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Appl Environ Microbiol. Apr 2010; 76(7): 2335–2344.
Published online Feb 12, 2010. doi:  10.1128/AEM.01790-09
PMCID: PMC2849233

Identification and Analysis of the Biosynthetic Gene Cluster Encoding the Thiopeptide Antibiotic Cyclothiazomycin in Streptomyces hygroscopicus 10-22[down-pointing small open triangle]

Abstract

Thiopeptide antibiotics are an important class of natural products resulting from posttranslational modifications of ribosomally synthesized peptides. Cyclothiazomycin is a typical thiopeptide antibiotic that has a unique bridged macrocyclic structure derived from an 18-amino-acid structural peptide. Here we reported cloning, sequencing, and heterologous expression of the cyclothiazomycin biosynthetic gene cluster from Streptomyces hygroscopicus 10-22. Remarkably, successful heterologous expression of a 22.7-kb gene cluster in Streptomyces lividans 1326 suggested that there is a minimum set of 15 open reading frames that includes all of the functional genes required for cyclothiazomycin production. Six genes of these genes, cltBCDEFG flanking the structural gene cltA, were predicted to encode the enzymes required for the main framework of cyclothiazomycin, and two enzymes encoded by a putative operon, cltMN, were hypothesized to participate in the tailoring step to generate the tertiary thioether, leading to the final cyclization of the bridged macrocyclic structure. This rigorous bioinformatics analysis based on heterologous expression of cyclothiazomycin resulted in an ideal biosynthetic model for us to understand the biosynthesis of thiopeptides.

The thiopeptides are a family of highly modified, sulfur-containing macrocyclic peptides, such as thiostrepton, thiocillins, and micrococcinic acid (3, 11). Their structures have several common features: a tri- or tetrasubstituted nitrogen heterocycle central domain, a macrocyclic framework, and heavily modified amino acid residues, including thiazoles, oxazoles, and dehydroamino acids (Fig. (Fig.1)1) (3). Members of this family exhibit various biological properties, such as inhibition of ribosomal protein synthesis (24), rennin inhibitory activity (2), and induction of TipA (20). Moreover, many thiopeptide antibiotics show bioactivity against some bacterial strains resistant to most conventional treatments, including methicillin-resistant Staphylococcus aureus (MRSA), penicillin-resistant Streptococcus pneumoniae (PRSP), and vancomycin-resistant enterococci (VRE) (3, 17).

FIG. 1.
Structures of thiostrepton, thiocillin, microncoccinate, and cyclothiazomycin (3).

Early in vitro investigations of these special heterocycles of thiopeptides were performed by organic chemists and included stereoselective synthesis of a γ-lactam acidic hydrolysate of cyclothiazomycin (4) and total synthesis of thiostrepton (21). Extensive research on microccins (5, 19) and lantibiotics (6, 29) described biosynthesis of the thiazole- and dehydroamino acid-containing polypeptides that were derived from ribosomally synthesized prepeptides. Similarly, Lee et al. described a widely conserved gene cluster for toxin biosynthesis and suggested a ribosome biosynthetic pathway for the modified polypeptide containing thiazoles and oxazoles (16).

Recently, Wieland Brown et al. (28) and Kelly et al. (14) identified the gene clusters encoding thiocillin and thiostrepton, respectively, with a probe that targeted hypothetic prepeptide genes, whereas Liao and coworkers (17) took advantage of the conservation of one putative cyclodehydratase. Although most of the biochemical reactions involved in the biosynthetic pathway remain obscure, it is clear that thiopeptides are synthesized ribosomally and then there is a series of posttranslational modifications.

Cyclothiazomycin, which was isolated as a novel selective inhibitor of human plasma rennin, is a unique bridged macrocyclic thiopeptide (2) whose stereo structure was recently revealed by degradation experiments and spectroscopic analysis (10). It contains a dehydroserine, two dehydrothreonine residues, three thiazolines, three thiazoles, and a trisubstituted pyridine. Compared with common thiopeptides, it lacks the characteristic 2- and 3-azole substituent on the central pyridine domain; instead, it has an alanine-derived heterocyclic residue with the (R) configuration, a quaternary sulfide, and two macrocyclic peptide loops (Fig. (Fig.1).1). Moreover, a pair of convertible isomers of cyclothiazomycin B, the cyclothiazomycin analogues produced by Streptomyces sp. strain A307 (10), were identified as Z and E configurations caused by the tautomerization of the dehydrated threonine. These structural traits may indicate that some new genetic elements are likely involved in posttranslational modification.

