BINARY CO-CULTURE SELECTION FROM MARINE-DERIVED MICROORGANISMS FOR DIFFERENTIAL PRODUCTION OF SPECIALIZED METABOLITES

Martínez-Buitrago, Paola A.; Ramos, Freddy A.; Castellanos, Leonardo

doi:10.21577/0100-4042.20170388

Abstract

Nowadays the discovery of new compounds from microorganisms has substantially decreased. Genomic studies have shown that certain genes are not expressed under standard laboratory conditions. In order to overcome this problem, several methods including microorganism co-culture have been developed. The aim of this work was to select binary co-cultures of marine-derived microorganisms to pursue further chemical studies. From 15 microorganisms, 151 interactions assays in solid media were performed using two different methodologies: distance assays and contact assays that allowed to distinguish between interactions due to diffusible compounds or due to cell-cell contact. For distance assays, the metabolic production changes were evaluated using 3 zones: two corresponding to each microorganism colony, and a third zone corresponding to the interaction zone. This division zone strategy allowed to assess the diffusion compounds gradient, and to suggest the producer microorganism of the induced compounds. The metabolic production of the co-cultures was evaluated using HPLC-DAD and NMR. Seven co-cultures were identified to be able to induce changes in the metabolic production. Remarkably, the co-culture between the fungus Purpureocillium sp. PNM-67 and the bacteria Rhodococcus sp. RKHC-26 or Gordonia sp. PNM-25 induce production of a red dye in the fungus. These are the first successful examples of interaction between a fungus and a mycolic acid-containing bacteria.

Keywords:
microbial co-culture; mixed fermentation; interspecies interaction; mycolic acid-containing bacteria; marine natural products

INTRODUCTION

Over the years, compounds isolated from microorganisms have played an important role in the treatment of human diseases and have revolutionized the pharmaceutical industry. However, redundant isolation of microbial compounds is increasingly common.¹1 Katz, L.; Baltz, R. H.; J. Ind. Microbiol. Biotechnol. 2016, 43, 155. Recent research on microorganisms' genome has shown that there are silent and cryptic biosynthetic pathways, which are not expressed in standard laboratory growth conditions. To promote the activation of these routes, different methods have been developed, including microorganism co-culture.²2 Ochi, K.; J. Antibiot. (Tokyo) 2017, 70, 25.

This approach takes into account that microorganisms normally grow in complex environments, in this way inter- or intraspecies interactions are prevalent in nature, and the growth of a microorganism in the presence of others, can alter or stimulate their specialized metabolism.³3 Okada, B. K.; Seyedsayamdost, M. R.; FEMS Microbiol. Rev. 2017, 41, 19. In fact, some studies have shown that when microorganisms interact with others, they produce specialized metabolites that can have positive (e.g. communication with other microorganisms) or negative (e.g. antibiotics) effects on others.⁴4 Abrudan, M. I.; Smakman, F.; Grimbergen, A. J.; Westhoff, S.; Miller, E. L.; van Wezel, G. P.; Rozen, D. E.; Proc. Natl. Acad. Sci. U. S. A. 2015, 112, 11054.^,⁵5 de Weert, S.; Kuiper, I.; Lagendijk, E. L.; Lamers, G. E. M.; Lugtenberg, B. J. J.; Mol. Plant-Microbe Interact. 2004, 17, 1185. Both scenarios are equally interesting on the discovery of novel compounds, and on the understanding of the role of specialized metabolites in nature.

Microorganism co-culture consists in the cultivation of two or more microorganisms in the same confined environment.⁶6 Bertrand, S.; Bohni, N.; Schnee, S.; Schumpp, O.; Gindro, K.; Wolfender, J.-L.; Biotechnol. Adv. 2014, 32, 1180. One of the first successful examples of co-cultivation was reported by Cueto and collaborators in 2001.⁷7 Cueto, M.; Jensen, P. R.; Kauffman, C.; Fenical, W.; Lobkovsky, E.; Clardy, J.; J. Nat. Prod. 2001, 64, 1444. In this study, a co-culture between the fungus Pestalotia sp. and the bacteria Thalassospira sp. was evaluated for its metabolic production, and led to the isolation and structural elucidation of pestalone, a benzophenone that showed antibacterial activity, and whose production was only associated with co-culture. Since then, studies have spread to bacteria-bacteria,⁸8 Dashti, Y.; Grkovic, T.; Abdelmohsen, U.; Hentschel, U.; Quinn, R.; Mar. Drugs 2014, 12, 3046.

