Abstract
In this study, the extracts of lignocellulosic materials such as sawdust, hay, and rapeseed press cake were used as medium for the production of laccase of the non-ligninolytic fungus Myrothecium roridum. Media prepared from hay extract and rapeseed press cake extract contributed to the highest quantity of the enzyme produced (ranging from 465 to 728 U/L after 24 h of cultivation). It could have resulted from the high content of reducing sugars and phenolic compounds such as gallic or ferulic acid identified in media by liquid chromatography coupled with tandem mass spectrometry. The enzyme was found to be stable in the pH ranging from 2 to 8 and decolorized up to 90% of Amaranth (400 mg/L) after 24-h incubation in the presence of a selected redox mediator. After 24 h of incubation, laccase almost completely (97%) decolorized the simulated dye effluent containing several dyes, metal ions, reducing agents, and detergents. An environment-friendly approach for dyes removal by laccase immobilized together with rapeseed press cake was proposed. After 24-h incubation of a dye (acid orange 7, trypan blue, and Amaranth) with laccase–rapeseed press cake alginate beads, more than 70% decolorization was obtained. The rate of Amaranth removal was found to be about 50% after five successive batches. Low-cost production and high decolorization efficiency in the presence of additional compounds make M. roridum laccase and its newly developed immobilization technique a promising option as a green catalyst for azo dyes containing wastewater treatment.
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Introduction
Textile and dyeing industries play a major role in the economy of many countries, but have also become one of the serious causes of water pollution. They releases large amounts of wastewaters containing hazardous chemicals such as dyes, surfactants, suspended solids, and organic matter, which cause aesthetically unacceptable coloring of water bodies and block the passage of light to the lower depths of aquatic systems, resulting in the inhibition of photosynthesis. It has an adverse effect on organisms at all levels of the trophic chain (Balarak et al. 2015). Based on their chemical structure, textile dyes have been classified into azo dyes, nitro dyes, indigo dyes, anthraquinone dyes, phthalein dyes, triphenyl dyes, nitrated dyes, etc. Azo dyes comprise about 60–70% of all synthetic colorants used worldwide (Sen et al. 2016). They find application as colorants of synthetic and natural textile fibers, plastic, leather, food, hair dyes, waxes, pharmaceuticals, inks, and paints. Their popularity and usefulness result from their stability to oxygen, light, washing, and heating processes (Jasińska et al. 2016). Nevertheless, some azo dyes have been banned for use due to toxic side effects. Although they are not always toxic by themselves, their degradation products are (e.g., aromatic amines (AA)). AA are formed as a result of chemical reduction, which causes cleavage of the N=N bond and the production of the corresponding amines (Chung 2016). This process can occur in textiles, cosmetics, or foods that are colored with azo dyes when the object is exposed to sweat, saliva, or symbiotic bacteria that inhabit the human skin or the gastrointestinal tract. Azo intermediates especially containing benzidine have been linked to genotoxicity, mutagenicity, and carcinogenicity in humans as well as in animals (Nguyen and Saleh 2016). According to the European Commission Regulation (Annex XVII of the REACH regulation; No. 1907/2006) (EC 2009), azo dyes that release one of the 22 aromatic amines (e.g., benzidine, 4-chloroaniline, 2-naphthylamine, and 4,4′-oxydianiline) are prohibited in all EU Member States. However, in some countries, these dyes are still being used in industries and can be illegally exported, thus endangering human life and health.
