Expression of esterase gene in yeast for organophosphates biodegradation |
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Authors: | Devaiah M. Kambiranda Kye Man Cho Young Han Lee Han Dae Yun |
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Affiliation: | a Division of Applied Life Science (BK21 Program) and Research Institute of Agriculture and Life Science, Gyeongsang National University, Chinju 660-701, Republic of Korea b Department of Food Science, Jinju National University, Chinju 660-758, Republic of Korea c Division of Plant Environmental Research, Gyeongsangnam-do Agricultural Research and Extension Service, Chinju 660-360, Republic of Korea d Department of Agricultural Chemistry, Sunchon National University, Suncheon 540-742, Republic of Korea |
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Abstract: | Organophosphates are esters of phosphoric acid and can be hydrolyzed and detoxified by carboxylesterase and phosphotriesterase. In this work esterase enzyme (Est5S) was expressed in yeast to demonstrate the organophosphorus hydrolytic activity from a metagenomic library of cow rumen bacteria. The esterase gene (est5S) is 1098 bp in length, encoding a protein of 366 amino acid residues with a molecular weight of 40 kDa. Est5S enzyme was successfully produced by Pichia pastoris at a high expression level of approximately 4.0 g L−1. With p-nitrophenol butyrate as the substrate, the optimal temperature and pH for enzyme activity were determined to be 40 °C and pH 7.0, respectively. The esterase enzyme was tested for degradation of chlorpyrifos (CP). TLC results obtained inferred that CP could be degraded by esterase enzyme (Est5S) and HPLC results revealed that CP could be efficiently degraded up to 100 ppm. Cadusafos (CS), coumaphos (CM), diazinon (DZ) dyfonate (DF), ethoprophos (EP), fenamiphos (FM), methylparathion (MPT), and parathion (PT) were also degraded up to 68, 60, 80, 40, 45, 60, 95, and 100%, respectively, when used as a substrate with Est5S protein. The results highlight the potential use of this enzyme in the cleanup of contaminated insecticides. |
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Keywords: | Rumen metagenome est5S gene Esterase Yeast expression OP degradation |
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