2.1. Bacterial growth

The Escherichia coli strain used in this study was BL21(DE3) F⁻ ompT gal [dcm] [lon] hsdS_B (r_B^–m_B^–; an E. coli B strain) with DE3, a λ prophage carrying the T7 RNA polymerase gene (Studier & Moffat, 1986). The plasmids used were pEnirsp-1 (Kan^R) (Prudêncio et al., 1999) and pTAZU-1 (R. L. Harris, R. R. Eady, S. S. Hasnain and R. G. Sawers, unpublished observations), which is a pT7-7 (Ap^R) derivative (Novagen). Antibiotics were used at a final concentration of 50 µg ml⁻¹.

E. coli strains were grown routinely in Luria Broth (LB) [1% w/v, bactotryptone (Difco), 0.5% w/v yeast extract (Difco), 1% w/v NaCl] at 310 K. Small-scale cultures (up to 10 ml) for testing protein overproduction were grown aerobically in sterile conical flasks filled to approximately 10% of their volume with growth medium. For large-scale isolation of NiR and azurin I, 1 l fermentor cultures were grown in HYE 50 medium [per liter; 3 g KH₂PO₄, 6 g Na₂HPO₄, 0.5 g NaCl, 2 g casein hydrolysate, 10 g (NH₄)₂SO₄, 35 g glycerol, 20 g yeast extract, 0.5 g MgSO₄·7H₂O, 40 mg FeSO₄·2H₂O, 20 mg citric acid, 30 mg CaCl·2H₂O, 8 mg thiamin hydrochloride and 0.5 ml trace-element solution]. Media were also supplemented with CuSO₄ (0.1 mM). Overproduction of NiR was performed at 303 K and achieved by adding 0.25 mM isopropyl-β-D-thiogalactopyranoside (IPTG). Cells were harvested approximately 4 h after induction had been initiated. For overproduction of azurin I the fermentor was run at 310 K and with a constant stirring speed of 300 r.p.m. until the cultures had attained an OD_600nm of 10 when the stirring speed was increased to 1000 r.p.m. The pH of the cultures was maintained at 7.1. Induction of high-level protein production was initiated when the cultures had reached a turbidity (OD_600nm) of 25, through the addition of 0.5 mM IPTG. The temperature of the culture was reduced to 301.5 K. The cells were cultured for a further 3 h (final OD_600nm of 40) prior to harvesting by centrifugation. Generally, 40–50 g wet weight of cells were derived from each fermentation. Antibiotics were purchased from Sigma and stock solutions were prepared in water and filter-sterilized through sterile 0.2 µm syringe filters (Sartorius). Cells were used immediately for the isolation of recombinant protein or were stored frozen at 193 K until required.

2.2. Protein purification

Native NiR and native azurin I were purified from A. xylosoxidans as described previously (Abraham et al., 1993; Dodd et al., 1995). Recombinant NiR was purified from the periplasmic fraction of E. coli as described (Prudêncio et al., 1999) and recombinant azurin I was purified from the crude extract of recombinant E. coli cells using a single carboxy­methyl cellulose step in a similar procedure to that described for NiR. Briefly, after cell disruption by French press (16000 p.s.i.) and centrifugation, the crude extract was passed over a DEAE cellulose column equilibrated with 100 mM tris-HCl pH 7.4 buffer. Under these conditions azurin I did not bind to the column and the flow-through was collected and precipitated with solid ammonium sulfate, which was added to a final saturation of 75%. After collection of the ammonium sulfate precipitate by centrifugation, the material was resuspended in 50 ml of water and dialyzed for 48 h against water. After clarification of the dialysate by centrifugation, the suspension was loaded onto a CM cellulose column (10 cm × 5 cm) that had been equilibrated with 500 mM MES [2-(N-morpholino)ethanesulfonic acid], pH 6.0, followed by washing with two column volumes of water. The overproduced azurin I has a pronounced absorbance band at 620 nm, which is characteristic of oxidized type-1 Cu sites. Recombinant azurin I bound as a tight blue band to the top of the column. After washing the column extensively with water, azurin was eluted with 200 mM tris-Cl pH 8 containing 200 mM NaCl. The pure azurin I preparation was then dialyzed against 50 mM MES buffer, pH 6. Generally, approximately 0.5 mg of pure NiR and 2 mg of pure azurin I were obtained per g wet weight of cell paste.

2.3. Metal determination

The copper and zinc content of samples of NiR and azurin I were measured on wet-ashed samples (Abraham et al., 1993), using inductively coupled plasma emission spectroscopy by Southern Analytical (Sussex, UK).

