Abstract

Introduction

The St. Peter and St. Paul Archipelago (SPSPA) is a remote group of islets located off the Brazilian coast. It is a rare case of geological formation, as this is the single portion of the Atlantic Ocean where the mantle has surfaced, permeating an area just about 17,000 m² above sea level.¹1 Vieira, L. M.; Farrapeira, C. M. R.; Amaral, F. D.; Lira, S. M. A.; Cah. Biol. Mar. 2012, 53, 159. Peripheral habitats such as SPSPA and surroundings are a potential source of marine biodiversity with high degree of endemism.¹1 Vieira, L. M.; Farrapeira, C. M. R.; Amaral, F. D.; Lira, S. M. A.; Cah. Biol. Mar. 2012, 53, 159.

2 Bowen, B. W.; Rocha, L. A.; Toonen, R. J.; Karl, S. A.; Trends Ecol. Evol. 2013, 28, 359.

3 Vaske-Jr, T.; Lessa, R. P. T.; Nóbrega, M. F.; Montealegre-Quijano, S.; Marcante-Santana, F.; Bezerra, J. L. A.; J. Appl. Ichthyol. 2005, 21, 75.^-44 Viana, D. F.; Hazin, F. H.; Andrade, H. A.; Nones, D. M.; Viana, D. L.; Bol. Inst. Pesca 2015, 41, 239. Microbial diversity studies, however, are still very scarce,⁵5 Moreira, A. P. B.; Duytschaever, G.; Tonon, L. A. C.; Froes, A. M.; de Oliveira, L. S.; Amado-Filho, G. M.; Francini-Filho, R. B.; DeVos, P.; Swings, J.; Thompson, C. C.; Thompson, F. L.; PeerJ 2014, 2, e427. while the biotechnological potential of microorganisms has only recently been described by our group in a preliminary assessment of the chemical diversity and prospection of anticancer compounds in extracts derived from culturable actinobacteria recovered from sediments collected therein.⁶6 Ferreira, E. G.; Torres, M. C. M.; da Silva, A. B.; Colares, L. L. F.; Pires, K.; Lotufo, T. M. C.; Silveira, E. R.; Pessoa, O. D. L.; Costa-Lotufo, L. V.; Jimenez, P. C.; Chem. Biodiversity 2016, 13, 1149. Essentially, this work showed a high incidence of bioactive extracts among those obtained from the 268 isolates, and dereplication studies demonstrated the presence of notorious bioactive compounds, such as, but not restricted to, staurosporines, piericidins, saliniketals and rifamycins. Such preliminary results merely hinted on the biological and metabolic diversity that is predicted for the SPSPA. In this scenario, the strain, thereby coded as BRA 177, showed remarkable cytotoxicity against a human tumor cell line,⁶6 Ferreira, E. G.; Torres, M. C. M.; da Silva, A. B.; Colares, L. L. F.; Pires, K.; Lotufo, T. M. C.; Silveira, E. R.; Pessoa, O. D. L.; Costa-Lotufo, L. V.; Jimenez, P. C.; Chem. Biodiversity 2016, 13, 1149. and was, thus, bidden for broader investigations.

In fact, traditional bioprospective efforts have long merged chemical studies and biological assays in search for functional natural products. While these well-used equipment and methodologies have been ever evolving into more sensitive and high-throughput analytical tools, for the past decade or so, another perspective, based on screening of genetic information, has irrefutably leveraged, and refreshed, biodiscovery investigations.⁷7 Bachmann, B. O.; Van Lanen, S. G.; Baltz, R. H.; J. Ind. Microbiol. Biotechnol. 2014, 41, 175. This so-called genome mining approach is, in truth, supporting the field as a third pillar by enabling exploration of the DNA itself, targeting clusters of genes that may encode information for the biosynthesis of relevant molecules.⁸8 Ziemert, N.; Alanjary, M.; Weber, T.; Nat. Prod. Rep. 2016, 33, 988. This technique has been particularly handy in mining secondary metabolites in bacterial DNA, as these are shorter, easier to assemble and intron-free, but packed with purposeful pathways.⁹9 Harvey, A. L.; Edrada-Ebel, R.; Quinn, R. J.; Nat. Rev. Drug Discovery 2015, 14, 111.

Therefore, aiming at expanding the knowledge on the biotechnological potential of microbes from SPSPA, this work examined, by means of both, chemical and genomic assessments, the capacity to produce bioactive metabolites of a cytotoxic actinobacteria strain (BRA 177) recovered from sediments collected at the Archipelago's vicinities.

Results and Discussion

Chemical investigation and anticancer potential

Chemical investigation of the crude EtOAc extract of the fermentation broth of BRA 177 led to the isolation of three prodiginine derivatives, as shown in Figure 1. Their structures were determined by mass spectrometry (MS), ¹H and ¹³C nuclear magnetic resonance (NMR) data, and confirmed by comparison with previously reported data (see Supplementary Information).

The three compounds, all red pigments, exhibited magenta spots on TLC (thin layer chromatography) and absorption bands at 530 nm on UV-Vis, a characteristic feature of the prodiginine skeleton.¹⁰10 Farzaneh, A.; Kou-San, J.; Jozsef, L.; Bruce, D. H.; Gang, S.; Biotechnol. Prog. 2008, 24, 742. Compounds 1 and 3 were obtained in small amounts, compared to 2. Thus, the structure of 2 was well established by high-resolution electrospray ionization mass spectrometry (HRESIMS), ¹H and ¹³C NMR-HSQC (heteronuclear single quantum correlation) and HMBC (heteronuclear multiple bond correlation) data, whereas the structures of 1 and 3 were supported by HRESIMS and ¹H NMR and comparison with the NMR data of 2 (see Supplementary Information).

