Flavin
HomeHome > News > Flavin

Flavin

Jun 07, 2023

Nature Communications volume 13, Article number: 4896 (2022) Cite this article

5104 Accesses

5 Citations

22 Altmetric

Metrics details

Epoxide ring opening reactions are common and important in both biological processes and synthetic applications and can be catalyzed in a non-redox manner by epoxide hydrolases or reductively by oxidoreductases. Here we report that fluostatins (FSTs), a family of atypical angucyclines with a benzofluorene core, can undergo nonenzyme-catalyzed epoxide ring opening reactions in the presence of flavin adenine dinucleotide (FAD) and nicotinamide adenine dinucleotide (NADH). The 2,3-epoxide ring in FST C is shown to open reductively via a putative enol intermediate, or oxidatively via a peroxylated intermediate with molecular oxygen as the oxidant. These reactions lead to multiple products with different redox states that possess a single hydroxyl group at C-2, a 2,3-vicinal diol, a contracted five-membered A-ring, or an expanded seven-membered A-ring. Similar reactions also take place in both natural products and other organic compounds harboring an epoxide adjacent to a carbonyl group that is conjugated to an aromatic moiety. Our findings extend the repertoire of known flavin chemistry that may provide new and useful tools for organic synthesis.

Epoxides are important building blocks in organic synthesis and biosynthesis1,2. Due to the significant strain of the three-membered oxirane ring and polarized oxygen-carbon bonds, epoxides can readily undergo regioselective and stereoselective ring-opening under the control of an appropriate catalyst3,4. Epoxide ring opening generally proceeds via nucleophilic addition with inversion of stereochemistry; however, the regioselectivity can be sensitive to whether the reaction is conducted under acidic or alkaline conditions as shown in Fig. 1a5. Accordingly, a number of nucleophiles have been developed to react with epoxides in order to yield 1,2-difunctionalized systems with trans stereochemistry6. Epoxide ring-opening can also be catalyzed by enzymes such as epoxide hydrolases (EHs) or oxidoreductases (ORs) (Fig. 1b)7. EHs catalyze the hydrolysis of epoxides to trans-vicinal diols8,9; ORs catalyze the stereoselective reduction of an epoxide to an alcohol (Fig. 1b)10,11.

a Nonenzymatic epoxide ring-opening reactions involving addition of a nucleophile (Nuc) under basic or acidic conditions. b Enzymatic epoxide ring-opening reactions by epoxide hydrolases (EHs) and oxidoreductases (ORs). c Epoxide ring-opening reactions of fluostatin C (1), either enzymatically catalyzed by the hydrolase Alp1U, or nonenzymatically mediated by FAD and NADH as reported in this study.

Epoxides are also an important structural element found in a wide variety of natural products and reactive intermediates in biosynthetic pathways1. In particular, the fluostatins (FSTs, e.g. 1)12,13,14,15,16,17,18,19,20,21,22, kinamycins23, lomaiviticins24,25, and nenestatins26,27,28 constitute a family of atypical angucyclines with a benzofluorene core (Supplementary Fig. 1). The benzofluorene core of the kinamycins and lomaiviticins is further decorated with a diazo group endowing these compounds with potent antitumor activities that has attracted considerable attention29,30. The atypical angucyclines are often characterized by a highly oxygenated A-ring that can undergo further modifications such as acylation, epoxidation, glycosylation, and dimerization leading to significant structural diversity18,21,27,31,32. The α/β hydroxylases Alp1U and Lom6 were recently reported to catalyze stereoselective epoxide hydrolysis reactions during the biosynthesis of kinamycins and lomaiviticin23. Alp1U has also been shown to hydrolyze the epoxide of FST C (1) to afford the two stereoisomeric FSTs C1 (2) and C2 (3) (Fig. 1c)18,33.

The α/β-hydrolase FlsH from the FST pathway in the South China Sea-derived Micromonospora rosaria SCSIO N160 has been shown to catalyze deacylation of acyl FSTs;18 however, it is unable to catalyze hydrolysis of the epoxide in FSTs despite its homology to Alp1U18. Naturally isolated FSTs (Supplementary Fig. 1), such as FST B12, pyrazolofluostatins A‒C16, and FST R17 have been proposed to derive from the corresponding epoxide precursors; however, given the activity of FlsH it is not entirely clear how the epoxide would be cleaved and what enzymes if any would be responsible.

In this work, the 2,3-epoxide ring in FST C (1) is shown to open nonenzymatically in the presence of flavin adenine dinucleotide (FAD, 4) and nicotinamide adenine dinucleotide (NADH) with reduced FADH2 (5) or C4a-hydroperoxyflavin (FADOOH, 6) serving as the reactive flavin species (Fig. 1c). The epoxide ring-opening reactions can thus proceed in a reductive manner to generate a putative enol intermediate, which is tautomerized to products possessing a single hydroxyl group at C-2 (7 and 8), or is further modified by 6 to products with a vicinal diol at C-2 and C-3 (3 and 9). In the presence of molecular oxygen, the epoxide ring opening reactions can also proceed in an oxidative manner leading to a peroxylated intermediate, which can be further reduced by NADH to 3 and 9, or can undergo ring rearrangements to afford products with a contracted five-membered A-ring (10) or a bridged and expanded seven-membered A-ring (11). As a result, this non-enzymatic epoxide cleavage reaction may account for the formation of several different FST derivatives observed in Nature. Additional experiments show that similar reactions also take place in both natural products and other organic compounds harboring an epoxide adjacent to a carbonyl group that is conjugated to an aromatic moiety. Thus, this nonenzyme catalyzed ring-opening reaction holds promise as a useful tool in organic synthesis.

The α/β hydroxylase Alp1U was previously shown to hydrolyze the epoxide of FST C (1) to afford FST C1 (2) and FST C2 (3) (Fig. 2a, traces i-ii)18,33. In contrast, the Alp1U homologue FlsH is unable to catalyze hydrolysis of the epoxide ring in 1 (Fig. 2a, trace iii)18. A possible explanation is that FlsH might require a protein partner or an exogenous cofactor to catalyze the epoxide hydrolysis. In order to test these hypotheses, several flavin reductases including Fre from E. coli34 were selected to examine their competence as putative protein partners for FlsH. It was found that incubation of FST C (1) with FlsH and Fre in the presence of NADH led to multiple products (Fig. 2a, trace vi). However, further experiments showed that formation of the same set of products was also observed in the absence of FlsH (Fig. 2a, trace vii), suggesting that Fre alone was able to mediate the same decomposition of FST C (1). Moreover, incubation of 1 with several other flavoenzymes including FlsO2 (prejadomycin oxidase)35, TiaM (tiacumicin halogenase)36,37, and XiaK (xiamycin N-hydroxylase)38 also led to the same result (Supplementary Fig. 2). Given that the activities of these flavoenzymes all rely on the reduction of FAD by NADH, the reduced flavin alone was proposed to serve as the actual catalyst of FST C (1) consumption. Indeed, similar products were observed upon incubation of FST C (1) with FAD and NADH in the absence of any enzymes, such that FAD and NADH are both sufficient (Fig. 2a, traces viii & xii) and necessary (Fig. 2a, traces ix‒xi) to facilitate the nonenzymatic decomposition of FST C (1).

a HPLC analysis of reactions involving FST C (1). (i) 1 std.; (ii) 1 + Alp1U; (iii) 1 + FlsH; (iv) 1 + FlsH + Fre; (v) 1 + FlsH + NADH; (vi) 1 + FlsH + Fre + NADH; (vii) 1 + Fre + NADH; (viii) 1 + FAD + NADH; (ix) 1 + Fre; (x) 1 + NADH; (xi) 1 + FAD; (xii) 1 + FAD + NADH. HPLC was performed using a reversed phase C18 column (i–xi) or in a polar column (xii). Reactions were run for 30 min at 30 °C in 50 mM PBS buffer (pH 7.0) containing 5 μM enzyme(s) (Alp1U, FlsH or Fre), 100 μM FAD and 10 mM NADH. b The X-ray crystal structures of 7 and 10. c Experimental ECD spectrum of 9 (black line) compared with the B3LYP/TZVP PCM/MeCN // ωB97X/TZVP PCM/MeCN spectrum of (1R,2S,3R)-9 (red line). The bars represent rotational strength values for the lowest energy solution conformers.

Reaction products (3 and 7‒11) were isolated from a scaled up reaction of FST C (1) with FAD and NADH and structurally characterized as shown in Fig. 1c. The first product was identified to be FST C2 (3) (Supplementary Fig. 3 and Table 1), which is also a product of the Alp1U-catalyzed hydrolysis reaction33. The second reaction product 7 (Supplementary Fig. 4 and Table 2) was established to have the same planar structure as FST B, an FST naturally isolated from Streptomyces sp. TA-339112 and Streptomyces strain Acta 1383;13 however, the absolute configuration of FST B was not determined12. The (1R,2R,3S) absolute configuration of 7 was established by the solution TDDFT-ECD methodology (Supplementary Fig. 5) and confirmed by single crystal X-ray analysis (Fig. 2b, CCDC 2036399; Supplementary Table 3). The third product 8 (Supplementary Fig. 6 and Table 2) was determined to have the same planar structure as 7 and the (1R,2R,3R) absolute configuration of 8 was assigned by comparison of the experimental and calculated ECD spectra carried out on the (1R,2R,3R) stereoisomer (Supplementary Fig. 7)39. In order to distinguish the two stereoisomers of FST B, 7 and 8 were named FST B1 and FST B2 (Fig. 1), respectively. The product 9 (designated FST C3, Fig. 1) was isolated with the same retention time as that of 3 during in the HPLC analysis with a reversed-phase C18 column. Analysis of the assay using a polar HPLC column allowed separation of these two species (Fig. 2a, trace xii). Finally, 9 was identified to be a stereoisomer of 3 by HRESIMS and NMR data (Supplementary Fig. 8 and Table 4), and the (1R,2S,3S) absolute configuration of 9 was established by TDDFT-ECD methodology (Fig. 2c, Supplementary Fig. 9).