9 Patin, N. V.; Floros, D. J.; Hughes, C. C.; Dorrestein, P. C.; Jensen, P. R.; Microbiology 2018, 164, 946.^-¹⁰10 Adnani, N.; Chevrette, M. G.; Adibhatla, S. N.; Zhang, F.; Yu, Q.; Braun, D. R.; Nelson, J.; Simpkins, S. W.; McDonald, B. R.; Myers, C. L.; Piotrowski, J. S.; Thompson, C. J.; Currie, C. R.; Li, L.; Rajski, S. R.; Bugni, T. S.; ACS Chem. Biol. 2017, 12, 3093. fungus-fungus¹¹11 Bertrand, S.; Schumpp, O.; Bohni, N.; Monod, M.; Gindro, K.; Wolfender, J.-L.; J. Nat. Prod. 2013, 76, 1157.

12 Bohni, N.; Hofstetter, V.; Gindro, K.; Buyck, B.; Schumpp, O.; Bertrand, S.; Monod, M.; Wolfender, J.-L.; Molecules 2016, 21, 370.^-¹³13 Serrano, R.; González-Menéndez, V.; Rodríguez, L.; Martín, J.; Tormo, J. R.; Genilloud, O.; Front. Microbiol. 2017, 8, 649. and bacteria-fungus¹⁴14 Yu, L.; Ding, W.; Wang, Q.; Ma, Z.; Xu, X.; Zhao, X.; Chen, Z.; Tetrahedron 2017, 73, 907.

15 Wakefield, J.; Hassan, H. M.; Jaspars, M.; Ebel, R.; Rateb, M. E.; Front. Microbiol. 2017, 8, 1284.^-¹⁶16 Wu, C.; Zacchetti, B.; Ram, A. F. J.; van Wezel, G. P.; Claessen, D.; Hae Choi, Y.; Sci. Rep. 2015, 5, 10868. interactions. As a result of co-culture, increased metabolite yields have been reported, as well as the production of analogues of known metabolites and the induction of new bioactive metabolites.¹⁷17 Pettit, R. K.; Appl. Microbiol. Biotechnol. 2009, 83, 19.

One of the challenges of using this co-culture approach is the microorganisms selection for co-culture establishment. In most of the reports, the selected microorganisms come from a screening of multiple pairs of microorganisms, or the authors do not mention the reason that support their choice. A revision of specialized literature allowed us to identify the following criteria to select the microorganisms: (1) the use of mycolic acid containing bacteria,¹⁸18 Onaka, H.; Mori, Y.; Igarashi, Y.; Furumai, T.; Appl. Environ. Microbiol. 2011, 77, 400. (2) the establishment of interactions already observed in nature (ecological criteria),¹⁹19 Rateb, M. E.; Hallyburton, I.; Houssen, W. E.; Bull, A. T.; Goodfellow, M.; Santhanam, R.; Jaspars, M.; Ebel, R.; RSC Adv. 2013, 3, 14444. (3) the confrontation with pathogens,²⁰20 Burgess, J. G.; Jordan, E. M.; Bregu, M.; Mearns-Spragg, A.; Boyd, K. G.; J. Biotechnol. 1999, 70, 27. (4) the confrontation between bacteria of the genus Streptomyces²¹21 Ueda, K.; Kawai, S.; Ogawa, H.; Kiyama, A.; Kubota, T.; Kawanobe, H.; Beppu, T.; J. Antibiot. (Tokyo) 2000, 53, 979. and (5) the confrontation between bacteria of the genus Streptomyces with a bacteria from the phylum Proteobacteria.²²22 Carlson, S.; Tanouye, U.; Omarsdottir, S.; Murphy, B. T.; J. Nat. Prod. 2015, 78, 381. Other challenges in co-culture studies include the selection of factors such as culture media, the degree of contact between microorganisms, population density and fermentation time.²³23 Goers, L.; Freemont, P.; Polizzi, K. M.; J. R. Soc. Interface 2014, 11, 20140065.

The degree of contact between the microorganisms showed to be important because the effects can be the result of two types of interaction: interaction due to diffusible compounds (related to nutrient supply or production of an antibiotic or signaling molecule) and interaction due to cell-cell contact.³3 Okada, B. K.; Seyedsayamdost, M. R.; FEMS Microbiol. Rev. 2017, 41, 19. Taking this into account, in co-cultures, microorganisms may be perfectly mixed or partially separated. About the culture growth medium, solid or liquid broth can be used. The selection of the culture medium must take into account the two microorganisms involved.²³23 Goers, L.; Freemont, P.; Polizzi, K. M.; J. R. Soc. Interface 2014, 11, 20140065.