Here we reported cloning and sequencing of the cyclothiazomycin biosynthetic gene cluster of Streptomyces hygroscopicus 10-22 (23). In addition, an analysis of heterologous expression in Streptomyces lividans 1326 and a deletion analysis were also performed, which indicated that a gene cluster at least 22.7 kb long is required for biosynthesis. A bioinformatics-based approach to analysis of this gene cluster postulated that there is a posttranslational modification pathway in which eight proteins are involved in the biosynthetic machinery.

MATERIALS AND METHODS

Bacterial strains, plasmids, and media.

Strains and plasmids used in this work are listed in Table Table1.1. S. hygroscopicus 10-22 and S. lividans 1326, as well as derivatives of the latter strain, were grown at 30°C on SFM agar (20 g soy flour, 20 g mannitol, and 20 g agar in 1 liter tap water) plates for sporulation or in tryptic soy broth (TSB) that was supplemented with sucrose (10.3%, wt/vol) and yeast extract (1%, wt/vol) for growth of mycelia. Isolation of total DNA and manipulation of all Escherichia coli strains were performed as described by Sambrook et al. (26). For selection of Streptomyces transformants, the concentrations of apramycin, kanamycin, and thiostrepton that were used in agar were 30 mg ml−1, 10 mg ml−1, and 15 mg ml−1, respectively, and the concentrations that were used in liquid medium were 20 mg ml−1, 5 mg ml−1, and 5 mg ml−1, respectively. Heterologous expression mutations in S. lividans 1326 were obtained by interspecies conjugation by using E. coli ET12567::pUZ8002 as the donor and S. lividans 1326 as the recipient (Table (Table1)1) as described by Kieser et al. (15). Unless specified otherwise, restriction enzymes, T4 DNA ligase, Taq polymerase, and alkaline phosphatase were purchased from MBI Fermentas (Vilnius, Lithuania).

TABLE 1.
Bacterial strains, plasmids, and cosmids

Production and analysis of cyclothiazomycin.

S. hygroscopicus 10-22 was grown at 30°C for 5 to 7 days on SFM agar plates for production of cyclothiazomycin. For a quick bioassay of heterologous production of cyclothiazomycin in an S. lividans 1326 mutant, agar patches were transferred to PDA agar (200 g diced potatoes, 20 g glucose, and 15 g agar in 1 liter tap water) that contained Botrytis cinerea Persoon (Table (Table1).1). Inhibition zones were observed after 48 h of incubation at 28°C. For liquid chromatography (LC)-mass spectrometry (MS) analysis, strains were cultured on SFM agar at 30°C for 7 days. The fermentation agar was harvested and extracted by using the same volume of methanol. After overnight soaking, the resulting suspension was dried with solid Na2SO4, filtered, and syringe filtered before injection. LC-electrospray (ES)-quadrupole time of flight (QTOF) analysis was performed with an Agilent 1200 system (Agilent Co., CA) using a 2.1- by 30-mm C18 reverse-phase column (Agilent Co., CA) at a flow rate of 0.3 ml/min. Solvent A was 10% aqueous acetonitrile with 0.1% HCOOH, and solvent B was 0.1% HCOOH in acetonitrile. The gradient used was a gradient from 0 to 90% solvent B over 10 min. Mass spectra were obtained with a 6530 accurate-mass QTOF mass spectrometer (Agilent Co., CA) equipped with an electrospray ionization source. Tandem MS (MS/MS) was performed in the target-dependent mode.

Construction of S. hygroscopicus 10-22 genomic library.