Two additional products 10 and 11 were also identified and structurally characterized (Fig.1c; Fig. 2a, traces vi-viii & xii). The product 10, designated FST C4 (Fig. 1), was found to possess a contracted five-membered A-ring by NMR spectroscopic analysis (Supplementary Fig. 10 and Table 5) and was determined to have the (1R,2R) absolute configuration by single crystal X-ray analysis (Fig. 2b; Supplementary Table 6; CCDC 2129081). The product 11, designated FST C5 (Fig. 1), was structurally elucidated to have a bridged and expanded seven-membered A-ring (Supplementary Fig. 11 and Table 5). Assignment of the (1R,2R,3R) absolute configuration to 11 was based on its origin from 1 but otherwise remains tentative, because a definitive experimental characterization was not possible on account of its instability. Currently, there are no reports of 9‒11 having been isolated from a natural source.

To investigate the mechanism of the nonenzymatic epoxide ring opening reaction, FST C (1), FAD and NADH were coincubated in PBS buffer (pH 7.0) prepared with deuterium oxide (2H2O). Incorporation of a single deuteron into both 7 and 8 was indicated by the presence of a + 1 Da-shifted molecular ion peak at m/z 326.7 ([M ‒ H]‒) for both reduced products (Supplementary Fig. 12). In contrast, no changes in the molecular weights of 3, 9, 10 or 11 (Supplementary Fig. 12) were observed. Subsequently, 7-2H and 8-2H were isolated from scaled up reactions and analyzed by 1H and 13C NMR (Supplementary Figs. 13, 14 and Table 2). Comparison of the 1H NMR spectra of 7-2H and 7 revealed that the 3-H proton signal of 7 had vanished in 7-2H and meanwhile the 3-Me doublet of 7 had collapsed to a singlet in 7-2H (Fig. 3a), which located 2H at C-3 of 7-2H. In support of this assignment, the COSY correlation between the H-2 and H-3 protons observed in 7 was absent in 7-2H (Supplementary Figs. 4, 13). Likewise, a singlet was also observed for the 3-Me along with the absence of any COSY correlation between H-2 and H-3 in 8-2H (Fig. 3a; Supplementary Figs. 13, 14). Moreover, the 13C NMR spectra of 7-2H and 8-2H both showed broadening and reduced intensity of the signals from C-3, and 2H‒13C couplings at C-3 were also observed (Supplementary Figs. 13, 14)40. These observations demonstrate that a single solvent hydron is incorporated at C-3 during the reduction of 1 to both 7 and 8.

a NMR analysis of 2H or 18O incorporation in products and intermediates as well as potential interconversions. Deuterium incorporation from 2H2O at C-3 of 7 and 8 was inferred from 1H NMR spectroscopic analysis. The O18-labeling in 3-18O and 9-18O was supported by HRMS analysis. The assigned structures of 12 and 14 are shown, whereas the proposed structure of 13 remains speculative on account of its poor stability. b HPLC analysis of reactions under varying conditions. (i) 1 std.; (ii) 1 + FAD + NADH (in air); (iii) 1 + FAD + NADH (under 18O2); (iv) 1 + FAD + NADH (under N2); (v) 7 in 50 mM borax/NaOH buffer (pH 10) at 30 °C for 12 h; (vi) 100 μM 1 + 10 μM FAD + 2 mM NADH (30 °C for 30 min); (vii‒ix) incubation of 13 collected from (vi) with (vii) H2O; (viii) FAD; (ix) FAD + NADH; the reactions of (viii) and (ix) were performed in O2 at 30 °C for 30 min in 50 mM PBS buffer (pH 7.0); (x) 14 in H2O; (xi) 14 + FAD; (xii) 14 + NADH; (xiii) 14 + FAD + NADH. The reactions of (x-xiii) were performed at 30 °C for 30 min. The reactions of (xiv‒xvii) involved incubation of 1 and NADH with different flavin cofactors: (xiv) FAD; (xv) FMN; (xvi) riboflavin; (xvii) isoalloxazine at 30 °C for 30 min. (xviii) The reaction containing 1, F420, glucose 6-phosphate and FGD was incubated at 30 °C for 10 h. HPLC analysis was run with UV detection at 304 nm using a polar column (traces i-v & x-xviii) or a reversed phase C18 column (traces vi-ix).

When FST C (1) was incubated with NADH and FAD under 18O2 (Fig. 3b, traces i−iii), LC-MS analysis of the reaction products revealed an increase of +2 Da in the molecular mass of the oxidized products yielding 3-18O, 9-18O, 10-18O and 11-18O (Fig. 3a; Supplementary Fig. 15). These data indicate that the conversion of 1 to 3, 9, 10, and 11 involves incorporation of one oxygen atom from O2. Furthermore, the relative production of 3/9 and 10/11 versus 7/8 was O2 dependent, because incubation of FST C (1) with FAD and NADH after saturating the reaction buffer with O2 led to a significant increase in the levels of the former (3, 9‒11) versus the latter (7 and 8); in contrast, saturating the reaction buffer with N2 led to 7 and 8 as the dominant products (Fig. 3b, traces iii and iv). To locate the exact position of 18O incorporation during the reaction (1 → 3/9), a scaled up reaction was performed by incubating 1, FAD, and NADH in 18O2-saturated PBS buffer (pH 7.0). Two products 3-18O ([M ‒ H]‒ m/z 343.0718) and 9-18O ([M ‒ H]‒ m/z 343.0722) (Fig. 3a; Supplementary Fig. 16) were isolated. NMR analysis showed that the 18O label was incorporated at C-3 of 9-18O (Supplementary Fig. 17). Specifically, comparison of the 13C NMR data for 9 and its 18O isotopolog 9-18O demonstrated a 3.8 Hz upfield shift of δC-3 in the latter relative to that of 9 (Supplementary Fig. 18 and Table 4), supporting the 18O label at C-3 (i.e., 9-18O)41,42.

The pH dependence of the FAD/NADH-dependent decomposition of 1 was subsequently investigated by performing the reaction in buffers over the pH range 3‒10. Following the incubation of 100 μM 1 with 100 μM FAD and 10 mM NADH for 2 h at 30 °C, 1 was more efficiently converted to the epoxide ring-opened products with buffers in the pH range 5‒7; however, the reaction was less efficient under more alkaline conditions at pHs 9–10 (Supplementary Fig. 19). FST B1 (7) was rather stable at pH 3–7; however, it readily converted to 8 at higher pH (Supplementary Fig. 20), where it also underwent oxidation to yield the previously reported natural product FST A (12) (Fig. 3b, trace v; Supplementary Fig. 20 and Table 1)12. FST B2 (8) was also stable at pH 3–6, and readily converted to 7 and 12 in more alkaline buffers (Supplementary Fig. 20). In contrast, FST C (1) was highly stable at pH 3‒10, even in the presence of FAD or NADH alone (Supplementary Fig. 21) again demonstrating that decomposition of the epoxide in 1 requires the presence of both FAD and NADH.

A time course analysis of 100 μM 1 with 100 μM FAD and 10 mM NADH demonstrated the transient formation of an intermediary species 13 that vanished after longer incubation (Supplementary Fig. 22). A fixed initial concentration of 1 (100 μM) was also incubated with varying concentrations of FAD (1, 10, and 100 μM) and NADH (2, 5, and 10 mM) for 30 min at 30 °C (Supplementary Fig. 22). The lifetime of the transient intermediate was significantly extended at decreased levels of FAD (Fig. 3b, trace vi). This allowed collection of the intermediate 13 followed by immediate reinjection on the HPLC demonstrating its conversion to 7 and 12 (Fig. 3b, trace vii). When the isolated intermediate 13 was immediately incubated with FAD under O2, the production of 7 and 12 was again observed (Fig. 3b, trace viii); however, if NADH was also included in the incubation, then 3 was instead observed as the major product with 12 as the minor product, and 7 was no longer observed (Fig. 3b, trace ix). The UV absorbance spectrum of the intermediate 13 was highly similar to those of 1, 3, and 7, and LC-MS analysis of the intermediate indicated an m/z 325.7 for the [M–H]– ion (Supplementary Fig. 23). Based on these measurements, the intermediate is tentatively proposed to be the enol 13 (Fig. 3b), which is essentially a tautomer of 7 and 8 and thus has the same oxidation state as these two products.

While several attempts were made to isolate the intermediate in order to confirm its structural assignment as 13, only 7 was obtained as the major product along with another minor compound 14. This is consistent with the poor stability of the intermediate and its facile conversion to 7 (Fig. 3b, trace vii, Supplementary Fig. 24). Nevertheless, 14 could be characterized and was thus identified as the C-3 peroxide designated hydroperoxyfluostatin (Fig. 3a; Supplementary Fig. 25 and Table 5); however, poor recovery of 14 hampered collection of sufficient spectra for a complete characterization of its absolute configuration at C-3. Hydroperoxyfluostatin (14) was stable in water, even in the presence of FAD (Fig. 3b, traces x and xi). While the coincubation of 14 with NADH alone led to multiple products 3, 9, 10 and 11, the inclusion of FAD with NADH did not change the product profile (Fig. 3b, traces xii and xiii; Supplementary Fig. 26). Given the observed conversion of 14 to both 3 and 9, compound 14 is likely a mixture of the (1S,2S,3R) and (1S,2S,3S) stereoisomers. The fact that isolation of 13 afforded a minor amount of 14 suggests that 14 is another intermediate that coelutes with 13 as opposed to being derived from 13. Furthermore, while 3/9 could be generated from both 13 and 14, 7/8 were only produced from 13, whereas 10/11 were exclusively derived from 14 (Fig. 3a).

