In Vivo Investigation of the Roles of FdmM and FdmM1 in Fredericamycin Biosynthesis Unveiling a New Family of Oxygenases*

Fredericamycin (FDM) A, a highly oxidized aromatic pentadecaketide natural product, exhibits potent cytotoxicity and has been studied as a new anticancer drug lead. The FDM biosynthetic gene cluster has been previously cloned from Streptomyces griseus ATCC 49344 and successfully expressed in the heterologous host Streptomyces albus J1074. The fdmM and fdmM1 genes code for two proteins with high sequence homology to each other but unknown function. In-frame deletion of each of the genes from the fdm cluster was accomplished in the S. albus host. Each mutant failed to produce FDM A and the key biosynthetic intermediate FDM E but produced various new metabolites, the titers of which were dramatically increased via overexpression of an fdm pathway-specific activator fdmR1. The ΔfdmM mutant strain accumulated three new compounds FDM M-1, FDM M-2, and FDM M-3, whereas the ΔfdmM1 mutant strain produced one new compound FDM M1-1. Isolation and structural characterization of these compounds enable us to propose that FdmM and FdmM1 catalyze the C-6 and C-8 hydroxylations for FDM biosynthesis, respectively. Homologs of FdmM and FdmM1 can be found in biosynthetic gene clusters of many other aromatic polyketides, ranging from dodecaketides to pentadecaketides, but to date all of them were annotated as proteins of unknown function. Based on the findings reported here for FdmM and FdmM1, we now propose similar functions for those proteins, and FdmM and FdmM1 therefore represent an emerging family of novel oxygenases responsible for hydroxylation of aromatic polyketide natural products.

Studies on natural product biosynthetic pathways have uncovered a number of intriguing oxygenases. For instance, the first reported metal-and cofactor-free monooxygenase TcmH is responsible for quinone moiety formation in tetracenomycin D3 and represents a rapidly growing family of antibiotic biosynthetic monooxygenases (1,2). Another example is DpgC, which is involved in the biosynthesis of vancomycin building block 3, 5-dihydroxyphenylglycine. The crystal structure of DpgC has been used to understand the reaction mechanism of metal-and cofactor-free dioxygenases (3). MomA, involved in mompain biosynthesis (4) is a metal ion-dependent monooxygenase belonging to the cupin superfamily of oxidases bearing no prosthetic group. The discovery of enzymes such as TcmH, DpgC, and MomA continually encourage the community to search for and characterize new oxygenases from proteins of unknown functions involved in natural products biosynthesis.
We report here in vivo investigations of the roles of FdmM and FdmM1 in the biosynthesis of 1 by (i) construction of ⌬fdmM and ⌬fdmM1 mutants, respectively and (ii) structural characterization of the accumulated metabolites for each mutant. These data provide new insights into the biosynthesis of 1 and unveil FdmM and FdmM1 as members of an emerging family of novel oxygenases involved in aromatic polyketide biosynthesis.

EXPERIMENTAL PROCEDURES
General-IR spectra were measured on a Bruker EQUINOX 55/S FT-IR/NIR spectrophotometer (Ettlingen). Electrospray ionization mass spectroscopy (ESI-MS) or high-resolution (HR) ESI-MS was performed on an Agilent 1100 HPLC-MSDSL ion trap mass spectrometer (Santa Clara, CA). Atmospheric pressure chemical ionization mass spectroscopy (APCI-MS) was performed on an Agilent 1100 VL APCI mass spectrometer (Santa Clara, CA). HR Matrix-Assisted Laser Desorption Ionization-Fourier Transform (MALDI-FT)-MS was measured on an IonSpec HiResMALDI FT mass spectrometer (Lake Forest, CA). NMR data were obtained using a Varian Unity Inova 500 MHz NMR spectrometer (Palo Alto, CA). Analytical or semipreparative HPLC was carried on a Varian HPLC system with in-line Prostar 330 PDA detector (Woburn, MA). The cytotoxity assay of FDM compounds was performed as described previously (14). Bacterial Strains and Culture Conditions-Streptomyces albus J1074 was used as heterologous expression host (12). For protoplast preparation, S. albus was grown in YEME medium (16). Escherichia coli ET12567/pUZ8002 (17) and BW25113 (18) were used for intergeneric conjugation and RED-mediated PCR-targeting mutagenesis, respectively. S. albus recombinant strains were cultured in R2YE medium to prepare seed cultures, and then inoculated to production medium and cultured at 28°C, 250 rpm for FDM production as described previously (12). The production medium consisted of 8 g of yeast extract, 20 g of malt extract, 2 g of NaCl, 10 g of MOPS sodium salt in 500 ml of tap water, and 380 ml of Milli-Q water (Millipore Corp, Bedford, MA). After autoclaving, 1 ml of 10% MgSO 4 , 1 ml of 1% FeSO 4 , 0.1 ml of 10% ZnSO 4 , and 120 ml of 50% glucose were added. The concentrations of antibiotics used for selection were ampicillin (100 g/ml), apramycin (50 g/ml), chloramphenicol (25 g/ml), and thiostrepton (10 g/ml) (16).