The solid medium has been used in co-cultures because, unlike the liquid broth, it enables to visualize the morphology and interaction patterns between microorganisms, that allow to observe phenotypic changes including developmental defects, growth inhibition, lysis, motility, pigment production, among others.²⁴24 Stubbendieck, R. M.; Vargas-Bautista, C.; Straight, P. D.; Front. Microbiol. 2016, 7, 1234. It also facilitates the spatial location of metabolites,²⁵25 Yang, Y.-L.; Xu, Y.; Straight, P.; Dorrestein, P. C.; Nat. Chem. Biol. 2009, 5, 885. which allows the identification of the organism responsible for the production of compounds induced by interaction.

Although co-cultivation is a promising strategy that has produced successful results, these have generally been a consequence of serendipity.²⁶26 Nai, C.; Meyer, V.; Trends Microbiol. 2018, 26, 538. For this reason, this strategy still presents disadvantages such as the lack of reproducibility and predictability. To address these drawbacks, this strategy still faces the challenge of developing standardized protocols, as well as establishing methodologies to evaluate a large number of interactions simultaneously.²⁶26 Nai, C.; Meyer, V.; Trends Microbiol. 2018, 26, 538. This could result in more specific criteria for the selection of microorganisms, or in the characterization of promoting factors produced by stimulating strains that could guide to the development of effective co-culture conditions.

In this study, a screening of binary interactions was performed in solid media using different methodologies in order to prioritize microorganisms' co-cultures for the evaluation of their metabolic production.

EXPERIMENTAL SECTION

General

Bacteriological agar (Scharlau), tryptose (Scharlau), sodium chloride (Merck), yeast extract (Oxoid), malt extract (Scharlau), glucose (Merck), potato dextrose agar (Scharlau), iron sulphate heptahydrate (Chemie Loba), manganese chloride tetrahydrate (Chemie Loba), zinc sulphate heptahydrate (Chemie Loba) and commercial oatmeal were used for culture media. Ethyl acetate (Panreac AppliChem) was used for extractions. For chromatographic analysis, acetonitrile HPLC grade (Honeywell) and deionized water were used. For nuclear magnetic resonance analysis CDCl₃ with deuteration grade 99.8 % (Merck) and methanol-d₄ with deuteration grade 99.8% (Merck) were used.

Microorganism selection

Based on criteria reported in the literature, 15 microorganisms (14 bacteria and 1 fungus) were selected from our in-home microorganism collection. This collection of microorganisms was built by the recovery of bacteria and fungi from samples of marine environments including sediments, invertebrates and algae collected at the reef of the island of Providencia and Santa Catalina.²⁷27 Betancur, L. A.; Naranjo-Gaybor, S. J.; Vinchira-Villarraga, D. M.; Moreno-Sarmiento, N. C.; Maldonado, L. A.; Suarez-Moreno, Z. R.; Acosta-González, A.; Padilla-Gonzalez, G. F.; Puyana, M.; Castellanos, L.; Ramos, F. A.; PLoS One 2017, 12, e0170148.

Primary selection of couples to be evaluated

In order to reduce the number of couples to be evaluated in bacteria-bacteria distance interactions, a first assay was carried out to prioritize those couples that showed phenotypic changes. The methodology developed by Seyedsayamdost et al. was adapted.²⁸28 Correa, H.; Haltli, B.; Duque, C.; Kerr, R.; Microb. Ecol. 2013, 66, 972.

Each bacteria was grown in 10 mL of Luria-Bertani medium (composition per liter: tryptose 10 g, NaCl 10 g, yeast extract 5 g) until reaching a OD_600nm between 0.6 and 0.8. From each of these cultures 1µL aliquots were taken and sown in 150*15 mm Petri dishes containing solid Luria-Bertani medium (composition per liter: tryptose 10 g, NaCl 10 g, yeast extract 5 g, agar 14 g). In each dish the interaction of 36 pairs was evaluated arranging them in 3 columns separated by 1 cm of distance. In each couple the bacteria were sown 5 mm away. At the left and right end of the Petri dish a column of each single bacteria was sown as control. The seeding arrangement of the bacteria is shown in Figure 1S of the supplementary material. Each pair was evaluated by triplicate. Petri dishes were incubated at 28 ºC for 5 days. After this time, the phenotypic changes induced by co-culture (growth inhibition, pigmentation, sporulation, macroscopic morphology) were evaluated by visual comparison with the respective controls.