A wide range of methods have been developed for the removal of dyes from wastewaters and decrease their impact on the environment. The main mechanisms involved in these technologies are physical dye separation, breakdown of the dyes by photocatalysis, and/or by oxidation processes or decolorization by biosorption/biodegradation (dos Santos et al. 2007; Brillas and Martínez-Huitle 2015). Application of microorganisms and their enzymes in the removal of toxic dyes from environment has gained popularity due to its safety, efficiency, and ability to transform hazardous chemicals into less toxic compounds (Jasińska et al. 2016). In particular, fungal ligninolytic enzymes such as laccase, manganese peroxidase, and lignin peroxidase, which are extracellular in nature and have relatively high stability, can be easily isolated and applied in the process of biodegradation. Laccases with low substrate specificity can catalyze the oxidation of different phenolic and non-phenolic compounds; therefore, they have found application in many industrial and environmental processes (Singh et al. 2015). They require only air as the co-substrate and release water as the by-product; therefore, they can be classified as green catalysts (Mate and Alcalde 2017). Laccases from Bacillus subtilis, B. licheniformis, Trametes trogii, Pleurotus ostreatus, Pycnoporus sangineus, Ganoderma lucidum, Cerrena unicolor have been suggested for the effective dye degradation (Kuhar et al. 2015; Campos et al. 2016; Jaszek et al. 2016; Zimbardi et al. 2016; Qiao et al. 2017; Wang et al. 2017; Bhavsar et al. 2018; Zhuo et al. 2018). However, enzymatic biodegradation has to meet several criteria in order for it to be profitable, effective, and environment-friendly. First of all, biosynthesis, isolation, and preparation of the enzyme should be fast and cheap (Osma et al. 2011). To achieve this, recently, some researchers have tested lignocellulosic wastes and by-products, such as fruits peel, cereal bran and straw, and sawdust and oilcakes as growth media for the biotechnological production of laccases, which has been found to be quite promising (Songulashvili et al. 2015; Daâssi et al. 2016; Schalchli et al. 2017). According to JRC Science for Policy Report, Bioeconomy Report 2016 (Ronzon et al. 2017), the use of lignocellulosic materials for the biosynthesis of enzymes seems to be economically justified and is in line with the concept of sustainable development goals. The use of waste products for the production of enzymes allows to manage wastes generated by various industries and significantly reduces the costs of obtaining the enzyme. Lignocellulosic materials, primarily composed of polysaccharides (cellulose and hemicellulose) and lignin, have been demonstrated to stimulate fungal growth and the production of laccase (Cavka and Jönsson 2014). They can also be utilized as adsorbents of pollutants. For example, canola residues, rice husks, rapeseed press cake (RPC), brewery grains, or plant leaves showed an excellent capability to remove contaminants, such as organic pollutants and heavy metals from aqueous solutions (Silva et al. 2004; Jasińska et al. 2013; Ashrafi et al. 2015; Balarak et al. 2015; Guerrero-Coronilla et al. 2015).
Immobilization of enzymes on lignocellulosic wastes seems to be a promising alternative for conventional supports. The use of alternative matrices could help to reduce the cost of the enzyme immobilization process and allows application on an industrial scale. Lignocellulosic materials were successfully applied for lipases, invertases, amylases and laccases immobilization (de Souza Bezerra et al. 2015). However, there are no reports showing the immobilization of laccase with the use of waste materials after the production of this enzyme. Therefore, the aim of the study was to produce the laccase of the non-ligninolytic fungus Myrothecium roridum in the eco-friendly and cost-effective approach and use it in the degradation of azo dyes. We used the extracts of a sawdust (SE), hay (HE), and rapeseed press cake extract(s) (RPCE) as the media. The media were preliminarily characterized for total proteins, phenols, and reducing sugars estimation, followed by liquid chromatography coupled with tandem mass spectrometry (LC–MS/MS)-based measurement of selected phenolic compounds. The enzyme was tested on decolorization of the azo dye Amaranth in a wide range of pH. Redox mediators’ influence on the elimination of dye was also tested. According to the assumption of zero-waste bioprocessing, RPC that remained after the preparation of the medium was successfully used for the novel cost-effective immobilization of the enzyme and removal of the dyes. The entire work was carried out in the Department of Industrial Microbiology and Biotechnology, University of Lodz, Poland, from April 2017 to March 2018.
