High-throughput screening system based on phenolics-responsive transcription activator for directed evolution of organophosphate-degrading enzymes

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Synthetic organophosphates (OPs) have been used as nerve agents and pesticides due to their extreme toxicity and have caused serious environmental and human health problems. Hence, effective methods for detoxification and decontamination of OPs are of great significance. Here we constructed and used a high-throughput screening (HTS) system that was based on phenolics-responsive transcription activator for directed evolution of OP-degrading enzymes. In the screening system, phenolic compounds produced from substrates by OP-degrading enzymes bind a constitutively expressed transcription factor DmpR, initiating the expression of enhanced green fluorescent protein located at the downstream of the DmpR promoter. Fluorescence intensities of host cells are proportional to the levels of phenolic compounds, enabling the screening of OP-degrading enzymes with high catalytic activities by fluorescence-activated cell sorting. Methyl parathion hydrolase from Pseudomonas sp. WBC-3 and p-nitrophenyl diphenylphosphate were used as a model enzyme and an analogue of G-type nerve agents, respectively. The utility of the screening system was demonstrated by generating a triple mutant with a 100-fold higher k(cat)/K-m than the wild-type enzyme after three rounds of directed evolution. The contributions of individual mutations to the catalytic efficiency were elucidated by mutational and structural analyses. The DmpR-based screening system is expected to be widely used for developing OP-degrading enzymes with greater potential.
Publisher
OXFORD UNIV PRESS
Issue Date
2012-11
Language
English
Article Type
Article
Keywords

METHYL PARATHION HYDROLASE; ICE NUCLEATION PROTEIN; CELL-SURFACE DISPLAY; SP STRAIN CF600; NERVE AGENTS; SWISS-MODEL; BACTERIAL PHOSPHOTRIESTERASE; HYDROLYSIS; ENVIRONMENT; EXPRESSION

Citation

PROTEIN ENGINEERING DESIGN & SELECTION, v.25, no.11, pp.725 - 731

ISSN
1741-0126
DOI
10.1093/protein/gzs071
URI
http://hdl.handle.net/10203/102423
Appears in Collection
BS-Journal Papers(저널논문)
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