Binary co-cultures

Two different methods were used: a distance assay and a contact assay. The methodology was divided into two types of interactions: bacteria-bacteria and bacteria-fungus. All tests were performed on 90 mm*15 mm Petri dishes. For bacteria the used inoculum was 10⁵5 de Weert, S.; Kuiper, I.; Lagendijk, E. L.; Lamers, G. E. M.; Lugtenberg, B. J. J.; Mol. Plant-Microbe Interact. 2004, 17, 1185. CFU per dish, and in the case of the fungus 10⁵5 de Weert, S.; Kuiper, I.; Lagendijk, E. L.; Lamers, G. E. M.; Lugtenberg, B. J. J.; Mol. Plant-Microbe Interact. 2004, 17, 1185. conidia per dish were used.

Bacteria-bacteria interactions

Luria-Bertani (composition per liter: tryptose 10 g, NaCl 10 g, yeast extract 5 g, and agar 14 g) was used as culture media. In the distance assay the microorganisms were sown at a distance of 5 mm from each other. For the contact assay, aliquots of each one of the microorganisms were mixed, and this mixture was inoculated on the surface of the agar. The seeding arrangement of the bacteria is shown in Figure 2S of the supplementary material. Three replicates were made of each co-culture. Monocultures of each of the bacteria were performed also by triplicate under the same conditions. In both cases, the dishes were incubated at 30 ºC for 5 days.

Bacteria-fungus interactions

Cultures were made in solid medium using 4 different culture media: a) LB supplemented with glucose (composition per liter: tryptose 10 g, NaCl 10 g, yeast extract 5 g, glucose 20 g, and agar 14 g), b) PDA (composition per liter: potato peptone 4 g, glucose 20 g, and agar 15 g), c) ISP2 (composition per liter: malt extract 10 g, yeast extract 4 g, glucose 4 g, and agar 20 g), and d) ISP3 (composition per liter: Oatmeal 20 g, agar 18 g, and trace solution 1 mL). For the distance assay, the bacteria were inoculated in the centre of the dish in a strip 1 cm wide, while the fungus was inoculated at opposite ends of the dish. For the contact assay, aliquots of each one of the microorganisms were mixed, and this mixture was then inoculated. The seeding arrangement of microorganisms is shown in Figure 3S of the supplementary material. three replicates of each co-culture were made. Monocultures of each of the bacteria and fungus were made by triplicate under the same conditions as the co-cultures. In both cases, the dishes were incubated at 30 ºC for 10 days.

In all established binary co-cultures, phenotypic changes induced by co-culture were visually assessed looking for changes in growth, pigmentation, sporulation, and macroscopic morphology.

Extraction

In contact assays the agar was cut into 1 cm*1 cm pieces using a sterile blade. In the distance assays, three different zones were previously defined, which can be seen in figure 4S of the supplementary material, and then each zone was cut into pieces separately. Each sample was freeze-dried using a LABCONCO lyophilizer (Freezone 4.5). The dry material was extracted twice with ethyl acetate, at a ratio of 70 mL of solvent per dish. The extractions were performed using a Cole-Parmer ultrasound bath at room temperature for 20 minutes. The samples were filtered and dried at reduced pressure.

Metabolic profiling

Organic extracts were analyzed by liquid chromatography using a UHPLC Thermo Dionex Ultimate 3000 (Germering) device with a DAD detector. The extracts were previously dissolved in methanol to have a final concentration of 2 mg mL^-1, and an injection of 20 µL was made. A Kinetex 2.6 µm C8 (100x4.6 mm) column was used. Solvents used in elution were: water (A) and acetonitrile (B). The analysis program for all the extracts was: a gradient that started with 10% of phase B, and increased linearly to 100% in 23 minutes, keeping this ratio for 2 more minutes. The flow was set to 0.5 mL min^-1. The spectra of ¹H NMR and COSY for organic extracts were obtained in a Bruker Avance 400, using as solvents CDCl₃ and methanol-d₄. Differences in the metabolic production of co-cultures, in comparison to monocultures and culture medium, were determined by comparison of HPLC-DAD chromatograms and ¹H NMR spectra.

