Enzyme-Based Organic Synthesis. Cheanyeh Cheng
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Название: Enzyme-Based Organic Synthesis
Автор: Cheanyeh Cheng
Издательство: John Wiley & Sons Limited
Жанр: Химия
isbn: 9781118995150
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The diversity of alkane oxygenases evolved in prokaryotes and eukaryotes has been strategically used in synthetic chemistry to catalyze the chemo‐, regio‐, and stereoselective oxygenation of alkanes and many other compounds for the production of useful alcohols, aldehydes, epoxides, and carboxylic acids [31]. In particular, cytochromes P450 are external monooxygenases that convert a broad variety of substrates and catalyze many interesting chemical reactions including the hydroxylation of hydrocarbons [32, 33]. As an example, cytochrome P450 BM3(CYP102A1) isolated from Bacillus megaterium catalyzes the hydroxylation of gaseous alkanes, such as methane, ethane, propane, and butane, and cyclohexane to corresponding primary alcohols and 2‐propanol and 2‐butanol together with a dummy substrate perfluorocarboxylic acids of different alkyl chain length (8–14 carbon atoms) [34]. The screening of the mutant library revealed that cytochrome P450 BM3 F87a/A328V mutant has the ability to effectively hydroxylate cyclooctane, cyclodecane, and cyclododecane to corresponding alcohols. Cytochrome P450 BM3 F87V/A328F mutant demonstrated the ability to hydroxylate acylic n‐octane to 2‐(R)‐octane with 46% e.e. and high regioselectivity of 92% [35]. For cytochrome P450 catalysis, the nicotinamide adenine dinucleotide cofactor in its reduced form (NADH or NADPH) is needed to provide the electrons necessary for the catalytic cycle. However, the transfer of electrons cannot be made directly and a cytochrome P450 reductase must be present to shuttle the electrons from NAD(P)H to the hydrolase domain (Figure 2.1). It was discovered that cytochrome P450 BM3 was the first natural self‐sufficient P450, which still makes it one of the most efficient cytochromes to date [36].
Medium‐chain alkanes (C5–C16) are usually oxidized by heme‐iron‐containing cytochrome P450 monooxygenases (P450s or CYPs) or by integral‐membrane non‐heme diiron monooxygenases (Alk B) [37, 38]. Alkane hydrolases of the CYP153A from Mycobacterium marinum (CYP153A16) and Polaromona sp. (CYP153A P. sp.) were examples to catalyze regioselectively ω‐hydrolation of C6–C11 alkanes, alkenes, cycloalkanes, and alicyclic compounds [39, 40]. The cloned and expressed CYP153A16 and CYP153A P. sp. monooxygenases were capable of performing the ω‐hydroxylation in vitro with C5–C12 alkanes and C6–C12 primary alcohols into their corresponding primary alcohols and α,ω‐diols [37]. However, a soluble three‐component diiron monooxygenase, butane monooxygenase (sBMO), has been purified from the gram‐negative β‐proteobacterium Pseudomonas butanovora (ATCC 43655), which was capable of hydroxylating C3–C6 linear and branched aliphatic alkanes (propane, butane, pentane, hexane, isobutene, and isopentane) at the terminal carbon atom mostly (≥80% regiospecificity) to produce primary alcohols with only small fractions of secondary and tertiary alcohols [41].
Figure 2.1 Hydroxylation of alkanes by cytochrome P450 monooxygenase (CYP).
Since long‐chain alkanes are more persistent in the environment than shorter alkanes, the degradation of long‐chain alkane is an important topic in synthetic chemistry for dealing with the crude oil contamination in environment. Enzymes used for the activation of alkanes with long chain length (≥C16) by hydroxylation have been found including yeast P450s [42], integral‐membrane monooxygenases (AlkM) [43], flavin‐containing alkane monooxygenases (LadA) [44], and dioxygenases [45]. It was acknowledged that thermophilic bacillus Geobacillus thermodenitrificans NG80‐2 degrades the long‐chain alkane (C15–C36) by utilizing a terminal oxidation pathway to convert long‐chain alkanes to their corresponding primary alcohols (Scheme 2.8). It is also found that LadA is the key initiating enzyme in the terminal oxidation pathway of G. thermodenitrificans NG80‐2 [46]. However, studies on the bacterial strain Acinetobacter venetianus 6A2 show that this bacterial strain can utilize n‐alkanes with chain lengths ranging from decane (C10H22) to tetracontane (C40H82) [47]. Two genes of the AlkB‐type alkane hydroxylase homologous, alkMa and alkMb, isolated from A. venetianus 6A2 were involved in the utilization of alkanes with chain lengths ranging from C10 to C18 implying that other enzyme(s) should be required for the utilization of C20‐C40 alkanes.
In addition to the notorious cytochrome P450 monooxygenase for alkane hydroxylation, a group of novel extracellular heme‐thiolate peroxygenases secreted by fungal Agrocybe aegerita have been demonstrated to catalyze efficiently the H2O2‐dependent hydroxylation of a variety of alkanes, which include linear, branched, and cyclic saturated hydrocarbons. As shown in Scheme 2.9, linear C3‐C16 alkanes can be hydroxylated at either 2‐ or 3‐positon of the carbon chain to yield corresponding secondary alcohols. For example, n‐propane and n‐butane were hydroxylated regioselectively to produce 2‐propanol and 2‐butanol, whereas n‐heptane and n‐octane were hydroxylated both stereoselectively and regioselectively to give 99.9% e.e. (R)‐enantiomer and the corresponding 3‐alcohol. Branched alkanes such as 2,3‐dimethylbutane were hydroxylated regioselectively to 2,3‐dimethylbutane‐2‐ol and isobutene was oxidized to 2‐methyl‐propan‐2‐ol. While cyclic alkanes of C5–C8 gave monohydroxylated products [48], there are also non‐heme enzymes that are capable of catalyzing the hydroxylation of alkanes [49]. Studies showed that non‐heme alkane hydroxylase involves high‐valent oxoiron moiety to catalyze the initial H abstraction from alkane followed by the rebound mechanism of FeOH/radical species. Examples are the enzyme taurine:α‐ketoglutarase dioxygenase (TauD) toward the cyclohexanol and cyclopentanol from cyclohexane and cyclopentane, respectively [50], and the diiron alkane monooxygenase of Pseudomonas oleovorans (AlkB) hydroxylates 2‐methyl‐1‐phenylcyclopropane to produce only 1‐phenyl‐3‐buten‐1‐ol and norcarane to produce approximately 85% cis‐ and trans‐2‐norcaranol [51].
Scheme 2.8 Terminal hydroxylation of long‐chain alkanes by LadA.
Scheme 2.9 Hydroxylation of alkanes by fungal peroxygenase.
2.1.3 Hydroxylation of Aromatic Compounds
Oxidative enzymes performing the introduction of one or two oxygen atoms on aromatic compounds is important in industrial applications [52, 53]. The four classes of enzyme: oxygenases, hydroxylases, peroxidases, and laccases are the most representative enzymes to perform the hydroxylation of aromatic compounds. The four classes of oxidative СКАЧАТЬ