For generation of a cosmid library, high-molecular-weight chromosomal DNA was prepared using the protocol described by Kieser et al., partially digested with MboI, dephosphorylated with calf intestinal alkaline phosphatase (Fermentas), and size fractionated in low-melting-temperature agarose by using pulsed-field gel electrophoresis (15). The chromosome DNA fragments that were between 35 and 45 kb long were recovered from the low-melting-temperature agarose gel digested with β-agarase (New England Biolabs). The DNA recovered was ligated with BamHI-digested cosmid vector pHZ1358 (Table (Table1)1) at a 1:1 molar ratio. Packaging and transfection into E. coli EPI300-T1 (Table (Table1)1) were done with λ-packaging mixtures prepared as described by Sambrook et al. (26). Ampicillin (Amp)-resistant colonies were picked individually and inoculated into LB (100 μl) supplemented with Amp in each well of 22 96-well plates. The plates were incubated at 37°C for 18 h, and then 50% glycerol (100 μl) was added to each well before storage at −80°C.

PCR primers and cosmid library screening.

Degenerate PCR primers designed using homologs of putative cyclodehydratases (17) were used to amplify a cyclodehydratase gene fragment from S. hygroscopicus 10-22. PCR products were purified from agarose gels (0.8%) by using a DNA gel extraction kit (V-gene Biotechnology Ltd.) and were subsequently inserted into the pMD18-T vector (TaKaRa, Dalian, China) for sequencing. Based on the fragment sequence, one pair of specific primers (CYCP primers) (Table (Table2)2) were designed and used to screen the genomic cosmid library of S. hygroscopicus 10-22. Each of the 22 96-well plates was screened by combining equal aliquots of cells from every well and using the resulting mixtures as templates for the first batch of PCR. For plates that yielded the desired PCR products, aliquots of cells from all wells in a row were combined and screened by a second PCR. Finally, each well in the positive rows was separately screened to identify individual clones that carried the target gene.

TABLE 2.
Primers used in this study

Construction of shuttle plasmids for heterologous production of cyclothiazomycin.

Shuttle plasmids pJTU4891 to pJTU4893 were constructed from restricted enzyme-digested cosmid 14E6 and pSET152 (Table (Table1),1), and pJTU4894 was constructed based on pJTU4891 using the PCR-targeting method (9) with the KT-IMN primers (Table (Table2).2). To confirm successful construction of the plasmids, restriction enzyme digestion was performed, and two pairs of primers (Table (Table2)2) were tested.

Sequence analysis.

DNA sequencing was done at Shanghai Ding'an Ltd. (Shanghai, China), and a multiple-sequence alignment was constructed with BioEdit 7.0. Open reading frames (ORFs) and ribosome binding sites (RBS) were predicted by using Frame-Plot 4.0 (12). Comparisons of nucleotide or amino acid sequences with sequences in public databases were performed by using the BLAST program and the NCBI website (http://blast.ncbi.nlm.nih.gov/Blast.cgi) (1).

Nucleotide and protein sequence accession number.

The DNA and deduced protein sequences described in this paper have been deposited in the GenBank database under accession number FJ472825.

RESULTS AND DISCUSSION

Cloning of the putative cyclothiazomycin biosynthetic gene cluster from S. hygroscopicus 10-22.

S. hygroscopicus 10-22, which was isolated by Zhou et al. in the 1980s, can produce three antifungal antibiotics, 5102-I, 5102-II, and 5102-III (23). One of these antibiotics, antibiotic 5102-I, has been identified and designated validamycin (13). Antibiotic 5102-II is a polypeptide containing Thr, Ser, and Cys and can protect corn plants against leaf spot (a disease caused by Cochliobolus heterostrophus). However, the lack of detailed structural information and an unsuccessful cloning strategy based on a nonribosomal peptide hypothesis have hampered cloning of the 5102-II biosynthesis gene cluster for years.

