The ability of the expressed laccase to polymerize β-naphthol (1) (ADWIC, Abu Zaabal, Egypt) was tested by incubating 440 nM of enzyme with 250 mg L⁻¹ β-naphthol (1) in 50 mM potassium phosphate buffer at pH 8. The reaction was incubated for 15 min at 60°C after which the reaction was stopped by heating the solution to 100°C for 5 min to deactivate the enzyme. The resulting precipitate was removed by centrifugation at 13,000 rpm for 10 min.

A one-gram scale conversion of β-naphthol (1) was carried out in a final volume of 500 mL in a screw-cap bottle following previously run procedure with some modifications (Habib et al., 2017). The reaction mixture contained 1 g β-naphthol (1) and 1 μM Bli-Lacc in 50 mM potassium phosphate buffer adjusted to a final pH of 10. The reaction was incubated at 37°C for 14 days (static state). The reaction mixture was then centrifuged, the supernatant decanted and the precipitate dried in the oven until constant weight to determine the yield.

Crystallization trials were performed using previously published results on other laccases (Brissos et al., 2022). The sitting-drop method was used with 2 M ammonium sulfate (Sigma Aldrich) as the reservoir and the drop was composed of a 3:1 ratio of protein (5 mg mL⁻¹): reservoir solution. All crystallization conditions were conducted at 20°C. Crystals started to appear within a few days and were stable for months in the sitting drop.

The crystals were soaked for ~1 h in a cryoprotectant solution containing 3 M ammonium sulfate and 20% glycerol (v/v). The crystals were directly frozen in the 100°K nitrogen stream. Data was collected using a Bruker D8 VENTURE diffractometer (Billerica, MA, USA) attached to a PHOTON 100 detector. Because of the long unit cell, oscillation images were collected using 0.1° steps, with 6 min exposures, and at a crystal to film distance of 100 mm. The diffraction intensities were integrated and scaled using the associated Bruker software. The crystals had a space group of P6(5) with cell dimensions of a = b = 94.8 Å, c = 271.7 Å, α = β = 90°, γ = 120°.

Using the Basic Local Alignment Search Tool (BLAST) on the NCBI online database, the laccase with the highest sequence similarity to the Bli-Lacc was the CotA laccase from Bacillus subtilis (PDB: 2X87; Bento et al., 2010). From Matthews probability calculations (Matthews, 1968), it was most likely that there were two copies of the protein in the crystallographic asymmetric unit. Assuming a dimer, two copies of CotA laccase was used for molecular replacement with the PHASER routine (McCoy et al., 2007) within the PHENIX software package (Afonine et al., 2005). This molecular replacement solution was then used as a starting model for refinement. Six amino acid sequences of copper-containing oxidases/laccases were aligned against the Bli-Lacc sequence using Clustal Omega (https://www.ebi.ac.uk/jdispatcher/msa/clustalo) and the alignment visualized using Jalview software Version 2.11.4.0 (Waterhouse et al., 2009).

β-naphthol (1) structure was characterized using ¹H and ¹³C 1D NMR spectroscopy to assign all the chemical shifts. In Figure 1A, H11 does not appear in the β-naphthol (1) sample due to its rapid exchange with the water molecules, while it appears in the β-naphthol precipitate in Figure 1B as the sample was dissolved in DMSO-d₆ (aprotic solvent). Carbons C1, C2, and C9 are quaternary carbons so they possess no protons. Protons H3 (7.43 ppm, d, 12 Hz, 1), H4 (7.19 ppm, t, 6 Hz, 1), H5 (7.09 ppm, t, 6 Hz, 1), H6 (7.51 ppm, d, 12 Hz, 1), H7 (7.53 ppm, d, 12 Hz, 1), H8 (6.86 ppm, d, 12 Hz, 1), and H10 (6.9 ppm, s, 1) are assigned according to the literature (Premachandran et al., 1996). In Figure 2A, the ¹³C peak assignment according to the literature is as the following; C1 129.3 ppm, C2 135 ppm, C3 126.7 ppm, C4 126.9 ppm, C5 124 ppm, C6 128 ppm, C7 130.3 ppm, C8 118 ppm, C9 153.6 ppm, and C10 109.9 ppm (Premachandran et al., 1996).

