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大豆过氧化物酶对瑞佐尔翠蓝 G133 的氧化降解。

Oxidative degradation of Remazol Turquoise Blue G 133 by soybean peroxidase.

机构信息

Università degli Studi di Torino, Department of Chemistry I.F.M., Via P. Giuria 7, 10125 Torino, Italy.

出版信息

J Inorg Biochem. 2011 Feb;105(2):321-7. doi: 10.1016/j.jinorgbio.2010.11.009. Epub 2010 Nov 26.

Abstract

Reactive dyes are widely employed in textile industries and their removal from wastewaters is a relevant environmental problem. In addition to chemical and physical methods, several bioremediation approaches, involving intact micro-organisms or isolated enzymes, have been proposed to decolorize dye solutions. In this paper, we report the complete and fast decolourization of a Cu(II)-phthalocyanine based reactive dye (Remazol Turquoise Blue G 133) by means of the soybean peroxidase/H(2)O(2) system. The oxidative degradation of the dye in aqueous solution at 25°C was studied as function of pH, revealing a quantitative decolourization yield at acidic pH values with a maximum of activity at pH 3.3. The reaction products were identified and characterized by HPLC-diode array detector (DAD)-mass spectrometry (MS), ionic chromatography and EPR techniques. This analysis showed that the enzyme catalyses the breaking of the phthalocyanine ring producing sulfophthalimide as the main degradation product, and the release of stoichiometric amount of ammonium and Cu(II) ions.

摘要

活性染料广泛应用于纺织工业,其从废水中去除是一个相关的环境问题。除了化学和物理方法外,还提出了几种生物修复方法,包括完整的微生物或分离的酶,以对染料溶液进行脱色。在本文中,我们报告了大豆过氧化物酶/H(2)O(2)系统对基于 Cu(II)酞菁的活性染料(Remazol 翠蓝 G 133)的完全快速脱色。研究了在 25°C 下在水溶液中染料的氧化降解作为 pH 的函数,在酸性 pH 值下表现出定量的脱色率,在 pH 3.3 时具有最大的活性。通过高效液相色谱-二极管阵列检测器(DAD)-质谱(MS)、离子色谱和 EPR 技术对反应产物进行了鉴定和表征。该分析表明,该酶催化酞菁环的断裂,生成主要降解产物磺基邻苯二甲酰亚胺,并释放出化学计量的铵和 Cu(II)离子。

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