2.4. Spectroscopic methods

Electron paramagnetic resonance (EPR) data were collected using a Bruker ER ER200 D-SRC spectrometer fitted with an ER042 MRH microwave bridge with an ER033C field frequency lock and an Oxford Instruments Ite⁵⁰³ temperature controller. EPR spectra were simulated using the program WINEPR (SimFonia, Bruker). Spin quantizations were made according to the method of Åasa & Vänngård (1975), by comparing the area of the experimental curve under non-saturating conditions to that obtained, under the same conditions, for a sample of Cu(II)-EDTA.

2.5. Other methods

Molecular weight determinations were undertaken using matrix-assisted laser desorption/ionization time-of-flight (MALDI-ToF) mass spectrometry and by quadrupole/time-of-flight (Q-ToF) mass spectrometry.

MALDI-ToF mass spectrometry was performed using a Reflex III MALDI-ToF mass spectrometer (Bruker UK, Coventry, UK). A 10 mg ml⁻¹ solution of 3,5-dimethoxy-4-hydroxycinnamic acid (Fluka, Dorset, UK) in acetone was prepared. This was mixed with the protein sample and spotted directly onto a stainless steel target plate. Mass spectra were acquired in positive-ion reflection mode. Accurate calibration was achieved with reference to the singly and doubly charged molecular ions of horse heart myoglobin (Sigma), spotted adjacent to the sample.

Q-ToF mass spectrometry was performed in the following way: protein was diluted in 50/50 water/acetonitrile + 0.1% formic acid to a concentration of 5 pmol µl⁻¹, loaded into coated borosilicate glass capillaries (Micromass, Manchester, UK) and sprayed into the nano-electrospray ion-source of a Q-ToF 2 mass spectrometer (Micromass, Manchester, UK) in positive-ion mode. Charge-states from the resulting spectra were deconvoluted using the MaxEnt algorithm (Micromass, Manchester, UK) to enable determination of exact molecular weights.

Polyacrylamide gel electrophoresis (PAGE) in the presence of sodium dodecyl sulfate (SDS-PAGE) was used routinely to check the purity of protein samples throughout the purification. SDS-PAGE was performed according to Laemmli (1970). Typically, 12.5% (w/v) or 15% (w/v) acrylamide gels were run. For whole cell extracts, OD_600nm was measured and a volume of 1.2/OD_600nm ml of cell suspension was centrifuged and the cell pellet was resuspended in 80 µl of SDS sample buffer.

3.1. Heterologous synthesis of NiR in E. coli

The nirA gene could be overexpressed in exponentially growing E. coli BL21(DE3) cells containing vector pEnirsp-1 by inducing the T7 RNA polymerase-directed transcription of this gene with IPTG. Overproduction of NiR was optimized on a small scale (5–10 ml cultures) with regard to growth temperature, IPTG concentration and duration of induction. Growth of the cultures at 303 K and inducing enzyme production by adding 0.25 mM IPTG when the cells had attained an optical density of ∼0.4–0.5, as determined by measuring the absorbance at 600 nm, were found to be optimal conditions (Prudêncio et al., 1999; and data not shown). The extent of cell growth subsequent to induction is also an important parameter and this was assayed in a 1 l batch-fed fermentor. Cells were grown at 303 K and induction with 0.25 mM IPTG was carried out when the OD_600nm was 0.5. Samples were then collected at 30 min intervals for up to 5 h and the production of NiR was analysed by SDS-PAGE (Fig. 1a). The overproduced protein is present in two different forms, which correspond to an unprocessed form of the protein, of higher apparent molecular mass (∼43 kDa), and a mature form of the protein, of lower apparent molecular mass (∼35 kDa). Overproduction of NiR worked well for a number of conditions analysed. However, incubating the cultures at 303 K for 3–4 h subsequent to induction yielded the highest ratio of mature:unprocessed forms of the protein, together with the highest levels of soluble mature enzyme (Fig. 1a).

Figure 1 Analysis of recombinant NiR. (a) SDS-PAGE containing 12.5% (w/v) acrylamide of whole cell extracts of BL21(DE3) containing pEnirsp1 grown at 303 K in a 1 l fermenter. Induction at OD600nm ≃ 0.5: lane S, molecular mass markers; lane 1, negative control, BL21(DE3); lane 2, sample taken immediately after addition of 0.25 mM IPTG; lanes 3 to 12, samples taken at 30 min intervals after induction. (b) EPR spectra of recombinant NiR in 20 mM MES buffer, pH 6.0. Spectrum 1. As-purified protein (T2D form) at 9.4 mg ml−1 (255 µM monomer). Spectrum 2. Protein incubated with 1 mM CuSO4 after purification (partially reconstituted form) at 6.1 mg ml−1 (165 µM monomer). Spectrum 3. Protein purified after incubation of the periplasmic fraction with CuSO4 (fully reconstituted form) at 4.8 mg ml−1 (135 µM monomer). The spectra were recorded at 60 K at a microwave frequency of 9.312 GHz and normalized for ease of comparison. The type-1 and type-2 features are indicated.

