From the Department of Molecular Biology, Stockholm
University, S-106 91 Stockholm, Sweden, the
Department of
Genetics & Microbiology, Faculty of Sciences, Autonomous University of
Barcelona, Bellaterra, 08193 Barcelona, Spain, and the
§§ Ludwig Institute for Cancer Research,
Biomedical Center, Box 595, S-751 24 Uppsala, Sweden
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ABSTRACT |
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Ribonucleotide reductases (RNRs) are key enzymes in living cells that provide the precursors of DNA synthesis. The three characterized classes of RNRs differ by their metal cofactor and their stable organic radical. We have purified to near homogeneity the enzymatically active Mn-containing RNR of Corynebacterium ammoniagenes, previously claimed to represent a fourth RNR class. N-terminal and internal peptide sequence analyses clearly indicate that the C. ammoniagenes RNR is a class Ib enzyme. In parallel, we have cloned a 10-kilobase pair fragment from C. ammoniagenes genomic DNA, using primers specific for the known class Ib RNR. The cloned class Ib locus contains the nrdHIEF genes typical for class Ib RNR operon. The deduced amino acid sequences of the nrdE and nrdF genes matched the peptides from the active enzyme, demonstrating that C. ammoniagenes RNR is composed of R1E and R2F components typical of class Ib. We also show that the Mn-containing RNR has a specificity for the NrdH-redoxin and a response to allosteric effectors that are typical of class Ib RNRs. Electron paramagnetic resonance and atomic absorption analyses confirm the presence of Mn as a cofactor and show, for the first time, insignificant amounts of iron and cobalt found in the other classes of RNR. Our discovery that C. ammoniagenes RNR is a class Ib enzyme and possesses all the highly conserved amino acid side chains that are known to ligate two ferric ions in other class I RNRs evokes new, challenging questions about the control of the metal site specificity in RNR. The cloning of the entire NrdHIEF locus of C. ammoniagenes will facilitate further studies along these lines.
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INTRODUCTION |
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Ribonucleotide reductases (RNRs)1 catalyze the reduction of ribonucleotides providing 2'-deoxyribonucleotides for DNA replication and repair. Three well-characterized classes of RNRs, with limited sequence similarities, have been described. They differ in their overall protein structure and cofactor requirement but have in common an allosteric regulation and the use of an organic radical to initiate catalysis through free radical chemistry (1, 2) .
Apart from the similarity in mechanism, the radical chain initiator and
the accompanying metal cofactor differ between the three classes. Class
I enzymes (2
2) contain a stable tyrosyl radical and a dinuclear iron center. Class II enzymes (
or
2) use adenosylcobalamin as cofactor and cleave it to
produce a 5'-deoxyadenosyl radical (3, 4). The anaerobic class III
enzymes (
2
2) possess a stable glycyl
radical and an iron-sulfur cluster (5). Moreover, the different RNRs
require their specific physiological reductants thioredoxin,
glutaredoxin, and formate, respectively (6-8). At the beginning of the
1990s, only these three classes of RNR were known, and they were found
to cover all major branches of the tree of life. However, additional
types of RNRs may remain to be discovered, and questions about
non-exhaustively characterized atypical RNRs have to be answered.
During the last few years, an additional operon, in practice silent under normal laboratory growth conditions, coding for a new type of RNR, was found in Salmonella typhimurium and Escherichia coli (9-11). These enzymes share with class I enzymes the subunit composition and distinct sequence similarity, including all highly conserved residues, such as the iron ligands, the tyrosyl radical, and active site cysteines. Thus, the discovery of these enzymes led to the division of the class I RNR in two subclasses, classes Ia and Ib (12). The class Ia reductase is encoded by the nrdA and nrdB genes, coding for the homodimeric proteins R1 and R2, respectively, and the class Ib reductase is encoded by the nrdE and nrdF genes, coding for the homodimeric proteins R1E and R2F, respectively. In E. coli and S. typhimurium, the low expression of the nrdE and nrdF genes of class Ib cannot support aerobic growth, and these bacteria are totally dependent on class Ia (11). Moreover, the physiological role of these "silent" enzymes is still unknown. However, the Lactococcus lactis RNR was found to be a functionally active reductase of the class Ib type (12), and the purified enzyme from Mycobacterium tuberculosis also turned out to belong to this class (13, 48). Class Ib genes have also been described in Bacillus subtilis, Mycoplasma genitalium, and M. pneumoniae (14-16).