Based on the obtained data, compounds 1, 2 and 3 were identified as methylcyclooctylprodigiosin,¹¹11 Laatsch, H.; Kellner, M.; Weyland, H.; J. Antibiot. 1990, 44, 187. [molecular formula C₂₃H₂₉N₃O (m/z 364.2383 [M + H]⁺)], cyclononylprodigiosin¹⁰10 Farzaneh, A.; Kou-San, J.; Jozsef, L.; Bruce, D. H.; Gang, S.; Biotechnol. Prog. 2008, 24, 742.^,1212 Gerber, N. N.; McInnes, A. G.; Smith, D. G.; Walter, J. A.; Wright, J. L. C.; Vining, L. C.; Can. J. Chem. 1978, 56, 1155. [molecular formula C₂₃H₂₉N₃O (m/z 364.2383 [M + H]⁺)] and nonylprodigiosin¹⁰10 Farzaneh, A.; Kou-San, J.; Jozsef, L.; Bruce, D. H.; Gang, S.; Biotechnol. Prog. 2008, 24, 742.^,1212 Gerber, N. N.; McInnes, A. G.; Smith, D. G.; Walter, J. A.; Wright, J. L. C.; Vining, L. C.; Can. J. Chem. 1978, 56, 1155. [molecular formula C₂₃H₃₁N₃O, m/z 366.2545 [M + H]⁺)], respectively. It is worth mentioning that nonylprodigiosin and cyclononylprodigiosin, isolated in 1969 and 1970, respectively, by Gerber from Actinomadura madurae, were originally named nonylprodiginine and cyclononylprodiginine.¹³13 Gerber, N. N.; Appl. Microbiol. 1969, 18, 1; Gerber, N. N.; Tetrahedron Lett. 1970, 11, 809; Gerber, N. N.; J. Antibiot. 1971, XXIV, 636. Indeed, due to their structural similarities with prodigiosin, the first tripyrrole alkaloid isolated from Serratia marcescens,¹⁴14 Wasserman, H. H.; McKeon, J. E.; Smith, L.; J. Am. Chem. Soc. 1960, 82, 506. and other prodiginine derivatives, there has been some conflict around the nomenclature of these compounds. Currently, it seems to be a consensus that the term "prodiginine" should be employed to denote the class of alkaloids in general, while "prodigiosin" should refer to the particular names of the red or magenta pigments.

Cytotoxicity of the isolated compounds was assessed using three tumor cell lines from different origins, HCT-116 (colon adenocarcinoma), MCF-7 (breast carcinoma) and SK-Mel-147 (melanoma), and a non-tumor cell line, MRC-5 (fibroblast). Doxorubicin was used as a positive control and displayed the lowest IC₅₀ values for all assayed cell lines. Prodigiosin was included in the assays as a reference compound, which showed higher activity than the other isolated prodiginine derivatives. Compounds 2 and 3 were cytotoxic against most cell lines, with comparable IC₅₀ for the tumor cells, as shown in Table 1. Nevertheless, Prodigiosin, compounds 2 and 3, showed the highest cytotoxicity towards MRC-5, the non-tumor cell line model accessed presently.

Bacterial prodiginines are characterized by a common pyrrolylpyrromethene skeleton, which retains interesting anticancer, antiparasitic, antibiotic and immunosuppressive activities.¹⁵15 Darshan, N.; Manonmani, H. K.; J. Food Sci. Technol. 2015, 52, 5393; Pérez-Tomás, R.; Viñas, M.; Curr. Med. Chem. 2010, 17, 2222. Considering the NCI 60-cell line panel, the mean average IC₅₀ value for prodigiosin is 2.1 µM,¹⁶16 www.dtp.nci.nih.gov under NSC47147, accessed in September 2016.
www.dtp.nci.nih.gov under NSC47147... a compatible value with those presented herein. The proposed mechanisms of action for this class of compounds includes four different possibilities: (i) potent DNA-damaging properties under oxidative conditions; (ii) intracellular acidification; (iii) interference with kynases; and (iv) induction of apoptosis.¹⁵15 Darshan, N.; Manonmani, H. K.; J. Food Sci. Technol. 2015, 52, 5393; Pérez-Tomás, R.; Viñas, M.; Curr. Med. Chem. 2010, 17, 2222. It seems, however, that the mechanism and target are highly dependent on cell type.

Furthermore, Fürstner¹⁸18 Fürstner, A.; Angew. Chem. Int. Ed. 2003, 42, 3582. pointed out particular structural requirements for the cytotoxic activity of prodiginines, arguing that replacement of individual pyrrole rings or removal of the peripheral methoxyl group at C3 of the B-ring significantly decreased cytotoxicity. The compounds tested herein shared these mentioned structural features, but compound 1 was consistently less active than both, 2 and 3, and prodigiosin itself. Thus, it is possible to speculate that the structure-activity relationships for prodiginine compounds are more complex than previously anticipated.

Genome mining

In order to unveil the biosynthetic origin of the isolated prodiginines (nonilprodigiosin; cyclononilprodigiosin and methylcyclooctylprodigiosin), shotgun sequencing of BRA 177 genome was performed at the Illumina MiSeq sequencher. A total of 6.2 gigabytes (Gb) of raw sequence data was generated, trimmed for quality and assembled into 735 contigs, composing BRA 177 draft genome.

To evaluate sequencing efforts, molecular taxonomy was accomplished by retrieving a 16S rRNA gene from BRA 177 genome and submitting it to phylogenetic analysis (Figure 2). The maximum likelihood phylogenetic tree recovered grouped BRA 177 within the actinobacteria Actinomadura genus (99% sequence identity), closely related to Actinomadura madurae. The estimated BRA 177 total genome length of 8,043,576 bp is in agreement with this strains phylogenetic inference, since the median length of Actinomadura madurae genomes was estimated as 9.46 Mb on the basis of previously sequenced and publicly available genomes.¹⁹19 Doroghazi, J. R.; Albright, J. C.; Goering, A. W.; Ju, K. S.; Haines, R. R.; Tchalukov, K. A.; Labeda, D. P.; Kelleher N. L.; Metcalf, W. W.; Nat. Chem. Biol. 2014, 10, 963; Vera-Cabrera, L.; Ortiz-Lopes, R.; Elizondo-González, E.; Campos-Rivera, M. P.; Gallardo-Rocha, A.; Molina-Torres, C. A.; Ocampo-Candiani, J.; Genome Announc. 2014, 2, e00201-14. Therefore, sequencing efforts covered BRA 177 genomic contents between 654 to over 770 fold, which guarantees a high quality draft genome.