RESULTS AND DISCUSSION

Co-culture as a tool of induction of bioactive metabolites is a relatively recent method, without not fully defined criteria for its establishment.²⁶26 Nai, C.; Meyer, V.; Trends Microbiol. 2018, 26, 538. Some selection criteria for establish the most promising interactions have been described in the literature, which are particularly true for bacteria-bacteria interactions, while for bacterial-fungus interactions this is limited to ecological criteria.

In this study, 14 bacteria and 1 fungus were selected from our collection of microorganisms that comprises mostly marine recovered isolates, as well as some soil recovered isolates, which are summarized in Table 1 where the inclusion criteria is also described.

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Table 1
Microorganisms selected for the establishment of binary co-cultures

Bacteria-bacteria co-cultures

Distance assays

Co-cultures assays enable to evaluate effects mediated by diffusible compounds. A first assay that would prioritize couples that would later be evaluated in individual Petri dish assays was conducted. For this purpose, the methodology proposed by Seyedsayamdost and collaborators²⁹29 Seyedsayamdost, M. R.; Traxler, M. F.; Clardy, J.; Kolter, R.; Methods Enzymol. 2012, 517, 89. was adapted to evaluate the phenotypic changes associated to interactions, taking into account that these could be indicators of changes in metabolic production. Phenotypic changes were observed in 27 out of 91 tested couples. Growth inhibition was observed in 18 out of the 27 cases and pigmentation changes and/or sporulation in 9 out of the 27 cases (detailed results are found in Figure 5S).

These 27 interactions that showed phenotypic changes were cultured in 9cm Petri dishes by triplicate, in order to obtain organic extracts that allowed evaluating the metabolic production. Each extract was analyzed by HPLC-DAD (in the range of 200-600 nm); however, no changes were observed in the metabolic production of 27 co-cultures in comparison with those of the corresponding monocultures. The 18 co-cultures that showed bacterial growth inhibition were analyzed by NMR. This technique did not showed changes in co-cultures spectra in comparison with those of the monocultures spectra. Thus, this methodology did not allow to select any co-cultures to evaluate their metabolite production.

It is worth to mention that co-cultures could be producing compounds in response to the presence of the other microorganism, but the analytical techniques here employed did not allow to detect such production changes. More sensitive analytical techniques such as HPLC-MS, could help to detect metabolic production changes in these distance assays.¹²12 Bohni, N.; Hofstetter, V.; Gindro, K.; Buyck, B.; Schumpp, O.; Bertrand, S.; Monod, M.; Wolfender, J.-L.; Molecules 2016, 21, 370.^,³⁰30 Caraballo-Rodríguez, A. M.; Dorrestein, P. C.; Pupo, M. T.; Sci. Rep. 2017, 7, 5373. The above since this technique is several orders of magnitude more sensitive than NMR.³¹31 Wolfender, J.-L.; Planta Med. 2009, 75, 719. Also, it is important to consider that while HPLC-MS is more sensitive, their isolation could be difficult because they can be found in small quantities, whereas compounds detected by NMR could be isolated by traditional methods.

Contact assays

For the selection of couples in this type of assay, there is no applicable methodology such as the phenotypic change assay performed in distance assays. For this reason, some bacteria were not considered in this study, the exclusion criteria are explained below.

Co-culture couples containing the bacteria Gordonia sp. PNM-25 and Dietzia sp. RKHC-59b were discarded because their growth rate in the selected culture medium was significantly slower in comparison with other strains. Co-culture couples including Brevibacillus sp. PNM-157, Paenibacillus sp. PNM-210, Paenibacillus sp, PNM-115 and Paenibacillus sp. PNM-123 were also discarded since in previous studies they showed potent antibiotic properties.

In order to reduce the number of interactions to be evaluated, 3 criteria derived from literature were used: (1) co-cultures involving 2 strains of the genus Streptomyces; (2) co-cultures involving strains of the genus Streptomyces and mycolic-acid containing bacteria; and (3) co-cultures involving 2 strains obtained from the same environmental sample. In this way, 13 selected pairs were grown in 9cm petri dishes by triplicate. Co-cultures results are summarized in Table 1S of the supplementary material. The ¹H NMR analyses of these 13 co-cultures allowed to identify Streptomyces sp. PNM-161a and Rhodococcus sp. RKHC-26 co-culture as producer of compounds absent in both, the broth blank and the monocultures. The signals for induced compounds are found at δ_H 1.5-1.7, 2.35-2.50, and 2.95 (bt, J=7.5Hz) for aliphatic protons, and at δ_H 7.15 (m) for aromatic protons (Figure 6S).