The isolation and characterization of a unique manganese-dependent RNR activity in Corynebacterium (formerly Brevibacterium) ammoniagenes was reported in the 1980s (17, 18). The specific Mn requirement of C. ammoniagenes was first observed in the 1960s during studies of factors controlling nucleotide overproduction (19, 20). Mn-starved cells showed so-called "unbalanced growth death" because they were arrested in DNA synthesis (17) due to inhibition of DNA precursor synthesis (21). Upon addition of manganese ions to the medium, DNA synthesis and growth were rapidly restored to the level of a nonstarved culture. The main target of Mn starvation was suggested to be RNR activity, which was very low in a Mn-depleted culture but was increased when manganese ions were supplied in vivo (17). Similar correlations between RNR activity and Mn-starvation conditions have been demonstrated in other coryneform bacteria, such as Arthrobacter citreus, A. globiformis, and A. oxydans, and in Micrococcus luteus, (17, 21, 22).
The partially purified C. ammoniagenes RNR was suggested to consist of two subunits (18, 23), a nucleotide-binding component called B1 (in this report renamed R1E) and a metal-containing component called B2 (in this report renamed R2F). The presence of Mn was suggested on the basis of specific 54Mn incorporation into the R2F subunit, as well as appearance of a characteristic Mn six-line EPR spectrum after denaturation of a protein preparation containing R2F. Recently, a novel type of stable organic free radical signal was reported for partially purified C. ammoniagenes RNR (24). However, the radical has not been characterized in detail. Generally, a new metal center and a novel organic radical would be enough to define a new class of RNR. However, other properties, such as the sensitivity to hydroxyurea and the polypeptide sizes of this C. ammoniagenes RNR, suggest a similarity with the well known class I. An intriguing question is therefore whether the C. ammoniagenes RNR is a prototype of a new class of RNR or a subtype of one of the existing classes.
In this study, we report that the Mn-containing RNR of C. ammoniagenes is of the class Ib type. We have followed two
parallel approaches: identification of class Ib genes in the C. ammoniagenes genome by PCR and purification to homogeneity of the
active RNR from C. ammoniagenes, followed by N-terminal and
internal peptide amino acid sequence analysis of the - and
-polypeptide chains. The amino acid sequences obtained from the
enzyme proper matched the cloned and sequenced class Ib genes
nrdE and nrdF. In addition, the sequence of the
neighboring genes nrdH and nrdI is reported.
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EXPERIMENTAL PROCEDURES |
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Materials, Strains, and Plasmids--
Wild type C. ammoniagenes (ATCC 6872), obtained from the collection of A. N. Bach (Institute of Biochemistry, Russian Academy of Sciences,
Moscow, Russia) and E. coli DH5F'
(CLONTECH) strains were used. Plasmid vectors used
were pBluescript SK(+) (pBSK, Stratagene) for subcloning and sequencing
and pGEM-T (Promega Corp.) for cloning of PCR-generated fragments.
Growth Conditions and General Recombinant DNA Techniques-- C. ammoniagenes ATCC 6872 and E. coli strains were grown aerobically in LB medium at 30 and 37 °C, respectively. Ampicillin was added at 50 µg/ml when selecting for plasmid-containing clones. Genomic DNA from C. ammoniagenes was extracted as described (26) and purified by ultracentrifugation on a cesium chloride gradient. ExoIII deletions were constructed by using the double-stranded nested deletions kit (Pharmacia Biotech Inc.) following the supplier's instructions. DNA sequencing was carried out using the dideoxynucleotide sequencing method with fluorescent universal primers (M13 direct and reverse) and the Automated Laser Fluorescent DNA sequencer (Pharmacia). Other general DNA manipulations and Southern hybridizations were done by standard procedures (27). Sequence analyses were made with the University of Wisconsin Genetics Computer Group package (version 9.0 for UNIX).