When other flavin-related cofactors were considered, FMN and riboflavin in place of FAD were also found to efficiently mediate the decomposition of 1 in the presence of NADH (Fig. 3b, traces xiv-xvi). Isoalloxazine and NADH were also able to facilitate the formation of 3 from 1, albeit with a much lower efficiency (Fig. 3b, trace xvii). Only the products 3, 9‒11 were observed using the cofactor F420 in the presence of the reducing system constructed from glucose 6-phosphate and F420-dependent glucose-6-phosphate dehydrogenase (FGD)43,44,45, but notably no production of the reduced species 7 and 8 was observed (Fig. 3b, trace xviii). The observation of oxygen incorporation in the presence of F420 and NADH was unexpected, because reduced 5-deazaflavin has generally be reported to react very slowly with molecular oxygen46,47. Nevertheless, the results with flavin cofactor compatibility shown in Fig. 3b (traces xiv-xviii) were found to be reproducible (Supplementary Fig. 27). NADPH was also found to be an effective cofactor similar to NADH and thus support the epoxide ring opening reactions (Supplementary Fig. 19).

To explore the generality of this reaction, an array of FST derivatives 15‒21 (Fig. 4) were tested as possible oxirane reactants. Although FST F (15) is inert to Alp1U18,33, it could be efficiently converted in the presence of FAD and NADH to 1-O-methyl-FST C2 (22), 1-O-methyl-FST B1 (23), 1-O-methyl-FST C3 (24), and 1-O-methyl-FST B2 (25) (Fig. 4 and Supplementary Fig. 28), which were structurally characterized by NMR and ECD spectroscopic analysis (Supplementary Tables 7, 8 and Figs. 29‒32), as well as single crystal X-ray diffraction analysis (e.g. 23, CCDCC 2036400, Supplementary Table 3).

FST derivatives 15‒20 could undergo epoxide-ring opening reactions upon treatment with FAD/NADH to produce multiple products related to 3, 7, 8, and 9. FST Q (21) was unreactive with FAD/NADH. The epoxides 28–35 displayed no activities with FAD/NADH. Treatment of auxarthrol H (36) or menadione 2,3-epoxide (37) with FAD/NADH yielded multiple products. The epoxides 42–46 were found to be unreactive with FAD/NADH. The oxidoreductase RslO5 catalyzed a reductive epoxide ring opening reaction on 43 to produce 44 during rishirilide biosynthesis and chalcone α,β-epoxide (46) was found to be a substrate of RlsO5 to yield the single product 47.

Similarly, 7-O-methyl-FST C (16), 6-O-methyl-FST C (17), FST D (18), FST S (19), and difluostatin H (DiFST H, 20) could also undergo epoxide-ring opening reactions upon treatment with FAD/NADH to produce a set of multiple products related to 3, 7, 8, and 9 (Fig. 4, Supplementary Figs. 33‒37). The major products from 16 and 17 were structurally characterized by 1D and 2D NMR as well as ECD spectroscopic analysis as FST M (26)17, and 6-O-methyl-FST B1 (27), respectively (Fig. 4, Supplementary Table 9 and Figs. 38, 39). The structures of the other products from reactions with 18‒20 were deduced based on LC-MS analyses. Notably, FST Q (21), which differs from 16 in terms of a C-4 hydroxyl instead of a C-4 carbonyl, was unreactive with FAD/NADH (Supplementary Fig. 40) highlighting the essential role of the C-4 carbonyl in this chemistry.

The epoxides 28–37 (Fig. 4) were also tested as putative oxirane substrates. No activities were observed with 28–35 (Supplementary Figs. 41‒46)16,40. In contrast, treatment of auxarthrol H (36)48 with FAD/NADH led to multiple products (Supplementary Fig. 47), one of which was determined to be 38, which is a structural analog of auxarthrol F (Fig. 5; Supplementary Fig. 48 and Table 10)49, by comparison with the experimental and calculated ECD spectra of 36 and 38 (Supplementary Fig. 49). Reaction with menadione 2,3-epoxide (37) yielded three products (Supplementary Table 11 and Figs. 50‒53) including 3-hydroxy-3-methyl-2,3-dihydronaphthalene-1,4-dione (39), 2-hydroxy-3-methyl-1,4-naphthoquinone (40, phthiocol, characterized by X-ray diffraction, CCDC 2036401; Supplementary Table 12), and 3-methylnaphthalene-1,4-dione (41).

The reaction can proceed via reductive and oxidative pathways leading to multiple products of different redox states depending on the presence of NADH and O2. The key transformations in the reductive reactions (yellow background) are proposed to involve a flavin N5‒C4′ adduct (49) to produce the enol intermediate 13, which can undergo tautomerization to yield 7 (major) or 8 (minor), and oxidation to produce 3 (major) or 9 (minor). 7 can be further autooxidized to 12. Whereas the oxidative ring opening is likely to involve a flavin C4a‒O‒O‒C3′ adduct (50) to give the peroxylated intermediate 14 (gray background), which can undergo reduction to 3 and 9 by NADH, and further rearrangements leading to 10 and 11.

Two common structural features shared by all compounds that can react with FAD/NADH to undergo the epoxide ring opening reactions include (i) the presence of a carbonyl adjacent to the epoxide and (ii) the presence of an aromatic moiety adjacent to the carbonyl/epoxide pair (Fig. 4). The absence of a carbonyl group neighboring the epoxide ring in 21 and 28–31 may account for the observed lack of reactivity. While 36 and 37 underwent ring opening in the presence of FAD/NADH, no reaction was observed for 32–35 despite the presence of an epoxide/carbonyl pair in these compounds. This implies that conjugation of the carbonyl/epoxide pair to an aromatic system is also necessary for ring opening of the epoxide.

The commercial compound vitamin K1 2,3-epoxide (42) was also tested as a putative substrate, which features both an epoxide/carbonyl pair and an adjacent aromatic ring. However, incubation of 42 with FAD/NADH led to no changes in either its TLC retention profile or spectroscopic properties implying no reaction (Supplementary Fig. 54). A recent study demonstrated that the flavoenzyme RslO5 catalyzed a hydride-mediated reductive epoxide ring opening reaction to convert 43 to 44 during rishirilide biosynthesis (Fig. 4)11. The reaction proceeded in a manner that was highly similar to the conversion of 1 to 7. However, the production of 44 from 43 was confirmed to be strictly RslO5-dependent, and 43 was unreactive in the presence of FMN and NADH11. A possible explanation is that the presence of a long side chain next to the epoxide in both 42 and 43 might hinder both approach and orientation of the flavin thereby preventing suitable interactions for ring opening (Supplementary Fig. 55). Two additional commercial compounds trans-1,3-diphenyl-2,3-epoxypropan-1-one (45) and chalcone α,β-epoxide (46) were found to be unreactive with FAD/NADH; however, 46 but not 45 was accepted as a substrate by RlsO5 to yield the single product 47 (Supplementary Table 13 and Figs. 56, 57), which indicates that RslO5 is specific for only one of the two enantiomers. Deuterium incorporation into 47 was not observed from the RslO5 reaction in buffered 2H2O but was indeed observed when carrying out the RslO5 reaction in a coupled assay either with the glucose dehydrogenase from Bacillus megaterium DSM 2894 (BmGDH) to provide (S)-[4-2H]NADH50, or with the glucose dehydrogenase from Thermoplasma acidophilum ATCC 25905 (TaGDH) to provide (R)-[4-2H]NADH51, respectively, employing d-[1-2H]glucose as the deuterium donor (Supplementary Fig. 58)52. Previous studies demonstrated that the RslO5-H172N mutant had a deficiency in FMN binding and was inactive with the native substrate 4311, suggesting the critical role of FMN in the RslO5-catalyzed reaction. Taken together, a hydride from FMNH2 originating from NADH is proposed to be the effective nucleophile for RslO5-catalyzed epoxide opening reactions. In contrast, no deuterium incorporation into 7 was observed in reactions of 1 and FAD with either (S)-[4-2H]NADH or (R)-[4-2H]NADH generated as described above (Supplementary Figs. 58, 59). Therefore, nonenzymatic reduction of 1 to 7 in the presence of FAD/NADH differs from that of RslO5 catalysis with respect to the ultimate origin of the C-3 hydrogen.

Epoxide ring opening reactions are common and important in both biological processes and synthetic applications1,2. Nonenzymatic epoxide ring opening reactions are typically redox neutral proceeding through nucleophilic addition with the preferred regioselectivity and stereoselectivity contingent upon the nature of the epoxide and on the reaction conditions to generally yield products with a trans-vicinal diol3,4. Similar chemistry is encountered among the α/β-epoxide hydrolases that also generate trans-vicinal diol products53. For example, the hydrolase AlpU catalyzes the epoxide hydrolysis of the FST C (1) epoxide to afford 2 and 3, each of which exhibits a trans-vicinal diol (Fig. 1)33. In contrast, the flavoenzyme RslO5 was recently reported to catalyze a reductive epoxide ring opening of rishirilide thereby yielding a monohydroxylated product11. The RslO5 chemistry is thus distinctly different from that of the previously reported hydrolytic reactions and instead represents hydrogenation of an epoxide by reduced flavin, which is evident from the results using isotopically labeled substrates (Supplementary Fig. 58).

In this study, FAD/NADH is shown to induce the ring opening of suitably activated epoxides leading to a variety of products with different redox states. Under anaerobic conditions epoxide ring opening proceeds reductively in the presence of FAD/NADH via a mechanism that may be unrelated to that of RslO5 catalysis. The resulting monohydroxylated species, however, are highly susceptible to oxidation by molecular oxygen resulting in quinones (e.g., 12) and vicinal alcohols in reactions that can also be accelerated by the presence of FAD. Under aerobic conditions, the epoxide ring opening appears to proceed through the formation of an α-ketoperoxylated species which can be reduced by NADH to again generate vicinal diols. Alternatively, the peroxylated intermediate can undergo further rearrangement leading to both ring contracted (e.g., the five-membered species 10) as well as ring expanded (e.g., the seven-membered species 11) oxidized products.