Bacteria-fungus co-cultures

Most of successful co-culture examples involve at least one fungus.³²32 Adnani, N.; Rajski, S. R.; Bugni, T. S.; Nat. Prod. Rep. 2017, 34, 784. Thus, pairings between the fungal isolate Purpureocillium sp. PNM-67 and 14 different bacteria were performed. As initial criterion for matching, the capability of growing in four different culture media was used (Table 2). All co-cultures were initially evaluated in a distance assay, and those couples that had a phenotypic change when the two microorganisms came into contact, were also evaluated in a contact assay. The results of both approaches are summarized below.

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Table 2
Results of the binary co-cultures between the bacteria and the fungus Purpureocillium sp. PNM-67 in distance assays using different culture media

Distance assays

Distance assays were performed on 4 different culture media (PDA, LBG, ISP2, ISP3). A total of 45 assays were conducted and phenotypic changes were observed in 13 cases. The predominant phenotypic change was inhibition of fungal growth in response to its interaction with several bacteria. In order to obtain the organic extracts from these assays, three zones at Petri dish were defined, the first one where the fungus was inoculated; the second one where the bacteria was inoculated; and a third zone, which will be called “interaction zone” because it was spatially between the two inoculums. This division allowed to suggest which was the producer of the compounds due to their diffusion gradient.

The obtained results are summarized in Table 2. Phenotypic changes were observed in 13 out of 45 assays; in all cases inhibition of fungal growth was observed. Extracts from the interaction zones of these 13 co-cultures were analyzed by HPLC-DAD, and changes were observed in 8 cases (1 case in PDA, 3 in ISP2 and 4 in ISP3). It is important to observe that the bacteria involved in these co-cultures belong to the genera Streptomyces sp. (PNM-9 and IBUN-5.1.), Paenibacillus sp. (PNM-115, PNM-123 and PNM-210) and Brevibacillus sp. (PNM-157). These 8 co-cultures were also analyzed by ¹H NMR, and changes were found in 5 cases which are described below.

In the first co-culture, between the fungus Purpureocillium sp. PNM-67 and the bacterium Paenibacillus sp. PNM-123 in PDA; changes in phenotype, in HPLC-DAD and ¹H NMR were observed. HPLC analysis for the interaction zone, showed two peaks (maximum absorbance at 320 nm) that are not present in the monocultures. These peaks are also present in the bacteria zone in the co-culture dish, so the diffusion gradient of these compounds indicates that they are produced by the bacteria in response to its interaction with the fungus. This co-culture was also analyzed by ¹H NMR, where signals exclusive to co-culture extracts in bacterial and interaction zones were found between 7.6 and 7.8 ppm. Changes induced by co-culture are showed in Figure 1. Both analytical techniques suggest that compounds induced by co-culture have aromatic features.

Figure 1
Comparison of HPLC-DAD chromatograms (320nm) at the left and comparison of 1H NMR spectra at the right for the organic extracts of: (a) culture medium PDA, (b) monoculture of Purpureocillium sp. PNM-67, (c) monoculture of Paenibacillus sp. PNM-123 and the three zones of the co-culture dish (d) fungus zone, (e) interaction zone and (f) bacteria zone

The co-cultures of the fungus PNM-67 with the bacteria Paenibacillus sp. PNM-115, Paenibacillus sp. PNM-123, Paenibacillus sp. PNM-210 and Streptomyces sp. IBUN-5.1, in medium ISP3 showed by HPLC one same peak (both in retention time and UV spectrum) in all cases that can be associated to co-culture. This peak was obtained from interaction zone of the co-culture extracts and was absent in the corresponding monocultures. The ¹H NMR analyses for these extracts showed the presence of the same signals but in different proportions (Figure 2).

Figure 2
Comparison of HPLC-DAD chromatograms (320nm) at the left and 1H NMR spectra (expansion 6-8ppm) at the right for organic extracts of the interaction zones of the co-cultures between Purpureocillium sp. PNM-67 and: (a) Paenibacillus sp. PNM-123, (b) Paenibacillus sp. PNM-115, (c) Streptomyces sp. IBUN-5.1 and (d) Paenibacillus sp. PNM-210. (e) Monoculture of the fungus Purpureocillium sp. PNM-67

The results indicate that the induced compounds were produced by the fungus because the signals (HPLC-DAD and ¹H NMR) were found in both, the interaction zone and the fungus zone of the 4 co-cultures. In addition, the possible role of these compounds is the defense of the fungus against the bacteria, taking into account that there is inhibition of fungal growth in the 4 co-cultures. Using the COSY experiment, it was found that the signals at 7.28 and 6.37 ppm coupled among them, indicating that they are part of the same compound. Further studies will enable to establish if the signals in NMR and the peak in HPLC-DAD correspond to the same compound(s).

