Resumo
Oxidative enzymes secreted by white rot fungi can be applied in several technological processes within the paper industry, biofuel production and bioremediation. The discovery of native strains from the biodiverse Misiones (Argentina) forest can provide useful enzymes for biotechnological purposes. In this work, we evaluated the laccase and manganese peroxidase secretion abilities of four newly discovered strains of Trametes sp. that are native to Misiones. In addition, the copper response and optimal pH and temperature for laccase activity in culture supernatants were determined.The selected strains produced variable amounts of laccase and MnP; when Cu2+ was added, both enzymes were significantly increased. Zymograms showed that two isoenzymes were increased in all strains in the presence of Cu2+. Strain B showed the greatest response to Cu2+ addition, whereas strain A was more stable at the optimal temperature and pH. Strain A showed interesting potential for future biotechnological approaches due to the superior thermo-stability of its secreted enzymes.(AU)
Assuntos
Trametes/classificação , Trametes/genética , Lacase/análise , PeroxidasesResumo
Thermophilic and thermotolerant micro-organisms strains have served as the natural source of industrially relevant and thermostable enzymes. Although some strains of the Trametes genus are thermotolerant, few Trametes strains were studied at the temperature above 30 °C until now. In this paper, the laccase activity and the mycelial growth rate for Trametes trogii LK13 are superior at 37 °C. Thermostability and organic cosolvent tolerance assays of the laccase produced at 37 °C indicated that the enzyme possessed fair thermostability with 50% of its initial activity at 80 °C for 5 min, and could remain 50% enzyme activity treated with organic cosolvent at the concentration range of 25%50% (v/v). Furthermore, the test on production of laccase and lignocellulolytic enzymes showed the crude enzymes possessed high laccase level (1000 U g−1) along with low cellulose (2 U g−1) and xylanase (140 U g−1) activity. Thus, T. trogii LK13 is a potential strain to be applied in many biotechnological processes.(AU)
Assuntos
Lacase/metabolismo , Trametes/enzimologia , Trametes/crescimento & desenvolvimento , Análise por Conglomerados , DNA Fúngico/química , DNA Fúngico/genética , DNA Espaçador Ribossômico/química , DNA Espaçador Ribossômico/genética , Estabilidade Enzimática , Lacase/químicaResumo
Aspergillus flavus was isolated from soil and exhibited laccase activity under both constitutive and copper induced conditions. Spiking the medium with 1 mM copper sulfate resulted in an increase in the activity which reached 51.84 U/mL, a distinctive protein band was detected at 60 kDa. The extracellular enzyme was purified 81 fold using gel filtration chromatography and resulted in two different laccase fractions L1 and L2, the latter had a higher enzymatic activity which reached 79.57 U/mL and specific activity of 64.17 U/μg protein. The analysis of the spectrum of the L2 fraction showed a shoulder at 330 nm which is characteristic for T2/T3 copper centers; both copper and zinc were detected suggesting that this is an unconventional white laccase. Primers of laccase gene were designed and synthesized to recover specific gene from A. flavus. Sequence analysis indicated putative laccase (Genbank ID: JF683612) at the amino acid level suggesting a close identity to laccases from other genera containing the copper binding site. Decolorization of textile waste water under different conditions showed possible application in bioremediation within a short period of time. The effect of copper on A. flavus was concentration dependent.(AU)
Assuntos
Aspergillus flavus , Aspergillus flavus/enzimologia , Cobre/metabolismo , Regulação Enzimológica da Expressão Gênica , Aspergillus flavus/genética , Aspergillus flavus/isolamento & purificação , Cromatografia em Gel , Meios de Cultura/químicaResumo
aguardando
Three experiments were carried out to examine the effect of lignocellulolytic enzymes on the nutritive value of whole-plant corn silage (WPCS). In experiment 1, we examined the effect of spent substrate from Pleurotus ostreatus cultivation (SSPO) on the chemical composition, antioxidant capacity, lignin monomers, and in vitro 5 digestibility of WPCS. In experiment 2, we evaluated the performance of lactating goats fed WPCS treated with different levels of SSPO. In experiment 3, we verified the activity of an enzymatic complex at different pH and the effects of adding increasing levels of that enzymatic complex produced by Pleurotus ostreatus on the fermentative profile, chemical composition, and ruminal digestibility along of the days on the onset of fermentation of WPCS. In experiment 1, four levels of lignocellulolytic enzymes from spent substrate of Pleurotus ostreatus were tested in a completely randomized design: 0, 10, 20, and 30 mg of lignocellulosic enzymes/kg of fresh matter, and four replicates per treatment (vacuum-sealed bags). The bags were opened 60 d after ensiling. The NDF, ADF, lignin, and cellulose concentration decreased quadratically. At the nadir point, SSPO decreased NDF by 14.1%, ADF by 19.5%, lignin by 9.07%, and cellulose by 22.1% compared to the untreated silage. Therefore, SSPO led to a quadratic increase in IVDMD of WPCS (+10.3 % at vertex). In experiment 2, WPCS treated with three enzyme levels (0, 10, or 30 mg/kg fresh