Plasmids and DNA Manipulation-General DNA manipulations were performed as described (17). MYME was used for genomic DNA isolation (16). Protoplast transformation and intergeneric conjugation were performed as previously described (19). PCR reactions were performed with the GoTaq DNA polymerase kit (Promega, Madison, WI) or Platinum Pfx DNA polymerase kit (Invitrogen, Carlsbad, CA). RED-mediated recombination was carried out according to the standard procedure (18). Plasmids pSET152, pWHM1250, pKC1218, and pBS4028 were described previously (19).

Construction of the ⌬fdmM and ⌬fdmM1
In-frame Deletion Mutant Strains-The inactivation of fdmM and fdmM1 took advantage of the successful heterologous expression of the fdm cluster carried by pBS4028 in S. albus (12). The fdmM gene in pBS4028 was disrupted by replacing a 0.4-kb fragment internal fdmM with the 1.4-kb aac(3)IVϩoriT cassette through REDmediated recombination; the primers fdmMf and fdmMr (supplemental Table S1) were used for cloning the aac(3)IVϩoriT cassette used in fdmM inactivation. The ⌬fdmM in-frame-deleted fdm heterologous expression plasmid pBS4052 was obtained by excising the aac(3)IVϩoriT cassette with XbaI and self-ligation. Correct construction of pBS4052 was confirmed by DNA sequencing and PCR using primers fdmMM1a and fdmMM1b (supplemental Table S1 and Fig. S2). The ⌬fdmM recombinant mutant strain SB4021 was afforded by transforming pBS4052 into S. albus J1074.
The ⌬fdmM1 in-frame-deleted fdm heterologous plasmid pBS4053 was constructed from pBS4028 in a similar way as pBS4052 using the primers fdmM1f and fdmM1r (supplemental Table S1). Following confirmation by sequencing and PCR using fdmMM1a and fdmMM1b as primers (supplemental Table S1), pBS4053 was transformed to S. albus to afford the ⌬fdmM1 recombinant mutant strain SB4022 (supplemental Fig. S3).
Complementation of SB4021 and SB4022-The 2.5-kb BamHI/NcoI fragment containing fdmKLM was excised and inserted into the same sites of pET28a. The resultant plasmid was cut off a 0.7-kb ApaLI fragment and self-ligated. Then, the entire fdmM gene together with its native promoter was removed as a 1.9-kb EcoRI/XbaI fragment and inserted into the same sites of pKC1218 to generate pBS4054. Plasmid pBS4054 was introduced into SB4021 by E. coli-Streptomyces conjugation, affording the ⌬fdmM-complemented strain SB4023. The 1.0-kb EcoRV/KpnI fragment, containing fdmM1 and its native promoter, was inserted into the same sites of pET29a. The same locus was then removed as a 1.1-kb EcoRI/XbaI fragment and inserted into the same sites of pKC1218 to yield pBS4055. Introduction of pBS4055 into SB4021 finally afforded the ⌬fdmM1 complemented strain SB4024.
Overexpression of fdmR1 in SB4021 and SB4022-Plasmid pBS4045 (19) was cut by HindIII and blunted by DNA polymerase I large (Klenow) fragment (Promega). A 2.5-kb fragment containing fdmR1 downstream of ErmE * promoter was excised by EcoRI and inserted into the EcoRI/EcoRV sites of pSET152 to generate pBS4056. Introducing pBS4056 into SB4021 and SB4022 by E. coli-Streptomyces conjugation afforded SB4025 and SB4026, respectively.