Previous failures raised the possibility that the polypeptide antibiotic 5102-II is synthesized by a ribosomal pathway, followed by posttranslational modification. Alignment of putative docking proteins encoded by the biosynthetic gene clusters of MccB17 (18) and streptolysin S, a ribosomally synthesized toxin secreted from the human pathogen Streptococcus pyogenes (16), suggested that there is a common domain belonging to the Ycao family that occurs in most putative toxin gene clusters (16). Accordingly, a pair of degenerate primers, ThioF and ThioR (17), was designed based on the common domain. Subsequently, a 700-bp fragment was obtained by performing PCR with the genomic DNA of S. hygroscopicus 10-22 as the template, and its sequence was found to be a segment of the YcaO family domain by BlastP analysis. Based on this nucleotide sequence, a pair of specific nested primers (CYCP primers [Table [Table2])2]) was designed to screen the S. hygroscopicus 10-22 genomic library constructed in pHZ1358. One of the positive cosmids, 14E6 with a 35-kb insertion, was sequenced (accession number FJ472825), and 27 ORFs were predicted in its sequence.

Significantly, a 180-nucleotide ORF, designated cltA, in the sequence was found to encode a 60-amino-acid precursor peptide (Fig. (Fig.2A)2A) whose C-terminal sequence (SNCTSTGTPASCCSCCCC) from S43 to C60 is perfectly consistent with the structural peptide of cyclothiazomycin (Fig. (Fig.3C,3C, from S1 to C18) (10), and the N-terminal 42-amino-acid sequence from M1 to A41 is likely to be the leader peptide (LP) (Fig. (Fig.4,4, compound 7). This putative cleavage site in the precursor is very similar to the cleavage sites in thiocillins (28) and two other putative thiopeptides, Sare_2569 and SGR_4418 (17), but very different from the cleavage site of another ribosomal synthesized polypeptide, where Gly is usually considered the initial residue recognized by some peptidase (16). In addition, the organization of all of the ORFs in this sequence (Fig. (Fig.2A)2A) is also similar to that of thiostrepton (14, 17), thiocillin (28), and other putative ribosomally produced polypeptide gene clusters (16). Moreover, cyclothiazomycin was reported to be active against some important plant-pathogenic fungi (2, 10), including Cochliobolus miyabeanus, which belongs to the same genus as C. heterostrophus, and Botrytis cinerea Persoon, which was used as the indicator in a bioassay of the production by S. hygroscopicus 10-22 in this study (Fig. (Fig.5).5). These findings suggested that the polypeptide antibiotic 5102-II is likely to be cyclothiazomycin, and they indicated a successful strategy for cloning the cyclothiazomycin biosynthetic gene cluster.

FIG. 2.
Heterologous expression of the cyclothiazomycin biosynthesis gene cluster cloned from S. hygroscopicus 10-22. (A) Organization of the ORFs in the gene cluster. The putative functions of the ORFs are indicated and are summarized in Table Table ...
FIG. 3.FIG. 3.
LC-ES-QTOF and MS/MS analysis of methanol extract of an S. hygroscopicus 10-22 culture. (A) LC-ES-QTOF analysis of methanol extract from an S. hygroscopicus 10-22 culture. Two distinct peaks were extracted with m/z 737.1515 ± 5 from total ion ...
FIG. 4.
Proposed pathway for biosynthesis of cyclothiazomycin. Eight proteins, CltB, CltC, CltD, CltE, CltF CltG, CltM, and CltN, are the candidate enzymes involved in posttranslational modification, and one transport protein, CltO, is predicted to transport ...
FIG. 5.
Bioassay for cyclothiazomycin production by S. hygroscopicus 10-22 with B. cinerea Persoon. An agar patch containing S. hygroscopicus 10-22 was placed on B. cinerea Persoon growing on medium to determine the zone of inhibition due to cyclothiazomycin ...

Characterization of the cyclothiazomycin produced by S. hygroscopicus 10-22.

To confirm production of cyclothiazomycin by S. hygroscopicus 10-22, the active components were extracted with methanol from a fermentation agar plate, and structural characterization was subsequently performed by using LC-ES-QTOF mass spectrometry analysis.

