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Rapid cultivation of stable aerobic phenol-degrading granules using acetate-fed granules as microbial seed |
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| Authors: | Tay Stephen Tiong-Lee Moy Benjamin Yan-Pui Jiang He-Long Tay Joo-Hwa |
| Affiliation: | aLaboratory of Enzyme Technology, Institute of Microbiology, Academy of Sciences of the Czech Republic, Vídeňská 1083, 142 20 Prague 4, Czech Republic bROQUETTE Microbiology and Genetic Department, Molecular Biology Laboratory, 62080 Lestrem Cedex, France |
| Abstract: | cDNA-encoding pyranose 2-oxidase (P2O) from Trametes pubescens was sequenced and cloned into Escherichia coli strain BL21/DE3 on a multicopy plasmid under the control of trc promoter. The synthesis of P2O was studied in a batch culture in M9-based mineral medium: the enzyme was synthesized constitutively at 28 °C in amount corresponding to 8% of the cell soluble protein (0.6 U mg−1). Only small portion of P2O (11%) was in the form of non-active inclusion bodies. Purified recombinant enzyme has similar physico-chemical and kinetic parameters with other P2Os. When compared to the expression of p2o of Trametes ochracea, a ratio of the mature enzyme to inclusion bodies found in the same E. coli host at 28 °C is as much as nine times higher. The finding makes the enzyme from T. pubescens preferable for the large-scale production by recombinant bacteria. The difference in amino acid sequences of the P2O from T. ochracea and T. pubescens may explain the favourable trait of the latter enzyme regarding protein folding. |
| Keywords: | Pyranose 2-oxidase Recombinant protein Inclusion bodies Heterologous expression |
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