PCR Amplification of Partial nrdF Gene-- For PCR amplification of the nrdF gene of C. ammoniagenes, two primers were designed from conserved R2F peptide sequences (GYKYQ and NHDFFS, respectively; indicated in Fig. 3): CoryFup, 5'-GGCTACAAGTACCAG-3', and CoryFlow, 5'-AACCACGACTTCTTCTC-3' (antisense). Genomic DNA (0.2 µg) was used as template in a 50-µl PCR amplification reaction with 50 pmol of each primer, all dNTPs (0.2 mM each), 5 µl of 10× PCR buffer (Boehringer Mannheim), and 1.5 units of Taq polymerase. The reaction was run with the following program: (a) 3 min at 94 °C; (b) 30 cycles of 1 min at 94 °C, 1 min at 50 °C, and 1 min at 72 °C; and (c) 7 min at 72 °C. The amplification product was purified from an ethidium bromide, 3% Nusieve-agarose gel by melting the band in 6 M NaI at 50 °C and using the Wizard DNA Clean-up system (Promega Corp.), and cloned in pGEM-T according to the manufacturer's protocol. This fragment was labeled with the DIG DNA labeling and detection kit (Boehringer Mannheim).
Construction and Screening of a Chromosomal C. ammoniagenes Phage Library--
The library of C. ammoniagenes ATCC 6872 genomic DNA consisted of a mixture of partially digested DNA. Freshly
prepared genomic DNA (15 µg) was partially digested with
Sau3A. Fragments of 6-11 kb were pooled, and
restriction-generated ends were filled in with A and G nucleotides by
incubation at 37 °C for 30 min with 10 units of Klenow DNA
polymerase (Boehringer Mannheim). Lambda GEM-12 vector (Promega) was
prepared by filling in XhoI-generated ends with T and C
nucleotides. After ligation of insert DNA to vector, the library was
packaged using Packgene extracts (Promega).
Fermentation and Purification of RNR--
C. ammoniagenes ATCC
6872 was inoculated from a slant (1% yeast extract, 1% glucose, 1%
CaCO3, 2% agar; Difco) grown at 30 °C for 24 h in
100 ml of inoculate medium (2% glucose, 1% peptone, 1% yeast
extract, 0.3% NaCl, 0.05 mg/ml biotin) and cultivated at 30 °C
overnight. The overnight culture was used to inoculate several 1-liter
batches of minimal fermentation medium (21), and cultivation was
continued in 5-liter flasks at 30 °C and 220 rpm. After 10 h of
growth, 10 µM MnCl2 was added to the medium, and 1 h after Mn repletion, cells were harvested by
centrifugation. The cell paste was washed with Buffer A (85 mM potassium phosphate buffer, pH 7.0, 2 mM
DTT), frozen on dry ice, and stored at 80 °C.
Enzyme Activity Assay-- RNR activity was assayed in 50-µl mixtures containing 120 mM potassium phosphate buffer, pH 7.0, 1 mM dATP as a positive effector, 1 mM magnesium acetate, 10 mM DTT, 13 µM E. coli thioredoxin, 5-20 µl of the concentrated protein solution. The reaction was started by addition of [3H]CDP (specific activity, 60,000-80,000 cpm/nmol) to a final concentration of 0.5 mM. Assay mixtures were incubated for 20 min at 30 °C and stopped by addition of 0.5 ml of ice-cold 1 M perchloric acid. One unit of enzyme activity corresponds to 1 nmol of dCDP formed per min of incubation (30).
SDS-PAGE and Protein Blotting--
To obtain partial peptide
amino acid sequences, SDS-PAGE was used. Protein samples (50 µg of
total protein) were first denatured in a mixture of 125 mM
Tris-HCl, pH 6.8, 2.5% SDS, 10 mM DTT, 15% glycerol, and
0.01% bromphenol blue. After boiling for 2-3 min and cooling to room
temperature, the incubation was continued with 20 mM
iodoacetamide for another 20 min in darkness at room temperature.