Materials and methods
Chemicals
All chemicals used in this study were of certified reagent analytical grade. The following azo dyes were used: Amaranth, acid orange 7 (AO7), Acid blue 113 (AB113), trypan blue (TB), and Sunset Yellow FCF (SY FCF). Dyes were purchased from Sigma-Aldrich (USA). Stock dye solutions (50 mg/mL in water) were sterilized and stored in the dark at 4 °C. In addition, 2,2-azinobis-3-ethylbenzothiazoline-6-sulfonic acid (ABTS); 2,6-dimethoxyphenol (DMP); 2,2,6,6-tetramethylpiperidine 1-oxyl (TEMPO); gallic acid (GA); caffeic acid (CA); vanillin (V); p-hydroxybenzoic acid (HBA); and syringaldehyde (S) were purchased from Sigma-Aldrich (USA). The other chemicals were obtained from Idalia (Poland) and POCh (Poland). Sawdust, RPC, and hay were purchased from a local market in Lodz, Poland.
Microorganism
Filamentous fungus M. roridum IM 6482 was isolated from soil samples collected around a textile dyeing factory (Zgierz, Poland). The strain was identified by molecular techniques and preserved in the strain collection of the Department of Industrial Microbiology and Biotechnology, University of Lodz (Poland). The strain was regularly subcultured on ZT slants and maintained at 4 °C. Laccase production was proven in both static and submerged cultures by using ABTS and syringaldazine as the substrates (Jasińska et al. 2012).
Media preparation
In this study, sawdust (5 × 5 × 2 mm), RPC (2 × 2 × 2 mm), and hay (5 × 5 × 2 mm) were used as the substrates for the production of laccase by M. roridum under submerged conditions. Hot water extracts of the media were prepared according to a previous study (Atlas 2010). pH was adjusted to 6.8. Media were used as pure extracts with or without the supplementation of 0.75% (w/v) of glucose and 0.3% (w/v) of yeast extract. Next, the media were supplemented with 1 mM CuSO4 as an inducer of laccase. The extracts were analyzed for the content of total proteins, reducing sugars, and phenols.
Protein concentration was determined using the BCA method (according to the Pierce™ BCA Protein Assay Kit protocol).
Reducing sugars were determined according to the method described by Miller (1959) with some modifications. Specifically, the diluted samples and 3,5-dinitrosalicylic acid (DNS) solvent (prepared by dissolving 1 g of DNS in 20 mL of 2 M NaOH and the volume adjusted to 100 mL with citrate–phosphate buffer pH 8.0) were thoroughly mixed and reacted in boiling water bath for 5 min. The absorbance of the sample was measured at 540 nm, and the amount of sugar was determined based on the absorbance of the glucose as the standard.
Determination of phenolic compounds was performed by the modified Folin–Ciocalteu method (Singleton et al. 1965). Briefly, 188 µL of deionized water, 12 µL of Folin–Ciocalteu reagent, and 30 µL of Na2CO3 (200 g/L) were added to the sample (20 µL). Then, the samples were incubated in the dark at room temperature for 1 h. Next, deionized water (50 µL) was added and the absorbance was measured at 765 nm. Simultaneously, a standard curve was prepared using GA solutions with the following concentrations: 0.00, 0.05, 0.10, 0.25, 0.50, 0.75, and 1.00 mg/L.
LC–MS/MS was performed to determine the phenolic contents in extracts using Agilent 1200 chromatograph (Agilent, USA) coupled with QTRAP 3200 mass spectrometer (SCIEX, USA). Chromatographic separation was performed on a Synergi Hydro-RP column (2 × 150 mm, 4 µm) (Phenomenex, Germany) according to parameters described in Table S1. The flow rate was set to 600 µL/min at 50 °C, and the injection volume was set to 10 µL. The applied eluents were water (A) and acetonitrile (B), both supplemented with 0.1% formic acid. The 10-min separation time was started from 5% B for 1 min followed by a linear increase to 95% B for 5 min and held for 2 min and then decreased to 5% B and held for 2 min. The MS parameters (in negative ionization mode) were as follows: IS: − 4500 V, Cur: 25, GS1: 50, GS2: 60, temperature: 500 °C. Ionization polarity, optimal declustering potential (DP), product ion, and collision energy (CE) for all compounds were manually tuned using standard solutions as presented in Table S1.