matter, chosen based on experiment 1) were fed to lactating goats as part of TMR. Nine lactating Saanen goats (62.68±7.62 kg BW; 44±8 days in milk; 2.91±0.81 kg of milk/day, mean±SD) were assigned to three 3 × 3 Latin squares. Intake and digestibility of dry matter and nutrients, microbial protein syntheses, and milk production and composition were examined. The SSPO increase the in vivo total-tract ADF digestibility quadratically. Additionally, the concentration of polyphenols in milk increased linearly with the addition of SSPO in WPCS; however, no other differences were detected among treatments. In experiment 3, the lignocellulolytic enzymatic complex was obtained through in vitro cultivation of Pleurotus ostreatus, and the activities of laccase, lignin peroxidase, manganese peroxidase, endo and exoglucanase, xylanase, and mannanase were determined at pH 3, 29 4, 5, and 6. Following, five different enzymatic complex levels were tested in a completely randomized block design: 0; 9; 18; 27, and 36 mg of lignocellulosic enzymes/kg of fresh matter (FM) of whole-plant corn, with four replicates per treatment (vacuum-sealed bags). The bags were opened after 1, 2, 3, and 7 d of ensiling to evaluate the onset of fermentation and after 30 d of storage to evaluate the fermentation, chemical composition, and in situ digestibility of WPCS. Laccase showed highest activity at pH 5 (P < 0.01), whereas manganese peroxidase and lignin peroxidase had a higher activity at pH 4 (P < 0.01;< 0.01, respectively). There was no interaction between the enzymatic complex and days of fermentation (P > 0.11). The concentration of WSC decreased quadratically at the onset of fermentation (P = 0.02) due to its consumption that led to a quadratic increase of lactic acid (P = 0.01) and a linear increase of acetic acid (P = 0.02). As a result of increasing those organic acid concentrations, pH decreased quadratically (P = 0.01). Lignin concentration decreased linearly (P = 0.04) with the enzymatic complex at 30 d of storage. The collective interpretation of these results leads to the conclusion that 10 mg of lignocellulolytic enzymes from SSPO per kg of FM of WPC presented the best effect in silage production due to more evident reduction in NDF, ADF, and lignin concentration and increased ADF digestibility of lactation goats
Resumo
Laccases are blue copper oxidases (E.C. 1.10.3.2) that catalyze the one-electron oxidation of phenolics, aromatic amines, and other electron-rich substrates with the concomitant reduction of O2 to H2O. A novel laccase gene pclac2 and its corresponding full-length cDNA were cloned and characterized from Phytophthora capsici for the first time. The 1683 bp full-length cDNA of pclac2 encoded a mature laccase protein containing 560 amino acids preceded by a signal peptide of 23 amino acids. The deduced protein sequence of PCLAC2 showed high similarity with other known fungal laccases and contained four copper-binding conserved domains of typical laccase protein. In order to achieve a high level secretion and full activity expression of PCLAC2, expression vector pPIC9K with the Pichia pastoris expression system was used. The recombinant PCLAC2 protein was purified and showed on SDS-PAGE as a single band with an apparent molecular weight ca. 68 kDa. The high activity of purified PCLAC2, 84 U/mL, at the seventh day induced with methanol, was observed with 2,2'-azino-di-(3-ethylbenzothialozin-6-sulfonic acid) (ABTS) as substrate. The optimum pH and temperature for ABTS were 4.0 and 30 ºC, respectively . The reported data add a new piece to the knowledge about P. Capsici laccase multigene family and shed light on potential function about biotechnological and industrial applications of the individual laccase isoforms in oomycetes.(AU)
Assuntos
Lacase/genética , Lacase/metabolismo , Phytophthora/enzimologia , Clonagem Molecular , Sequência Conservada , Estabilidade Enzimática , Expressão Gênica , Concentração de Íons de Hidrogênio , Lacase/química , Lacase/isolamento & purificação , Peso Molecular , Fases de Leitura Aberta , Estrutura Terciária de Proteína , Phytophthora/genética , Pichia/genética , Sinais Direcionadores de Proteínas/genética , Proteínas Recombinantes/química , Proteínas Recombinantes/genética , Proteínas Recombinantes/isolamento & purificação , Proteínas Recombinantes/metabolismo , Homologia de Sequência de Aminoácidos , TemperaturaResumo
Pleurotus species secrete phenol oxidase enzymes: laccase (Lcc) and manganese peroxidase (MnP). New genotypes of these species show potential to be used in processes aiming at the degradation of phenolic compounds, polycyclic aromatic hydrocarbons and dyes. Hence, a screening of some strains of Pleurotus towards Lcc and MnP production was performed in this work. Ten strains were grown through solid-state fermentation on a medium based on Pinus spp. sawdust, wheat bran and calcium carbonate. High Lcc and MnP activities were found with these strains. Highest Lcc activity, 741 ± 245 U gdm-1 of solid state-cultivation medium, was detected on strain IB11 after 32 days, while the highest MnP activity occurred with strains IB05, IB09, and IB11 (5,333 ± 357; 4,701 ± 652; 5,999 ± 1,078 U gdm-1, respectively). The results obtained here highlight the importance of further experiments with lignocellulolytic enzymes present in different strains of Pleurotus species. Such results also indicate the possibility of selecting more valuable strains for future biotechnological applications, in soil bioremediation and biological biomass pre-treatment in biofuels production, for instance, as well as obtaining value-added products from mushrooms, like phenol oxidase enzymes.(AU)