Reduced and alkylated protein samples were separated on 7.5%
SDS-polyacrylamide gel, stained with 0.1% Coomassie Brilliant Blue
R-250 in 50% methanol, and destained in 50% methanol, 10% acetic
acid. Protein bands corresponding to the - and
-polypeptide chains of RNR were excised from the gel and used for subsequent proteolytic digestions.
Proteolytic Digestion and Amino Acid Sequence Analysis--
The
two excised gel bands containing the alkylated - and
-polypeptides, respectively, were treated for in-gel digestion to
prepare internal peptides for amino acid sequence analysis. Briefly,
the gel pieces were washed with Tris-HCl/acetonitrile to remove SDS and
the Coomassie dye and to put the gel pieces in the appropriate
digestion environment. After complete drying of the gel pieces, a
solution containing 0.5 µg of Achromobacter lyticus
protease Lys-C (Wako Chemicals GmbH, Neuss, Germany) was allowed to
absorb into the gel pieces. Rehydration with digestion buffer was
continued until the gels were soaked, and incubation was carried out
overnight at 30 °C. After acidifying the incubation mixtures,
generated peptides were extracted from the gels and isolated by
narrow-bore reversed phase liquid chromatography on a µRPC C2/C18 SC
2.1/10 column operated in the SMART System (Pharmacia). A full
description is found elsewhere (31). Of the collected peptides, some
were selected for automated Edman degradation in a Perkin-Elmer-Applied
Biosystems Model 494A sequencer, operated according to the
manufacturer's instructions.
Spectroscopic Methods-- EPR spectra at 9.36 GHz measured at 77 K were recorded on a Bruker ESP 300 spectrometer using a cold finger Dewar flask for liquid nitrogen. Subtractions were performed using the ESP 300 software. Denaturation was done by adjusting the sample to pH 1 by addition of 1 M nitric acid. Buffer from the flow-through of the centricon concentration step prior to the EPR analysis was used as background control for the native sample. For the denatured sample, the same amount of nitric acid as added to the protein sample was added to the background control sample. Background spectra were recorded under conditions identical to those for the native and denatured protein and thereafter subtracted from the total spectrum to give the spectra presented in Fig. 7.
Atomic absorption measurements were made on a Perkin-Elmer Z3030 graphite furnace. Calibrations for each metal were made by the use of several solutions of known metal concentration in the same buffer as used for the sample.Other Methods-- Protein concentration was determined either by the modified Lowry method (32) or the Bradford method (33) using bovine serum albumin as standard. Analytical protein gel electrophoresis was done by the Phast gel system (Pharmacia) in 7.5% or 10-15% denaturing polyacrylamide gels with Coomassie or silver staining.
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RESULTS |
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PCR Isolation of an Internal Fragment of the C. ammoniagenes nrdF Gene-- The deduced amino acid sequences of all known RNR class Ib nrdF genes contain some highly conserved regions that allow the design of NrdF-specific oligonucleotides for PCR amplification. Primers CoryFup and CoryFlow (see "Experimental Procedures") were designed from the R2F conserved regions GYKYQ and NHDFFS, respectively, according to the Corynebacterium codon usage (34) and used for PCR amplification of selected parts of genomic DNA extracted from C. ammoniagenes. A single 297-bp product, which was of the expected size range, was amplified, cloned in pGEM-T plasmid DNA, and sequenced in both directions. The sequence of the amplified and cloned product corresponded to a nrdF gene fragment according to its high homology to the S. typhimurium nrdF gene (60.7% identity at the nucleotide sequence level). The cloned fragment was used as a probe for screening a genomic C. ammoniagenes library.