¹H spectrum (Figure 1B) for poly-β-naphthol (3,4) precipitate dissolved in DMSO-d₆ showed a broad peak in the aromatic region between 6.5 and 8.5 ppm indicating the presence of a polymeric compound formed from β-naphthol (1). A sharp and high intensity peak at 8.29 ppm was assigned to the proton in the hydroxylic functional group (H11). This peak appeared in the aprotic solvent, DMSO-d₆, as it was not exchanging with the solvent surrounding it. In Figure 2B, the ¹³C spectrum showed no peaks in the aromatic region between 120 and 150 ppm. This could indicate the high molecular weight for the formed polymeric material.

As depicted in Figure 3, the presence of a prominent OH stretching region in the polymer signifies its notable naphthol character (Premachandran et al., 1996). Furthermore, the OH stretching region exhibited a shift to higher frequencies in comparison to the monomer, likely due to weakened hydrogen bonding interactions among the hydroxyl groups within the polymer, as opposed to the self-associations present in the monomer. A notable observation pertains to the bands within the 900–650 cm⁻¹ range, attributed to CH out-of-plane bending frequencies. These bands are distinct indicators of substitution patterns in an aromatic ring. The disappearance of the 844 cm⁻¹ band, corresponding to the CH out-of-plane bending of a lone hydrogen upon polymerization, suggests the involvement of the 1 position in the polymerization process. The bands at 814 and 748 cm⁻¹, however, remain intact. Notably, there is a discernible peak with very low intensity between 1,270 and 1,280 cm⁻¹, signifying the presence of low content of aromatic ether linkages (Ar-O-Ar). The polymer still retains vibrational bands indicative of unbound naphthol hydroxyl groups, including the phenolic CO stretch at ~1,210 cm⁻¹ and the OH stretch spanning from 3,100 to 3,500 cm⁻¹, thus confirming its fundamental naphthol nature. After careful analysis, the peak at around 1,050 cm⁻¹ is attributed to C-O stretching in alcohols and was due to ethanol traces from the reaction mixture. Furthermore, the peak at ~ 1,060 cm⁻¹ is attributed to the C=C stretching in aromatic compounds. Based on NMR and FTIR results, we depicted a hypothetical structure for our generated poly-β-naphthol (3,4) (Scheme 1).

To maximize yield and attain the highest degree of polymerization of β-naphthol (1), optimization experiments using various parameters must be conducted. To do this, three levels of each parameter were selected covering high, middle and low ends. The variables chosen were temperature, pH and enzyme concentration. Polymer yield was determined based on the OD_600nm readings after 4 and 9 days. Out of the different variables tested, the optimal conditions for polymerization of β-naphthol (1) were found to be a temperature of 37°C, a working pH of 10, and an enzyme concentration of 440 nM over a period of 9 days (see Supplementary Table 1). Different colors of residue formed after drying from the different reaction conditions were recorded (Supplementary Figure 4). Further future analysis of these residues by NMR could reveal different sized polymers.

One-gram conversions are used to determine if a reaction could be extrapolated to a pilot scale for industrial applications. To apply this hypothesis, a one-gram scale conversion of the β-naphthol (1) polymerization was conducted. It was found that one gram of β-naphthol (1) produced 216 mg poly-β-naphthol (3,4) (≈ 21.6% conversion yield) as dry weight.

To be able to study and elucidate important characteristics/features of the Bli-Lacc enzyme, a crystal structure needs to be solved. To achieve this, the purity level of the expressed enzyme needs to be enhanced. This is achieved using IMAC followed by ion-exchange chromatography to remove any non-specifically bound proteins from the column. The purified enzyme is then crystallized followed by X-ray diffraction. Analysis of the structure using computational tools can then identify molecular details important for determining function, binding and other parameters necessary for laccase activity.