Contact assays

In distance assays, two co-cultures stood out due to their reddish pigmentation that happened when the fungus came into contact with the bacteria Gordonia sp. PNM-25 as well as with Rhodococcus sp. RKHC-26. It is noteworthy that these two bacteria were initially included in the set of microorganisms because they are mycolic acid-containing bacteria. In the case of bacteria-bacteria co-cultures, bacteria containing mycolic acid have been shown to be able to induce the production of specialized metabolites in bacteria from the Streptomyces genus.³³33 Onaka, H.; Mori, Y.; Igarashi, Y.; Furumai, T.; Appl. Environ. Microbiol. 2011, 77, 400. Recent studies have shown that the effect of mycolic acid containing bacteria also extends to other Actinobacteria;³⁴34 Hoshino, S.; Okada, M.; Awakawa, T.; Asamizu, S.; Onaka, H.; Abe, I.; Org. Lett. 2017, 19, 4992. however, there are no reports showing that they also have such effect on fungus³⁵35 Hoshino, S.; Onaka, H.; Abe, I.; J. Ind. Microbiol. Biotechnol. 2018, 1.. In this way, these two co-cultures could be of great interest, as they constitute the first examples of the effect of mycolic acid containing bacteria on fungi. The fact that these two co-cultures show changes only when performed by a contact assay methodology support the reports that show that mycolic acid containing bacteria exert their effect only when they are alive and have cell to cell contact with the other organism.³⁵35 Hoshino, S.; Onaka, H.; Abe, I.; J. Ind. Microbiol. Biotechnol. 2018, 1.

In an effort to increase the production of this red pigment, these two co-cultures were evaluated in a contact assay. In the case of the co-culture between PNM-67 and RKHC-26, the red pigment could be observed in the whole dish.On the other hand Gordonia sp. PNM-25 did not survive to the assay conditions. Changes to the methodology of the contact assay (like inoculation timing) could lead to the survival of Gordonia sp. PNM-25. There are many reports of microbial pigments functions, ranging from their protective activity against ultraviolet radiation, antimicrobial oxidants or compounds produced by other microorganisms, until its antimicrobial activity against other microorganisms.³⁶36 Liu, G. Y.; Nizet, V.; Trends Microbiol. 2009, 17, 406. In addition, the production of this red pigment can be used as an indicator of change in another metabolites production.²⁸28 Correa, H.; Haltli, B.; Duque, C.; Kerr, R.; Microb. Ecol. 2013, 66, 972.^,³³33 Onaka, H.; Mori, Y.; Igarashi, Y.; Furumai, T.; Appl. Environ. Microbiol. 2011, 77, 400.^,³⁷37 Yang, Y.-L.; Xu, Y.; Kersten, R. D.; Liu, W.-T.; Meehan, M. J.; Moore, B. S.; Bandeira, N.; Dorrestein, P. C.; Angew. Chem., Int. Ed. 2011, 50, 5839. HPLC-DAD analyses showed no single peak for co-culture while ¹H NMR analyses showed signals in δ_H 0.84-0.87, 4.54 (td, J=11.0; 4.2 Hz), and 7.85-7.88 exclusive for co-culture, as is showed in Figure 3.

Figure 3
Comparison of 1H NMR spectra for organic extracts of a) culture medium LB, (b) monoculture of Purpureocillium PNM-67, (c) monoculture of Rhodococcus sp. RKHC-26 and (d) co-culture of them

The most relevant information of the selected co-cultures during this study is summarized in Table 3.

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Table 3
Selected binary co-cultures that induce changes in metabolic production

CONCLUSIONS

From a set of 15 microorganisms (14 bacteria and 1 fungus), co-cultures between bacteria-bacteria and bacteria-fungus were evaluated through 151 assays, using distance interactions and contact interactions in solid media. The main advantage of distance assays over contact assays is that the former facilitates the survival of the two strains. Seven co-cultures induce changes in the metabolic production, five of them due diffusible compounds, and two of them due to cell-to-cell contact.