Cloning of the C. ammoniagenes nrdEF Genes--
Our cloning
strategy assumed that the nrdE and nrdF genes
would be located in close proximity to each other in the C. ammoniagenes genome as in all bacterial nrdEF operons
studied thus far (9, 11, 12, 14-16). The amplified nrdF
fragment was used as a hybridization probe for screening a phage
genomic C. ammoniagenes library enriched for 6-11 kb
fragments (see "Experimental Procedures"). Several positive phage
plaques were purified, and their DNA was extracted and checked by
restriction endonuclease analysis and Southern hybridization and found
to contain the nrdF gene. Several fragments derived from the
endonuclease digestion of these
phage DNA clones were cloned into
pBSK(+) and sequenced from both extremes to localize the
nrdE and nrdF genes. A 10 kb SacI
fragment from one of these positive plaques was assumed to contain both
genes and was subcloned into SacI-digested pBSK(+),
resulting in plasmid pUA728.
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Analysis of the nrdHIEF Gene Sequence-- Five different open reading frames are present in the nucleotide sequence obtained from plasmid pUA728 (Fig. 1). Four of them correspond to the previously reported genes nrdH (228 bp), nrdI (435 bp), nrdE (2 163 bp), and nrdF (990 bp). The fifth putative open reading frame (714 bp), located between nrdE and nrdF, would be transcribed in the opposite direction to the nrd genes. The function of this open reading frame still remains unknown, although comparison with the current data bases shows the highest homologies to several bacterial transcription regulatory proteins of similar size.
The G+C contents of the nrd genes (nrdH, 53.5%; nrdI, 50%; nrdE, 51.5%; and nrdF, 48.5%), as well as their codon usage, are in accordance with those described for genes of corynebacterial origin (34). The putative translational start codon of genes nrdE, nrdF, and nrdI is GTG; that of nrdH is ATG. Putative RBS sequences complementary to the 3' end of the 16S rRNA of B. subtilis (35) are located 14 nucleotides upstream of nrdE (GAAAGG), 13 nucleotides upstream of nrdF (AGCAGGG), 14 nucleotides upstream of nrdH (AAAGG), and 10 nucleotides upstream of nrdI (AAAGGAGG). When we searched for a hypothetical promoter region, we found a putative TATA box (TATAGT) 111 bp upstream of the nrdH gene. Sixteen base pairs upstream of the TATA box, a
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Purification of Active RNR from C. ammoniagenes-- To correlate our genetic results with previously published biochemical observations, we essentially followed the published strategy (18) for cell growth and the first steps of enzyme purification. Cells grown in Mn-deficient medium lost their colony-forming ability after about 10 h of fermentation, but addition of 10 µM MnCl2 at that time fully preserved the viability of the cells. The cells were harvested 1 h after manganese repletion and used as a starting material for purification of enzymatically active RNR.
Purification of the holoenzyme (described in detail under "Experimental Procedures") involved three major steps: precipitation by dialysis of cell-free extract against low salt buffer, chromatography on a weak anion exchanger, and size fractionation by Superdex 200 gel filtration. At this stage, the specific enzyme activity was 6.5 units/mg, and the overall yield was 35% (Table I). Separation of the R1E and R2F components was achieved by fast protein liquid chromatography anionic chromatography (Fig. 4), resulting in preparations of 70 and >90% purity, respectively (Fig. 5). Mixing of the two components resulted in a specific activity of 34 units/mg. In general, the specific activities obtained by us in the different purification steps are approximately an order of magnitude higher than those reported earlier (18) .
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Identification of the Active RNR as a Class Ib Enzyme by Amino Acid
Sequence Analyses--
The enzyme preparation after DEAE-cellulose
chromatography contained several protein bands when analyzed by
SDS-PAGE, but after Superdex 200 chromatography, the two most prominent
bands were of the expected sizes for RNR - and
-polypeptides
(Fig. 5). Material from the 80- and 40-kDa bands was subjected to
partial amino acid sequence analyses using the techniques described
under "Experimental Procedures." N-terminal sequences, as well as
partial internal peptide sequences, were obtained for both subunits
(Table II). The peptides were analyzed by
comparison to the deduced NrdE (deposited in GenBank) and NrdF (Fig. 3)
sequences of C. ammoniagenes and found to match
perfectly in all positions of the internal peptides. The N-terminal
peptides obtained from the blotted
- and
-polypeptide bands were
also in accordance with the gene sequences. The N-terminal sequencing
results indicate that the initiator methionines have been processed
during protein maturation, confirming that both genes, as suggested
from the nucleotide sequence results, start with a GTG initiator codon
that is read as methionine instead of valine.