Assuntos
Genótipo , Pleurotus/fisiologia , Lacase/análise , Biotecnologia/tendências , Enzimas/ultraestruturaResumo
The mushroom Pleurotus ostreatus has nutritional and medicinal characteristics that depend on the growth substrate. In nature, this fungus grows on dead wood, but it can be artificially cultivated on agricultural wastes (coffee husks, eucalyptus sawdust, corncobs and sugar cane bagasse). The degradation of agricultural wastes involves some enzyme complexes made up of oxidative (laccase, manganese peroxidase and lignin peroxidase) and hydrolytic enzymes (cellulases, xylanases and tanases). Understanding how these enzymes work will help to improve the productivity of mushroom cultures and decrease the potential pollution that can be caused by inadequate discharge of the agroindustrial residues. The objective of this work was to assess the activity of the lignocellulolytic enzymes produced by two P. ostreatus strains (PLO 2 and PLO 6). These strains were used to inoculate samples of coffee husks, eucalyptus sawdust or eucalyptus bark add with or without 20 % rice bran. Every five days after substrate inoculation, the enzyme activity and soluble protein concentration were evaluated. The maximum activity of oxidative enzymes was observed at day 10 after inoculation, and the activity of the hydrolytic enzymes increased during the entire period of the experiment. The results show that substrate composition and colonization time influenced the activity of the lignocellulolytic enzymes.(AU)
Assuntos
Enzimas/análise , Pleurotus/classificação , Lacase/análise , Celulose , Agaricales/crescimento & desenvolvimentoResumo
Cascas de café são fonte de carboidratos e nutrientes que podem ser bioconvertidos em produtos de interesse como enzimas. Lacases são cobre polifenol oxidases que oxidam compostos fenólicos, enquanto reduzem oxigênio molecular à água e; sua baixa especificidade a substratos permite sua aplicação em várias áreas como indústria têxtil, de alimentos e biorremediação. Os objetivos desse trabalho foram avaliar a capacidade de produção de lacase de três linhagens de fungos basidiomicetos (Lentinula edodes U6/1, Pleurotus ostreatus U6/9 e Pleurotus florida U6/10) por fermentação submersa com cascas de café e avaliar o uso de cobre como indutor dessa enzima. A casca de café mostrou ser um bom substrato para produção de lacases e das três linhagens testadas Pleurotus ostreatus (U6/9) foi a mais produtiva (22,5 U mL-1). A melhor fonte de nitrogênio para produção de lacases de Pleurotus ostreatus (U6/9) foi o extrato de levedura na concentração de 9 g/L (20 U mL-1). A adição de 150 μM de CuSO4 resultou na indução significativa na produção de lacases nessa linhagem (21 U mL-1) no 12° dia de cultivo.
Coffee husks are a source of carbohydrates and nutrients that may be bioconverted into products of interest, such as enzymes. Laccases are copper polyphenol oxidases that oxidize phenolic compounds while reducing molecular oxygen to water. Laccases low specificity to substrates allows its application in several areas such as textiles, food processing and bioremediation industries. The aims of this study were to evaluate the potential to produce laccase from three strains of basidiomycetous fungi (Lentinula edodes U6/1, Pleurotus ostreatus U6/9, and Pleurotus florida U6/10) by submerged fermentation with coffee husks, and to evaluate the use of copper as an inducer of the enzyme. Coffee husk proved to be a good substrate for laccase production, with Pleurotus ostreatus (U6/9) being the most productive strain (22.5 U mL-1). The best source of nitrogen for laccase production of Pleurotus ostreatus (U6/9) was yeast extract 9 g/L (20 U mL-1). The addition of CuSO4 (150 μM) resulted in significant induction of laccase (21 U mL-1) on the 12th day of cultivation.
Cáscaras de café son fuente de carbohidratos y nutrientes que pueden ser bioconvertidos en productos de interés, tales como enzimas. Lacases son cobre polifenol oxidasas que oxidan compuestos fenólicos, mientras reducen el oxígeno molecular a el agua y; su baja especificidad a sustratos permite su aplicación en diversas áreas, como la industria textil, de alimentos y de biorremediación. Los objetivos de este estudio fueron evaluar la capacidad de producción de lacase de tres linajes de hongos basidiomicetos (Lentinula edodes U6/1, Pleurotus ostreatus U6/9 y Pleurotus florida U6/10) por fermentación sumergida con cáscaras de café, y evaluar el uso del cobre como inductor de esta enzima. La cáscara de café resultó ser un buen sustrato para la producción de lacases y, de las tres linajes probadas, Pleurotus ostreatus (U6/9) fue la más productiva (22,5 U mL-1). La mejor fuente de nitrógeno para la producción de lacases de Pleurotus ostreatus (U6/9) fue el extracto de levadura a una concentración de 9 g L-1 (20 U mL-1). La adición de 150 μM de CuSO4 resultó en la inducción significativa de Cáscaras de café son fuente de carbohidratos y nutrientes que pueden ser bioconvertidos en productos de interés, evadura a una concentración de 9 g L-1 (20 U mL-1). La adición de 150 μM de CuSO4 resultó en la inducción significativa de la producción de lacases en esa linaje (21 U mL-1), en el 12º día de cultivo.