On the basis of the accumulated experimental evidence, a putative mechanism is proposed for the FAD/NADH enabled nonenzymatic epoxide-ring opening reactions (Fig. 5). Since both FAD and excess NADH are required for the observed epoxide ring opening reactions, NADH is proposed as the reductant with FAD serving as a redox catalyst. When the reaction is conducted aerobically, O2 is proposed to act as the oxidant. Given that NADH alone could not initiate the reaction, the reduced flavin is proposed to be the species directly responsible for the reduction of 1. It is possible that 7 is directly formed via a hydride transfer from a reduced flavin species (e.g., N5-H of FADH2) to C3 of 1 thereby opening the epoxide ring, which would resemble the RslO5 catalyzed epoxide reduction reaction (Fig. 4). In this case, the observation that the product 7 has its H-3 derived from solvent could be explained by ready exchange of N5-H of the reduced flavin with solvent. This would imply that 7 should be the immediate reduction product prior to tautomerization to the observed intermediate 13. However, a time course assay using 0.5 μM 1 with 10 μM FAD and 2 mM NADH demonstrated that 13 accumulates first followed by conversion to 7 and 8. In contrast, no significant accumulation of 13 was observed in incubations of 7 under similar conditions (Supplementary Fig. 60). These results imply that 13 is the initial reduction product rather than 7 or 8, and thus nonenzymatic reduction of 1 in the presence of FAD/NADH does not proceed via direct hydride transfer to C-3 as is proposed for RslO5 catalysis.

An alternative mechanism involves activation of the oxirane by the adjacent carbonyl coupled to an aromatic ring and undergoes reduction leading to an unstable intermediate. This intermediate is unlikely to be 7-demethyl-FST Q (48) (Fig. 4), which is the product of a direct C-4 carbonyl reduction in 1, because the previously isolated FST Q (21)17 is inert to the FAD/NADH reaction system (Supplementary Fig. 40). Instead, the intermediate during reduction of FST C (1) is hypothesized to be an enol species such as 13, which is consistent with the observation that 13 readily tautomerizes to yield 7 and 8. This mechanism is also consistent with the incorporation of deuterium at H-3 of 7 and 8 when the reaction is carried out in 2H2O. Compound 13 is also expected to be susceptible to autoxidation to yield 3 and 9 in a manner that is sensitive to the presence of O2, FAD, and NADH.

Formation of 13 may proceed via the addition of the nucleophilic N-5 of the reduced flavin to 1. This model is supported by the fact that no formation of 7 was observed using the reduced F420 cofactor, which lacks the nucleophilic N-5 but is still able to serve as a hydride donor54. Nucleophilic addition of FADH2 to 1 may occur at either C-3 or C-4. Given the presence of a sterically bulky CH3 group at C-3 of 1, C-4 is proposed to be the likely site of nucleophilic attack, which is consistent with the requirement for a carbonyl adjacent to the epoxide and thus the different reactivity of 16 (C-4 carbonyl) versus 21 (C-4 hydroxyl). Considering that N-5 in FADH2 possesses a lone pair, and C-4 in 1 is a trigonal carbonyl carbon, the redox reaction is proposed to happen via an n→π* interaction. Specifically, the nucleophilic N-5 donates the lone-pair (n) electron density into the trigonal carbene center (empty π* orbital) along the Burgi–Dunitz trajectory55. Mixing of these orbitals is thermodynamically favorable resulting in a covalent adduct 49 (Fig. 5)56. Subsequent N-1 deprotonation of the flavin moiety in 49 leads to the breakage of the N5‒C4' linkage and release of the oxidized flavin thereby completing the reduction of 1 to the enol intermediate 13 with a Δ3,4 double bond (Fig. 5).

Intermediate 13 is highly unstable and undergoes facile tautomerization to incorporate a solvent hydron at the α-carbon (C-3) either from the si face (the major route) or the re face (the minor route) of the sp2 planar structure, to yield 7 or 8, respectively57. This mechanism is consistent with the site-specific incorporation of deuterium at C-3 in 7 and 8 from buffered 2H2O (Fig. 3a). Despite the 2,3-cis configuration of 7 compared to 8, the former appears to be the thermodynamically favored tautomer with an equilibrium constant of approximately [7]eq/[8]eq = 5.4 (Supplementary Fig. 61). Moreover, 7, 8 and the putative enol intermediate 13 are also susceptible to autooxidation to yield 12 (Supplementary Fig. 62).

The putative enol intermediate 13 also appears to be sensitive to molecular oxygen and can undergo autoxidation in the presence of FAD and NADH. Reduced flavin is known to react with O2 to form the covalent Fl4aOOH adduct (FAD → FADOOH)58, and in some cases, H2O2 may be released from FADOOH to serve as the oxidant37,59. However, neither 1 nor 13 can react with H2O2 (Supplementary Figs. 24, 63). Thus, the intermediate 13 is proposed to react with the electrophilic C(4a)-hydroperoxy group of FADOOH to afford the C-3 monooxygenated products (see Supplementary Fig. 64). Hydroxylation can occur either from the si face (major route) or the re face (minor route) of the planar double bond (Δ3,4) to produce 3 or 9, respectively, with concomitant release of the oxidized flavin (Fig. 5). The proposed mechanism is supported by the observations that (i) the O incorporated into both 3 and 9 at C-3 originates in O2, and (ii) the conversion of 13 to 3 and 9 requires the presence of FAD, NADH and O2.

Isolation of intermediate 14 indicates that 3 and 9 can also be produced in an alternative way that does not involve 13. In the presence of molecular oxygen, the flavin C(4a)-peroxide (FADOO‒) may serve as a nucleophile to regioselectively attack C-3 of 1 at either the si face (major route) or the re face (minor route) to open the epoxide ring, resulting in the putative adduct 50 (Fig. 5). The presence of the C-4 carbonyl oxygen with electron-withdrawing effect may cause changes of the electron density of C-360, to make C-3 a better site for nucleophile substitutions than C-2 of the epoxide in 1. Deprotonation of the flavin N-5 in 50 breaks the C4a‒O covalent bond to release 14 and FAD (Fig. 5). The product 14 is a mixture of C-3 isomers and easily reduced to 3 and 9 by NADH (Fig. 5, Supplementary Fig. 65). Coincubation of 14 with NADH also leads to 10 and 11, which is proposed to involve a Baeyer-Villiger reaction-like mechanism. The C-3 hydroperoxide in 14 may thus perform an intramolecular nucleophilic addition at the C-4 carbonyl to form the putative intermediate 51, which can partition to generate 10 and 11. In the former case, intermediate 51 may undergo a Criegee rearrangement to yield a seven-membered lactone ring61,62, followed by an intramolecular backbiting addition of the C-1 hydroxy at the C-4 carbonyl that leads to 10 after dehydration (Fig. 5)63. Alternatively, the 1,2-dioxetane unit of 51 may undergo heterolytic cleavage, followed by Grob-like fragmentation to yield an oxoheptanoate intermediate64,65, which eventually generates the hemiacetal 11 after successive intramolecular cyclizations and dehydration66.

In conclusion, the reductive epoxide ring opening is suggested to proceed mechanistically via a transient adduct (49) with an N5‒C4', covalent bond that is formed between N-5 of the flavin cofactor and C-4 of the substrate FST C (1) (Fig. 5). While tautomerization of the resulting product can yield 7 and 8, nucleophilic reaction with FADOOH can also afford the diol products 3 and 9. Oxidative epoxide ring opening of 1 produces the intermediate 14 via a putative C4a‒O‒O‒C3' covalent adduct (50, Fig. 5). The canonical reactivity of flavin cofactors involves redox chemistry through N-5 hydride transfer or oxygen activation at C-4a in the majority of cases67. However, a few flavoenzymes have been reported to catalyze the formation of covalent flavin N-5‒substrate adducts in a redox-neutral manner68, with examples including the iminium-adducts in the catalytic cycle of UDP-galactopyranose mutase69, alkyl-dihydroxyacetone phosphate synthase70, flavin prenyltransferase71, thymidylate synthase72, and 2-haloacrylate hydratase73.

The present study provides an example likely involving flavin N-5 adduct formation during flavin-catalyzed nonenzymatic reactions (Fig. 5). Furthermore, in addition to serving as a nucleophile in mediating hydroxylation, epoxidation and Baeyer-Villiger oxidation in flavoenzyme catalysis58, the flavin C(4a)-peroxide (FADOO‒) is proposed to also facilitate the formation of peroxylated intermediates such as 14 (Fig. 5). Flavin and flavin derivatives are well known to participate as cofactors in a wide variety of reactions found in nature67,74. Previous reports have shown that natural flavins can catalyze nonenzymatic oxidative decarboxylation of picolinic acid derivatives75 and the nonenzymatic iodination of diverse aromatic compounds37,59. In this study, the chemistry of flavins is expanded to epoxide ring opening reactions in both a reductive and an oxidative manner to generate multiple ring-opened products. Consequently, the flavin chemistry identified in this study may be applicable to other epoxides and thus holds promise as a useful tool in organic synthesis.

The strain Micromonospora rosaria SCSIO N160 was used for the isolation of FSTs15. FST Q (21) was previously isolated from Streptomyces sp. PKU-MA0004517. Chemicals, enzymes, and other molecular biological reagents were purchased from standard commercial sources and used according to the recommendations of the manufacturer.

HPLC analysis of reactions was generally carried out on an Agilent 1260 Infinity series instrument (Agilent Technologies Inc., USA) using a reversed phase C18 column (Kinetex® 5 µm C18 100 Å, LC Column 150 × 4.6 mm, Phenomenex, USA) or a polar column (Comixsep®, P/N FMG-BPF5-EONU, Polar BiPFP 5 u, 250 × 4.6 mm, China) with UV detection at 256 or 304 nm under the following program: solvent A, 10% acetonitrile (MeCN) in water supplementing with 0.1% formic acid; solvent B, 90% MeCN in water; 5% B to 80% B (0–20 min), 80% B to 100% B (20–21 min), 100% B (21–24 min), 100% B to 5% B (24–25 min), 5% B (25–30 min); flow rate at 1 mL min−1.