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Preliminary Characterization of C. ammoniagenes RNR-- The nucleoside triphosphates ATP, dTTP, and dATP were found to be positive allosteric effectors for CDP reduction. At low concentrations of effector, dATP was more effective than ATP (Fig. 6a). Optimal activity with dATP was obtained at nucleotide concentrations as low as 0.02 mM, and no significant inhibition was seen even with 1 mM dATP. When ATP was used, a concentration of at least 0.12 mM was needed for optimal activity (Fig. 6a). This type of allosteric regulation is typical of class Ib enzymes and differs from that of class Ia enzymes (10, 12) .
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The Purified C. ammoniagenes R2F Protein Contains Bound Manganese Ions-- EPR analysis of the active R2F component obtained after the MonoQ purification step showed no signal corresponding to an organic free radical or a metal center (Fig. 7a and data not shown). However, upon denaturation of R2F by nitric acid, a 6-line EPR spectrum typical of Mn2+ in solution (S = 5/2) was observed. This shows that the native R2F protein contained EPR-silent Mn bound to the polypeptide chain. Preliminary atomic absorption spectroscopic analysis of the nitric acid-denatured R2F protein showed that it contained approximately 0.5 mol of manganese ions/mol of R2F polypeptide (Table III). In contrast, the content of iron in the R2F preparation was close to that of the buffer control, and essentially no cobalt was found, confirming that we have purified the previously described Mn-containing RNR of C. ammoniagenes.
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DISCUSSION |
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To date, three different classes of RNR have been described in detail. Suggestions had been put forward as to the existence of a fourth, manganese-dependent class, based on the presence of metal ion and the radical signal in C. ammoniagenes RNR (18, 24). This enzyme was, however, shown to have certain features (e.g. hydroxyurea sensitivity and polypeptide sizes) in common with the well characterized class I RNR of eukaryotes and bacteria (18, 23). Our purpose was to establish whether the manganese-dependent RNR really is a new class that could be fitted into the evolutionary pattern described by the other three classes. We therefore purified the active RNR of C. ammoniagenes to obtain partial amino acid sequence results of its components and to clone the genes for this enzyme. We also wanted to establish whether C. ammoniagenes has the widespread (in bacteria) class Ib RNR.
In this report, we show that the active Mn-containing RNR of C. ammoniagenes is of the class Ib type and that the nrd genomic region contains the same open reading frames as previously seen for the class Ib operon in enterobacteria and L. lactis (11, 12). These are the two genes for R1E and R2F, as well as the gene for a thioredoxin-like protein called NrdH-redoxin and a fourth open reading frame of unknown function called nrdI. The nrdH gene is not present in all nrdEF clusters; it is absent in B. subtilis and in Mycoplasma species (14-16). As in other class Ib systems, we found that the species-specific NrdH-redoxin was the preferred reductant for the C. ammoniagenes RNR. The nrdI gene is present in all known nrdEF loci, and preliminary studies with the S. typhimurium system have shown that the NrdI protein stimulates the NrdEF-dependent CDP reduction in the presence of NrdH-redoxin (37). As shown in Fig. 2, the gene organization of the nrd locus of C. ammoniagenes is homologous to the ones present in enterobacteria, L. lactis, B. subtilis, and Deinococcus radiodurans and to M. tuberculosis (in which the two nrdF genes are less closely linked to the rest of the operon). A different organization is found in Mycoplasma species, in which the nrdF gene is located upstream from the nrdI and nrdE genes.