Assuntos
Cogumelos Shiitake , Fungos/ultraestrutura , Pleurotus/ultraestrutura , Café/classificação , FermentaçãoResumo
Cascas de café são fonte de carboidratos e nutrientes que podem ser bioconvertidos em produtos de interesse como enzimas. Lacases são cobre polifenol oxidases que oxidam compostos fenólicos, enquanto reduzem oxigênio molecular à água e; sua baixa especificidade a substratos permite sua aplicação em várias áreas como indústria têxtil, de alimentos e biorremediação. Os objetivos desse trabalho foram avaliar a capacidade de produção de lacase de três linhagens de fungos basidiomicetos (Lentinula edodes U6/1, Pleurotus ostreatus U6/9 e Pleurotus florida U6/10) por fermentação submersa com cascas de café e avaliar o uso de cobre como indutor dessa enzima. A casca de café mostrou ser um bom substrato para produção de lacases e das três linhagens testadas Pleurotus ostreatus (U6/9) foi a mais produtiva (22,5 U mL-1). A melhor fonte de nitrogênio para produção de lacases de Pleurotus ostreatus (U6/9) foi o extrato de levedura na concentração de 9 g/L (20 U mL-1). A adição de 150 μM de CuSO4 resultou na indução significativa na produção de lacases nessa linhagem (21 U mL-1) no 12° dia de cultivo.(AU)
Coffee husks are a source of carbohydrates and nutrients that may be bioconverted into products of interest, such as enzymes. Laccases are copper polyphenol oxidases that oxidize phenolic compounds while reducing molecular oxygen to water. Laccases low specificity to substrates allows its application in several areas such as textiles, food processing and bioremediation industries. The aims of this study were to evaluate the potential to produce laccase from three strains of basidiomycetous fungi (Lentinula edodes U6/1, Pleurotus ostreatus U6/9, and Pleurotus florida U6/10) by submerged fermentation with coffee husks, and to evaluate the use of copper as an inducer of the enzyme. Coffee husk proved to be a good substrate for laccase production, with Pleurotus ostreatus (U6/9) being the most productive strain (22.5 U mL-1). The best source of nitrogen for laccase production of Pleurotus ostreatus (U6/9) was yeast extract 9 g/L (20 U mL-1). The addition of CuSO4 (150 μM) resulted in significant induction of laccase (21 U mL-1) on the 12th day of cultivation.(AU)
Cáscaras de café son fuente de carbohidratos y nutrientes que pueden ser bioconvertidos en productos de interés, tales como enzimas. Lacases son cobre polifenol oxidasas que oxidan compuestos fenólicos, mientras reducen el oxígeno molecular a el agua y; su baja especificidad a sustratos permite su aplicación en diversas áreas, como la industria textil, de alimentos y de biorremediación. Los objetivos de este estudio fueron evaluar la capacidad de producción de lacase de tres linajes de hongos basidiomicetos (Lentinula edodes U6/1, Pleurotus ostreatus U6/9 y Pleurotus florida U6/10) por fermentación sumergida con cáscaras de café, y evaluar el uso del cobre como inductor de esta enzima. La cáscara de café resultó ser un buen sustrato para la producción de lacases y, de las tres linajes probadas, Pleurotus ostreatus (U6/9) fue la más productiva (22,5 U mL-1). La mejor fuente de nitrógeno para la producción de lacases de Pleurotus ostreatus (U6/9) fue el extracto de levadura a una concentración de 9 g L-1 (20 U mL-1). La adición de 150 μM de CuSO4 resultó en la inducción significativa de Cáscaras de café son fuente de carbohidratos y nutrientes que pueden ser bioconvertidos en productos de interés, evadura a una concentración de 9 g L-1 (20 U mL-1). La adición de 150 μM de CuSO4 resultó en la inducción significativa de la producción de lacases en esa linaje (21 U mL-1), en el 12º día de cultivo.(AU)
Assuntos
Fungos/ultraestrutura , Cogumelos Shiitake , Pleurotus/ultraestrutura , Café/classificação , FermentaçãoResumo
Fourteen strains of Grifola frondosa (Dicks.) S. F. Gray, originating from different regions (Asia, Europe and North America) were tested for lignin degradation, ligninolytic enzyme activities, protein accumulation and exopolysaccharide production during 55 days of cultivation on oak sawdust. Lignin degradation varied from 2.6 to7.1 % of dry weight of the oak sawdust substrate among tested strains. The loss of dry matter in all screened fungi varied between 11.7 and 33.0%, and the amount of crude protein in the dry substrate varied between 0.94 to 2.55%. The strain, MBFBL 596, had the highest laccase activity (703.3 U/l), and the maximum peroxidase activity of 22.6 U/l was shown by the strain MBFBL 684. Several tested strains (MBFBL 21, 638 and 662) appeared to be good producers of exopolysaccharides (3.5, 3.5 and 3.2 mg/ml respectively).
