Two β-xylanases from Aspergillus terreus: Characterization and influence of phenolic compounds on xylanase activity

Moreira, Leonora Rios de Souza; Campos, Marcela de Carvalho; Siqueira, Pedro Henrique Vieira Martins de; Silva, Luciano; Ricart, Carlos André Ornelas; Martins, Pedro Alves; Queiroz, Rayner Myr Lautherjung; Filho, Edivaldo Ximenes Ferreira

doi:10.1016/j.fgb.2013.07.006

Cited by 43 publications

(9 citation statements)

References 32 publications

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“…Brazil is the second biggest producer of soybean worldwide, harvesting 96.5 kton in 2016, just behind United States, with 106.9 kton in 2016 [ 10 , 11 ]. Therefore, soybean residues represent the major byproduct of processing soybean industry [ 12 ], which could be used as a carbon source for the production of enzymes [ 13 ].…”

Section: Introductionmentioning

confidence: 99%

Optimization of Xylanase Production from Aspergillus foetidus in Soybean Residue

et al. 2018

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Enzymatic hydrolysis is an important but expensive step in the process to obtain enzyme derived products. Thus, the production of efficient enzymes is of great interest for this biotechnological application. The production of xylanase by Aspergillus foetidus in soybean residues was optimized using 2 × 23 factorial designs. The experimental data was fitted into a polynomial model for xylanase activity. Statistical analyses of the results showed that variables pH and the interaction of pH and temperature had influenced the production of xylanase, with the best xylanase production level (13.98 U/mL) occurring at fermentation for 168 hours, pH 7.0, 28°C, and 120 rpm.

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Section: Introductionmentioning

confidence: 99%

Optimization of Xylanase Production from Aspergillus foetidus in Soybean Residue

et al. 2018

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“…With previous purification and characterization in A. terreus ( Soni et al, 2016 ), here we observed four CAZyme-encoding DEGs associated with degradation of these polysaccharides. Whilst the pectin content in SB and SH is considerably lower than for hollocellulose ( de Souza Moreira et al, 2013 ; Li et al, 2017 ), evidence was also observed for pectin degradation on both, with considerable exclusive up-regulation of genes on SH likely reflecting differences in pectin content between the different carbon sources. Up-regulation of genes related to pectinolytic activity have also been reported previously on SB for A. niger (PL4 family), A. fumigatus (PL4 family) and for A. tamarii (PL1, PL9, GH28 families) ( Borin et al, 2017 ; de Gouvêa et al, 2018 ; Midorikawa et al, 2018 ).…”

Section: Discussionmentioning

confidence: 92%

“…related to biomass degradation comprise CreA (carbon catabolite repression), within the Cys2His2 class and the HAP complex (Cazy regulation), within the CBF class ( Benocci et al, 2017 and references therein). Whilst mechanisms for regulation of expression of sugar transporter genes during sugar utilization in fungi is only partially understood at present, a number of the above transcription factors, such as XlnR, CreA, ClrA/ClrB, GalX and AraR, are also known to regulate sugar transporter genes in model Aspergillus species (e. g. Vankuyk et al, 2004 ; Andersen et al, 2008 ; de Souza Moreira et al, 2013 ). Our data revealed considerable numbers of transcription factor genes with significant differential expression on SB and/or SH at a probability level of p ≤ 0.01, with 15 at log2 fold change (FC) at least ≥2-fold and 84 at log2 fold change (FC) <2-fold.…”

Section: Discussionmentioning

confidence: 99%

“…In this study, we examine differential expression of CAZyme-encoding genes through transcriptome profiling of A. terreus strain BLU24 after growth on sugarcane bagasse and soybean hulls, which are both considered promising lignocellulosic substrates for biorefinery applications, in terms of the high concentration of carbohydrates that can be converted into fermentable sugar residues ( Cheng and Zhu, 2013 ). This fungal strain has previously been reported to efficiently secrete xylanases on lignocellulosic biomass residues ( de Souza Moreira et al, 2013 ). Increased understanding of plant cell wall degradation mechanisms will contribute to downstream rational engineering of improved microorganisms for efficient enzymatic degradation of agricultural plant biomass residues.…”

Section: Introductionmentioning

confidence: 99%

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Transcriptome Profiling-Based Analysis of Carbohydrate-Active Enzymes in Aspergillus terreus Involved in Plant Biomass Degradation

Corrêa

Midorikawa

Filho

et al. 2020

Front. Bioeng. Biotechnol.