Two peaks were present in the extract ion current chromatogram extracted from the total ion current chromatogram of the methanol extract by m/z searching with the molecular weight of protonized cyclothiazomycin (m/z 1473.2967 ± 2) (Fig. (Fig.3B),3B), suggesting that in solution cyclothiazomycin includes a pair of isomers, very similar to those of cyclothiazomycin B (10). The QTOF mass spectrum of each isomer had an accurate [M+1]+ signal at m/z 1473.2933 and an accurate [M+2]2+ signal at m/z 737.1515. Within the error of the instrument, these results matched the theoretical value for protonized cyclothiazomycin (C59H64N18O14S7+) (m/z 1473.2967) well (Fig. (Fig.3B).3B). According to a Beynon table, isotope abundances could be calculated with the formulas [M+2]+ = 1.1x + 0.2z + 0.4S and [M+3]+ = (1.1x)2/200 + 4.4S, where x, z, and S are the numbers of C, O, and S atoms, respectively; these calculations resulted in abundances of 87 and 55, respectively (5a). The calculated results for [M+2]+ and [M+3]+ matched the measured results shown in Fig. Fig.3D3D well. This isotope analysis, together with the high-resolution mass spectrum, allowed assignment of a unique formula to cyclothiazomycin using the Masshunter qualitative analysis software (Agilent Co., CA).

The role of cleavage of cyclothiazomycin, a bridged macrocyclic thiopeptide, in a mass spectrometer is difficult to determine, and the number of possible cleavage sites is much less than the number for a normal peptide. Most fragments were generated by double cleavage at the acrylamide bond or at the C—S bond between the modified S5 and C18 residues; three examples are fragments 4, 5, and 6 with [M+1]+ signals at m/z 283, 441, and 1231, respectively. Ions 2 and 3 generated from the neutral loss of ion 4 were observed at m/z 784 and 1163, respectively. Therefore, these important fragments in the tandem MS spectrum were characterized as fragments of cyclothiazomycin (Fig. (Fig.3C)3C) and confirmed that this thiopeptide is produced by S. hygroscopicus 10-22.

Minimal biosynthetic gene cluster indicated by the heterologous expression study.

To define the functional gene cluster in the sequenced cosmid 14E6, a series of plasmids derived from pSET152 were constructed (Table (Table1;1; see Fig. S1 in the supplemental material). First, pJTU4891, containing a large XbaI-EcoRI fragment from 14E6 (Fig. (Fig.2B),2B), was transformed into S. lividans 1326, resulting in a transformant with bioactivity against B. cinerea Persoon. Then a 4-kb NdeI fragment that is close to the 3′ end of the gene cluster was removed from pJTU4891 to create pJTU4892. Activity against B. cinerea Persoon confirmed that pJTU4892 contains all of the essential genes for producing cyclothiazomycin. Further deletion of cltIMN from the inserted sequence of pJTU4891 was obtained by a PCR targeting method to generate pJTU4894, which resulted in a failure to produce cyclothiazomycin (Fig. (Fig.2B2B).

To detect the cyclothiazomycin produced by S. lividans 1326::pJTU4892, a similar LC-ES-QTOF analysis was done to screen the transformant's product. Two peaks that were characterized as a pair of isomers of cyclothiazomycin were also detected at the same retention time (see Fig. S2 in the supplemental material), and the mass spectrum of each peak had two signals, one at m/z 737.1511 ([M+2]2+) and one at m/z 1473.2907 ([M+1]+) (Fig. (Fig.3C).3C). Together with the isotope abundances of [M+2]+ and [M+3]+, these high-resolution mass spectra also allowed assignment of a unique formula to cyclothiazomycin.

Successful heterologous production of cyclothiazomycin by S. lividans 1326::pJTU4891 did not include expression of ORFs 5, 6, 7, 8, 9, and 10 in the cyclothiazomycin biosynthetic gene cluster. Since pJTU4892 lacks the 4-kb NdeI fragment that includes cltL, ORF 1, ORF 2, and most of cltK and ORF 3, expression of these genes was also not included, and ORF 4 at the 3′ end is unlikely to encode a functional protein involved in biosynthesis. Moreover, the failure of pJTU4894 to produce cyclothiazomycin suggested that at least one gene in the cltIMN cluster is essential for production of cyclothiazomycin (Fig. (Fig.2B).2B). Thus, a 22.7-kb gene cluster containing 15 ORFs was the minimal cluster to govern biosynthesis of cyclothiazomycin.