The deduced NrdEF proteins from C. ammoniagenes are currently most closely related to the R1E and the active R2F protein of M. tuberculosis. Both species belong to the phylogenetic group of Gram-positive eubacteria with a high G+C content. It was recently reported that M. tuberculosis contains a second nrdF gene, which is inactive (48). We have not been able to find a second C. ammoniagenes nrdF gene by PCR amplification or Southern blotting. The identification of the active RNR from C. ammoniagenes as belonging to class Ib helps to replace the initial idea, based on the enterobacterial loci, that nrdEF genes are generally silent. As exemplified in the phylogenetic tree of R2F proteins (Fig. 2), class Ib enzymes are widely spread among eubacteria, and the completely sequenced genomes of B. subtilis, Mycoplasma genitalium, and M. pneumoniae code only for class Ib RNRs (15, 16, 49).
The specific activity of the Mn-containing RNR of C. ammoniagenes obtained by us, even if improved at least an order of magnitude compared with previous studies (18, 23), is only 12 and 18% of the specific activities described for class Ib RNR from S. typhimurium and L. lactis, respectively (10, 12). There are some obvious reasons for the low enzyme activity obtained by us. First, our preliminary studies indicate that inclusion of species-specific NrdH-redoxin will increase the C. ammoniagenes RNR activity at least 2-fold. Second, the substoichiometric amount of metal ion per R2F polypeptide observed after the four-step purification procedure may lead to substoichiometric levels of organic free radical.
Atomic absorption analysis of the isolated C. ammoniagenes R2F protein showed about 0.5 mol/mol Mn/R2F polypeptide chain. Because of the homology with the well known diiron-RNRs, 2 metal ions per R2F was expected. The EPR analysis suggests that the manganese ions may be magnetically coupled, but the substoichiometric amount of metal ion does not allow a definitive conclusion about the structure of the metal center at this point. However, our EPR and atomic absorption analyses clearly confirm earlier published observations (18) that the active C. ammoniagenes RNR contains manganese, and as we show here, in essence, it lacks iron. The strong amino acid sequence homology between active Mn-containing RNR from C. ammoniagenes and class Ib RNRs is thus in many respects remarkable: (a) all previously described class I enzymes are diiron proteins, including the class Ib enzyme from S. typhimurium (10); (b) all iron binding residues in the Fe-RNRs (class Ia and Ib) are conserved in the C. ammoniagenes RNR (Fig. 3); and (c) even though both E. coli class Ia R2 and mouse R2 can bind manganese at their metal centers, Mn substitutions have invariably led to nonactive enzymes (41, 42).
Our results bring a series of new fascinating questions to the field of RNR research, in particular concerning metal specificity and diversity despite high sequence similarities. The metal ion content of the class Ib enzymes has currently only been investigated for the recombinant S. typhimurium (10) and native C. ammoniagenes enzymes. Even though the S. typhimurium R2F has a diiron center, it is not known whether it can also work with manganese. Likewise, it is not yet known whether the C. ammoniagenes enzyme will work with iron. A clear definition of the metal ion dependence of the C. ammoniagenes RNR will have to await the design of an overproducing system. In addition, manganese activation experiments should be performed with other class Ib enzymes. Interestingly, the R2F sequences in the two Mycoplasma species both lack 3 of the metal ligating residues conserved in the rest of the class I enzymes. However, because it is not known which metal ions are present in other class Ib reductases, neither the deduced C. ammoniagenes NrdF amino acid sequence nor the phylogenetic tree can yet be used for predictions about metal ion specificity. Specific three-dimensional features in the vicinity of the metal site may have to be identified to explain a Mn dependence.