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Given the global abundance of plant biomass residues, potential exists in biorefinery-based applications with lignocellulolytic fungi. Frequently isolated from agricultural cellulosic materials, Aspergillus terreus is a fungus efficient in secretion of commercial enzymes such as cellulases, xylanases and phytases. In the context of biomass saccharification, lignocellulolytic enzyme secretion was analyzed in a strain of A. terreus following liquid culture with sugarcane bagasse (SB) (1% w/v ) and soybean hulls (SH) (1% w/v ) as sole carbon source, in comparison to glucose (G) (1% w/v ). Analysis of the fungal secretome revealed a maximum of 1.017 UI.mL –1 xylanases after growth in minimal medium with SB, and 1.019 UI.mL –1 after incubation with SH as carbon source. The fungal transcriptome was characterized on SB and SH, with gene expression examined in comparison to equivalent growth on G as carbon source. Over 8000 genes were identified, including numerous encoding enzymes and transcription factors involved in the degradation of the plant cell wall, with significant expression modulation according to carbon source. Eighty-nine carbohydrate-active enzyme (CAZyme)-encoding genes were identified following growth on SB, of which 77 were differentially expressed. These comprised 78% glycoside hydrolases, 8% carbohydrate esterases, 2.5% polysaccharide lyases, and 11.5% auxiliary activities. Analysis of the glycoside hydrolase family revealed significant up-regulation for genes encoding 25 different GH family proteins, with predominance for families GH3, 5, 7, 10, and 43. For SH, from a total of 91 CAZyme-encoding genes, 83 were also significantly up-regulated in comparison to G. These comprised 80% glycoside hydrolases, 7% carbohydrate esterases, 5% polysaccharide lyases, 7% auxiliary activities (AA), and 1% glycosyltransferases. Similarly, within the glycoside hydrolases, significant up-regulation was observed for genes encoding 26 different GH family proteins, with predominance again for families GH3, 5, 10, 31, and 43. A. terreus is a promising species for production of enzymes involved in the degradation of plant biomass. Given that this fungus is also able to produce thermophilic enzymes, this first global analysis of the transcriptome following cultivation on lignocellulosic carbon sources offers considerable potential for the application of candidate genes in biorefinery applications.

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“…O ácido ferúlico já foi descrito como responsável tanto pelo aumento na atividade da xilanase (XylT2) de Aspergillus terreus (Moreira et al, 2013), quanto pela inibição de celulases comerciais da Novozyme que tem origem de diversos microrganismos (Tejirian e Xu, 2011 (Moreira et al, 2013), e não afetou a atividade de xilanase de CPP. Outra vantagem da amostra CPP, é que ela não teve alteração em suas atividades enzimáticas quando incubada com o ácido 4-hidroxibenzóico, enquanto que esse fenol só foi observado atuando de forma repressora em outras atividades celulolíticas de enzimas comerciais oriundas de diversos microrganismos, descritas anteriormente (Ximenes, 2010;Ximenes et al, 2010a;Tejirian e Xu, 2011).…”

Section: Efeito Dos Compostos Fenólicos Nas Atividades De Cmcases E Xunclassified

Identificação e caracterização do secretoma e celulossoma de um novo isolado de Clostridium thermocellum (B8) para a sacarificação de biomassas lignocelulósicas