Production and Isolation of 12, 13, and 14-Growth of S. albus SB4025 to produce 12, 13, and 14 was done in a fashion similar to that for FDM production in S. griseus (14). Briefly, the seed cultures were prepared by inoculating spores into R2YE medium and growing at 28°C, 250 rpm for 1 day, added to the production medium (2%, v/v), and the resulting cultures were grown for 8 days under the same conditions. For preparation of compound 12 cultures were grown for 5 days instead of the usual 8 days. Cultures were acidified to pH 2.0 with 2 M HCl and centrifuged. The pellet (mycelia and any other precipitate) was harvested and extracted three times with acetone. Follow-ing solvent removal in vacuo, the resulting residue was extracted with EtOAc three times. Solvent removal in vacuo was followed by chromatography over a polyamide 6 column (Fluka, Steinheim, Germany) using CHCl 3 (14). Solvents tested for NMR data collection of 13 included acetone, MeOD, CDCl 3 , MeOD-CDCl 3 in different ratios, DMSO, DMF, pyridine, and trifluoroacetic acid.
Production and Isolation of 15-Compound 15 was produced by SB4026 using the same culture procedures described for SB4025. Isolation of 15 was executed using the same procedure applied to 13 and 14, except that 15 was eluted from the polyamide 6 column with a solvent of 200:50:1.0 (CHCl 3 -MeOH-HCO 2 H). When subjected to silica gel chromatography, 15 was eluted by CHCl 3 -MeOH-AcOH 140:60:0.4 and was completely eluted by a solvent ratio of 140:60:1.0. Partially purified 15 was further refined by semi-preparative HPLC affording pure 15 for NMR spectroscopy.

Construction and Evaluation of the ⌬fdmM and ⌬fdmM1
In-frame Deletion Mutants-Inactivation of both fdmM and fdmM1 was carried out on the basis of successful heterologous expression of the fdm cluster in S. albus (12). For fdmM, a 0.4-kb internal fragment of fdmM was replaced by the aac(3)IVϩoriT cassette through RED-mediated PCR-targeting protocol (18) in plasmid pBS4028 (19). The cassette was then removed by XbaI leaving an 81-bp scar in the resultant construct pBS4052. The ⌬fdmM in-frame deletion recombinant mutant strain SB4021 was generated by transforming pBS4052 into S. albus. When cultured in production medium, SB4021 failed to produce 1 and 10 but instead yielded three new compounds FDM M-1 (12), FDM M-2 (13), and FDM M-3 (14) in very low titer. SB4021 was complemented by in trans expression of fdmM with its native promoter to afford SB4023, in which production of 1 and 10 was restored with the concomitant disappearance of 12, 13, and 14. Titers of 12, 13, and 14 were dramatically increased (Ͼ12-fold) by overexpression of an fdm pathway specific activator fdmR1 (19) in SB4021 to afford SB4025 (Fig. 3a). The titer enhancement in SB4025 vastly hastened isolation and characterization of the three accumulated compounds.
The ⌬fdmM1 in-frame deletion expression plasmid pBS4053 was constructed from pBS4028 in a fashion similar to that used to make pBS4052, affording the mutated fdm cluster with a 0.4-kb internal fragment of fdmM1 being substituted with an 81-bp scar. Transformation of pBS4053 into S. albus afforded the ⌬fdmM1 in-frame deletion recombinant mutant strain SB4022, in which production of 1 and 10 was abolished. HPLC analysis of the SB4022 metabolite profile revealed two minor peaks at 12.8 and 15.4 min. When the activator FdmR1 was overproduced in SB4022 to afford SB4026, the titer of FDM M1-1 (15), with retention time at 12.8 min, was increased by ϳ25-fold. In contrast, there was almost no change for the compound eluting at 15.4 min in SB4022 and SB4026, implying that this compound has no relationship to the fdm biosynthetic pathway. Complementation of the ⌬fdmM1 mutation was achieved by introducing a plasmid, pBS4055 carrying fdmM1 with its native promoter into SB4022, restoring the production of both 1 and 10 (Fig. 3b).
