Isolated enzymes epoxidation

Another very recent development in the field of enzymatic domino reactions is a biocatalytic hydrogen-transfer reduction of halo ketones into enantiopure epoxides, which has been developed by Faber, Bornscheuer and Kroutil. Interestingly, the reaction was carried out with whole lyophilized microbial cells at pH ca. 13. Investigations using isolated enzymes were not successful, as they lost their activity under these conditions [26]. 

Based on knowledge of a biosynthetic pathway one can select certain steps which could be of interest for bioconversion of (a) readily available precursor(s). This could, for example, be stereospecific reactions, like the reduction of quinidinone in quinine or quinidine and the epoxidation of atropine to scopolamine. For the bioconversion one can consider using plant cells [e.g., the production of L-dopa from tyrosine by immobilized cells of Mucuna pruriens (10)] or isolated enzymes from the plant itself. An interesting example of the latter is the (5)-tetrahydroprotoberberine oxidase (STOX) enzyme, which oxidizes (5)-reticuline but not its stereoisomer (11). This feature can be used in the production of (i )-reticuline from a racemic mixture (see below). Immobilized strictosidine synthase has been successfully used to couple secologanin and tryptamine. The gene for this enzyme has been isolated from Rauvolfia (6) and cloned in Escherichia coli, in which it is expressed, resulting in the biosynthesis of active enzyme (7). The cultured bacteria produced 20 times more enzyme... 

The maximum aetivity of the isolated enzyme was observed at 30 °C and pH 6.5 in a buffer system with 5% (v/v) DMSO as a eosolvent. The enzyme was very stable at pH 7.5 and retained full activity after ineubation at 40 °C for 6 h. Interestingly, when the eosolvent DMSO was replaced by an emulsifier (Tween-80, 0.5% w/v) as an alternative modulator to disperse the water-in-soluble substrate, the apparent activity of the epoxide hydrolase significantly increased by 1.8-fold, while the optimum temperature shifted from 30 to 40 °C and the half-life of the enzyme at 50 °C increased by 2.5 times (Figure 2.5). The enzymatic hydrolysis of rac-PGE was highly enantioselective, with an B-value (enantiomeric ratio) of 69.3 in the Tween-80 emulsion system, which is obviously superior than that (41.2) observed in the DMSO-modulated system. ... 

Biocatalytic asymmetric epoxidation of alkenes catalyzed by monooxygenases cannot be performed on a preparative scale with isolated enzymes due to their complex nature and their dependence on a redox cofactor, such as NAD(P)H. Thus, whole microbial cells are used instead. Although the toxic effects of the epoxide formed, and its further (undesired) metabolism by the cells catalyzed by epoxide hydrolases (Sect. 2.1.5), can be reduced by employing biphasic media, this method is not trivial and requires bioengineering skills [1151]. Alternatively, the aUcene itself can constitute the organic phase into which the product is removed, away from the cells. However, the bulk apolar phase tends to damage the cell membranes, which reduces and eventually abolishes all enzyme activity [1152]. 

Nucleophilic. In view of the ability of epoxides to become hydrated to the diol under aqueous alkaline conditions, the analogous addition of water to epoxides by enzymes will be considered in this section. The en mes responsible for epoxide hydration (epoxide hydrases) in animal liver systems have been purified, assayed using [7- H]styrene oxide,and tested for substrate and inhibitor -ass specificity. The current interest in these epoxide hydrases is mainly due to their close association with aryl monooxygenase enzymes and thus the total metabolism of olefinic and arene substrates via epoxides) in animals. The isolation of the antibacterial compounds aeroplysinin-1 (358) and aeroplysinin-2 (359) from the sponge Verongia aerophoba might be explained by the initial enzymatic formation of the unstable arene oxide (357), which can subsequently be hydrated by an epoxide hydrase enzyme, to form what the authors consider... 

The isolated enzyme chloroperoxidase from Caldariomyces fumago is reported to perform stereoselective epoxidation reactions and in one example, oxidation of a-meth-... 