The DNA fragment of rslO5 (GenBank: KJ437438.1 [https://www.ncbi.nlm.nih.gov/nuccore/KJ437438.1]) from the rishirilide biosynthetic gene cluster in Streptomyces bottropensis11 was synthesized and cloned into pET28a to afford the plasmid pCSG8112 (Supplementary Table S14). When the cultures of E. coli BL21(DE3)/pCSG8112 in LB media containing kanamycin (50 μg mL−1) were grown to an OD600 of about 0.6 at 37 °C, the production of RslO5 was induced by the addition of isopropyl-β-d-thiogalactopyranoside (IPTG) to a final concentration of 0.1 mM. The cultures were grown at 16 °C for an additional 12 h. The cells were then collected by centrifugation and were resuspended in the lysis buffer (20 mM Tris-Cl, 500 mM NaCl, and 5 mM imidazole, pH 8.0) for sonication. Purification of N-His6-tagged RslO5 was conducted using Ni-NTA affinity chromatography according to the manufacturer's manual (Novagen, USA). After desalting with PD-10 column (GE Healthcare, USA), the purified RslO5 was stored in the storage buffer (10% glycerol, 1 mM DTT, 50 mM Tris-Cl, 100 mM NaCl, pH 8.0) at −80 °C for further use. The expression and purification of Fre34, Alp1U18, FlsH18, XiaK38, TiaM36, and FlsO235 were performed similar as described for RslO5. The standard in vitro enzyme assays (Alp1U, FlsH, Fre, XiaK, TiaM, Fre, or FlsO2) contained 100 μM FST C (1) and 10 μM of purified recombinant enzyme in 50 mM PBS (phosphate buffered saline) buffer (pH 7.0) in a total volume of 100 μL with incubation at 30 °C for 0.5‒2 h. The reactions were stopped by adding 100 μL of ice-cold MeOH and were monitored using the general analytical HPLC methods.

A typical reaction mixture included 100 µM 1, 100 µM FAD and 10 mM NADH in 50 mM PBS buffer (pH 7.0) in a total volume 100 µL with incubation at 30 °C for 0.5‒2 h. In general, the reactions were terminated by adding 100 μL of ice-cold MeOH and analyzed by HPLC using the general analytical HPLC method or subjected to LC-MS analysis. For reactions under anaerobic conditions, the reaction buffers were flushed in N2 for 5 min before adding 1, cap-sealed using Parafilm and flushed with N2 during incubation at 30 °C for 30 min. For reactions under aerobic conditions, the reaction buffers were flushed in O2 for 5 min before adding 1, cap-sealed using Parafilm and flushed with O2 during incubation at 30 °C for 30 min. For isotope labeling reactions with 2H, each reaction was carried out in 50 mM PBS buffer (pH 7.0) prepared with deuterated water (2H2O). For isotope labeling reactions with 18O2, a reaction mixture containing 100 µM FAD and 10 mM NADH in 50 mM PBS buffer (pH 7.0) was degassed and flushed with 18O2 for 5 min; after the addition of 100 µM 1, 18O2 gas was continuously bubbled into the reaction mixture for 2 h at room temperature with occasional shaking.

For determining the pH effects on the reactions, the assays were performed in a total volume of 100 μL containing 100 μM 1, 100 μM FAD and 10 mM NADH in 50 mM buffers with pH values ranging from 3 to 10 with incubation at 30 °C for 2 h. The buffers were prepared as follows: citric acid/Na2HPO4 buffer (pH 3‒6); PBS buffer (pH 7); boric acid/borax buffer (pH 8‒9), borax/NaOH buffer (pH 10). As controls, 100 μM 1 was incubated in different pH buffers (pH 3‒10) in the presence of 100 μM FAD alone (or 10 mM NADH alone) at 30 °C for 2 h.

For time course assay, reactions were performed by incubating 100 µM 1, 100 µM FAD, and 10 mM NADH in 50 mM PBS buffer (pH 7.0) at 30 °C with sampling at different time points of 0, 2, 4, 6, 8, 10, 12, 14, 16, 20, 25, and 30 min. For assaying the effects of different FAD/NADH concentrations, reactions were carried out with 100 µM 1 in 50 mM PBS buffer (pH 7.0) with varying concentrations of FAD and NADH. The first set of reactions were conducted with 100 μM 1, 1 μM FAD, and 2 (or 5 or 10 mM) NADH. The second set of reactions were performed with 100 μM 1, 10 μM FAD, and 2 (or 5 or 10) mM NADH. The third set of reactions were carried out with 100 μM 1, 100 μM FAD, and 2 (or 5 or 10) mM NADH. The reaction mixtures were incubated in 50 mM PBS buffer (pH 7.0) at 30 °C for 30 min.

To test cofactor compatibility, assays containing 100 μM of 1, 100 μM FAD (or FMN/riboflavin/isoalloxazine) and 10 mM NADH in 50 mM PBS buffer (pH 7.0) in a total volume of 100 μL were incubated at 30 °C for 30 min. For testing F420 as a cofactor, assays containing 100 μM of 1, 200 μM F420, 2.5 mM glucose-6-phosphate, 10 μM F420-dependent glucose-6-phosphate dehydrogenase (FGD) in 50 mM Tris-HCl buffer (pH 7.5) in a total volume of 100 μL were incubated at 30 °C for 1 h.

The FAD/NADH-mediated epoxide ring opening reactions were tested with various substrates including both FST-related substrates 15‒21 and FST-nonrelated substrates 28–37, 42, 45, and 46. A typical reaction mixture contains 100 µM substrate (15‒21, 28–37, 42, 45, or 46), 100 µM FAD and 10 mM NADH in 50 mM PBS buffer (pH 7.0) in a total volume of 100 µL.

To test the reactivity of H2O2 with FST C (1), the assays were performed in a total volume of 100 μL containing 100 μM 1 and 30% H2O2 in 50 mM buffers at pH 3.0 (or pH 7.0 or pH 10.0) by incubation at 30 °C for 2 h.

A scaled up reaction of 1 in a total volume of 1 L was performed in 50 mM PBS buffer (pH 7.0) containing 100 μM 1, 10 mM NADH and 100 μM FAD at 30 °C for 2 h with occasional shaking. The reaction was quenched by the addition of an equal volume of ice-cold butanone and centrifuged at 2057 × g for 20 min at 4 °C. The reaction mixtures were then extracted with an equal volume of butanone three times and the solvents were removed under vacuum on an ice bath. The crude extracts were dissolved in 1.5 mL MeOH and subjected to semi-preparative HPLC using an Agilent Eclipse XDB-C18 column (250 mm × 9.4 mm, 5 μm; Agilent technology Ltd., USA) with an isocratic elution gradient of 70% A (H2O with 0.8% formic acid) and 30% B (MeCN) at a flow rate of 2.5 mL min−1. In this way, compounds 3 (8.5 mg, 22.0%), 7 (22.0 mg, 57.0%), 8 (6.0 mg, 15.5%), 9 (2.6 mg, 6.7%), 10 (1.6 mg, 4.1%) and 11 (3.4 mg, 8.8%) were obtained. Similarly, a 40 mL scale of reaction with 100 μM FST F (2) afforded 22 (2.0 mg, 15%), 23 (6.0 mg, 46.0%), 24 (0.9 mg, 7.0%), and 25 (1.2 mg, 9.0%). The 30 mL scale reactions of 16, 17 or 36 yielded 26 (1.3 mg, 44.0%), 27 (1.5 mg, 46.0%), or 38 (1.3 mg, 67.0%), respectively. A 30 mL scale reaction of 37 yielded 39 (1.8 mg, 11.0%), 40 (4.8 mg, 30.0%) and 41 (4.3 mg, 27.0%).

For the isolation of 3-18O and 9-18O, a 400 mL scale reaction of 1 was carried out under 18O2, consisting of 100 µM 1, 100 µM FAD, and 10 mM NADH in 50 mM PBS buffer (pH 7.0) by incubation at 30 °C for 2 h. The reaction products were purified via semi-preparative HPLC as described above to afford 3-18O (3.0 mg, 33.0%) and 9-18O (1.2 mg, 16.0%). For the isolation of 7-2H and 8-2H, a 400 mL scale reaction of isotope labeling with 2H, was set up in 50 mM PBS buffer (pH 7.0) prepared with buffered 2H2O, containing 100 µM 1, 100 µM FAD, and 10 mM NADH, by incubation at 30 °C for 2 h. The reaction products were purified via semi-preparative HPLC to afford 7-2H (11.5 mg, 65.0%) and 8-2H (3.2 mg, 19.0%).

A reaction mixture containing 100 µM 1, 10 µM FAD, and 2 mM NADH in 50 mM PBS buffer (pH 7.0) in a total volume 100 µL was incubated under a normal atmosphere at 30 °C for 20 min. The reactions were quenched by adding 100 μL of ice-cold MeOH. To check the stability of 13, the intermediate 13 was collected from a general analytical HPLC run and was immediately reinjected for HPLC analysis. Similarly, to monitor the changes of 13 under various conditions, the freshly collected 13 was immediately incubated in 50 mM PBS buffer (pH 7.0) containing (i) 10 µM FAD; (ii) 30% H2O2; (iii) 2 mM NADH; (iv) 10 µM FAD and 2 mM NADH (in presence of excess of O2) at 30 °C for 30 min. The reactions were quenched by adding 100 μL of ice cold MeOH and monitored by the general analytical HPLC method using a C18 column as well as a polar column.

Scaled up reactions in a total volume of 50 mL (100 µL × 500 Eppendorf tubes) were performed containing 100 µM 1, 10 µM FAD, and 2 mM NADH in 50 mM PBS buffer (pH 7.0) at 30 °C for 20 min with the aim of isolating 13 for structure elucidation. The reactions in each Eppendorf tube were stopped by extracting three times with 100 μL of ice-cold butanone and the solvents were removed under vacuum on an ice bath. The crude extracts were then collected and dissolved in 1.0 mL MeOH and subjected to general analytical HPLC using a polar column. The collections were kept at −80 °C prior to lyophilization. The collected fractions were purified a second time to remove 7, which had been generated from the decomposition of 13. This process finally afforded a pure and stable compound (0.8 mg), which was dissolved in DMSO-d6 for NMR analysis and confirmed to be 14.