Laccase production and purification
Laccase was produced by submerged cultures. To prepare the inoculum, 7 mL of the WHI medium containing peptone (5 g/L), yeast extract (5 g/L), KH2PO4 (5 g/L), glucose (2% (v/v)), and soybean oil (0.025% (v/v)) was added to a fully sporulated culture slant. A preculture was prepared by using spore suspension of approximately 5 × 109 spores/mL, which was incubated at 28 °C with shaking at 140 rpm for 24 h. These precultures were transferred to a fresh medium (10%, v/v) and incubated for another 24 h. Cultures of M. roridum IM 6482 prepared in 1-L Erlenmeyer flasks containing 270 mL of each test medium prepared according to “Media preparation” section were inoculated with 30 mL of a homogenous preculture. Cultures were incubated with shaking (150 rpm) at 28 °C. At appropriate time intervals, the cultures were centrifuged (3500×g, 15 min). Fungal biomass was washed with distilled water and dried overnight in an air oven at 80 °C. Laccase activity in the extracellular fluid was determined spectrophotometrically according to the method described earlier with ABTS as a substrate (Eggert et al. 1996). The obtained filtrate with the highest laccase activity was used for the protein precipitation and purification according to the method described by Jasińska et al. (2018).
Effects of pH on laccase activity and stability
Optimum pH values for the laccase activity were determined at a pH range of 2.2–8.0 using Mcllvaine buffer at room temperature and ABTS as the substrate. For pH stability testing, the enzyme was incubated at pH values ranging from 2.2 to 8.0 in Mcllvaine buffer for 4 h at room temperature. Then, the residual laccase activity was determined under standard reaction conditions with ABTS as the substrate.
Decolorization experiment
The decolorization experiment was performed at room temperature. The course of decolorization was studied by measuring the absorbance at the appropriate wavelength (λmax) for a given dye (AO7, 485 nm; AB113, 556 nm; Amaranth, 521 nm; TB, 607 nm; and SY FCF, 482 nm). The reaction mixture contained a dye prepared at a specified concentration (50, 100, 200, or 400 mg/L) in a buffer of the appropriate pH (2.2, 3, 4, 5, 6, 7, or 8). The effect of reaction mediators such as ABTS, TEMPO, DMP, GA, CA, and V (100 µM) was analyzed. The decolorization of Amaranth was also evaluated from simulated dye effluent (SDE) containing additional compounds: Zn(CH3COOH)2 × 2H2O; Co(CH3COOH)2 × 4H2O; Cd(CH3COOH)2 × 2H2O; and NaCl (at concentration 0.1 mM); Tween 80; SDS; urea; and EDTA (at concentration 0.1%) and the mixture of dyes AB113; AO7; SY FCF; Amaranth; and TB (each at concentration 50 mg/L). The decolorization was expressed as a percentage of color loss with reference to the control sample without enzyme. All measurements were repeated thrice, and the average values were used for all calculations.
Immobilization and reusability experiment
For immobilization of laccase, 2 g of sodium alginate was prepared by dissolving in 10 mL water. To the sodium alginate solution, an equivalent amount of enzyme extract (25 IU), RPC (10 g/L), or both of them were added under continuous stirring. Then, the mixture was dropped into chilled CuSO4 × 5H2O solution (150 mM), and the resulting beads were allowed to harden in the same solution for 2 h under mild agitation. After this, the beads were collected and washed several times by using deionized water, until there was no detectable laccase activity in the solution. Then, these beads were used in the decolorization experiment according to method described in “Decolorization experiment” section. The reusability of the immobilized laccase for the decolorization of dyes was tested for up to five successive batches of 24-h incubation each. After every decolorization cycle, alginate beads were filtered and washed thrice with deionized water. The cleaned beads were reused for the next decolorization cycle.