The draft genome was then annotated at the RAST server,²⁰20 Aziz, R. K.; Bartels, D.; Best, A. A.; DeJongh, M.; Disz, T.; Edwards, R. A.; Formsma, K.; Gerdes, S.; Glass, E. M.; Kubal, M.; Meyer, F.; Olsen, G. J.; Olson, R.; Osterman, A. L.; Overbeek, R. A.; McNeil, L. K.; Paarmann, D.; Paczian, T.; Parrello, B.; Pusch, G. D.; Reich, C.; Stevens, R.; Vassieva, O.; Vonstein, V.; Wilke, A.; Zagnitko, O.; BMC Genomics 2008, 9, 75. presenting an average GC content of 71.1%, 68 RNA and 7588 protein encoding genes (PEG). Within automated predicted proteins, a fraction of 31% (2320) could be assigned to 427 subsystems of the Subsystem ontology. Functions related to "Amino acids and derivatives" (16%), "Carbohydrates" (15%), "Cofactors, Vitamins, Prosthetic Groups, Pigments" (12%) and "Protein Metabolism" were the most enriched Subsystems (Figure 3A). Sequentially, BRA 177 annotated draft genome was mined for natural products biosynthetic gene clusters (BGCs) with the Antibiotics & Secondary Metabolite Analysis SHell (ANTISMASH).²¹21 Weber, T.; Blin, K.; Duddela, S.; Krug, D.; Kim, H. U.; Bruccoleri, R.; Lee, S. Y.; Fischbach, M. A.; Müller, R.; Wohlleben, W.; Breitling, R.; Takano, E.; Medema, M. H.; Nucleic Acids Res. 2015, 43, 237. A total of 22 BGCs were detected, including pathways for production of ribosomally (lantipeptides) and non-ribosomally (NRPS) derived bioactive peptides, terpenes, siderophores and polyketides (Figure 3B).

Within the polyketides group, a total of 37.347 bp BGC (NODE_44) was detected, containing thirteen PEGs with homology to genes of the highly related red and mar BGCs, respectively responsible for the biosynthesis of undecylprodigiosin and its cyclic derivative streptorubin B by S. coelicolor, and mariniosins by the marine Streptomyces sp. CNQ-617 (Figure 4, Table S1).²²22 Feitelson, J. S.; Malpartida, F.; Hopwood, D. A.; J. Gen. Microbiol. 1985, 131, 2431.^,2323 Salem, S. M.; Kancharla, P.; Florova, G.; Gupta, S.; Lu, W.; Reynolds, K. A.; J. Am. Chem. Soc. 2014, 136, 4565.

Undecylprodigiosin, mariniosins and other related prodiginines derived all from the condensation of the same two precursor moieties: 2-undecylpyrrole (2-UP) and 4-methoxy-[2,2'-bipyrrole]-5-carboxaldehyde (MBC). Therefore, this group of prodiginines diverges from prodigiosin isolated from Serratia species and other gram-negative bacteria, where the MBC precursor is condensed with 2-methyl-3-n-amyl-pyrrole (MAP) instead of 2-UP.²⁴24 Williamson, N. R.; Fineran, P. C.; Leeper, F. J.; Salmond, G. P.; Nat. Rev. Microbiol. 2006, 4, 887. The enzymology involved in biosynthesis of prodiginines precursors have been exhaustively studied and recently reviewed.²⁵25 Hu, D. X.; Withall, D. M.; Challis, G. L.; Thomson, R. J.; Chem. Rev. 2016, 116, 7818. In fact, nonylprodigiosin and its cyclic derivatives isolated from BRA 177 are structurally related to undecylprodigiosin and the only difference detected is that the hydrocarbon moiety is 2 methylene shorter.²⁵25 Hu, D. X.; Withall, D. M.; Challis, G. L.; Thomson, R. J.; Chem. Rev. 2016, 116, 7818.

In agreement with the chemical structure, multilocus sequence analysis (MLSA) performed with the amino acid sequences of eight protein homologs encoded on undecylprodigiosin red and prodigiosin pig clusters, and involved in biosynthesis the MBC precursor (RedWIOMNYV/PigAFGHIKM) and precursors condensation (RedH/PigC), separated gram-negative prodiginiosin producers from actinobacteria undecylprodigiosin-related prodiginine producers in two main clades.²⁶26 Li, P.; Kwok, A. H.; Jiang, J.; Ran, T.; Xu, D.; Wang, W.; Leung, F. C.; PLoS One 2015, 10, e0123061. Therefore, the enzymology codified on the detected contig NODE_44 is in agreement with that expected for the biosynthesis of nonylprodigiosin and derivatives.

In the prototypic undecylprodiginine red BGC, 2-UP is assembled by RedPQRL enzymes, while RedMOWUXNVI components produce MBC.²⁵25 Hu, D. X.; Withall, D. M.; Challis, G. L.; Thomson, R. J.; Chem. Rev. 2016, 116, 7818.^,2727 Cerdeno, A. M.; Bibb, M. J.; Challis, G. L.; Chem. Biol. 2001, 8, 817.