A set of assays were performed to check the stability of 14. A typical reaction mixture included 100 µM 14, 10 µM FAD, and 2 mM NADH in 50 mM PBS buffer (pH 7.0) in a total volume 100 µL. Control reactions were run in parallel by omitting FAD or NADH in the assays. Co-incubation of 100 µM 14 in 30% H2O2 were also performed in a total volume of 100 μL. The reaction mixtures were incubated at 30 °C for 30 min. The reactions were quenched after adding 100 μL of ice-cold MeOH and were analyzed by HPLC using a polar column following the general analytical HPLC method.

A standard RslO5 in vitro reaction mixture contained 100 μM trans-1,3-diphenyl-2,3-epoxypropan-1-one (45) or chalcone α,β-epoxide (46), 10 μM RslO5 and 5 mM NADH in 50 mM PBS buffer (pH 7.0) in a total volume of 100 μL and incubated at 30 °C for 2 h. The reaction with 46 was also performed in 50 mM PBS buffer (pH 7.0) prepared with deuterated water (2H2O) and subjected to LC-HRESIMS analysis to investigate 2H incorporation into 47 from the solvent. To isolate 47 for structural elucidation, 15 mL reactions were performed in 50 mM PBS buffer (pH 7.0) containing 100 μM 46, 10 μM RslO5 and 5 mM NADH at 30 °C for 6 h. The reaction was quenched with an equal volume of pre-chilled butanone. After centrifugation at 2057 × g for 20 min at 4 °C, the supernatants were extracted three times with an equal volume of pre-chilled butanone. The butanone was removed under vacuum on an ice bath. The crude extracts were dissolved in 500 μL of MeOH and were purified by semi-preparative HPLC using a C18 column (250 mm × 10.0 mm, 5 μm; Phenomenex, USA), with an isocratic elution gradient of 60% A (H2O with 0.8% formic acid)/40% B (MeCN) at a flow rate of 2.5 mL min−1 to yield 47 (3.0 mg, 41.0%).

The purification of d-glucose dehydrogenases BmGDH from Bacillus megaterium DSM 2894 in E. coli BL21(DE3)/pRSF-BmGDH and TaGDH from Thermoplasma acidophilum in E. coli BL21(DE3)/pCSG3622, was carried out according to our previous study76. In case of the RslO5/GDH coupling assays, the reduction of NADP to NADPH was first performed in a 100 μL reaction containing 10 μM TaGDH (or BmGDH), 2 mM NADP and 100 mM [1-2H]d-glucose in 50 mM sodium phosphate buffer (pH 7.0) by incubation for 1 h at 37 °C for BmGDH or 50 °C for TaGDH, followed by the addition of 100 μM 46 and 10 mM RslO5 and further incubation at 30 °C for 6 h. The in situ generated 2H-labeled NADH was also reacted with 1 and FAD to monitor the incorporation of 2H in to the product 7. The reactions were quenched with an equal volume of ice-cold MeOH and analyzed by LC-HRESIMS using the general analytical HPLC method.

Mixed torsional/low-mode conformational searches were carried out by means of the Macromodel 10.8.011 software using the MMFF with an implicit solvent model for CHCl3 applying a 21 kJ/mol energy window77. Geometry re-optimizations of the resultant conformers were carried out at the ωB97X/TZVP level with the PCM solvent model for MeCN. TDDFT ECD calculations were performed with Gaussian 09 for ECD using various functionals (B3LYP, BH&HLYP, CAM-B3LYP, PBE0) and the TZVP basis set with the same solvent model as in the preceding DFT optimization step78. ECD spectra were generated as the sum of Gaussians with 3000 and 3600 cm−1 half-height widths, using dipole-velocity-computed rotational strength values79. Boltzmann distributions were estimated from the ωB97X energies. The MOLEKEL software package was used for visualization of the results80.

A single crystal of 7, 10, and 23 was obtained in a mixed solvent of MeOH and water, and single crystals of 40 were obtained in a mixed solvent of CH3CN and H2O. The suitable crystals were selected, and the crystal data were recorded on an XtaLAB AFC12 (RINC): Kappa single diffractometer, with Cu Kα radiation (λ = 1.541 84 Å). The crystals were kept at 99.9(7) K for 7, 99.8(9) K for 23, 100.00(10) K for 10 and 100.01(12) K for 40 for during data collection. Using Olex281, the structure was solved with the ShelXT82 structure solution program using intrinsic phasing and refined with the ShelXL refinement package using least squares minimization.

The data and code in this manuscript have been appropriately deposited into a public data repository or provided in the supplementary information for public availability. Crystallographic data can be obtained free of charge for 7 (CCDC 2036399), 10 (CCDC 2129081), 23 (CCDC 2036400), and 40 (CCDC 2036401) via www.ccdc.cam.ac.uk/data_request/cif, or by emailing [email protected], or by contacting The Cambridge Crystallographic Data Centre, 12 Union Road, Cambridge CB2 1EZ, UK; fax: +44 1223 336033. The GenBank accession number for DNA fragment of rslO5 is KJ437438.1 (https://www.ncbi.nlm.nih.gov/nuccore/KJ437438.1).

Thibodeaux, C. J., Chang, W.-c. & Liu, H.-w. Enzymatic chemistry of cyclopropane, epoxide, and aziridine biosynthesis. Chem. Rev. 112, 1681–1709 (2012).

Article CAS PubMed Google Scholar

Guengerich, F. P. & Yoshimoto, F. K. Formation and cleavage of C–C bonds by enzymatic oxidation–reduction reactions. Chem. Rev. 118, 6573–6655 (2018).

Article CAS PubMed Google Scholar

Meninno, S. & Lattanzi, A. Organocatalytic asymmetric reactions of epoxides: recent progress. Chem. Eur. J. 22, 3632–3642 (2016).

Article CAS PubMed Google Scholar

He, J., Ling, J. & Chiu, P. Vinyl epoxides in organic synthesis. Chem. Rev. 114, 8037–8128 (2014).

Article CAS PubMed Google Scholar

Parker, R. E. & Isaacs, N. S. Mechanisms of epoxide reactions. Chem. Rev. 59, 737–799 (1959).

Article CAS Google Scholar

Posner, G. H. & Rogers, D. Z. Organic reactions at alumina surfaces. Mild and selective opening of epoxides by alcohols, thiols, benzeneselenol, amines, and acetic acid. J. Am. Chem. Soc. 99, 8208–8214 (1977).

Article CAS Google Scholar

Swaving, J. & de Bont, J. A. M. Microbial transformation of epoxides. Enzym. Microb. Technol. 22, 19–26 (1998).

Article CAS Google Scholar

Fretland, A. J. & Omiecinski, C. J. Epoxide hydrolases: biochemistry and molecular biology. Chem. Biol. Interact. 129, 41–59 (2000).

Article CAS PubMed Google Scholar

Morisseau, C. & Hammock, B. D. Epoxide hydrolases: mechanisms, inhibitor designs, and biological roles. Ann. Rev. Pharmacol. Toxicol. 45, 311–333 (2005).

Article CAS Google Scholar

Steckbeck, S. R., Nelson, J. A. & Spencer, T. A. Enzymic reduction of an epoxide to an alcohol. J. Am. Chem. Soc. 104, 893–895 (1982).

Article CAS Google Scholar

Tsypik, O. et al. Oxidative carbon backbone rearrangement in rishirilide biosynthesis. J. Am. Chem. Soc. 142, 5913–5917 (2020).

Article CAS PubMed Google Scholar

Akiyama, T. et al. Fluostatins A and B, new inhibitors of dipeptidyl peptidase III, produced by Streptomyces sp. TA-3391. I. Taxonomy of producing strain, production, isolation, physico-chemical properties and biological properties. J. Antibiot. 51, 553–559 (1998).

Article CAS Google Scholar

Baur, S. et al. Fluostatins C-E, novel members of the fluostatin family produced by Streptomyces strain Acta 1383. J. Antibiot. 59, 293–297 (2006).

Article CAS Google Scholar

Feng, Z., Kim, J. H. & Brady, S. F. Fluostatins produced by the heterologous expression of a TAR reassembled environmental DNA derived type II PKS gene cluster. J. Am. Chem. Soc. 132, 11902–11903 (2010).

Article CAS PubMed PubMed Central Google Scholar

Zhang, W. et al. Fluostatins I-K from the South China Sea-derived Micromonospora rosaria SCSIO N160. J. Nat. Prod. 75, 1937–1943 (2012).

Article CAS PubMed Google Scholar

Zhang, W. et al. Pyrazolofluostatins A-C, pyrazole-fused benzo[a]fluorenes from South China Sea-derived Micromonospora rosaria SCSIO N160. Org. Lett. 19, 592–595 (2017).

Article CAS PubMed Google Scholar

Jin, J. et al. Fluostatins M-Q featuring a 6-5-6-6 ring skeleton and high oxidized A-rings from marine Streptomyces sp. PKU-MA00045. Mar. Drugs 16, 87 (2018).

Article PubMed Central CAS Google Scholar

Huang, C. et al. Molecular basis of dimer formation during the biosynthesis of benzofluorene-containing atypical angucyclines. Nat. Commun. 9, 2088 (2018).

Article ADS PubMed PubMed Central CAS Google Scholar

Huang, C. et al. Marine bacterial aromatic polyketides From host-dependent heterologous expression and fungal mode of cyclization. Front. Chem. 6, 528 (2018).

Article ADS CAS PubMed PubMed Central Google Scholar

Huang, C. et al. Discovery of stealthin derivatives and implication of the amidotransferase FlsN3 in the biosynthesis of nitrogen-containing fluostatins. Mar. Drugs 17, 150 (2019).

Yang, C. et al. Inactivation of flavoenzyme-encoding gene flsO1 in fluostatin biosynthesis leads to diversified angucyclinone derivatives. J. Org. Chem. 86, 11019–11028 (2021).

Article CAS PubMed Google Scholar

Huang, C. et al. Discovery of an unexpected 1,4-oxazepine-linked seco-fluostatin heterodimer by inactivation of the oxidoreductase-encoding gene flsP. J. Nat. Prod. 84, 2336–2344 (2021).

Article CAS PubMed Google Scholar

Wang, B. et al. Identification of Alp1U and Lom6 as epoxy hydrolases and implications for kinamycin and lomaiviticin biosynthesis. Nat. Commun. 6, 7674 (2015).