Some other enzymatic systems are known to use, alternatively, iron or manganese and have similar or identical metal binding residues (43). In the superoxide dismutase family, the enzyme from Propionibacterium shermanii is functional with either Fe or Mn, i.e. cambialistic, whereas other superoxide dismutases are strictly manganese- or iron-dependent. Comparisons of their three-dimensional structures revealed that the metal ligands are the same in all three types and that differences are localized to the second coordination sphere of the metal center (44). A similar phenomenon seems to occur among extradiol-cleaving catechol dioxygenases. All members of this family are iron enzymes except the 3,4-dihydroxyphenylacetate 2,3-dioxygenase from Arthrobacter globiformis, which contains manganese instead of iron (45). Comparison using the structure of one iron enzyme, sequence alignment, and site-directed mutagenesis of the 3,4-dihydroxyphenylacetate 2,3-dioxygenase suggests that differences can be seen only in the second coordination sphere and that all direct ligands of the two metal ions are the same. These observations suggest a major role for the residues of the second coordination sphere in determining the metal specificity. The hypothesis may also apply to the metal specificity in RNR, because the well known diiron-binding site of E. coli class Ia R2 is intrinsically capable of binding manganese, albeit without activating the protein (41). Perturbations of the second coordination sphere might modify the redox properties of such a Mn center and lead to an active enzyme. One striking difference between prokaryotic class Ia and Ib R2 proteins is the substitution of Gln-43 and Ser-114, which form hydrogen bonds to the iron ligand His-241 in E. coli R2, for hydrophobic counterparts in the class Ib NrdF sequences. However, a preliminary modeled structure of the C. ammoniagenes R2F protein, based on the E. coli R2 structure, highlights only differences between class Ia and class Ib but none that are specific to the C. ammoniagenes RNR and absent from the other NrdF sequences.3
The characterization of the C. ammoniagenes RNR as a class Ib enzyme evokes new, challenging questions. The cloning of the NrdHIEF locus will facilitate future studies on this RNR, whereby new insights in the design and fine-tuning of metal-active sites may be gained.
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ACKNOWLEDGEMENTS |
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We are grateful to Margareta Sahlin for help with the EPR analyses and evaluations and for constructive discussions and to Agneta Slaby for help with purification of E. coli thioredoxin. We thank the Institute for Genomic Research for availability of sequence data prior to publication.
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Note Added in Proof |
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Preliminary experiments indicate that binding of manganese ions to S. typhimurium apo R2F protein results in enzymatically inactive protein (P. Reichard, personal communication) and that cloned and overproduced C. ammoniagenes R2F can bind either manganese or ferrous ions and generate a characteristic tyrosine radical EPR signal.
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FOOTNOTES |
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* This work was supported by grants from the Swedish Cancer Society, the Swedish Research Council for Engineering Sciences and the Swedish National Board for Technical Development (to B.-M. S.); from the Spanish DGICYT (PB94-0687) and the CUR de la Generalitat de Catalunya (GRQ93-2049) (to I. G. and J. B.); and from Stiftelsen Lars Hiertas Minne, Magn. Bergvalls stiftelse, and Jeanssonska stiftelserna (to M. K.).
The nucleotide sequence(s) reported in this paper has been submitted to the GenBankTM/EMBL Data Bank with accession number(s) Y09572.
§ These three authors, listed in alphabetical order, contributed equally to the study.
¶ Supported by the European Molecular Biology Organisation and the Human Frontier Science Project Organisation. Present address: Institut de Biologie Structurale/CEA-CNRS/Université Joseph Fourier, 41 Ave. des Martyrs, F-38027 Grenoble Cedex 1, France.
** Supported by a predoctoral fellowship from Direcci-General d'Universitats de la Generalitat de Catalunya.
Supported by the Swedish Institute and the Stockholm University
Science Faculty program for East European collaborations. Present
address: Dept. of Biochemistry & Biophysics, University of
Pennsylvania, 3700 Hamilton Walk, Philadelphia, PA 19104-6089.The costs of publication of this
article were defrayed in part by the
payment of page charges. The article
must therefore be hereby marked
"advertisement" in
accordance with 18 U.S.C. Section
1734 solely to indicate this fact.
¶¶ To whom correspondence should be addressed. Tel.: 46-8-164150; Fax: 46-8-152350; E-mail: Britt-Marie.Sjoberg{at}molbio.su.se.
1 The abbreviations used are: RNR, ribonucleotide reductase; DTT, dithiothreitol; EPR, electron paramagnetic resonance; PAGE, polyacrylamide gel electrophoresis; PCR, polymerase chain reaction; bp, base pair(s); kb, kilobase pair(s).
2 E. Torrents, unpublished data.
3 J. Nilsson, personal communication.
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