Resumo
Enzyme application in biotechnological and environmental processes has had increasing interest due to its efficiency, selectivity and mainly for being environmentally healthful, but these applications require a great volume of enzymes. In this work the effect of different concentrations of ethanol and 2,5 - xylidine on growth and production of laccase by Pycnoporus sanguineus was investigated. In a medium containing 200 mg.L-1 of 2,5 - xylidine or 50 g.L-1 of ethanol, the maximum activity of laccase was 2019 U.L-1 and 1035 U.L-1, respectively. No direct correlation between biomass and activity of laccase was observed for any of the inducers used during the tests. Ethanol concentrations, larger than or equal to 20 g.L-1, inhibited the radial growth of P. sanguineus. This study showed that ethanol, which has less toxicity and cost than the majority of the studied inducers, presents promising perspectives for laccase production by P. sanguineus.
Resumo
Various genotoxic textile dyes, xenobiotics, substrates (10 µM) and agrochemicals (100 µg/ml) were tested for enhancement of alkalophilic laccase activity in-proteobacterium JB. Neutral Red, Indigo Carmine, Naphthol Base Bordears and Sulphast Ruby dyes increased the activity by 3.7, 2.7, 2.6 and 2.3 fold respectively. Xenobiotics/substrates like p-toluidine, 8-hydroxyquinoline and anthracine increased it by 3.4, 2.8 and 2.3 fold respectively. Atrazine and trycyclozole pesticides enhanced the activityby 1.95 and 1.5 fold respectively.
Vários corantes têxteis genotóxicos, xenobióticos, substratos (10 mM) e agroquímicos (100 mM/mL) foram testados quanto ao aumento da atividade de lacase em -Proteobacterium JB. Os corantes Neutral Red, Indigo Carmine, Naphtol Base Bordears e Sulphast Ruby aumentaram a atividade em 3,7, 2,7, 2,6 e 2,3 vezes, respectivamente. Xenobióticos/substratos como p-toluidina, 8-hidroxiquinolina e antracina aumentaram a atividade em 3,4, 2,8 e 2,3 vezes, respectivamente. Atrazina e pesticidas triciclozol aumentaram a atividade em 1,95 e 1,5 vezes, respectivamente.
Resumo
Wood rotting Basidiomycetes collected in the "Estação Ecológica do Noroeste Paulista", São José do Rio Preto, São Paulo State, Brazil, concerning Aphyllophorales order and identified as Coriolopsis byrsina SXS16, Lentinus strigellus SXS355, Lentinus sp SXS48, Picnoporus sanguineus SXS 43 and Phellinus rimosus SXS47 were tested for ligninases production by solid state fermentation (SSF) using wheat bran or rice straw as culture media. C. byrsina produced the highest laccase (200 U mL-1) and Lentinus sp produced the highest activities of manganese peroxidase (MnP) and lignin peroxidase (LiP) (7 and 8 U mL-1, respectively), when cultivated on wheat bran. The effect of N addition on enzyme production was studied in medium containing rice straw and the data showed an increase of 3 up to 4-fold in the laccase production compared to that obtained in SSF on wheat bran. The laccases presented optimum pH at 3.0-3.5 and were stable at neutral pH values. Optimum pH for MnP and LiP activities was at 3.5 and between 4.5 and 6.0, respectively. All the strains produced laccase with optimum activities between 55-60°C while the peroxidases presented maximum activity at temperatures of 30 to 55°C. The crude enzymes promoted decolorization of chemically different dyes with around 70% of decolorization of RBBR and cybacron blue 3GA in 6h of treatment. The data indicated that enzymes from these basidiomycetes strains are able to decolorize synthetic dyes.