Putative functional enzymes for the cyclothiazomycin biosynthesis model.

According to the bioinformatics analysis of the insert of pJTU4892 (Table (Table3),3), besides the 60-amino-acid precursor peptide, the products of 9 of the 15 ORFs in the biosynthetic cluster were candidates for molecules involved in biosynthesis of cyclothiazomycin. Several mutagenesis experiments were done using in-frame deletion of cltD, the C-domain of cltC, and cltA, but none of the mutants was able to generate cyclothiazomycin (see Fig. S2 in the supplemental material). Other genes, the cltHPOIQ genes, were likely to encode two regulators, a transporter, and two transposases, respectively.

TABLE 3.
Putative functions of ORFs in cyclothiazomycin biosynthesis gene cluster

Similar to the tsrJKLMNOS and sioJKLMNOS genes in thiostrepton and siomycin A gene clusters, respectively (17), six ORFs, cltBCDEFG flanking cltA, are likely to encode the components of the main framework of cyclothiazomycin: dehydramino acids, thiazolines or thiazoles, and the trisubstituted pyridine. Two of the gene products, CltE and CltF, which are homologous to the lantibiotic dehydratases, were candidates for dehydration of Ser and Thr residues (Fig. (Fig.4,4, reaction c). About 4.5 kb from the main structural genes, the cltMN genes were likely to encode the enzymes involved in production of the tertiary thioether (Fig. (Fig.4,4, reactions f and g). cltJ, which was located at the 3′ end of the gene cluster, encoded a homolog of an epoxide hydrolase with high levels of identity (47%) and similarity (62%). According to the model proposed for other thiopeptides (14, 17, 28) and the thioether synthetic pathway in lantibiotic biosynthesis (6), cltJ was unlikely to be a functional gene for either the main framework or tertiary thioether biosynthesis.

Specific dehydrogenation of the thiazolines in the biosynthetic precursor.

Thiazoles and thiazolines are known to be generated by nucleophilic attack on each Cys side chain on the adjacent carbonyl group, followed by dehydration and selective dehydrogenation (19, 25). CltB is likely to be a candidate for cyclodehydratase, governing the formation of thiazolines (Fig. (Fig.4,4, reaction a), since CltB has a putative C-terminal domain belonging to the YcaO superfamily and an N-terminal domain homologous to the uncharacterized protein DUF181. Similarly, in MicroB17 biosynthesis, McbD, which has a YcaO family domain, was proposed to dock protoxin with other subunits to form thiazolines and oxazolines (19). In addition, TclJ, also a YcaO-DUF181 double-domain protein, was suggested to be a cyclodehydratase that catalyzes the formation of a similar heterocycle in thiocillins (28).

Interestingly, in accordance with the prepeptide sequence, only the N-terminal thiazoline of a bithiazoline can be dehydrogenated to produce thiazole, resulting in the three thiazolines that are unchanged in cyclothiazomycin (compound 7) (Fig. (Fig.4,4, reaction b). Selective dehydrogenation of thiazolines to form thiazoles would be expected to be catalyzed by CltC, a putative NADH oxidase with two McbC-like domains, since it has been suggested that McbC catalyzes a similar dehydrogenation in pro-MccB17 and belongs to the nitro-flavin mononucleotide (FMN) reductase superfamily (19). Thus, with two “reductase” domains, CltC is likely to recognize a bithiazoline residue as a substrate but exhibit the dehydrogenation function only with the N-terminal thiazoline residue. The consecutive dehydrogenations of the two thiazoline residues on the prethiazoline chain illustrated by C15*-C16*-C17* (compound 8) (Fig. (Fig.4)4) suggest that CltC is capable of searching the bithiazoline residue from the N terminus and play a role as an LP-dependent enzyme.

Simultaneous reaction involved in LP cleavage and biosynthesis of a trisubstituted pyridine.