Purification of the mature NiR polypeptide was from the periplasmic fraction of E. coli (Prudêncio et al., 1999). The N-terminal amino acid sequence of the mature polypeptide was determined to be Q-D-A-D-K-L, which is in perfect agreement with that predicted for the mature NiR protein lacking the signal sequence and is identical to that determined for native NiR isolated from A. xylosoxidans (Vandenberghe et al., 1998). Taken together, these data provide clear evidence that the native NiR signal peptide is recognized and efficiently and specifically cleaved by the E. coli export apparatus.

Recombinant NiR purified from various growths of E. coli cells was characterized in terms of its catalytic, spectroscopic and biochemical properties. These were compared with those of the wild-type NiR (wt-NiR) from A. xylosoxidans and the two proteins were shown to be indistinguishable with regard to the parameters studied (see Prudêncio et al., 1999, 2001).

The final confirmation that the recombinant NiR protein is indeed indistinguishable from the native enzyme isolated from A. xylosoxidans was confirmed by the determination of the X-ray crystal structures of both enzymes (Ellis et al., 2001, 2003).

3.2. Correlation between Cu content and activity of NiR

Purified concentrated recombinant NiR is dark blue in colour. The colour is due to absorbance maxima at 595 nm and 470 nm and is an indication of the occupancy of the type-1 Cu centre (Abraham et al., 1993). Measurement of the ratio of the absorbance at 280 nm compared with that at 595 nm gives a good indication of the type-1 centre occupancy. Type-1 centres fully loaded with Cu have an absorbance ratio of between 12 and 16. Higher ratios indicate incomplete occupancy. NiR that was purified without treatment has a ratio of ∼20. The EPR spectrum of this protein shows the typical features of type-1 Cu and a complete absence of a type-2 Cu EPR signal (Fig. 1b). Metal analysis indicated that this protein contains ∼2.1 Cu atoms per trimer and the specific activity of this enzyme measured with the MV/dithionite assay (Abraham et al., 1993) is only 11 units per mg of protein (Table 1), where one unit is defined as 1 µmol of nitrite reduced per minute. This shows that this form of the enzyme is deficient in the type-2 Cu centre (T2D) and also does not have a full type-1 Cu complement.

Upon incubation of the purified protein with 1 mM CuSO₄, type-2 Cu EPR features appear in the spectrum of NiR (Fig. 1b, trace 2). The intensity of these features is lower than that of the type-1 signal, the ratio Abs_280nm/Abs_595nm is reduced to ∼16 and the Cu content is increased to ∼3.8 Cu atoms per trimer, based on metal analysis (Table 1). This indicates that the type-2 Cu sites in the protein have been only partially reconstituted, whilst there is a full complement of type-1 Cu. Again, this result is consistent with the approximate fourfold increase in activity observed for this form of the enzyme.

It is possible to isolate recombinant NiR that has a full complement of type-1 and type-2 Cu after incubation of the periplasmic fraction with 1 mM CuSO₄ (Fig. 1b, trace 3). The Abs_280nm/Abs_595nm ratio of this enzyme was ∼13 and the protein was shown to have ∼6.3 Cu atoms per trimer and a maximal activity of 168 per mg of protein (Table 1). The correlation between the presence of type-2 Cu centres and the activity of NiR is consistent with the notion that these centres are the sites of catalysis (Libby & Averill, 1992; Howes et al., 1994; Abraham et al., 1997; Suzuki et al., 1997; Dodd et al., 1998; Farver et al., 1998).

Owing to its location at the subunit boundary, it is likely that the type-2 Cu is readily removed from the enzyme during purification. The results above suggest that the incorporation of Cu into the type-2 centres of NiR in vivo is facilitated by the activity of a periplasmic enzyme. The fact that when the purified enzyme is incubated with CuSO₄ only partial reconstitution of the type-2 Cu sites occurs is in accord with previous observations that suggested the presence of a metal chaperone in A. xylosoxidans, involved in the insertion of type-2 Cu into NiR (R. Eady, unpublished data). The fact that activation of the enzyme is more effective on a concentrated periplasmic protein extract than on a diluted periplasmic fraction is in accord with the presence of such an activity in the periplasm of E. coli cells and suggests that, in vivo, recombinant NiR is fully loaded with Cu. The role of metal chaperones in the assembly of the CuZn superoxide dismutases is well documented (Lamb et al., 2001; Bartnikas & Gitlin, 2003).