28 Mo, S.; Sydor, P. K.; Corre, C.; Alhamadsheh, M. M.; Stanley, A. E.; Haynes, S. W.; Song, L.; Reynolds, K. A.; Challis, G. L.; Chem. Biol. 2008, 15, 137.^-2929 Stanley, A. E.; Walton, L. J.; Kourdi-Zerikly, M.; Corre, C.; Challis, G. L.; Chem. Commun. 2006, 38, 3981. BLASTx searches using the amino acid sequence of Red/Mar proteins missed by the ANTISMASH screening as query against the genome of BRA 177 recovered an additional 31.335 bp contig (NODE_60) containing the respective red (mar) gene homologs clustered (Figure 4, Table 1). Therefore, the genome mining strongly supports that contigs NODE_44 and NODE_60 gene composition includes BRA 177 putative prodiginine BGC, named from now on as the non cluster (Figure 4).

On Actinomadura spp. BRA 177 non cluster, the homologs to genes redXWYD, which, in Streptomyces spp. prodiginine BGCs are organized as a separated transcript unit, appear rearranged upstream and on same transcriptional direction of redG homolog nonG (Figure 4). Such operon-like organization indicates that a major portion of the prodiginines biosynthetic enzymes are co-transcribed as one huge polycistronic mRNA (Figure 4, arrows for hypothetical transcript units). Although physical mapping of NODE_44 and 60 was not yet addressed, it is possible that these contigs are placed at a single genomic locus. In such case, NODE_60 putative nonP gene would appear upstream to NODE_44 putative nonD, possibly increasing the predicted larger transcriptional unit up to gene nonP (in Figure 4 this arrangement is not shown since NODE_60 contig 5' fragment is shown downstream to NODE_44 3' fragment in order to facilitate comparative analysis between prodiginine BGCs).

The only relevant absence noticed on the BRA 177 putative non cluster, was for a redK (marK) homologous, that in both red and mar BGCs follows redL in the clusters biggest transcriptional unit (Figure 4).²³23 Salem, S. M.; Kancharla, P.; Florova, G.; Gupta, S.; Lu, W.; Reynolds, K. A.; J. Am. Chem. Soc. 2014, 136, 4565.^,2727 Cerdeno, A. M.; Bibb, M. J.; Challis, G. L.; Chem. Biol. 2001, 8, 817. RedK oxidoreductase is responsible for reduction and dehydration of 4-keto-2-undecyl-4,5-dihydropyrrole at the final step for generation of 2-UP precursor.²⁴24 Williamson, N. R.; Fineran, P. C.; Leeper, F. J.; Salmond, G. P.; Nat. Rev. Microbiol. 2006, 4, 887.^,2828 Mo, S.; Sydor, P. K.; Corre, C.; Alhamadsheh, M. M.; Stanley, A. E.; Haynes, S. W.; Song, L.; Reynolds, K. A.; Challis, G. L.; Chem. Biol. 2008, 15, 137. A thorough analysis showed, however, that BRA 177 putative NonL protein is larger than its homologs RedL and MarL, presenting additional 347aa at the C-terminus portion (in relation to MarL). BLASTp analysis using NonL C-terminus extra amino acid sequence reveals that it codifies an oxidoreductase highly similar (69/80% identity/similarity) to MarK (Figure 5A).

The catalytic domains constellation found in the putative NonL PKS, where a RedK-like oxidoreductase appears as a C-terminal domain, indicates a possible ancestry of this protein in relation to its homologous RedL and MarL. In order to evaluate that, phylogenetic reconstitution of RedL-like PKSs was executed. The obtained ML tree topology showed that NonL and a RedL-like homolog proteins from Actinomadura spp. form a robust clade (100% bootstrap support) apart from the respective proteins from Streptomyces spp., (e.g., RedL and MarL) (Figure 5B). Moreover, BRA 177 and Actinomadura latina putative PKSs were shown to be closely related, corroborating the fact that only these RedL PKS variants present RedK-like oxidoreductase embedded as a C-terminal catalytic domain (Figures 5A and 5B). Curiously, RphL, the RedL homologous from Streptomyces griseoviridis that, likewise, does not contain the C-terminus oxidoreductase, did not group within the Streptomyces PKSs, but as an outgroup of the prodiginine-PKS clade (Figure 5B). In S. griseoviridis, the prodiginine BGC is related with production of prodigiosin R1 and the structurally related antibiotic roseophilin, where the central pyrrole ring is replaced by a furan ring.³⁰30 Kawasaki, T.; Sakurai, F.; Nagatsuka, S. Y.; Hayakawa, Y.; J. Antibiot. (Tokyo) 2009, 62, 271.

Interestingly, the production of nonylprodigiosin and its cyclic derivatives in A. madurae was hypothetically related with altered specificities of the catalytic activities of RedJ or RedL N-terminal adenylation domain (RedL_A). These proteins selectively interact with the fatty acyl thioester tethered to RedQ (acyl carrier protein, ACP), which, in turn, is generated at the beginning of the 2-undecylpyrrole biosynthetic pathway by action of RedP (FabH-like beta-ketoacyl-acyl carrier protein synthase III), RedR (FabF-like beta-ketoacyl-acyl carrier protein synthase II), and RedQ combined with the full reduction set of FAS enzymology, ketoreductase (KR), dehydratase (DH) and enoylreductase (ER).²⁵25 Hu, D. X.; Withall, D. M.; Challis, G. L.; Thomson, R. J.; Chem. Rev. 2016, 116, 7818. RedJ thioesterase is proposed to hydrolyze dodecanoyl-RedQ generating the dodecanoic acid. Then, RedL_A would activate and attach the dodecanoyl acid to RedL first acyl carrier protein domain (RedL_ACP₁) by a thioester linkage. The dodecanoyl group then suffers further elongations/modifications that lead on 2-UP precursor.²⁵25 Hu, D. X.; Withall, D. M.; Challis, G. L.; Thomson, R. J.; Chem. Rev. 2016, 116, 7818.^,2727 Cerdeno, A. M.; Bibb, M. J.; Challis, G. L.; Chem. Biol. 2001, 8, 817.^,2828 Mo, S.; Sydor, P. K.; Corre, C.; Alhamadsheh, M. M.; Stanley, A. E.; Haynes, S. W.; Song, L.; Reynolds, K. A.; Challis, G. L.; Chem. Biol. 2008, 15, 137.

