plant cell mitochondria.
Our results also suggest an essential role of a mitochondrial cysteine desulfurase protein (Nfs1) in the restoration of Arabidopsis biotin synthase activity in vitro, when cysteine is used as a sulfur donor. This result strongly supports the idea that cysteine is the initial sulfur donor for biotin in plant mitochondria. However, the mechanism by which the sulfur atom is mobilized from cysteine and next transferred into DTB remains unclear. For E. coli biotin synthase, two different models are presently proposed. First, the sulfur atom is extracted from cysteine by a cysteine desulfurase. It is next incorporated into DTB via the [2Fe-2S] cluster of biotin synthase, which is the final sulfur donor (10, 15, 51). Second, a pyridoxal 5'-phosphate-dependent cysteine desulfurase activity recently attributed to E. coli biotin synthase could provide, via a protein-bound persulfide, the sulfur atom for biotin (52). Amino acids proposed to be involved in the [2Fe-2S] formation by Ugulava et al. (10) and in the persulfide binding by Ollagnier-de-Choudens et al. (52) are the same. Consequently, the two models are incompatible. In Arabidopsis, Nfs1 protein addition led to a marked increase in biotin synthase activity. This confirms and strengthens the results obtained by Kiyasu et al. (53) with a crude bacterial cell-free system. Indeed, they have shown that IscS protein (cysteine desulfurase encoded by the isc operon) of E. coli significantly stimulated the biotin synthase reaction in the presence of cysteine. Interestingly, in the absence of exogenously added cysteine desulfurase, we observe a slight but significant biotin production when the bio2 gene product is associated with purified Adx and AdxR with cysteine as sulfur donor (Fig. 6A). As a result, we cannot exclude an endogenous pyridoxal 5'-phosphate-dependent cysteine desulfurase activity for the bio2 gene product. However, contrary to what is observed for the bacterial enzyme (52), pyridoxal 5'-phosphate addition has no effect on Arabidopsis biotin synthase activity (data not shown). Finally, as discussed above, plant mitochondria might contain a complex iron-sulfur cluster assembly machinery, including Nfs1, similar to that found previously (36) in yeast. Whether all or part of its components in addition to Nfs1 participates or not in the plant biotin synthase reaction remains to be established (Fig. 9).
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FOOTNOTES |
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* The costs of publication of this article were defrayed in part by the payment of page charges. This article must therefore be hereby marked "advertisement" in accordance with 18 U.S.C. Section 1734 solely to indicate this fact.
Present address: UMR 5019 CNRS/Commissariat à l'Energie Atomique (CEA)/Université Joseph Fourier/INRA, CEA-Grenoble, Dépt. Réponse et Dynamique Cellulaires, Laboratoire de Physiologie Cellulaire Végétale, 17 rue des Martyrs, 38054 Grenoble Cedex 9, France.
Present address: Institut de Biologie Structurale, 41, rue Jules Horowitz, 38027 Grenoble Cedex 1, France.
¶ To whom correspondence should be addressed: UMR 5019 CNRS/Commissariat à l'Energie Atomique (CEA)/Université Joseph Fourier/INRA, CEA-Grenoble, Dépt. Réponse et Dynamique Cellulaires, Laboratoire de Physiologie Cellulaire Végétale, 17 rue des Martyrs, 38054 Grenoble Cedex 9, France. Tel.: 33-438-78-23-63; Fax: 33-438-78-50-91; E-mail: calban{at}cea.fr.
1 The abbreviations used are: DTB, dethiobiotin; AdoMet, S-adenosylmethionine; Adx, adrenodoxin; AdxR, adrenodoxin reductase; Fdx, ferredoxin.
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ACKNOWLEDGMENTS |
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REFERENCES |
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