Isolation and Characterization of 12, 13, and 14-Compounds 12, 13, and 14 were extracted from the pellet of acidified SB4025 culture with acetone. Following re-extraction with ethyl acetate, the concentrated extract was subjected to several rounds of chromatography. The three compounds were separated by silica gel chromatography and refined using semi-preparative reverse phase HPLC. Compounds 12, 13, and 14 were isolated as yellow, purple, and red solids, respectively. Compound 12 was found to be very unstable; com-  (Table 1). After exhaustive testing, 13 was found to be soluble in trifluoroacetic acid. However, the use of trifluoroacetic acid rapidly and quantitatively converted 13 to the dehydration product FDM M-4 (16) (Fig. 2) Fig. 4). The right half of 16 (C-1 to C-4 and C-19 to C-30) showed NMR data almost identical to that of previously reported FDM C1 (17) (13), strongly supporting the notion that 16 and 17 possess the same ring D, E, F, and diene side chain structures. Ring A of 16 was assigned to be in the quinone oxidation state based on gHMBC correlations from H-12 (6.43 ppm) to C-10 (180.0 ppm) and C-13 (188.0 ppm). Comparison of the 1 H NMR spectra of 16 and 17 revealed that 16 possessed two extra proton signals at 8.14 ppm and 8.51 ppm. One proton was assigned as H-8 (8.14 ppm) in ring B based on its HSQC correlation to C-8 (129.1 ppm) and gHMBC correlations to C-10 and C-14 (106 ppm); the other was determined as H-6 (8.51 ppm) by its HSQC correlation to C-6 (124.6 ppm) and gHMBC correlations to C-4 (119.4 ppm), C-8, and C-18 (127.6). The structures of ring B and C of 16 were confirmed by gHMBC correlations originating from H-6, H-8, and H-12 (Fig. 4). The angular ring structure of 16, supported by NMR data, was consistent with the proposed FDM biosyn-thetic pathway. Comparison of the molecular weight of 13 and 16 suggested that 16 was generated from 13 via dehydrative cyclization (Fig. 2). This was confirmed by analysis of the 1 H NMR spectra of 13 and 16. The two ␣-proton signals at C-24 (4.21 ppm) of 13 were shifted and replaced to a single proton signal at C-24 (6.35 ppm) of 16, supporting the formation of lactone ring F in going from 13 to 16. Further evidence supporting this transformation was that 16 lacked the peak at 1593 cm Ϫ1 present in the IR spectrum of 13; the C-25 keto group of 13 is absent in 16.
HR  (Fig. 2). The mass detected for 18 supported its formula as C 31 H 23 O 9 (calculated 539.1337 for the [MϩH] ϩ ion). Analyses of the 1 H, 13 C, and two-dimensional (gCOSY, HSQC, and gHMBC) NMR spectra of 18 enabled us to propose its structure (Table 1 and Fig. 4). The only difference between 17 and 18 is the C-6 hydroxyl group of 17, which is absent in 18. This was consistent with the almost identical nature of 1 H and 13 C NMR data for 17 and 18 except for data relating to ring C. The 1 H NMR signal at 8.81 ppm, HSQC correlation to C-6 (120.4 ppm) and gHMBC correlations from H-6 to C-8 (187.2 ppm) and C-18 (133.8 ppm) support the C-6 phenyl proton of 18. Compound 18 was proposed to be the dehydrated derivative of 14 according to their mass difference. By analogy to the conversion of 13 to 16, dehydrative cyclization of 14 affords the lactone ring F of 18. As with 16, this is substantiated by the absence of the carbonyl IR stretch at 1592 cm Ϫ1 for 18, which is present in 14.
Compound 12 was found to be very unstable and, consistent with its predicted reactivity, converts to oxidized species 13 and 14 during culture and isolation. Accordingly, SB4025 was cultured in production medium for 5 days, instead of 8 days, to optimize the chance of isolating 12. All manipulations were carried out under 20°C to minimize loss of 12. Subsequent HR ESI-MS analysis of purified 12 revealed an [M-H] Ϫ ion at m/z 541.1479, consistent with formula C 31 H 25 O 9 (calculated 541.1504 for the [M-H] Ϫ ion). The tentative formula for 12 bore two protons more than 13. 1 H NMR of 12 (Table 1) revealed a spectrum almost identical to that of 13, with the notable exception that 12 was determined to be in the hydroquinone oxidation state. This structure assignment was supported by the fact that 12 can be converted to 13 and 14 spontaneously in air. Furthermore, IR spectra revealed that 12 lacks IR bands typically associated with the presence of quinones (1684 cm Ϫ1 in 13 and 1676 cm Ϫ1 in 14).
Conversion of 12 to 13 and 14-During the growth of SB4025 in production medium it was noted that 12 is produced prior to 13 and 14. It was also observed that 12 was very unstable and was primarily converted to 13 during the course of isolations at room temperature. When 12 was dissolved in acetone (922 M) under aerobic conditions at 30°C for 6 h, it was almost completely converted to 13 and 14 in a ratio of 1:3 (supplemental Fig. S4a). Analogous conditions devoid of O 2 led to significantly reduced production of 13 and 14 from 12 (supplemental Fig.  S4b). To exclude the possibility that 12 was converted to 14 via 13 as an intermediate, a 370 M solution of 13 in acetone was exposed to air at 30°C for 6 h, followed by HPLC analysis of the mixture. No loss of 13 was observed nor was any new product detected.