In order to explore this hypothesis, we carried out a phylogenetic analysis using amino acid sequences of RedL_A and of RedJ protein homologs from both Steptomyces and Actinomadura species (Figures 5C and 5D). Once the phylogenetic analysis of the entire RedL proteins were performed treating gaps missing data as "complete deletion", which would discard the extra oxidoreductase domain (OXR) of BRA 177 RedL from the distance calculations, it was anticipated that RedL_A could be a hotspot of divergence among the RedL homologs. Indeed, the topology recovered for RedL_A domains phylogeny mirrored the one obtained with RedL full proteins, where Actinomadura and Streptomyces spp. sequences grouped apart from each other on well supported genera-specific clades (Figures 5B and 5C). The same pattern of species-specific clade was also observed on RedJ thioesterase phylogeny (Figure 5D). Therefore, the present results sustain the hypothesis of the discrimination of Actinomadura spp., RedL_A and RedJ homologs, including putative NonL_A and NonJ, to process decanoyl instead of dodecanoyl-ACP substrates.

RedJ biochemical characterization corroborates the proposed activity by proving this thioesterase strong selectivity for long and saturated acyl chains that are linked to prodiginine specific RedQ ACP in detriment to substrates attached to FabC, the fatty acid synthase ACP of streptomycete.³¹31 Whicher, J. R.; Florova, G.; Sydor, P. K.; Singh, R.; Alhamadsheh, M.; Challis, G. L.; Reynolds, K. A.; Smith, J. L.; J. Biol. Chem. 2011, 286, 22558. However, no differential kinetics was observed for RedJ when cleaving dodecanoyl or decanoyl-AcpP substrates, indicating that this thioesterase may also have editing activities related to deacetylation of ACP/PCP (peptidyl carrier protein) domains miss-acetylated by 4'-phosphopantetheinyl transferase (PPTase) RedU.²⁵25 Hu, D. X.; Withall, D. M.; Challis, G. L.; Thomson, R. J.; Chem. Rev. 2016, 116, 7818.^,3131 Whicher, J. R.; Florova, G.; Sydor, P. K.; Singh, R.; Alhamadsheh, M.; Challis, G. L.; Reynolds, K. A.; Smith, J. L.; J. Biol. Chem. 2011, 286, 22558. In this case, RedJ would not have the fine capability to discriminate between the two long chain substrates, and RedL_A would be the key component for selecting decanoyl substrate on the prodiginine biosynthetic pathway of Actinomadura spp.

Another key enzyme clustered on red and related prodiginine BGCs is RedG and homologs, since these Rieske oxygenase-like were proven to mediate regio and stereodivergent oxidative cyclizations that lead to a diversity of cyclic prodiginines.³²32 Sydor, P. K.; Barry, S. M.; Odulate, O. M.; Barona-Gomez, F.; Haynes, S. W.; Corre, C.; Song, L.; Challis, G. L.; Nat. Chem. 2011, 3, 388. Therefore, we also conducted phylogenetic analysis on RedG homologs, including the putative NonG. Aminoacid sequence alignment showed that NonG predicted protein presents all three Rieske oxigenases universal His and Asp containing conservative motifs related to iron binding: the amino terminal motifs CXH and CXXH, and the carboxy-terminal motif DXHX₄H.³²32 Sydor, P. K.; Barry, S. M.; Odulate, O. M.; Barona-Gomez, F.; Haynes, S. W.; Corre, C.; Song, L.; Challis, G. L.; Nat. Chem. 2011, 3, 388. Maximum likelihood phylogenetic inference showed, once again, that Actinomadura spp. and Streptomyces spp. Rieske oxigenases grouped apart on well supported genera-specific clades (100 and 98% bootstrap support, respectively) (Figure 5C). Interestingly, Streptomyces spp. RedG, McpG and MarG enzymes are involved on cyclization of 10 and 12-membered carbon rings, forming streptorubin B, metacycloprodigiosin, and mariniosins, respectively.²³23 Salem, S. M.; Kancharla, P.; Florova, G.; Gupta, S.; Lu, W.; Reynolds, K. A.; J. Am. Chem. Soc. 2014, 136, 4565.^,3232 Sydor, P. K.; Barry, S. M.; Odulate, O. M.; Barona-Gomez, F.; Haynes, S. W.; Corre, C.; Song, L.; Challis, G. L.; Nat. Chem. 2011, 3, 388. On the other hand, the nonylprodiginine cyclic prodiginines derivatives methylcyclooctylprodigiosin and cyclononylprodigiosin, exclusively found in Actinomadura spp.,²⁴24 Williamson, N. R.; Fineran, P. C.; Leeper, F. J.; Salmond, G. P.; Nat. Rev. Microbiol. 2006, 4, 887. present functionalization of ring A, indicating a unique oxidative carbocyclization reaction performed by NonG Rieske oxygenase.

Conclusions

Actinomadura sp. recovered from SPSPA sediments, is a singular source for bioprospection and biotechnological studies. While the chemical analysis of the EtOAc extract led to the isolation of three cytotoxic known prodiginine derivatives, the genome mining showed the presence of a total of 22 BGCs, including pathways for production of ribosomally (lantipeptides) and non-ribosomally (NRPS) derived bioactive peptides, terpenes, siderophores and polyketides. The analysis of the two contigs encoding enzymes with high homology to those from prodiginine BGC in actinobacteria implies the presence of unique RedL-like type I PKS and RedG-like Rieske oxygenase, diverging from the Streptomyces spp. homolog ones. These results suggest that cyclononilprodigiosin and methylcyclooctylprodigiosin could be considered as chemical signatures of Actinomadura spp. Comparative genomics of BRA 177 and other prodiginine producers are underway to achieve a better characterization of the diversity of prodiginine BGCs and to explore the BGCs diversity of these prolific natural product-producing bacteria.