Cyclothiazomycin harbors a central trisubstituted pyridine, which is very different from that of thiocillin (Fig. (Fig.1).1). Since the central substituted pyridine and dehydropiperidine were considered a common feature of thiopeptides (3), the trisubstituted pyridine is likely to be synthesized via a piperidine intermediate, which was proposed to be formed by an intramolecular hetero-Diel-Alder reaction (14, 17) (Fig. (Fig.4,4, reaction d). According to the bioinformatics analysis, CltD can be deduced to be a double-domain protein involved in pyridine biosynthesis (Table (Table3).3). Significantly, the N-terminal domain of CltD is homologous to that of a putative M14peptidase, carboxypeptidase A (41% similarity and 28% identity), providing a clue for the timing of LP cleavage. Although LP cleavage of thiocillins and LP cleavage of thiostrepton were thought previously to be the final step in thiopeptide biosynthesis (17, 28), we believe that processing of the prepeptide precursor of cyclothiazomycin happens during pyridine formation. The C-terminal domain of CltD, a member of the YcaO family, may provide a docking site for the hetero-Diel-Alder reaction to form a piperidine intermediate (Fig. (Fig.4,4, reaction d). To complete the formation of pyridine, CltG is expected to participate in the deamination that is required to eliminate the amine group generated by LP cleavage, since it shows similarity to SioL and NosO (23% and 29% similarity, respectively), which were previously proposed to be involved in the six-member nitrogen heterocycle formation in siomycin (17) and nosiheptide (30) synthesis.

Tertiary thioether biosynthesis resulting in the final bridged macrocyclic structure of cyclothiazomycin.

An unusual tertiary thioether was found between the dehydrated S5 and C18 residues of cyclothiazomycin (Fig. (Fig.1)1) in the bridged macrocyclic structure. Intramolecular thioether cross-linking within a peptide through Michael addition of Cys to a dehydroamino acid originating from Ser or Thr was observed previously in lantibiotic biosynthesis (31). However, the tertiary thioether of cyclothiazomycin is very different from the primary thioether of a lantibiotic, implying that there is rearrangement after the intramolecular Michael addition reaction (Fig. (Fig.4,4, reactions f and g). With 34% sequence identity to EthD, which was proven to be an essential protein involved in ethyl tert-butyl ether degradation (7), CltN is likely to be one of the enzymes involved in the final formation of the tertiary thioether. Although no function can be determined from the bioinformatics analysis, CltM is the only unassigned candidate left for biosynthesis. It is likely to be involved in biosynthesis of the tertiary thioether rather than biosynthesis of the framework. Unlike CltD, neither CltM nor CltN possesses the docking subunit, implying that the cyclothiazomycin intermediate with a central pyridine can be properly folded, allowing the —SH group of C18 to approach the double bond of the dehydrated S5 residue.

Conclusion.

In this study, a novel and complete gene cluster involved in posttranslational modification of a ribosomally synthesized prepeptide was elucidated based on heterologous production. Based on the heterologous expression study and the bioinformatics analysis of the minimal intact gene cluster, we propose an eight-enzyme biosynthetic model for posttranslational modification of cyclothiazomycin (Fig. (Fig.4).4). In this model, three proteins, CltC, CltD, and CltN, might be important for biosynthesis of the characteristic structural elements: the selectively dehydrogenated thiazolines, trisubstituted central pyridine, and tertiary thioether. Importantly, LP cleavage was deduced to be catalyzed by the C-terminal domain of CltD during pyridine formation. Although this bioinformatics-based biosynthetic model needs to be substantiated, it may provide clues for further cyclothiazomycin bioengineering.

Supplementary Material

[Supplemental material]

Acknowledgments

This work was supported by 863 Funds from the Ministry of Science and Technology, the National Science Foundation of China, the Ph.D. Training Fund of the Ministry of Education, and the Shanghai Municipal Council of Science and Technology.

We thank Jie Chen for the gift of B. cinerea Persoon.

Footnotes

[down-pointing small open triangle]Published ahead of print on 12 February 2010.

Supplemental material for this article may be found at http://aem.asm.org/.

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