Isolation and Characterization of 15-Compound 15, a dark blue solid, was isolated from SB4026 culture in a process similar to that used for 13 and 14. It was proposed as an isomer of 14, in that its molecular formula was also determined to be C 31 H 23 (Table 1 and Fig. 4). This molecule has the same right hemisphere as 9 (rings C, D, and E and the diene moiety) as supported by almost identical 1 H and 13 C NMR resonances for C-1 to C-4 and C-19 to C-30. The ring A of 15 was assigned to be in the quinone oxidation state based on gHMBC correlations originating from H-12 (6.49 ppm) to C-10 (175.9 ppm) and C-13 (185.5 ppm). This assignment was confirmed by the similarity of 1 H and 13 C NMR data to that of the ring A of 16. H-8 was assigned based on the chemical shift at 8.49 ppm in 1 H NMR, HSQC correlation to C-8 (121.2 ppm) and the gHMBC correlations from H-8 to C-6 (150 ppm) and C-10. The structure of ring B was determined by the gHMBC correlations from H-8 and H-12 while the structure of ring C was elucidated according to the gHMBC correlations originating from H-8 to C-6 and C-16 (114 ppm) and from H-19 (2.84 ppm) to C-5 (127.5 ppm) and C-18 (129.8 ppm). The structure of 15 as elucidated on the basis of NMR data acquired in d 6 -DMSO was confirmed by NMR experiments conducted in CDCl 3 -MeOD (supplemental Table S2).

DISCUSSION
The FDMs are aromatic polyketides originating from a pentadecaketide (C-30) precursor, representing aromatic polyketides derived from the longest polyketide chain whose biosynthetic machinery has been characterized. With its unique carbaspirocycle, 1 exhibits potent cytotoxicities against selected cancer cell lines, exerts its activities via several novel mode of actions, and has been studied as a new anticancer drug lead (14). Biosynthesis of 1 includes several oxidative reactions, which cannot be assigned to specific enzymes on the basis of bioinformatics analysis of the gene cluster alone (12). These features of 1 heighten the interest in investigations of the biosynthetic pathway for this unique natural product. Feeding experiments (20) and cloning of its biosynthetic gene cluster confirm the polyketide origin of 1 (12). Characterization of intermediates 8, 9, and 10 unveils the final steps en route to 1 and suggests that its carbaspirocycle moiety is formed through a benzilic acid rearrangement process from 10 to 1 (Fig. 2 and Ref. 14). The pathway from 7 to 9, previously unaccounted for, is now significantly illuminated by this work.
Inactivation of two functionally unknown genes, fdmM and fdmM1, was facilitated by successful expression of the fdm cluster in S. albus, a model heterologous host with expedient enabling tools for in vivo genetic pathway manipulations (12). Abolishment of 1 and 10 production in each of the mutant strains could be readily complemented confirming that both genes are essential to FDM biosynthesis. The titers of compounds accumulated in both ⌬fdmM and ⌬fdmM1 in-frame deletion mutant strains were dramatically improved by overexpression of the well studied activator fdmR1 (17). Compound 15 was isolated from SB4026, the ⌬fdmM1 mutant overexpressing FdmR1. Structural comparison of 9 and 15 suggests that FdmM1 catalyzes C-8 hydroxylation of 15 followed by tautomerization to afford 9 (Fig. 2). Compounds 12, 13, and 14 were produced by SB4025, the ⌬fdmM in-frame deletion recombinant mutant strain in which FdmR1 was overproduced. Compound 12 was unstable, rapidly oxidizing to both 13 and 14, under aerobic conditions. The enrichment of 12 prior to 13 and 14 observed during culture, suggests that 12 is the intermediate accumulated in SB4025 whereas 13 and 14 are shunt products derived from 12 by spontaneous oxidization. There are two proposed pathways from 12 to 15 (Fig. 2). The first invokes that 12 is either spontaneously or enzymatically oxidized to 13. Subsequent C-6 hydroxylation of 13 by FdmM would afford 15 (Route A). A second route (Route B) that cannot be excluded, invokes C-6 hydroxylation of 12 by FdmM prior to formation of the quinone-type ring A. Accumulation of 12 in SB4025 clearly demonstrates that the modification steps, including ring D reduction, O-11 methylation, and C-10 hydroxylation, occur prior to C-6 and C-8 hydroxylation.