Experimental

General procedures

¹H (500 or 300 MHz) and ¹³C (125 or 75 MHz) NMR spectra were performed either on a Bruker Avance DRX-500 or Avance DPX-300 spectrometer. High resolution electrospray ionization mass spectrometry (HRESI-MS) was acquired by a LCMS-IT-TOF (Shimadzu) spectrometer consisting of an ultra fast liquid chromatography (UFLC) system coupled to an ion trap - time of flight (IT-TOF) mass spectrometer equipped with electrospray ionization (ESI) source operating either in positive or negative mode. High performance liquid chromatography (HPLC) analysis was carried out using an UFLC (Shimadzu) system equipped with a SPD-M20A diode array UV-Vis detector and a Phenomenex C₁₈ column, 5 µm (4.6 × 250 mm). The mobile phase consisted of CH₃CN:H₂O with a flow rate of 4.72 mL min^-1 and UV detection wavelength of 210-600 nm. For the column chromatographic procedures, silica gel 60 [70-230 mesh (Vetec) or 230-400 mesh (Merck)] were used, while the thin layer chromatography (TLC) was performed on precoated 0.2 mm silica gel aluminum sheets (silica gel 60 F₂₅₄, Merck) and spots visualized by heating (ca. 100 ºC) the plates sprayed with a vanillin/perchloric acid/EtOH solution.

Collection, isolation and identification of microorganism

BRA 177 was recovered from sediments collected by scuba diving (16 m) at the Enseada site, at the SPSPA, then dried and stamped on trace minerals agar [TMA, composed of 18% agar, 0.1% glucose, 0.1% yeast extract, K₂HPO₄, Na₂HPO₄, KNO₃, NaCl, MgSO₄⋅7H₂O, and CaCl₂⋅2H₂O in 75% seawater, with an added solution containing FeSO₄⋅7H₂O, ZnSO₄⋅7H₂O, MnSO₄⋅4H₂O, CuSO₄⋅5H₂O, CoSO₄⋅7H₂O, H₃BO₃, and (NH₄)6Mo₇O₂₄⋅4H₂O)] supplemented with 0.1 mg mL^-1 cycloheximide. A burgundy colored colony producing white spores was separated into a new dish layered with A1 agar (10% soluble starch, 4% yeast extract, 2% peptone and 18% agar in 75% filtered sea water) for purification.

Growth, extraction and isolation

Growth of BRA 177 was carried out in 10 L of A1 media (10% soluble starch, 4% yeast extract and 2% peptone), equally distributed in twenty 2 L Erlenmeyer flasks. Media was supplemented with calcium carbonate and solutions of iron(III) sulfate (Fe₂(SO₄)₃) and potassium bromide (KBr). Cultures were grown for 10 days at 28 ºC under 150 rpm agitation. The resulting fermentation broth (10 L) was filtered using a filter press to give filtrate and mycelia. The filtrate was extracted twice with 2.5 L of EtOAc, evaporated under reduced pressure at 35 ºC and dried to afford a dark crude extract (390.8 mg). This extract was chromatographed over silica gel eluted with n-hexane, EtOAc and MeOH in mixtures of increasing polarity to yield eleven fractions (Fr. A-K) after comparative TLC analyses. Fr. B (29.3 mg) was subjected to a silica gel column eluted with n-hexane/EtOAc gradients followed by HPLC using a semipreparative C₁₈ column and an isocratic solvent system of CH₃CN:H₂O (9:1) to afford methylcyclooctylprodigiosin¹¹11 Laatsch, H.; Kellner, M.; Weyland, H.; J. Antibiot. 1990, 44, 187. (1, 5.4 mg, t_R 12.6 min). Fr. C (97.7 mg) was subjected to successive silica gel column chromatograpies eluted with n-hexane/EtOAc gradients to yield cyclononylprodigiosin¹⁰10 Farzaneh, A.; Kou-San, J.; Jozsef, L.; Bruce, D. H.; Gang, S.; Biotechnol. Prog. 2008, 24, 742.^,1212 Gerber, N. N.; McInnes, A. G.; Smith, D. G.; Walter, J. A.; Wright, J. L. C.; Vining, L. C.; Can. J. Chem. 1978, 56, 1155. (2, 33.0 mg). Fr. F (15.0 mg) was further purified by HPLC using a semipreparative C₁₈ column with an isocratic mobile phase of CH₃CN:H₂O (9:1) to give nonylprodigiosin¹⁰10 Farzaneh, A.; Kou-San, J.; Jozsef, L.; Bruce, D. H.; Gang, S.; Biotechnol. Prog. 2008, 24, 742.^,1212 Gerber, N. N.; McInnes, A. G.; Smith, D. G.; Walter, J. A.; Wright, J. L. C.; Vining, L. C.; Can. J. Chem. 1978, 56, 1155. (3, 4.0 mg, t_R 10.8 min).

Methylcyclooctylprodigiosin (1)

¹H NMR (500 MHz, (CD₃)₂CO) δ 1.29 (d, 3H, J 6.8 Hz, H-9'), 1.37-1.77 (m, 10H, H-3'-H-7'), 1.92 (m, 2H, H-2'), 2.72 (m, 2H, H-1'), 2.98 (m, 1H, H-8'), 3.88 (s, 3H, OCH₃), 5.91 (d, 1H, J 3.4 Hz, H-c3), 6.00 (d, 1H, J 3.4 Hz, H-a4), 6.01 (s, 1H, H-b4), 6.44 (d, 1H, J 3.4 Hz, H-c4), 6.60 (d, 1H, J 3.4 Hz, H-a3), 6.65 (s, 1H, H-1''); HRESI-MS calcd. for C₂₃H₃₀N₃O, [M + H]⁺: 364.2383; found: 364.2387.