Fungos decompositores de madeira, do grupo Basidiomicetes, coletados na "Estação Ecológica do Noroeste Paulista", São José do Rio Preto, São Paulo, Brasil, pertencentes a ordem Aphyllophorales e identificados como Coriolopsis byrsina SXS16, Lentinus strigellus SXS355, Lentinus sp. SXS48, Picnoporus sanguineus SXS 43 e Phellinus rimosus SXS47 foram estudados para a produção de ligninases por FES (fermentação em estado sólido) usando farelo de trigo ou palha de arroz como meio de cultura. A espécie C. byrsina produziu a maior quantidade de lacase (200 U mL-1) enquanto que Lentinus sp. foi o melhor produtor de manganês peroxidase (MnP) e lignina peroxidase (LiP) (7 e 8 U mL-1, respectivamente), quando cultivados em meio composto por farelo de trigo. A avaliação do efeito da suplementação de nitrogênio do substrato sólido lignocelulósico (palha de arroz) indicou um aumento de 3 a 4 vezes na produção de lacase. A caracterização das enzimas mostrou que as lacases apresentaram atividade ótima em pH 3,0-3,5 e foram estáveis em pH de neutro a alcalino. O pH ótimo para atividade de MnP e LiP foi de 3,5 e entre 4,5 e 6,0, respectivamente. Todas as linhagens produziram lacase com atividade ótima a 55-60°C, enquanto as peroxidases apresentaram atividades máximas entre temperaturas de 30 e 55°C. A aplicação das soluções enzimáticas brutas, obtidas pelo cultivo das linhagens em meio de farelo de trigo, em testes de descoloração de corantes sintéticos de diferentes grupos químicos levou a mais 70% de perda de cor dos corantes RBBR e de cybacron blue 3GA, em 6h de tratamento. Os dados obtidos indicaram que as soluções enzimáticas contendo ligninases produzidas pelas linhagens de basidiomicetos estudadas promoveram a descoloração de corantes sintéticos.
Resumo
The expression of the enzymatic system produced by basidiomycetous fungi, which is involved in the degradation of xenobiotics, mainly depends on culture conditions, especially of the culture medium composition. Trametes villosa is a strain with a proven biotechnological potential for the degradation of organochlorine compounds and for the decolorization of textile dyes. The influence of glucose concentration, addition of a vegetable oil-surfactant emulsion, nature of the surfactant and the presence of manganese and copper on the growth, pH and production of laccase, total peroxidase and manganese-dependent peroxidase activities were evaluated. In general, acidification of the medium was observed, with the pH reaching a value close to 3.5 within the first days of growth. Laccase was the main activity detected under the different conditions and was produced throughout the culture period of the fungus, irrespective of the growth phase. Supplementation of the medium with vegetable oil emulsified with a surfactant induced manganese-dependent peroxidase activity in T. villosa. Higher specific yields of laccase activity were obtained with the addition of copper.
A expressão do sistema enzimático produzido por fungos basidiomicetos envolvido na degradação de xenobióticos é bastante dependente das condições de cultivo, principalmente da composição do meio de cultivo. Trametes villosa CCB176 é uma linhagem com comprovado potencial biotecnológico para degradação de compostos organoclorados e descoloração de corantes têxteis. Foi avaliada a influência da concentração de glicose, adição de emulsão de óleo vegetal e surfactante, natureza do surfactante e os metais manganês e cobre no crescimento, pH e na produção das atividades de lacase, de peroxidases totais e de peroxidase dependente de manganês. No geral, ocorreu acidificação do meio com pH atingindo valor próximo a 3,5, nos primeiros dias de crescimento. Lacase foi a principal atividade detectada nas diferentes condições e sua produção se deu durante todo o período de cultivo do fungo, independente da fase de crescimento. Suplementação do meio com óleo vegetal emulsificado com surfactante resultou em indução da atividade de peroxidase dependente de manganês produzida por T. villosa. Maiores valores de rendimento específico da atividade de lacase foram propiciados pelo cobre.
Resumo
Nine isolates of Botryosphaeria spp. were evaluated for their growth and the production of cell wall-lytic enzymes (laccase, pectinase and beta-1,3-glucanase) when grown on basal medium in the absence and presence of the laccase inducer, veratryl alcohol (VA). The genetic relationship among the nine isolates collected from different host plants was determined by RAPD analyses. ITS sequence analysis showed eight closely related isolates classified as Botryosphaeria rhodina, and one isolate classified as Botryosphaeria ribis. RAPD analysis resolved the isolates into three main clusters based upon levels of laccase and beta-1,3-glucanase activity. There appears to be no correlation between pectinase production and genetic diversity among the nine isolates. However, the strain characterized as B. ribis, positioned out of the main cluster, was found to be the highest producer of pectinases in the presence of VA.
Nove isolados de Botryosphaeria spp foram avaliados quanto ao crescimento e produção de enzimas líticas da parede celular (lacase, pectinase e beta-1,3-glucanase) quando cultivados em meio basal na ausência e presença do indutor de lacase álcool veratrílico (VA). As relações genéticas entre os nove isolados coletados de diferentes plantas hospedeiras foram determinadas por RAPD. A análise das seqüências de nucleotídeos da região ITS mostrou oito isolados estreitamente relacionados, os quais foram classificados como Botryosphaeria rhodina e um isolado como Botryosphaeria ribis. A análise por RAPD agrupou os isolados em três grupos principais condizentes com os níveis de atividades de lacase e beta-1,3-glucanase. Nenhuma correlação foi detectada entre a produção de pectinase e a diversidade genética nos nove isolados. Entretanto, a linhagem caracterizada como B. ribis, posicionada fora dos grupos principais, se mostrou maior produtora de pectinase na presença de álcool veratrílico.