Investigation of aromatic polyketide biosyntheses revealed that their hydroxylation steps could be accomplished by a diverse set of monooxygenases, including the typical phenol hydroxylase-like FAD-dependent monooxygenase (e.g. RdmE catalyzing aklavinone-11-hydroxylation in Streptomyces purpurascens) (21) and some novel oxygenases. Aclacinomycin 10-hydroxylase involved in rhodomycin biosynthesis in S. purpurascens was reported as the first unveiled hydroxylase using S-adenosyl-L-methionine as a cofactor (22). SnoaL2 and AclR are proposed to be hydroxylases responsible for the conversion from aklavinone to 1-hydroxyaklavinone in nogalamycin and cinerubin biosynthetic pathways, respectively. These hydroxylases are postulated to be evolutionarily related to cyclases based on their primary and tertiary structures (23). However, little is known about the hydroxylation of aromatic polyketide natural products derived from polyketide chains longer than 18 carbons prior to this work. Bioinformatics analysis of the biosyn-thetic gene clusters for these aromatic polyketide natural products fell short of identifying candidates to account for all of the proposed oxidative steps. Instead, these clusters are often characterized with several genes whose deduced products show no sequence homology to proteins of known functions, as exemplified by FdmM and FdmM1.
Characterization of the compounds accumulated from the ⌬fdmM and ⌬fdmM1 mutant strains has enabled us to assign FdmM and FdmM1 as hydroxylases involved in the biosynthesis of 9. Homologs of FdmM and FdmM1 are known, such as BenG (7), LlpB (8), LlpQ (8), Prm-Orf5 (9), GrhM (10), and RubQ (11) (supplemental Fig. S1) involved in the biosynthesis of other aromatic polyketide natural products ranging from dodecaketides to pentadecaketides, and, like FdmM and FdmM1; however, they were all annotated previously as proteins of unknown function. Based on the findings reported here for FdmM and FdmM1, we now propose similar functions for these proteins, catalyzing region-specific hydroxylations in their respective biosynthetic pathways.
Alignment of FdmM and FdmM1 and their homologs reveals that a conserved motif (G/AXGXXAG) embedded within the N-terminal domain of most of these proteins (supplemental Fig. S3), which is reminiscent of the classical N-terminal Rossman fold characteristic of FAD-dependent oxygenases (24). However, the small size of FdmM (149 amino acids) and FdmM1 (154 amino acids) distinguishes these enzymes from the FAD-dependent oxygenases (e.g. p-hydroxybenzoate hydroxylase from E. coli, 394 amino acids) (25). Very few of the known oxygenases are as small as FdmM and FdmM1, with the exception of the aforementioned TcmH family of metal-and cofactor-free monooxygenases (2). Future efforts are clearly warranted to determine the cofactor dependence of FdmM and FdmM1 and to ensure a complete mechanistic understanding of this family of novel oxygenases.
Previous cytotoxity assays of the carbaspirocyclic FDM analogs 1 and 10 revealed that they exhibited comparable bioactivities against the selected cancer cell lines (14). Bioassays of newly isolated planar FDM intermediates 13, 14, and 15, as well as 9, showed their cytotoxicities to be compromised (ranging from one to three orders of magnitude less relative to 1). The significantly reduced potency observed for 9 and 13-15 relative to 1 supports previous assertions that the carbaspirocyclic center of the FDMs is crucial to their bioactivity (14).
Taken together, our ability to correlate specific gene inactivation events, as exemplified here with FdmM and FdmM1, with specific structural modifications to FDM A, supports the significance of S. albus as a heterologous host for combinatorial biosynthesis efforts to produce new FDM analogs. More importantly, the data resulting from this work highlight FdmM and FdmM1 as novel oxygenases previously assigned simply as proteins of unknown function. FdmM and FdmM1 catalyze hydroxylations at the C-6 and C-8 positions of FDM A and, in the heterologous host S. albus, are compatible to genetic inactivations during overexpression of the pathway specific activator FdmR1. The coordination of genetic inactivations and tandem FdmR1 overexpression within a heterologous host highlights the plasticity of the fdm biosynthetic gene cluster establishing an excellent stage for future investigations of FDM A biosynthesis and engineering.