Results and discussion
Fungal growth and laccase production on waste materials
Biotechnological applications require large amounts of low-cost enzymes. Therefore, one of the appropriate approaches is to utilize the waste materials or cheap agricultural by-products for the preparation of growth medium. During media preparation as well as during solid-state fermentation, some soluble carbohydrates and inducers are released, which ensure efficient production of enzymes (Singhaniaa et al. 2009). In this study, different lignocellulosic materials (5% w/v) were used to prepare the medium (according to method described in “Media preparation” section). The type of waste material used to prepare the medium strongly influenced the growth of M. roridum and laccase production (Fig. 1). Growth of the fungus was similar in medium prepared from HE or RPCE. Dry weight of mycelium obtained after 24- and 48-h cultivation in the aforementioned media reached 6.93 and 6.68 mg/mL, and the activity of the enzyme in their supernatants reached 566 and 728 U/L, respectively, which was found to be almost 2 and 3 times higher than the activity assessed in SE medium. The better growth and laccase production in RPCE and HE media might be due to the availability of some nutrients that are necessary for the growth of the fungus. The initial characterization of media showed the highest content of reducing sugars (1490 µg/mL) in HE medium. Phenolic acids, which are natural products of lignin degradation, can affect the activity of laccase. Previously, many studies have demonstrated that a large proportion of phenolic compounds remain in the rapeseed meal after oil press (Szydłowska-Czerniak and Łaszewska 2015; Vuorela et al. 2004). In this study, the highest concentration of phenolic compounds was detected in RPCE medium (820 µg/mL). Rapeseed and grass hay are rich in phenolics, the major secondary metabolites obtained from plants (Yang et al. 2014). LC–MS/MS analysis revealed the presence of FA and HBA as well as V in all the tested media (Table 1). In addition, HE medium contained GA (59.4 ng/mL), which was not present in other media. Figure 2 presents the chromatograms of V obtained for standard, HE, RPCE, and SE. All extracts contained compounds with retention times similar to standards, which suggest the need to broaden the range of phenolic substances to be tested. The inductive effect of GA, HBA, CA, FA, p-coumaric, and sinapic acid on laccase has been reported earlier (Wang et al. 2014; Adekunle et al. 2017). The effect of supplementation of medium with RPC on the production of laccase, chitinase, and β-glucosidase by white rot fungus Cerrena unicolor has been previously described by Jaszek et al. (2016). The addition of RPC (3.5% w/v) distinctly stimulated the activities of enzymes. However, this is the first study reporting on HE and RPCE for the preparation of media. High content of reducing sugars and phenolic compounds in HE and RPCE makes them as an innovative, low-cost, and easily available media for the production of laccase.
Application of M. roridum laccase in the decolorization of Amaranth
Laccase decolorization potential was investigated with the use of Amaranth as a model azo dye. Amaranth (C.I. Name Acid red 24) has been widely used as a colorant of synthetic fiber, leather, paper, and phenol–formaldehyde resin in industries. The dye is also used in the food industry to color various food products. However, it is reported to be potentially cytotoxic and genotoxic. It can also cause allergic and asthmatic reactions, in some sensitive people, when it comes in contact with certain drugs such as aspirin (Mpountoukas et al. 2010; Zhang and Ma 2013; Basu and Kumar 2015). Since 1976, Amaranth has been banned by the United States Food and Drug Administration (USFDA) as a suspected carcinogen. However, it is still being used illegally in some countries. Therefore, considering the potential adverse effects of Amaranth on human health, there is an urgent need to regulate the consumption of this synthetic colorant as well as eliminate the residues of this dye from the environment. Degradation and decolorization of azo dyes by fungal laccases have gained more attention recently because of their environment-friendly and inexpensive nature. In our study, after 24-h cultivation of M. roridum in RPCE medium, laccase was precipitated and prepared as previously described (Jasińska et al. 2018). The purified laccase was tested for decolorization of Amaranth at different operational conditions.