It was recently reported that. >97% of BaP 4,5-epoxide metabolically formed from the metabolism of BaP in a reconstituted enzyme system containing purified cytochrome P-450c (P-448) is the 4S,5R enantiomer (24). The epoxide was determined by formation, separation and quantification of the diastereomeric trans-addition products of glutathione. Recently a BaP 4,5-epoxide was isolated from a metabolite mixture obtained from the metabolism of BaP by liver microsomes from 3-methylcholanthrene-treated Sprague-Dawley rats in the presence of the epoxide hydrolase inhibitor 3,3,3-trichloropropylene oxide, and was found to contain a 4S,5R/4R,5S enantiomer ratio of 94 6 (Chiu et. al., unpublished results). However, the content of the 4S,5R enantiomer was <60% when liver microsomes from untreated and phenobarbital-treated rats were used as the enzyme sources. Because BaP 4R,5S-epoxide is also hydrated predominantly to 4R,5R-dihydro-... 

As with an isolated double bond, epoxide formation in an aromatic ring, i.e., arene oxide formation, can occur mechanistically either by a concerted addition of oxene to form the arene oxide in a single step, pathway 1, or by a stepwise process, pathway 2 (Fig. 4.78). The stepwise process, pathway 2, would involve the initial addition of enzyme-bound Fe03+ to a specific carbon to form a tetrahedral intermediate, electron transfer from the aryl group to heme to form a carbonium ion adjacent to the oxygen adduct followed by... 

In contrast, a number of alkene epoxides (10.3) are chemically quite stable, i.e., intrinsically less reactive than arene oxides. Examples of epoxide metabolites that have proven to be stable enough to be isolated in the absence of degrading enzymes include 1,2-epoxyoctane (10.4), 1,2-epoxycyclohex-ane (10.5), 1-phenyl-1,2-epoxy ethane (styrene oxide, 10.6), and cis- 1,2-diphenyl-1,2-epoxyethane (cfv-stilbene oxide, 10.7) [12], The same is true of alclofenac epoxide (10.8), hexobarbital epoxide (10.9), and a few other epoxides of bioactive compounds. 

As explained in the Introduction, alkene oxides (10.3) are generally chemically quite stable, indicating reduced reactivity compared to arene oxides. Under physiologically relevant conditions, they have little capacity to undergo rearrangement reactions, one exception being the acid-catalyzed 1,2-shift of a proton observed in some olefin epoxides (see Sect. 10.2.1 and Fig. 10.3). Alkene oxides are also resistant to uncatalyzed hydration, thus, in the absence of hydrolases enzymes, many alkene oxides that are formed as metabolites are stable enough to be isolated. 

In connection with our own work on the enzyme-catalysed hydrolysis of cyclohexene epoxide with various fungi we made the unexpected observation that the microorganism Corynesporia casssiicola DSM 62475 was able to interconvert the (1R,2R) and (1S,2S) enantiomers of the product, trans cyclohexan-1,2-dioI 25. As the reaction proceeded the (1R,2R) enantiomer was converted to the (1S,2S) enantiomer [20]. If the racemic trans diol 25 was incubated with the growing fungus over 5 days, optically pure (> 99 % e. e.) (1 S,2S) diol 25 could be isolated in 85% yield. Similarly biotransformation of cis (meso) cycIohexan-1,2-diol 26 yielded the (1S,2S) diol 25 in 41 % (unoptimized) yield (Scheme 11). 

Very recently, the purification and characterisation of an epoxide hydrolase, catalysing the conversion of limonene-1,2-epoxide to limonene-1,2-diol has been described [90]. The enzyme was isolated from Rhodococcus erythropolis DCL14 and is induced when the microorganism is grown on monoterpenes. The authors found evidence that the enzyme, limonene-1,2-epoxide hydrolase is the first member of a new class (the third class) of epoxide hydrolases [91]. 

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