Molecular cloning of a copper-dependent laccase from the dye-decolorizing strain Stenotrophomonas maltophilia AAP56

Galai, Said; Lucas-Elı́o, Patricia; Marzouki, M. Néjib; Sánchez-Amat, Antonio

doi:10.1111/j.1365-2672.2011.05164.x

Cited by 20 publications

(26 citation statements)

References 47 publications

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“…In the case of the E. coli cuprous oxidase CueO it was suggested that the methionines are involved in binding cuprous oxide atoms which are oxidized by the enzyme [25]. For other enzymes it was suggested that copper binding at methionine-rich regions results in a conformational change required for the entry and oxidation of organic substrates [26], [27]. The question of whether these MCOs can be considered LMCOs or constitute a separate class of MCOs remains still open and may be solved by more closely at their substrate spectrum.…”

Section: Resultsmentioning

confidence: 99%

Laccase versus Laccase-Like Multi-Copper Oxidase: A Comparative Study of Similar Enzymes with Diverse Substrate Spectra

et al. 2013

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Laccases (EC 1.10.3.2) are multi-copper oxidases that catalyse the one-electron oxidation of a broad range of compounds including substituted phenols, arylamines and aromatic thiols to the corresponding radicals. Owing to their broad substrate range, copper-containing laccases are versatile biocatalysts, capable of oxidizing numerous natural and non-natural industry-relevant compounds, with water as the sole by-product. In the present study, 10 of the 11 multi-copper oxidases, hitherto considered to be laccases, from fungi, plant and bacterial origin were compared. A substrate screen of 91 natural and non-natural compounds was recorded and revealed a fairly broad but distinctive substrate spectrum amongst the enzymes. Even though the enzymes share conserved active site residues we found that the substrate ranges of the individual enzymes varied considerably. The EC classification is based on the type of chemical reaction performed and the actual name of the enzyme often refers to the physiological substrate. However, for the enzymes studied in this work such classification is not feasible, even more so as their prime substrates or natural functions are mainly unknown. The classification of multi-copper oxidases assigned as laccases remains a challenge. For the sake of simplicity we propose to introduce the term “laccase-like multi-copper oxidase” (LMCO) in addition to the term laccase that we use exclusively for the enzyme originally identified from the sap of the lacquer tree Rhus vernicifera.

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Section: Resultsmentioning

confidence: 99%

Laccase versus Laccase-Like Multi-Copper Oxidase: A Comparative Study of Similar Enzymes with Diverse Substrate Spectra

et al. 2013

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“…Previous results with Syringaldazine as substrate also showed that phosphate buffer pH 7.0 is the optimal for SmLac . These results and other media studies, show that phosphate buffer is a convenient one for SmLac activity towards a wide range of substrates …”

Section: Resultsmentioning

confidence: 92%

“…Laccase was obtained from a copper induced 24 h culture of S. maltophilia AAP56 by sonication of harvested bacterial cells . The crude extract obtained was concentrated approximately 3‐fold in two steps: ammonium sulphate precipitation (80%) and ultrafiltration.…”

Section: Resultsmentioning

confidence: 95%

“…Purification and biochemical characterization of SmLac Laccase was obtained from a copper induced 24 h culture of S. maltophilia AAP56 by sonication of harvested bacterial cells. 15 The crude extract obtained was concentrated approximately 3-fold in two steps: ammonium sulphate precipitation (80%) and ultrafiltration. The strong yellow colour characterizing the enzymatic extract was eliminated by the gel filtration chromatography step, the purification rate was determined as 21% from crude laccase enzyme.…”

Section: Resultsmentioning

confidence: 99%

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Characterization of yellow bacterial laccase SmLac/role of redox mediators in azo dye decolorization

Galai

Korri-Youssoufi

Marzouki

2013

J of Chemical Tech & Biotech

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BACKGROUND: The bacterial Stenotrophomonas maltophilia AAP56 laccase (SmLac) has been purified from cell extracts and its spectral and kinetic properties studied. It shows a high decolorization rate (99%) of the diazoic dye Reactive Black 5 (RB5) in the presence of redox mediators such as ABTS (2,2 -azino-bis(3-ethylbenzthiazoline-6-sulfonic acid), ASGN (Acetosyringone), SGA (Syringaldehyde) and HOBT (1-Hydroxy-Benzotriazole). The optimal pH has been determined as neutral or basic compatible with textile wastewater pH for further treatment application.

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“…R. pickettii is capable of degrading 2,4,6-trichlorophenol and chlorobenzene Hatta et al, 2012). S. maltophilia exhibits laccase activity and therefore it is able to degrade dye compounds (Galai et al, 2011). Stenotrophomonas sp.…”

Section: Figmentioning

confidence: 99%

Combination of photoreactor and packed bed bioreactor for the removal of ethyl violet from wastewater

2014

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Molecular cloning of a copper-dependent laccase from the dye-decolorizing strain Stenotrophomonas maltophilia AAP56

Cited by 20 publications

References 47 publications

Laccase versus Laccase-Like Multi-Copper Oxidase: A Comparative Study of Similar Enzymes with Diverse Substrate Spectra

Laccase versus Laccase-Like Multi-Copper Oxidase: A Comparative Study of Similar Enzymes with Diverse Substrate Spectra

Characterization of yellow bacterial laccase SmLac/role of redox mediators in azo dye decolorization

Combination of photoreactor and packed bed bioreactor for the removal of ethyl violet from wastewater

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