Influence of pH on laccase activity, stability, and Amaranth decolorization
First, the influence of pH on laccase activity and dye decolorization in the pH range 2.2–8.0 at room temperature was examined. The results are presented in Fig. 3. The optimum pH of fungal laccase reported in the literature for the substrate ABTS is in the range of 3.0–6.0 (Fang et al. 2015). In this study, the enzyme was active in solutions with pH ranging from 2.2 to 8.0, whereas optimum pH for laccase activity was found to be at pH 4.0 which was found to be similar to what has been reported previously (Koschorreck et al. 2008; Yang et al. 2015; Zhuo et al. 2018). This agrees with our results obtained in the decolorization experiment, where Amaranth was most effectively decolorized within the first hour of incubation in solutions with pH 2–4. Extending the time of incubation did not increase the elimination of the dye from solutions with pH 2–4, but allowed to obtain high removal of the dye from solutions with neutral and slightly alkaline pH (7–8). The highest decolorization of the dye (91.56%) was detected after 24-h incubation with laccase in solution with pH 8. It is compatible with the results of enzyme stability. Laccase was found to be most stable after 4-h incubation in solutions with pH 8. However, it demonstrated high stability over pH ranging from 5 to 8, retaining over 80% of its initial activity after 4-h incubation at relevant pH. Most textile effluents are characterized by their alkaline pH, where most fungal laccases can lose their activities. This indicates that M. roridum laccase is a good candidate for basic and applied research with potentials for various industrial and biotechnological applications employing varying levels of pH.
Laccase–mediator system for decolorization improvement
To improve the degree of decolorization of Amaranth, the substrate was treated with M. roridum laccase in combination with one of the mediators ABTS, DMP, TEMPO, V, GA, or CA. According to the results, no significant effect on the decolorization was observed when Amaranth was at 50 mg/L (Fig. 4). However, all tested mediators increased the level of decolorization of Amaranth at concentrations more than 100 mg/L. After 4 h of decolorization in the mixture without mediators, Amaranth at a concentration as high as 400 mg/L was not found to be decolorized, whereas the addition of mediators resulted in the decolorization of the dye ranging from 76 to 87%. Because of their toxicity, most of the previously reported microbial decolorization systems cannot remove high concentration of dyes. Thus, primarily physicochemical processes are applied in the wastewater treatment. However, the application of mediators that are naturally present in the environment and have no toxic effects seems to be a promising alternative for the treatment of wastewater containing high concentration of dyes.
SDE decolorization
Effluents from the dyeing industries are characterized by the presence of low contents of metal and suspended solids; high chemical oxygen demand (COD); chlorinated organic compounds; surfactants; and intense color (Yaseen and Scholz 2018). Thus, to initially evaluate the possibility of using laccase from M. roridum for the treatment of real wastewater, we examined the decolorization of SDE (Fig. 5). When compared to a single dye solution, decolorization of SDE was found to be faster and after just 15 min of incubation with M. roridum laccase decolorization of SDE was found to be twice greater than the decolorization of a single dye. This result may be due to the effect of induction by metal ions on the activity of laccases, for example, as a result of avertable conformational changes. Notably, the enhanced activity of laccase by copper ions may be due to the incorporation of copper ions into the type-2 copper-binding sites. Similarly, numerous studies have also indicated that the addition of surfactants, primarily nonionic, such as Triton X-100, rhamnolipid, and Tween 80, might increase the removal of some xenobiotics by laccases by the protection of the enzyme, by changing the activity center, and by enhancing the solubility of xenobiotics. Ionic surfactants cause adverse effects, which impair the removal processes (Liu et al. 2012a, b).