The expressed enzyme was pure after running through the monoQ anion exchange column, evident through crystal formation within 2–3 days using the sitting drop technique. Purity of the protein fractions eluted from the monoQ purification was assessed upon measuring activity using syringaldazine (SGZ) (5) as a substrate. SGZ (5) is known for its ability to detect laccase and peroxidase activities (Harkin et al., 1974; Leonowicz and Grzywnowicz, 1981). Laccase oxidation of SGZ (5) is detected by the formation of a violet color. This violet color corresponds to the formation of tetramethoxy azobismethylene quinone (TMAMQ) (6) (Scheme 2) a compound known for its ability to measure antioxidant activity in various foods (Nugroho Prasetyo et al., 2010). Using SGZ (5) as an indicator for presence of laccase activity, each of the fractions that were run on the protein gel were assessed for their ability to convert SGZ (5) to TMAMQ (6) based on violet color formation/intensity. All fractions collected before fraction 32 showed no laccase activity but starting from fraction 34 onwards, all fractions showed positive activity (Supplementary Figure 5). However, based on the protein gel, we decided to pool only fractions 40–42 having the highest and purest yield of intact laccase. The pooled fractions 40–42 were dialyzed against Tris (20 mM) pH 7.5, NaCl (200 mM) buffer. The protein was concentrated using centricon filter tubes to a final concentration of 5 mg mL⁻¹ (OD 1). The blue color of the protein was evident in this step indicating the successful binding of the copper to the protein.

Using the structure of CotA laccase from B. subtilis (PDB ID: 2X87; Bento et al., 2010), the PHASER routine within PHENIX found the predicted dimer in the P6(5) asymmetric unit. The data and refinement statistics are summarized in Supplementary Table 2. The current model at 2.7 Å resolution has an Rmodel of ~17% and an Rfree of ~23%. The model consisted of residues 2–509 and therefore the residues beyond 513 that were added during cloning were not visible in the density. As found in several other laccase structures, two loops were disordered hence not interpreted with an atomic model: residues 90–96 and 359–361. Not unexpectedly, the structure of Bli-Lacc was highly similar in sequence to other laccase structures. Shown in Figure 4A is a structure alignment of Bli-Lacc with CotA laccase from B. subtilis (PDB ID: 3ZDW) that was complexed with 2,2′-azinobis-(3-ethylbenzothiazoline-6-sulfonate; ABTS; Enguita et al., 2003). The root mean square deviation (RMSD) between the two structures was 0.5 Å sharing 66% sequence identity and 78% similarity. While the structures of Bli-Lacc complexed with other substrates was also attempted, the substrates were insoluble in the high concentration of ammonium sulfate used for crystallization. Noted in this figure are the locations of the mononuclear (MNC) and trinuclear (TNC) redox centers. Also noted are the areas with the largest divergence between the two structures. Notably, two loops, 213–219 and 319–327, are immediately adjacent to the substrate binding site. These are unlikely due to substrate binding since those loops in B. subtilis are the same in the presence and absence of substrate. This suggests possible differences in substrate specificity and/or affinity.

With this sequence variability and structural differences in the substrate binding pocket compared to B. subtilis CotA, the apparent structural flexibility was examined. Shown in Figure 4B, is a representation of conformational flexibility as per the refined B factors in the structure. Here the most flexible (i.e., highest B values) regions are colored red and represented by “swollen” tubes. Aside from the disordered region at 356–362, the most flexible is the 213–218 loop adjacent to the substrate binding pocket. Therefore, the most divergent and conformationally flexible regions appear to be involved with substrate selectivity and affinity.

To further examine the overall sequence similarity amongst the various sources of laccase, the structure was input into the CONSURF Server (https://consurf.tau.ac.il/consurf_index.php; Landau et al., 2005; Ashkenazy et al., 2010, 2016; Celniker et al., 2013; Yariv et al., 2023). For comparison, 150 sequences were aligned to Bli-Lacc (Supplementary Figure 6A) and the similarity between the sequences projected onto a ribbon diagram (Supplementary Figure 6B). For each residue in Bli-Lacc, the highest percent of a particular amino acid was calculated. The most highly conserved residues are in red, and the least are in cyan. As expected, the most highly conserved residues are those in the vicinity of the bound metals and/or those in the core of the protein. To further validate and confirm the resemblance of the Bli-Lacc against other laccases with solved crystal structures, a multiple sequence alignment using the amino acid sequences was executed and motifs characteristic of laccases were found conserved—HXHG, HXH, HXXHXH, and HCHXXXHXXXXM/L/F as can be seen in Figure 5 (Sharma et al., 2007).