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Applied and Environmental Microbiology, June 1999, p. 2794-2797, Vol. 65, No. 6
Department of Genetics and Biology of
Microorganisms1 and Department of
Organic and Industrial Chemistry,2
University of Milan, 20133 Milan, Italy
Received 28 December 1998/Accepted 26 March 1999
We developed a biocatalyst by cloning the styrene monooxygenase
genes (styA and styB) from Pseudomonas
fluorescens ST responsible for the oxidation of styrene to its
corresponding epoxide. Recombinant Escherichia coli was
able to oxidize different aryl vinyl and aryl ethenyl compounds to
their corresponding optically pure epoxides. The results of
bioconversions indicate the broad substrate preference of styrene
monooxygenase and its potential for the production of several fine chemicals.
Very few bacteria of the genus
Pseudomonas that are able to degrade styrene have been
studied (1, 9, 13, 17). Styrene degradation can occur
through two different routes: the first involves the oxidation of the
side chain and the second involves the oxidation of the aromatic ring
(3, 12, 15, 16). Recently, we localized and characterized
the genes responsible for the oxidation of styrene to phenylacetic acid
in Pseudomonas fluorescens ST. Sequence analysis and
biotransformation experiments allowed the identification of the
functions of the styA and styB genes, which encode the styrene monooxygenase responsible for the formation of
styrene oxide (1). In addition, we have verified that the product was (S)-styrene oxide in optically pure form. This
outcome has stimulated our interest in the development of a biocatalyst for the production of different chiral epoxides, whose formation is
interesting since they are valuable building blocks in the manufacture
of optically active compounds (4).
Biocatalyst construction.
In order to design a biocatalyst for
the production of optically pure epoxides, the 3.0-kb
PstI-EcoRI region identified from the genomic
library of P. fluorescens ST and cloned in pTZ19R, leading
to pTPE30, was investigated (1, 9). We amplified by PCR a
fragment of plasmid pTPE30 spanning the region from nucleotide 39 upstream to nucleotide 1947 downstream of styA and
styB, which encode styrene monooxygenase, using the
synthetic oligonucleotides OLI1 (5'-TTTCCTTTTTTGCTGCTGGTC-3')
and OLI2 (5'-TTTTGTTGTTTTGTTCGTTGC-3'). The 1.9-kb
amplified fragment was cloned in the pTZ18R vector, yielding plasmid
pTAB19. Then, we transformed Escherichia coli JM109 with
pTAB19 carrying the styA and styB genes, which
led to the recombinant strain JM109(pTAB19), which was used for the bioconversion of different substrates.
Biotransformation products obtained with styrene monooxygenase
of P. fluorescens ST.
To investigate the substrate
preference of the enzyme, biotransformation experiments were performed
with different substrates. Cells of E. coli
JM109(pTAB19) were grown with shaking at 37°C on mineral medium
(M9) supplemented with 20 mM glucose, 1 mM thiamine, and 200 µg of
ampicillin per ml. When the culture reached an
A600 of 0.5, transcription from the
lacZ promoter was induced by addition of
isopropyl-
0099-2240/99/$04.00+0
Copyright © 1999, American Society for Microbiology. All rights reserved.
A New Biocatalyst for Production of Optically Pure Aryl Epoxides
by Styrene Monooxygenase from Pseudomonas fluorescens
ST
ABSTRACT
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-D-thiogalactopyranoside (IPTG) to a final
concentration of 1 mM. Then, cells were harvested and resuspended to an
A600 of 2.0 in 50 mM sodium phosphate buffer (pH
6.8) containing 20 mM glucose. Cell suspensions (100 ml in 500-ml
flasks) were incubated at 30°C on a rotary shaker in the presence of
the substrates, supplied at 0.5 g/liter. After 4 h, the culture
samples were extracted with three equal amounts of ethyl acetate. The
solvent was evaporated under vacuum, unless volatile compounds were
extracted, in which case the solvent was evaporated at atmospheric
pressure. Compounds were then purified by standard chromatography on
silica gel with a hexane-ethyl acetate mixture (50:50).
TABLE 1.
NMR characteristics and optical activities of bioproducts
obtained with styrene monooxygenase from P. fluorescens
ST
Identification and characterization of the epoxides.
From the
biotransformation experiments we obtained five epoxides: 1A, 2A, 4A,
5A, and 6A (Table 1). They are all known compounds, and their
identification was made by comparison. Where possible, more nuclear
magnetic resonance (NMR) data have been added. Optical purity was
measured by two means: by comparison of [
]D values with reported values and by use of a chiral-phase high-performance liquid chromatography (HPLC) column (CHIRALCEL OD-H). All the epoxides
seemed to be optically pure, and the known epoxides also had the
expected absolute configuration. These data in addition to the already
determined optical purity of the styrene oxide confirm the geometric
selectivity of the enzyme.
Identification and characterization of the 1,2-diols.
The only
by-products obtained from the epoxides were the hydrolyzed products.
These were 1,2-diols, and they represented trace by-products from
the bioconversions of compounds 4, 5, and 6; however, they were the
only isolated products for compounds 3 and 7. Compound 8 showed trace
amounts only of the diol. The optical purity depended on the substrate,
and results demonstrated that hydrolysis is not stereoselective. In
fact, both with purified products, with which a comparison with
published []D values was possible (products 3B and
6B), and with an unpurified mixture (product 4B), with which the only
data came from chiral HPLC, the diols were always optically impure, but
the purity level varied from 20% (product 3B) to 40% (product 6B).
Conclusions. The reaction products obtained in bioconversion experiments performed with a recombinant strain producing styrene monooxygenase from aryl ethenyl compounds can be grouped into epoxides and hydrolyzed products. All the epoxides were optically pure and had the same absolute configuration. The epoxide yields depended on the structure characteristics; in particular, they were high for acyclic compounds without electron withdrawing groups. In two cases (Table 1, substrates 3 and 7) the only products were the 1,2-diols and they did not maintain the optical purity predicted for the epoxide intermediates.
In this work we have demonstrated that E. coli JM109(pTAB19) carrying styrene monooxygenase genes cloned from P. fluorescens ST converts aryl ethenyl compounds to the corresponding epoxides in optically pure forms and with good yields. Thus, the engineered E. coli strain shows great promise as an efficient biocatalyst for the production of important chiral building blocks.| |
ACKNOWLEDGMENTS |
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This work was supported by grants from the CNR, MURST-CNR
Biotechnology Program L.95/95, and the MURST Research Program of National Relevance
1997.
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FOOTNOTES |
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* Corresponding author. Mailing address: Department of Genetics and Biology of Microorganisms, University of Milan, Via Celoria 26, 20133 Milan, Italy. Phone: 39-2-26605227. Fax: 39-2-2664551. E-mail: Bestetti{at}imiucca.csi.unimi.it.
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Applied and Environmental Microbiology, June 1999, p. 2794-2797, Vol. 65, No. 6
0099-2240/99/$04.00+0
Copyright © 1999, American Society for Microbiology. All rights reserved.
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