Preliminary study on zero-waste approach for azo dyes removal
Previous work demonstrated that oilseed press cakes have the ability to absorb pollutants. Rapeseed, almond, sunflower, olive press cakes have been described as efficient sorbent materials for azo dye removal (Karagöz et al. 2008; Jasińska et al. 2013). Laccases have been immobilized on various types of supports, such as silica, activated carbon, chitosan, and alginate. Immobilization of enzymes on agroindustrial residues (e.g., coconut fiber, granular waste from a brewery, and rice straw) also has great potential because of its physical characteristics, chemical composition, and low-cost nature. To date, no research about the laccase immobilization on spent RPC has been reported. Therefore, considering the advantages of RPC as biosorbent and catalytic properties of laccase, a zero-waste approach in the removal of azo dyes was proposed in this study. It involved copper alginate immobilization of laccase together with RPC remained after the preparation of the growth medium for enzyme production. Decolorization of five azo dyes (AO7, Amaranth, AB113, SY FCF, and TB) was investigated using immobilized RPC, immobilized laccase, or immobilized mixture of both. After 24-h incubation, all the tested dyes were found to be decolorized at different extents (Fig. 6a). The highest rate of decolorization was found in solutions containing TB (83%), Amaranth (74%), and AO7 (81%) using immobilized mixture of laccase and RPC. Decolorization was found to be higher on 17–29% than in the presence of immobilized RPC and about 2–6 higher than when laccase was immobilized alone. To date, mainly physicochemical processes as well as adsorption using various adsorbents have been used to remove these dyes from aqueous solutions. Efficient elimination of TB, Amaranth, and AO7 was obtained by using some natural adsorbents such spent brewery grains (Silva et al. 2004) and plant leaves (Guerrero-Coronilla et al. 2015). Jung et al. (2016) applied activated carbon powder derived from spent coffee grounds into calcium alginate beads for the removal of AO7. After 24-h incubation, almost complete removal of the dye was achieved. However, this is the first study reporting the simultaneous immobilization of biosorbent and laccase for more efficient removal of dye.
As shown in Fig. 6b, the rate of removal of Amaranth by laccase immobilized with RPC even after five successive batches of 24-h incubation was found to be about 50%. Rate of Amaranth decolorization decreased clearly for immobilized RPC, whereas immobilized laccase decolorized the dye to the same extent. The decrease in the removal efficiency may be due to the reduction in the number of binding sites for the dye molecules, not due to the loss of the activity of laccase. Reusability of immobilized enzyme in the biodegradation process shows that the most important aspect for industrial application is being cost-effective, since it decreases the overall cost of the process.
Conclusion
Lignocellulosic materials such as sawdust, hay, and RPC have low economic value; therefore, their use as substrate for laccase production can significantly reduce the cost of the procurement of the enzyme. In this study, the use of water extracts of sawdust, hay, and RPC for the production of laccase from the fungus M. roridum was reported for the first time. The highest enzyme production was noted in HE and RPCE media and was correlated with the high concentration of reducing sugars and several phenolic compounds. Laccase occurred to be stable in the pH ranging from 2 to 8 and is able to decolorize the azo dye Amaranth (50 mg/L). Application of redox mediators allowed for 90% decolorization of up to 400 mg/L of Amaranth after 24 h of incubation. The enzyme decolorized the SDE containing several azo dyes, metal ions, reducing agents, and detergents. An environment-friendly approach involving copper alginate immobilization of laccase together with RPC remaining after the preparation of the medium for enzyme production was applied for azo dyes removal. After 24 h of incubation in dye solution, laccase/RPC alginate beads decolorized the AO 7, TB, and Amaranth by more than 70%. The removal rate of Amaranth by laccase immobilized with RPC was still about 50% after five successive batches of 24 h each. Due to the pH stability, high efficiency of decolorization of single azo dyes, as well as SDE, laccase seems to be an attractive candidate for different environmental purposes. Additionally, an innovative approach involving copper alginate immobilization of laccase and RPC remaining after the preparation of growth medium for the production of enzyme is a promising option as an eco-friendly catalyst for dyestuff treatment.
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This work is a result of Project No. UMO 2013/11/D/NZ9/02776 financed by the National Science Center of Poland.
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Jasińska, A., Góralczyk-Bińkowska, A., Soboń, A. et al. Lignocellulose resources for the Myrothecium roridum laccase production and their integrated application for dyes removal. Int. J. Environ. Sci. Technol. 16, 4811–4822 (2019). https://doi.org/10.1007/s13762-019-02290-x
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DOI: https://doi.org/10.1007/s13762-019-02290-x