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박성훈

Park, Sunghoon
Biochemical Engineering Lab.
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Development of recombinant Pseudomonas putida containing homologous styrene monooxygenase genes for the production of (S)-styrene oxide

Author(s)
Bae, Jong WanHan, Jul HeePark, Mi SoLee, Sun-GuLee, Eun YeolJeong, Yong JooPark, Sunghoon
Issued Date
2006-11
DOI
10.1007/BF02932079
URI
https://scholarworks.unist.ac.kr/handle/201301/25368
Fulltext
https://link.springer.com/article/10.1007/BF02932079
Citation
BIOTECHNOLOGY AND BIOPROCESS ENGINEERING, v.11, no.6, pp.530 - 537
Abstract
Recently isolated, Pseudomonas putida SN1 grows on styrene as its sole carbon and energy source through successive oxidation of styrene by styrene monooxygenase (SMO), styrene oxide isomerase (SOI), and phenylacetaldehyde dehydrogenase. For the production of (S)styrene oxide, two knockout mutants of SN1 were constructed, one lacking SOI and another lacking both SMO and SOL These mutants were developed into whole-cell biocatalysts by transformation with a multicopy plasmid vector containing SMO genes (styAB) of the SN1. Neither of these self-cloned recombinants could grow on styrene, but both converted styrene into an enantiopure (S)-styrene oxide (e.e. > 99%). Whole-cell SMO activity was higher in the recombinant constructed from the SOI-deleted mutant (130 U/g cdw) than in the other one (35 U/g cdw). However, the SMO activity of the former was about the same as that of the SOI-deleted SN1 possessing a single copy of the styAB gene that was used as host. This indicates that the copy number of styAB genes is not rate-limiting on SMO catalysis by whole-cell SN1.
Publisher
KOREAN SOC BIOTECHNOLOGY & BIOENGINEERING
ISSN
1226-8372
Keyword (Author)
styrene monooxygenase(S)-styrene oxidewhole-cell biocatalystPseudomonas putida SN1styABC-deleted mutantself-cloning
Keyword
WHOLE-CELL BIOCATALYSTMETHYLOSINUS-TRICHOSPORIUMEPOXIDE HYDROLASEORGANIC-SOLVENTSSTRAIN VLB120DEGRADATIONMECHANISMSRESISTANCEMETHANECA-3

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