Resumo
In order to identify alternatives for soil fumigation in bioremediation process, the addition of benomyl and vegetable oil on the growth of L. crinitus and mitosporic fungi were evaluated. Benomyl can be used as an alternative to methyl bromide. Addition of vegetable oil favors the growth of L. crinitus.
Para identificar alternativas para a fumigação de solo em processos de biorremediação, foi avaliada a adição de benomil e de óleo vegetal no crescimento de Lentinus crinitus e fungos mitospóricos. Benomil pode ser usado como alternativa ao brometo de metila. A adição de óleo vegetal favoreceu o crescimento de L. crinitus.
Resumo
Pleurotus ostreatus ("shimeji") is produced in Brazil on a commercial scale using various lignocellulosic residues. Efforts have been made to reuse the culture residue to obtain products of greater aggregate value such as enzymes or in processes of bioremediation. We evaluated the Remazol brilliant blue R (RBBR) degradation potential of extracts from solid substrate colonized by P. ostreatus and extracts from residue of the "shimeji" mushroom yield. Colonized substrates and residue were provided by Toyobo do Brasil Ltda. Extraction was performed with sodium acetate buffer (50 mM, pH 4.6). RBBR decolorization was monitored at 592 nm and peroxidase and laccase activities were measured by monitoring the oxidation of ABTS. Horseradish peroxidase was used as reference. The time of growth of P. ostreatus influenced RBBR degradation and peroxidase and laccase activities. Concentration of 1 mM H2O2 and pH 4.0 were the best for RBBR decolorization. Complete RBBR decolorization was obtained with the addition of only one aliquot of 50 µL of 1 mM H2O2. The stability of the extracts was higher when they were kept under refrigeration than when stored frozen. The potential application of the ligninolytic complex derived from P. ostreatus and mushroom residue for xenobiotic degradation was demonstrated.
Pleurotus ostreatus ("shimeji") é produzido no Brasil em escala comercial empregando-se vários resíduos lignocelulósicos. Esforços têm sido feitos para reaproveitamento do resíduo do cultivo em produtos de maior valor agregado, como enzimas ou sua aplicação em processos de biorremediação. Foi feita avaliação do potencial de degradação do azul brilhante de remazol (RBBR) por extratos obtidos de substratos sólidos colonizados por P. ostreatus e por extratos do resíduo da produção do cogumelo "shimeji". Substratos colonizados e o resíduo foram fornecidos pela Toyobo do Brasil Ltda. Extração foi feita com tampão acetato de sódio (50 mM, pH 4,6). Descoloração do RBBR foi acompanhada a 592 nm e atividades de peroxidases e lacase pela oxidação do ABTS. Peroxidase da raiz forte (HRP) foi usada como referência. O tempo de crescimento de P. ostreatus influenciou a degradação do RBBR e a produção das atividades enzimáticas de peroxidases e de lacase. Concentração de 1 mM de H2O2 e pH 4,0 mostraram-se ótimos para descoloração do RBBR. Descoloração total do RBBR foi obtida com adição de apenas uma alíquota de 50 µL de H2O2 (1 mM). Maior estabilidade dos extratos foi obtida por refrigeração que por congelamento. Foi evidenciado o potencial de aplicação de extratos enzimáticos de Pleurotus ostreatus e do resíduo da produção do cogumelo para a degradação de compostos xenobióticos.
Resumo
Laccases are enzymes involved in lignin degradation and are produced by various organisms. Due to their low substrate specificity their potential to be used in biotechnological applications has received attention. The addition of laccase inducers to the culture medium of microorganisms can enhance laccase production and facilitate its purification and utilization. The aim of this study was to investigate the effect of some compounds as laccase inducers in cultures of Lentinula edodes (shiitake). First, it was selected a culture medium suitable for laccase production by shiitake using two levels of N (2.6 and 26 mM) and seven levels of Cu (0, 50, 100, 150, 200, 250 and 300 µM). The medium with 2.6 mM N and 250 µM Cu was found to provide the highest laccase activity. To the selected medium it were added gallic acid (1 mM), catechol (1 mM), ammonium tartrate (55 µM), hydroxybenzoic acid (1 mM) and vanillin (1 mM). The two first compounds completely inhibited laccase activity and a 30 day time course experiment was carried out with the remaining compounds. Only cultures with ammonium tartrate exhibited laccase activity higher than control cultures, reaching 251 U/mL of extract after 30 days. A native-PAGE was performed and showed only one band, suggesting that no isozyme was produced.