Cyclononylprodigiosin (2)

¹H NMR (500 MHz, (CD₃)₂CO) δ 1.41 (m, 4H, H-3' and H-7'), 1.53 (m, 6H, H-4'-H-6'), 1.70 (m, 4H, H-2' and H-8'), 2.72 (m, 4H, H-1' and H-9'), 3.88 (s, 3H, OCH₃), 5.93 (d, 1H, J 3.2 Hz, H-c3), 5.96 (d, 1H, J 3.3 Hz, H-a4), 6.03 (s, 1H, H-b4), 6.44 (d, 1H, J 3.2 Hz, H-c4), 6.61 (d, 1H, J 3.3 Hz, H-a3), 6.62 (s, 1H, H-1''); HRESI-MS calcd. for C₂₃H₃₀N₃O, [M + H]⁺: 364.2383; found: 364.2380.

Nonylprodigiosin (3)

¹H NMR (300 MHz, (CD₃)₂CO) δ 0.87 (t, 3H, J 6.3 Hz, H-9'), 1.29 (br, 12H, H-3'-H-8'), 1.73 (m, 2H, H-2'), 2.85 (m, 2H, H-1'), 4.12 (s, 3H, OCH₃), 6.35 (d, 1H, J 3.9 Hz, H-c3), 6.44 (dd, 1H, J 2.5, 2.6 Hz, H-a4), 6.71 (s, 1H, H-b4), 7.21 (br, 1H, H-c4), 7.21 (s, 1H, H- 1''), 7.29 (d, 1H, J 2.6 Hz, H-a3), 7.35 (br, 1H, H-a5); HRESI-MS calcd. for C₂₃H₃₂N₃O, [M + H]⁺: 366.2545; found: 366.2537.

Cytotoxicity assay

For cytotoxicity assessment, three human tumor and one non-tumor cell lines were used: HCT-116 (colon carcinoma; ATCC CCL-247), MCF-7 (breast carcinoma; ATCC HTB-22), SK-Mel-147 (melanoma; MSKCC CVCL-3876), and MRC-5 (normal lung fibroblast; ATCC CCL-171). HCT-116 and MCF-7 cells were grown in RPMI-1640 medium supplemented with 2 mM glutamine, while SK-Mel-147 and MRC-5 was grown in DMEM-F12 medium. Both media contained 10% fetal calf serum, 100 µg mL^-1 streptomycin, and 100 U mL^-1 penicillin. Cells were maintained at 37 ºC in a 5% CO₂ atmosphere. Cultures were regularly split to keep them in a logarithmic growth phase.

Cytotoxic activity of 1-3 was evaluated by the MTT assay.³³33 Mosmann, T.; J. Immunol. Methods 1983, 16, 55. Briefly, 24 h before addition of compounds, cells were seeded at 10⁴ cells per well in 96-well plates. Compounds previously dissolved in DMSO were added over 5-fold dilutions to each well and cells were exposed for 72 h. Negative controls received DMSO, while positive controls received doxorubicin (Sigma-Aldrich Co., USA). Prodigiosin, isolated as described by Arthaud et al.,¹⁷17 Arthaud, I. D. B.; Rodrigues, F. A. R.; Jimenez, P. J.; Montenegro, R. C.; Angelim, A. L.; Maciel, V. M. M.; Silveira, E. R.; Freitas, H. P. S.; Sousa, T. S.; Pessoa, O. D. L.; Lotufo, T. M. C.; Costa-Lotufo, L. V.; Chem. Biodiversity 2012, 9, 418. was included in the assays as a reference compound. At the end of the incubation period, 0.5 mg mL^-1 of MTT (3-(4,5-dimethyl-2-thiazolyl)-2,5-diphenyl-2H-tetrazolium bromide) was added to each well and removed 3 h later. Viable cells reduced the yellow MTT to a purple precipitate, formazan. The precipitate was dissolved in DMSO and the absorbance was measured using a multiplate reader (ThermoFisher Scientific). The cytotoxic effect of each concentration was quantified as the percentage of the control absorbance at 570 nm, while the IC₅₀, along with the respective 95% CI (confidence interval), were obtained by non-linear regression using GraphPad Prism 5.0 software.

