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使用响应面法优化用于木质素分解酶生产和合成染料脱色的培养基。

Optimization of a culture medium for ligninolytic enzyme production and synthetic dye decolorization using response surface methodology.

作者信息

Trupkin S, Levin L, Forchiassin F, Viale A

机构信息

Micología Experimental, Universidad de Buenos Aires, Dpto. de Biodiversidad y Biología Experimental, Fac. de Cs. Exactas y Naturales, 1428 Capital Federal, Argentina.

出版信息

J Ind Microbiol Biotechnol. 2003 Dec;30(12):682-90. doi: 10.1007/s10295-003-0099-0. Epub 2003 Nov 29.

Abstract

A Box-Wilson central composite design was applied to optimize copper, veratryl alcohol and l-asparagine concentrations for Trametes trogii (BAFC 212) ligninolytic enzyme production in submerged fermentation. Decolorization of different dyes (xylidine, malachite green, and anthraquinone blue) by the ligninolytic fluids from the cultures was compared. The addition of copper stimulated laccase and glyoxal oxidase production, but this response was influenced by the medium N-concentration, with improvement higher at low N-levels. The medium that supported the highest ligninolytic production (22.75 U/ml laccase, 0.34 U/ml manganese peroxidase, and 0.20 U/ml glyoxal oxidase) also showed the greatest ability to decolorize the dyes. Only glyoxal oxidase activity limited biodecoloration efficiency, suggesting the involvement of peroxidases in the process. The addition of 1-hydroxybenzotriazole (a known laccase mediator) to the ligninolytic fluids increased both their range and rate of decolorization. The cell-free supernatant did not decolorize xylidine, poly R-478, azure B, and malachite green as efficiently as the whole broth, but results were similar in the case of indigo carmine and remazol brilliant blue R. This indicates that the mycelial biomass may supply other intracellular or mycelial-bound enzymes, or factors necessary for the catalytic cycle of the enzymes. It also implies that this fungus implements different strategies to degrade dyes with diverse chemical structures.

摘要

采用Box-Wilson中心复合设计优化了铜、藜芦醇和L-天冬酰胺的浓度,以提高栓菌(BAFC 212)在深层发酵中木质素分解酶的产量。比较了不同染料(二甲苯胺、孔雀石绿和蒽醌蓝)被培养物中木质素分解液脱色的情况。添加铜刺激了漆酶和乙二醛氧化酶的产生,但这种反应受培养基氮浓度的影响,在低氮水平下提高幅度更大。支持最高木质素分解产量的培养基(22.75 U/ml漆酶、0.34 U/ml锰过氧化物酶和0.20 U/ml乙二醛氧化酶)也表现出最大的染料脱色能力。只有乙二醛氧化酶活性限制了生物脱色效率,这表明过氧化物酶参与了该过程。向木质素分解液中添加1-羟基苯并三唑(一种已知的漆酶介体)增加了其脱色范围和速率。无细胞上清液对二甲苯胺、聚R-478、天青B和孔雀石绿的脱色效率不如全发酵液,但靛蓝胭脂红和活性艳蓝R的情况结果相似。这表明菌丝体生物质可能提供其他细胞内或与菌丝体结合的酶,或酶催化循环所需的因子。这也意味着这种真菌采用不同的策略来降解具有不同化学结构的染料。

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