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À minha orientadora, Professora Eliane Ferreira Noronha, por ter me acolhido desde a iniciação científica, e por todo apoio, conselhos, orientação e muita paciência durante esta jornada. Será sempre uma referência e um exemplo de profissional, obrigada por todos esses anos. À professora Nádia Skorupa Parachin, pelos conselhos e suporte. Obrigada por toda ajuda. À Elaine Nascimento, pela ajuda e amizade durante a pesquisa. Agradeço também por fazerem parte da minha banca de mestrado. Ao professor Carlos Roberto Félix, por ser um exemplo de profissional com um coração enorme. Aos professores Edivaldo Ximenes, Ricardo Krüger e Tatsuya Nagata, pelo conhecimento compartilhado. Às técnicas mais animadas e divertidas, Marísia e Margarete, por toda amizade, carinho e cafés. À Jackeline Leite, por todos os ensinamentos e principalmente pela grande amizade. À Brenda Camargo por ter sido uma grande amiga, e que deu força em grande parte dos experimentos deste trabalho. À Rachel Satomi, que estagiou comigo e me ajudou em vários experimentos, deixando eles mais divertidos. Às amizades que fiz no laboratório, obrigada a todos da enzimologia. Cada um de vocês contribuiu de alguma forma para minha dissertação e crescimento pessoal, seja com um conselho, tirando dúvidas, ou até mesmo pela companhia e amizade quando precisei. Agradeço por todos os momentos de confraternização, congressos, happy hours, e El Paso juntos. À Leonora e a Débora, por terem me ajudado no experimento de HPLC e à Mary-Ann e Amanda pela ajuda no DLS. Ao meu companheiro e melhor amigo Caio, que acompanhou de perto desde a minha entrada na UnB até este momento. Seu amor e cuidado foram essenciais para que eu chegasse até aqui, te amo. Aos meus amigos Raul, Mila e Fernando Hiro, vocês são pra vida toda. Aos meus amigos biólogos, Thaís, Tamara, Thales e Ana. Sem vocês eu não seria a mesma bióloga, vocês fazem parte de tudo isso e me ajudaram a manter o sorriso mesmo nas situações mais difíceis. Agradeço em especial à minha família, por serem à base de tudo. ♥ iv APOIO FINANCEIRO Este projeto foi realizado por meio do apoio financeiro das agências de fomento CNPq (Conselho Nacional de Desenvolvimento), FAPDF (Fundação de Apoio à Pesquisa do Distrito Federal) e com a concessão de bolsa de estudos fornecida pela CAPES (Coordenação de Aperfeiçoamento de Pessoal de Nível Superior). v RESUMO O presente trabalho tem como propósito a purificação de celulossomas, sua caracterização e do secretoma de um novo isolado de Clostridium thermocellum B8, obtido do rúmen de caprino. Para obtenção das amostras proteicas C. thermocellum foi cultivada em meio líquido contendo celulose como fonte de carbono. O secretoma que constitui a amostra de Proteínas Ligadas á Celulose (PLC) foi eluído a partir da celulose residual da cultura. As frações cromatográficas do principal pico de proteína resultante do fracionamento da amostra PLC em uma cromatografia de exclusão molecular (Superdex S-200) compõe a amostra de Celulossomas Parcialmente Purificados (CPP). Ambas as amostras apresentara...

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Two β-xylanases from Aspergillus terreus: Characterization and influence of phenolic compounds on xylanase activity

Cited by 43 publications

References 32 publications

Optimization of Xylanase Production from Aspergillus foetidus in Soybean Residue

Optimization of Xylanase Production from Aspergillus foetidus in Soybean Residue

Transcriptome Profiling-Based Analysis of Carbohydrate-Active Enzymes in Aspergillus terreus Involved in Plant Biomass Degradation

Identificação e caracterização do secretoma e celulossoma de um novo isolado de Clostridium thermocellum (B8) para a sacarificação de biomassas lignocelulósicas

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