Article ADS PubMed Google Scholar

Woo, C. M., Beizer, N. E., Janso, J. E. & Herzon, S. B. Isolation of lomaiviticins C-E, transformation of lomaiviticin C to lomaiviticin A, complete structure elucidation of lomaiviticin A, and structure-activity analyses. J. Am. Chem. Soc. 134, 15285–15288 (2012).

Article CAS PubMed Google Scholar

Kim, L. J. et al. Structure revision of the lomaiviticins. J. Am. Chem. Soc. 143, 6578–6585 (2021).

Article CAS PubMed PubMed Central Google Scholar

Jiang, X. et al. Isolation, structure elucidation and biosynthesis of benzo[b]fluorene nenestatin A from deep-sea derived Micromonospora echinospora SCSIO 04089. Tetrahedron 73, 3585–3590 (2017).

Article CAS Google Scholar

Fang, Z. et al. S-Bridged thioether and structure-diversified angucyclinone derivatives from the South China Sea-derived Micromonospora echinospora SCSIO 04089. J. Nat. Prod. 83, 3122–3130 (2020).

Article CAS PubMed Google Scholar

Jiang, X. et al. Discovery of a new asymmetric dimer nenestatin B and implications of a dimerizing enzyme in a deep sea actinomycete. Org. Biomol. Chem. 19, 4243–4247 (2021).

Article CAS PubMed Google Scholar

Colis, L. C. et al. The cytotoxicity of (-)-lomaiviticin A arises from induction of double-strand breaks in DNA. Nat. Chem. 6, 504–510 (2014).

Article CAS PubMed PubMed Central Google Scholar

Herzon, S. B. The mechanism of action of (-)-lomaiviticin A. Acc. Chem. Res. 50, 2577–2588 (2017).

Article CAS PubMed PubMed Central Google Scholar

Kharel, M. K. et al. Angucyclines: biosynthesis, mode-of-action, new natural products, and synthesis. Nat. Prod. Rep. 29, 264–325 (2012).

Article CAS PubMed Google Scholar

Wang, Y., Zhang, C., Zhao, Y. L., Zhao, R. & Houk, K. N. Understand the specific regio- and enantioselectivity of fluostatin conjugation in the post-biosynthesis. Biomolecules 10, E815 (2020).

Article PubMed CAS Google Scholar

Zhang, L. et al. Mutation of an atypical oxirane oxyanion hole improves regioselectivity of the alpha/beta-fold epoxide hydrolase Alp1U. J. Biol. Chem. 295, 16987–16997 (2020).

Article CAS PubMed PubMed Central Google Scholar

Niviere, V., Fieschi, F., Decout, J. L. & Fontecave, M. The NAD(P)H:flavin oxidoreductase from Escherichia coli. Evidence for a new mode of binding for reduced pyridine nucleotides. J. Biol. Chem. 274, 18252–18260 (1999).

Article CAS PubMed Google Scholar

Yang, C., Huang, C., Zhang, W., Zhu, Y. & Zhang, C. Heterologous expression of fluostatin gene cluster leads to a bioactive heterodimer. Org. Lett. 17, 5324–5327 (2015).

Article CAS PubMed Google Scholar

Xiao, Y. et al. Characterization of tiacumicin B biosynthetic gene cluster affording diversified tiacumicin analogues and revealing a tailoring dihalogenase. J. Am. Chem. Soc. 133, 1092–1105 (2011).

Article CAS PubMed Google Scholar

Zhang, H. et al. A simple and facile iodination method of didechlorotiacumicin B and aromatic compounds. Sci. China Chem. 64, 1736–1742 (2021).

Article CAS Google Scholar

Zhang, Q. et al. Characterization of the flavoenzyme XiaK as an N-hydroxylase and implications in indolosesquiterpene diversification. Chem. Sci. 8, 5067–5077 (2017).

Article CAS PubMed PubMed Central Google Scholar

Toth, L. et al. HPLC-ECD and TDDFT-ECD study of hexahydropyrrolo[1,2-a]quinoline derivatives. Chirality 30, 866–874 (2018).

Article CAS PubMed Google Scholar

Lee, J. H., Okuno, Y. & Cavagnero, S. Sensitivity enhancement in solution NMR: emerging ideas and new frontiers. J. Magn. Reson. 241, 18–31 (2014).

Article ADS CAS PubMed PubMed Central Google Scholar

Mega, T. L. & Van Etten, R. L. The oxygen-18 isotope shift in carbon-13 nuclear magnetic resonance spectroscopy. 15. Studies of [18O,1,4-13C2]succinic acid and [18O]dimethylmaleic anhydride. J. Am. Chem. Soc. 115, 12056–12059 (1993).

Article CAS Google Scholar

Lin, S., Horsman, G. P., Chen, Y., Li, W. & Shen, B. Characterization of the SgcF epoxide hydrolase supporting an (R)-vicinal diol intermediate for enediyne antitumor antibiotic C-1027 biosynthesis. J. Am. Chem. Soc. 131, 16410–16417 (2009).

Article CAS PubMed PubMed Central Google Scholar

Bashiri, G., Rehan, A. M., Greenwood, D. R., Dickson, J. M. & Baker, E. N. Metabolic engineering of cofactor F420 production in Mycobacterium smegmatis. PLoS One 5, e15803 (2010).

Article ADS CAS PubMed PubMed Central Google Scholar

Bashiri, G. et al. A revised biosynthetic pathway for the cofactor F420 in prokaryotes. Nat. Commun. 10, 1558 (2019).

Article ADS PubMed PubMed Central CAS Google Scholar

Bashiri, G. Cofactor F420, an emerging redox power in biosynthesis of secondary metabolites. Biochem. Soc. Trans. 50, 253–267 (2022).

Article CAS PubMed Google Scholar

Walsh, C. Flavin coenzymes - at the crossroads of biological redox chemistry. Acc. Chem. Res. 13, 148–155 (1980).

Article CAS Google Scholar

Greening, C. et al. Physiology, biochemistry, and applications of F420- and Fo-dependent redox reactions. Microbiol. Mol. Biol. Rev. 80, 451–493 (2016).

Article CAS PubMed PubMed Central Google Scholar

Xu, H. et al. Ocauxarthrol A from Auxarthron umbrinum SCSIO 40432 and configurational reassignment of chrysoqueen and auxarthrols. Tetrahedron Lett. 66, 152482 (2021).

Google Scholar

Ge, X. et al. Anthraquinone derivatives from a marine-derived Fungus Sporendonema casei HDN16-802. Mar. Drugs 17, 334 (2019).

Article CAS PubMed Central Google Scholar

Ye, Q. et al. Construction and co-expression of a polycistronic plasmid encoding carbonyl reductase and glucose dehydrogenase for production of ethyl (S)−4-chloro-3-hydroxybutanoate. Bioresour. Technol. 101, 6761–6767 (2010).

Article CAS PubMed Google Scholar

Su, J. et al. Engineered Thermoplasma acidophilum factor F3 mimics human aminopeptidase N (APN) as a target for anticancer drug development. Bioorg. Med. Chem. 19, 2991–2996 (2011).

Article CAS PubMed Google Scholar

Mostad, S. B., Helming, H. L., Groom, C. & Glasfeld, A. The stereospecificity of hydrogen transfer to NAD(P)+ catalyzed by lactol dehydrogenases. Biochem. Biophys. Res. Commun. 233, 681–686 (1997).

Article CAS PubMed Google Scholar

Saini, P. & Sareen, D. An overview on the enhancement of enantioselectivity and stability of microbial epoxide hydrolases. Mol. Biotechnol. 59, 98–116 (2017).

Article CAS PubMed Google Scholar

Bashiri, G. & Baker, E. N. Convergent pathways to biosynthesis of the versatile cofactor F420. Curr. Opin. Struct. Biol. 65, 9–16 (2020).

Article CAS PubMed Google Scholar

Singh, S. K. & Das, A. The n → π* interaction: a rapidly emerging non-covalent interaction. Phys. Chem. Chem. Phys. 17, 9596–9612 (2015).

Article CAS PubMed Google Scholar

Newberry, R. W. & Raines, R. T. The n→π* interaction. Acc. Chem. Res. 50, 1838–1846 (2017).

Article CAS PubMed PubMed Central Google Scholar

Chang, J. A., Kresge, A. J., Nikolaev, V. A. & Popik, V. V. The 2-oxocyclohexanecarboxylic acid keto−enol system in aqueous solution. J. Am. Chem. Soc. 125, 6478–6484 (2003).

Article CAS PubMed Google Scholar

Romero, E., Gomez Castellanos, J. R., Gadda, G., Fraaije, M. W. & Mattevi, A. Same substrate, many reactions: oxygen activation in flavoenzymes. Chem. Rev. 118, 1742–1769 (2018).

Article CAS PubMed Google Scholar

Zhang, Y. et al. Aryl C–H iodination: are there actual flavin-dependent iodinases in nature? Sci. China Chem. 64, 1730–1735 (2021).

Article CAS Google Scholar

Donnet, J. B. The chemical reactivity of carbons. Carbon 6, 161–176 (1968).

Article CAS Google Scholar

Leisch, H., Morley, K. & Lau, P. C. K. Baeyer−Villiger monooxygenases: more than just green chemistry. Chem. Rev. 111, 4165–4222 (2011).

Article CAS PubMed Google Scholar

Wang, Y. S. et al. Molecular basis for the final oxidative rearrangement steps in chartreusin biosynthesis. J. Am. Chem. Soc. 140, 10909–10914 (2018).

Article CAS PubMed Google Scholar

Peris, G. & Miller, S. J. A nonenzymatic acid/peracid catalytic cycle for the Baeyer−Villiger oxidation. Org. Lett. 10, 3049–3052 (2008).

Article CAS PubMed PubMed Central Google Scholar

Shibuya, M. et al. Origin of structural diversity in natural triterpenes: direct synthesis of seco-triterpene skeletons by oxidosqualene cyclase. J. Am. Chem. Soc. 129, 1450–1455 (2007).