gDNA sequencing, annotation and BGC mining

BRA 177 gDNA was purified as previously described for environmental samples³⁴34 Garcia, G. D.; Gregoracci, G. B.; Santos-Ede, O.; Meirelles, P. M.; Silva, G. G.; Edwards. R.; Sawabe, T.; Gotoh, K.; Nakamura, S.; Iida, T.; deMoura, R. L.; Thompson, F. L.; Microb. Ecol. 2013, 65, 1076. with minor modifications. Briefly, a cell pellet from 1.5 mL of BRA 177 cultures on A1 broth (28 ºC, 5 days, 150 rpm) was suspended in 1 mL of CTAB lyses buffer for freezing/thawing lyses cycles (5 min at -80 ºC and 5 min at 65 ºC). DNA was then purified by two phenol/chloroform extractions, precipitated with sodium acetate and isopropanol, washed with 70% ethanol and eluted with 10 mM Tris buffer (4 ºC, overnight). Resulting DNA solution was evaluated for integrity, purity and double-stranded DNA concentration by running an agarose gel (1% agarose, 0.5X TBE buffer) and by reading the DNA solution on a NanoDrop spectrophotometer (Thermo Fisher Scientific) and a Qubit fluorometer (Thermo Fisher Scientific). Approximately 4 ng of pure gDNA was used to generate a genomic library preparation with Nextera XT DNA Library Preparation Kit (Illumina), following manufacturer's instructions. Sequencing was performed at MiSeq platform (Illumina) with the MiSeq Reagent Kits v3 (600 cycles) chemistry. Raw sequence data was submitted to quality analysis and trimming with Prinseq³⁵35 Schmieder, R.; Edwards, R.; Bioinformatics 2011, 27, 863. and quality data assembled into contigs with SPAdesa new assembler for both single-cell and standard (multicell,³⁶36 Bankevich, A.; Nurk, S.; Antipov, D.; Gurevich, A. A.; Dvorkin, M.; Kulikov, A. S.; Lesin, V. M.; Nikolenko, S. I.; Pham, S.; Prjibelski, A. D.; Pyshkin, A. V.; Sirotkin, A. V.; Vyahhi, N.; Tesler, G.; Alekseyev, M. A.; Pevzner, P. A.; J. Comput. Biol. 2012, 19, 455. using default parameter for Illumina paired reads. Assembled genomic contigs were annotated with RAST server²⁰20 Aziz, R. K.; Bartels, D.; Best, A. A.; DeJongh, M.; Disz, T.; Edwards, R. A.; Formsma, K.; Gerdes, S.; Glass, E. M.; Kubal, M.; Meyer, F.; Olsen, G. J.; Olson, R.; Osterman, A. L.; Overbeek, R. A.; McNeil, L. K.; Paarmann, D.; Paczian, T.; Parrello, B.; Pusch, G. D.; Reich, C.; Stevens, R.; Vassieva, O.; Vonstein, V.; Wilke, A.; Zagnitko, O.; BMC Genomics 2008, 9, 75. using default parameters. Genome mining for natural products BGCs, was performed with ANTISMASH 3.0 software³⁷37 Blin, K.; Medema, M. H.; Kazempour, D.; Fischbach, M. A.; Breitling, R.; Takano, E.; Weber, T.; Nucleic Acids Res. 2013, 41, 204. using BRA 177 GenBank genomic annotations as input, with default parameters.

Alignment and phylogenetic analysis of 16S rRNA gene

BRA 177 16S rRNA gene sequence was analyzed and compared by SINA and BLASTn tools at SILVA³⁸38 Quast, C.; Pruesse, E.; Yilmaz, P.; Gerken, J.; Schweer, T.; Yarza, P.; Peplies, J.; Glöckner, F. O.; Nucleic Acids Res. 2013, 41, 590. and NCBI³⁹39 http://www.ncbi.nlm.nih.gov/, accessed in September 2016.
http://www.ncbi.nlm.nih.gov/... databases, respectively. The species related with strain BRA 177 were downloaded and aligned by MAFFT v7.017.⁴⁰40 Katoh, K.; Standley, D. M.; Mol. Biol. Evol. 2013, 30, 772. A phylogenetic tree was constructed using maximum likelihood in the PhyML program⁴⁰40 Katoh, K.; Standley, D. M.; Mol. Biol. Evol. 2013, 30, 772. with 1000 bootstrap replicates and GTR+G model. The best nucleotide model was chosen with Akaike Information Criterion (AIC) by jModelTest v2.1.4.⁴¹41 Darriba, D.; Taboada, G. L.; Doallo, R.; Posada, D.; Nat. Methods 2012, 9, 772.^,4242 Guindon, S.; Gascuel, O.; Syst. Biol. 2003, 52, 696. Alignment and inference of the tree were performed using plugins implemented in the Geneious R7 program. Mycobacterium tuberculosis was used as outgroup. The tree obtained was visualized using Figtree v.1.4.0.⁴³43 Rambaut, A. FigTree. http://tree.bio.ed.ac.uk/software/figtree, 2007.
http://tree.bio.ed.ac.uk/software/figtre...

Phylogenetic analysis of prodiginine synthases

RedL, RedJ and RedG proteins were chosen by literature search and SmartBlast⁴⁴44 https://blast.ncbi.nlm.nih.gov/smartblast/?LINK_LOC=BlastHomeLink, accessed in September 2016.
https://blast.ncbi.nlm.nih.gov/smartblas... with putative proteins homologs from BRA 177 prodiginine BGC. Amino acids sequences were retrieved from the GenBank⁴⁵45 http://www.ncbi.nlm.nih.gov/genbank/, accessed in September 2016.
http://www.ncbi.nlm.nih.gov/genbank/... and Uniprot⁴⁶46 Consortium U.; Nucleic Acids Res. 2015, 43, 204. databases, and amino acid protein sequences were aligned with CLustalW.⁴⁷47 Thompson, J. D.; Higgins, D. G.; Gibson, T. J.; Nucleic Acids Res. 1994, 22, 4673. Maximum likelihood trees were then constructed at MEGA 6.0 software.⁴⁸48 Tamura, K.; Stecher, G.; Peterson, D.; Filipski, A.; Kumar, S.; Mol. Biol. Evol. 2013, 30, 2725. The best fitting amino acid substitution model within the 48 evaluated models were, respectively: Whelan-Goldman matrix (WAG)⁴⁹49 Whelan, S.; Goldman, N.; Mol. Biol. Evol. 2001, 18, 691. improved by a gamma distribution (+G) for RedL, and also amino acids frequency (+F) for RedG, WAG +F assuming that a certain fraction of sites are evolutionarily invariable (+I) for RedJ, and LG +G +F for RedL adenylation domain. Node support was accessed by Bootstrap method with 1000 replicates.⁵⁰50 Le, S. Q.; Gascuel, O.; Mol. Biol. Evol. 2008, 25, 1307.

Supplementary Information

Supplementary information is available free of charge at http://jbcs.sbq.org.br as a PDF file.

Acknowledgments

This work was supported by Conselho Nacional de Desenvolvimento Científico e Tecnológico (CNPq No. 458548/2013-8 and 473030/2013/6). The authors also thank Dr Lucas Buruaem for constructing the SPSPA map. The scientific expedition and all logistic support were provided by the Secretaria da Comissão Interministerial dos Recursos do Mar (SECIRM) as part of the Program PROARQUIPELAGO.

References

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