Lacases são enzimas envolvidas na degradação da lignina e produzidas por diversos organismos. Devido à sua baixa especificidade por substratos, seu potencial para utilização em aplicações biotecnológicas tem sido objeto de investigação. A adição de indutores de lacases ao meio de cultivo de microrganismos aumenta a produção dessas enzimas, facilitando sua purificação e utilização. Este trabalho teve como objetivo investigar o efeito de alguns compostos utilizados como indutores de lacases em fungos na produção destas enzimas por Lentinula edodes (shiitake). Previamente a utilização de indutores, foi selecionado um meio de cultura para a produção de lacases por shiitake, utilizando-se duas concentrações de N (2,6 mM e 26 mM) e sete de Cu (0, 50, 100, 150, 200, 250 e 300 µM). O meio no qual maior atividade de lacases foi detectada continha 2,6 mM N e 250 µM de Cu. Posteriormente, ao meio selecionado foram adicionados ácido gálico (1 mM), catecol (1 mM), tartarato de amônio (55 µM), ácido hidroxibenzóico (1 mM) e vanilina (1 mM). Os dois primeiros compostos inibiram completamente a atividade de lacases por shiitake, e um experimento com os restantes foi conduzido por 30 dias. Apenas as culturas com tartarato de amônio apresentaram atividade de lacase maior que o tratamento controle, alcançando 251 U/mL de extrato após 30 dias de cultivo. Um gel de atividade (native PAGE) exibiu apenas uma banda, sugerindo não haver produção e isozimas.
Resumo
Remazol Brilliant Blue R (RBBR) dye was used as substrate to evaluate ligninolytic activity in 125 basidiomycetous fungi isolated from tropical ecosystems. The extracellular RBBR decolorizing activity produced when selected fungi were grown in solid media and in soil contaminated with organochlorines was also evaluated. A total of 106 fungi decolorized the RBBR during the growth in malt extract agar (MEA, 2%); 96 fungi showed a mycelia growth and decolorization activity stronger than the P. chrysosporium used as reference. Extracellular extracts of 35 selected fungi grown on solid medium with sugar cane bagasse (BGS) were evaluated for RBBR decolorization and peroxidase activity. All fungi showed peroxidase activities, but 5 of those were unable to decolorize the RBBR. Different patterns of ligninolytic enzymes were detected in 12 fungi extracts. Mn-dependent peroxidase (MnP) was produced by Peniophora cinerea, Psilocybe castanella, three strains of Trametes villosa, T. versicolor, Melanoporia nigra and Trichaptum byssogenum. All 12 fungi had laccase activity. Trogia buccinalis showed the highest RBBR decolorization and did not produce MnP activity. RBBR decolorization without MnP production was also observed for three strains of Lentinum tested. Higher levels of peroxidase and laccase cannot be related to high RBBR decolorization. RBBR decolorization by extracellular extract was also detected during the growth of P. castanella, L. crinitus, P. cinerea and two strains of T. Villosa in pentachlorophenol- and hexachlorobenzene-contaminated soils. These fungi showed higher RBBR decolorization when grown in the presence of organochlorine compounds than when in non contaminated soil.
O corante azul brilhante Remazol R (RBBR) foi usado como substrato para avaliar 125 fungos basidiomicetos isolados de ecossistemas tropicais brasileiros quanto a atividade ligninolítica. A descoloração do RBBR por extratos obtidos do crescimento de fungos em meio sólido e em solo contaminado com organoclorados foi também avaliada. Cento e seis fungos descoloriram o RBBR durante o crescimento em meio sólido (agar extrato malte); noventa e seis desses fungos mostraram crescimento micelial e descoloração superiores a uma cepa de Phanerochaete chrysosporium usada como referência. Trinta e cinco fungos foram crescidos em meio sólido contendo bagaço de cana-de-açúcar (BGS) e seus extratos foram avaliados quanto a descoloração do RBBR e a produção de atividade de peroxidases. Todos os fungos mostraram atividade de peroxidases, mas 5 foram incapazes de descolorir o RBBR. Diferentes padrões de enzimas lignolíticas foram detectados em 12 desses extratos fúngicos, porém todos mostraram atividade de laccase. Atividade de peroxidase dependente de manganês (MnP) foi produzida por Melanoporia nigra, Peniophora cinerea, Psilocybe castanella, três cepas de Trametes villosa, T. versicolor e Trichaptum byssogenum. Trogia buccinalis apresentou a maior descoloração do RBBR e não produziu MnP. Descoloração do RBBR sem produção de MnP foi também observada para as três cepas de Lentinus testadas. Altos níveis de atividades de peroxidases e laccases não mostraram relação com significativa descoloração do RBBR. Foi observada descoloração do RBBR por extratos obtidos de P. castanella, L. crinitus, P. cinerea e duas cepas de T. Villosa durante crescimento em solos contaminados com pentaclorofenol e hexaclorobenzeno. Estes fungos mostraram maior descoloração de RBBR na presença de compostos organoclorados do que em solos não contaminados.
Resumo
A Lepista sordida laccase has been characterized. Laccase and manganese peroxidase were detected in liquid medium with ammonium phosphate, yeast extract and ammonium molybdidate as nitrogen sources after 3 days of cultivation. Laccase optimal temperature and pH were 45ºC and 3.5, respectively.
Uma lacase de Lepista sordida foi caracterizada. O fungo produziu lacase e manganês peroxidase em meio líquido com fosfato de amônio, extrato de levedura e molibdato de amônio como fontes de nitrogênio 3 dias após a inoculação. Temperatura e pH ótimos para lacase foram 45ºC e 3,5, respectivamente.