Article CAS PubMed Google Scholar

Harmata, M. & Elahmad, S. An intramolecular 4+3 cycloaddition-vinylogous grob fragmentation route to a tricyclo[6.3.0.02,4] undecene ring system. Tetrahedron Lett. 34, 789–792 (1993).

Article CAS Google Scholar

Valente, P., Avery, T. D., Taylor, D. K. & Tiekink, E. R. T. Synthesis and chemistry of 2,3-dioxabicyclo[2.2.2]octane-5,6-diols. J. Org. Chem. 74, 274–282 (2009).

Article CAS PubMed Google Scholar

Drenth, J. & Fraaije, M. W. In Flavin‐Based Catalysis: Principles and Applications (eds Cibulka, R. & Fraaije, M.). (Wiley‐VCH Verlag GmbH & Co. KGaA, 2021).

Piano, V., Palfey, B. A. & Mattevi, A. Flavins as covalent catalysts: new mechanisms emerge. Trends Biochem. Sci. 42, 457–469 (2017).

Article CAS PubMed Google Scholar

Mehra-Chaudhary, R., Dai, Y., Sobrado, P. & Tanner, J. J. In crystallo capture of a covalent intermediate in the UDP-galactopyranose mutase reaction. Biochemistry 55, 833–836 (2016).

Article CAS PubMed Google Scholar

Sobrado, P. Noncanonical reactions of flavoenzymes. Int. J. Mol. Sci. 13, 14219–14242 (2012).

Article CAS PubMed PubMed Central Google Scholar

White, M. D. et al. UbiX is a flavin prenyltransferase required for bacterial ubiquinone biosynthesis. Nature 522, 502–506 (2015).

Article ADS CAS PubMed PubMed Central Google Scholar

Mishanina, T. V. et al. An unprecedented mechanism of nucleotide methylation in organisms containing thyX. Science 351, 507–510 (2016).

Article ADS CAS PubMed PubMed Central Google Scholar

Dai, Y. et al. Flavin-N5 covalent intermediate in a nonredox dehalogenation reaction catalyzed by an atypical flavoenzyme. ChemBioChem 19, 53–57 (2018).

Article CAS PubMed Google Scholar

Mansoorabadi, S. O., Thibodeaux, C. J. & Liu, H. W. The diverse roles of flavin coenzymes-nature's most versatile thespians. J. Org. Chem. 72, 6329–6342 (2007).

Article CAS PubMed PubMed Central Google Scholar

Wo, J. et al. Transformation of streptonigrin to streptonigrone: flavin reductase-mediated flavin-catalyzed concomitant oxidative decarboxylation of picolinic acid derivatives. ACS Catal. 6, 2831–2835 (2016).

Article CAS Google Scholar

Zhang, G. et al. Mechanistic insights into polycycle formation by reductive cyclization in ikarugamycin biosynthesis. Angew. Chem. Int. Ed. 53, 4840–4844 (2014).

Article CAS Google Scholar

MacroModel; Schrödinger LLC. http://www.schrodinger.com/MacroModel (2015).

Frisch, M. et al. Gaussian 16. Gaussian, Inc. Wallingford, CT (2016).

Stephens, P. J. & Harada, N. ECD cotton effect approximated by the Gaussian curve and other methods. Chirality 22, 229–233 (2010).

CAS PubMed Google Scholar

Varetto, U. Molekel 5.4. 0.8. Swiss National Supercomputing Centre, Manno, Switzerland (2009).

Gildea, R. J. et al. iotbx.cif: a comprehensive CIF toolbox. J. Appl. Crystallogr. 44, 1259–1263 (2011).

Article CAS PubMed PubMed Central Google Scholar

Sheldrick, G. M. SHELXT - integrated space-group and crystal-structure determination. Acta Crystallogr. A Found. Adv. 71, 3–8 (2015).

Article PubMed PubMed Central MATH CAS Google Scholar

Download references

This work is supported in part by the National Natural Science Foundation of China (31820103003 to C.Z., 42176127 to W.Z., 41676165 to W.Z., 31630004 to C.Z., and 31700042 to C.Y.); Key Science and Technology Project of Hainan Province (ZDKJ202018 to C.Z.); MOST (2018YFA0901903 to Y.Z.); K.C. Wong Education Foundation (GJTD-2020-12 to C.Z.); the Guangdong Provincial Special Fund for Marine Economic Development Project (GDNRC[2021] 48 to C.Z.); Southern Marine Science and Engineering Guangdong Laboratory (Guangzhou) (GML2019ZD0406 to C.Z.); Youth Innovation Promotion Association CAS (2022349 to C. Y.) and the Science and Technology Planning Project of Guangzhou (202102020471 to C.Y.). B.C.D. acknowledges the support of CAS-TWAS President's PhD Fellowship. H.-w.L. acknowledges the support of Welch Foundation (F-1511). G.B. is supported by a Sir Charles Hercus Fellowship through the Health Research Council of New Zealand. We appreciate Professor Keqiang Fan from Institute of Microbiology, Chinese Academy of Sciences, for the generous gift of compound 30. We would like to thank Professor Tadhg Begley of Texas A& M University for useful discussion. We are grateful to Dr. Z. H. Xiao, X. H. Zheng, A. J. Sun, Y. Zhang, and X. Ma in the equipment public service center at SCSIO for recording spectroscopic data. We also thank the data archive support from the National Earth System Data Center, National Science & Technology Infrastructure of China (http:// www.geodata.cn).

These authors contributed equally: Bidhan Chandra De, Wenjun Zhang.

Key Laboratory of Tropical Marine Bioresources and Ecology, Guangdong Key Laboratory of Marine Materia Medica, South China Sea Institute of Oceanology, Chinese Academy of Sciences, Guangzhou, 510301, China

Bidhan Chandra De, Wenjun Zhang, Chunfang Yang, Chunshuai Huang, Liping Zhang, Wei Liu, Yiguang Zhu & Changsheng Zhang

University of Chinese Academy of Sciences, 19 Yuquan Road, Beijing, 100049, China

Bidhan Chandra De, Wenjun Zhang, Chunfang Yang, Liping Zhang, Yiguang Zhu & Changsheng Zhang

Southern Marine Science and Engineering Guangdong Laboratory (Guangzhou), 1119 Haibin Road, Nansha District, Guangzhou, 511458, China

Wenjun Zhang, Chunfang Yang, Liping Zhang, Yiguang Zhu & Changsheng Zhang

Sanya Institute of Ocean Eco-Environmental Engineering, Yazhou Scientific Bay, Sanya, 572000, China

Wenjun Zhang, Chunfang Yang, Yiguang Zhu & Changsheng Zhang

Department of Organic Chemistry, University of Debrecen, P.O. Box 400, H-4002, Debrecen, Hungary

Attila Mándi & Tibor Kurtán

Division of Chemical Biology & Medicinal Chemistry, College of Pharmacy, and Department of Chemistry, University of Texas at Austin, Austin, TX, 78712, USA

Mark W. Ruszczycky & Hung-wen Liu

State Key Laboratory of Natural and Biomimetic Drugs, School of Pharmaceutical Sciences, Peking University, 38 Xueyuan Road, Haidian District, Beijing, 100191, China

Ming Ma

Laboratory of Molecular and Microbial Biochemistry, School of Biological Sciences, The University of Auckland, Auckland, New Zealand

Ghader Bashiri

You can also search for this author in PubMed Google Scholar

You can also search for this author in PubMed Google Scholar

You can also search for this author in PubMed Google Scholar

You can also search for this author in PubMed Google Scholar

You can also search for this author in PubMed Google Scholar

You can also search for this author in PubMed Google Scholar

You can also search for this author in PubMed Google Scholar

You can also search for this author in PubMed Google Scholar

You can also search for this author in PubMed Google Scholar

You can also search for this author in PubMed Google Scholar

You can also search for this author in PubMed Google Scholar

You can also search for this author in PubMed Google Scholar

You can also search for this author in PubMed Google Scholar

You can also search for this author in PubMed Google Scholar

B.C.D., W.Z., C.Y., H.C., L.P., and W.L. performed epoxide opening reactions, compound isolation, and structure determination. A.M. and T.K. conducted the ECD calculations. M.M. and G.B. contributed key compound and reagents. B.C.D., W.Z., M.W.R., Y.Z., T.K., H.w.L., and C.Z. analyzed the data and wrote the manuscript. C.Z. and H.w.L. directed the research. B.C.D. and W.Z. contributed equally to this work.

Correspondence to Hung-wen Liu or Changsheng Zhang.

The authors declare no competing interests.

Nature Communications thanks Xudong Qu, and the other anonymous reviewer(s) for their contribution to the peer review of this work. Peer reviewer reports are available.

Publisher's note Springer Nature remains neutral with regard to jurisdictional claims in published maps and institutional affiliations.

Open Access This article is licensed under a Creative Commons Attribution 4.0 International License, which permits use, sharing, adaptation, distribution and reproduction in any medium or format, as long as you give appropriate credit to the original author(s) and the source, provide a link to the Creative Commons license, and indicate if changes were made. The images or other third party material in this article are included in the article's Creative Commons license, unless indicated otherwise in a credit line to the material. If material is not included in the article's Creative Commons license and your intended use is not permitted by statutory regulation or exceeds the permitted use, you will need to obtain permission directly from the copyright holder. To view a copy of this license, visit http://creativecommons.org/licenses/by/4.0/.

Reprints and Permissions

De, B.C., Zhang, W., Yang, C. et al. Flavin-enabled reductive and oxidative epoxide ring opening reactions. Nat Commun 13, 4896 (2022). https://doi.org/10.1038/s41467-022-32641-1

Download citation

Received: 09 April 2022

Accepted: 08 August 2022

Published: 20 August 2022

DOI: https://doi.org/10.1038/s41467-022-32641-1

Anyone you share the following link with will be able to read this content:

Sorry, a shareable link is not currently available for this article.

Provided by the Springer Nature SharedIt content-sharing initiative

Nature Communications (2022)

By submitting a comment you agree to abide by our Terms and Community Guidelines. If you find something abusive or that does not comply with our terms or guidelines please flag it as inappropriate.