3.3. Isolation of recombinant azurin I with a fully occupied type-1 Cu centre

The cloning and characterization of the gene encoding azurin I will be described elsewhere (R. L. Harris, R. R. Eady, S. S. Hasnain and R. G. Sawers, unpublished observations). For overexpression purposes the azu-1 gene was cloned into the expression vector pT7-7 to create plasmid pTAZU-1, which is under the control of the phage T7 ϕ10 promoter. Optimization of azurin I overproduction was achieved on a small scale in the same manner as for NiR. Induction was achieved by adding 0.5 mM IPTG, with growth of the culture at 303 K.

Although azurin I could be shown to be exported to the periplasm of E. coli BL21, when the protein was purified from the periplasmic fraction it was colourless and contained no type-1 Cu (data not shown). However, when the enzyme was purified from the crude cell extract (Fig. 2) the protein was a deep blue colour and had an absorption maximum at 620 nm, characteristic of type-1 cupredoxin (Abraham et al., 1997). The A_280nm:A_620nm ratio was 2.6, which was a value indistinguishable from that of the native protein (Dodd et al., 1995). The N-terminal sequence of recombinant azurin I was determined to be AEXSVD. If the residue X is assumed to be due to oxidation of a cysteinyl residue, the sequence matches exactly the first six amino acids of native azurin I (Inoue et al., 1994; Dodd et al., 1995).

Figure 2 Purification profile of azurin I. SDS-PAGE (15% w/v polyacrylamide) analysis of various stages of protein purification is shown. Lane S, molecular mass standards; lane 1, whole cell lysate (50 µg protein); lane 2, crude cell extract (50 µg protein); lane 3, pool of DEAE flow-through (50 µg protein); lane 4, purified azurin I after CM-cellulose chromatography (5 µg protein).

3.4. Mass spectrometry of recombinant and native azurin I

MALDI-ToF and Q-Tof mass spectrometry are powerful techniques that allow the determination of the precise masses of proteins. Aliquots (50 pmol) of recombinant and native azurin I were analysed initially by MALDI-ToF, which revealed the presence of several different species (Fig. 3a). These species had a mass difference of either 38 or 22 Da. It is likely that the 38 Da species is due to bound potassium and that the 22 Da species is due to sodium binding. It is clear from the profiles, however, that azurin I isolated from E. coli and azurin I isolated from A. xylosoxidans are indistinguishable. The predicted mass of both azurins as determined by MALDI-ToF was 13960 Da. This is in accord with the monomeric nature of these electron transfer proteins.

Figure 3 Analysis of recombinant azurin I. (a) The MALDI-ToF profiles of recombinant azurin (full line) and native azurin I (dotted line) are shown (see Experimental for details). The three most prominent peaks are highlighted. (b) Q-ToF of RecAz showing the four sets of doublets. The doublets are the Cu-containing and apo-forms of the protein. The four sets are consistent with up to three MES molecules binding to the protein.

Q-ToF analysis of recombinant azurin I showed additional features not identified by the MALDI-ToF analysis. Four pairs of repeating peaks were identified (Fig. 3b). The mass difference between the two peaks within each doublet was 63 Da, consistent with the loss or retention of copper. Each set of doublets was separated by a mass of 194–196 Da. MES buffer has a MW of 195.03, and these patterns suggest that up to three MES molecules were bound to the protein. Q-ToF calculated the mass of RecAz to be 14015 Da.

For comparison, the mass of azurin was computationally determined using ExPASy's ProtParam tool (https://ca.expasy.org/cgi-bin/protparam ). The program calculated the mass of the protein based on the amino acid sequence to be 13840 Da. This program did not take into account any cofactors, therefore Cu (63 Da) had to be added to give a final mass of 13903 Da. This is significantly different to the MALDI-ToF (13960) and the Q-ToF (14015) results. The reason for the differences between the deduced molecular mass and that derived from MALDI-ToF might result from the minimal ionic species in the MALDI-ToF experiment having one bound potassium plus one bound sodium ion. The discrepancy in size between the MALDI-ToF and Q-ToF data could signify some post-translational modification or tight binding of a non-specific unidentified species.