The use of HPLC-DAD and NMR techniques, as a strategy for monitoring metabolic production, can be used to detect and monitor larger changes in metabolic profile, with the advantage that this technique gives information about the isolable compounds. However, the use of LC-MS/MS for co-culture monitoring could be a valuable technique in order to follow small metabolic changes related to interactions.

The co-culture between the fungus Purpureocillium sp. PNM-67 and the bacteria Rhodococcus sp. RKHC-26 or Gordonia sp. PNM-25 induce red pigmentation in the fungus Purpureocillium sp. PNM-67, that could be associated with a change in the metabolic production. These are the first successful examples of interactions between a fungal isolate and a mycolic acid-containing bacterium. This kind of interaction could be considered as criteria for selecting couples for co-culture studies.

ACKNOWLEDGMENTS

P. Martínez thanks to Colciencias for the program “Jóvenes Investigadores Convocatoria 761 de 2016”. This work was supported in part by research grants from Colciencias and Universidad Nacional de Colombia-DIB. We would like to thank to ANLA and Ministerio de Ambiente y Desarrollo Sostenible for the permission to collect samples and perform this research (Permiso No. 4 de 10/02/2010, Anexo 2, Contrato de Acceso a Recurso Genético No. 108 Otrosi No. 6 al contrato marco de acceso a recurso genético y sus productos derivados No. 121 del 22 de enero del 2016).

SUPPLEMENTARY MATERIAL

The figures related to the experimental part and some details about the results obtained are in the supplementary material that is available in http://quimicanova.sbq.org.br in the form of an open PDF file.

REFERENCES

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Yu, L.; Ding, W.; Wang, Q.; Ma, Z.; Xu, X.; Zhao, X.; Chen, Z.; Tetrahedron 2017, 73, 907.
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Pettit, R. K.; Appl. Microbiol. Biotechnol. 2009, 83, 19.
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Onaka, H.; Mori, Y.; Igarashi, Y.; Furumai, T.; Appl. Environ. Microbiol. 2011, 77, 400.
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Correa, H.; Haltli, B.; Duque, C.; Kerr, R.; Microb. Ecol. 2013, 66, 972.
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Seyedsayamdost, M. R.; Traxler, M. F.; Clardy, J.; Kolter, R.; Methods Enzymol. 2012, 517, 89.
³⁰
Caraballo-Rodríguez, A. M.; Dorrestein, P. C.; Pupo, M. T.; Sci. Rep. 2017, 7, 5373.
³¹
Wolfender, J.-L.; Planta Med. 2009, 75, 719.
³²
Adnani, N.; Rajski, S. R.; Bugni, T. S.; Nat. Prod. Rep. 2017, 34, 784.
³³
Onaka, H.; Mori, Y.; Igarashi, Y.; Furumai, T.; Appl. Environ. Microbiol. 2011, 77, 400.
³⁴
Hoshino, S.; Okada, M.; Awakawa, T.; Asamizu, S.; Onaka, H.; Abe, I.; Org. Lett. 2017, 19, 4992.
³⁵
Hoshino, S.; Onaka, H.; Abe, I.; J. Ind. Microbiol. Biotechnol. 2018, 1.
³⁶
Liu, G. Y.; Nizet, V.; Trends Microbiol. 2009, 17, 406.
³⁷
Yang, Y.-L.; Xu, Y.; Kersten, R. D.; Liu, W.-T.; Meehan, M. J.; Moore, B. S.; Bandeira, N.; Dorrestein, P. C.; Angew. Chem., Int. Ed. 2011, 50, 5839.

Publication Dates

Publication in this collection
26 Aug 2019
Date of issue
July 2019

History

Received
18 Jan 2019
Accepted
26 June 2019
Published
29 July 2019

This is an Open Access article distributed under the terms of the Creative Commons Attribution License, which permits unrestricted use, distribution, and reproduction in any medium, provided the original work is properly cited.

[1] ¹
Katz, L.; Baltz, R. H.; J. Ind. Microbiol. Biotechnol. 2016, 43, 155.

[2] ²
Ochi, K.; J. Antibiot. (Tokyo) 2017, 70, 25.

[3] ³
Okada, B. K.; Seyedsayamdost, M. R.; FEMS Microbiol. Rev. 2017, 41, 19.

[4] ⁴
Abrudan, M. I.; Smakman, F.; Grimbergen, A. J.; Westhoff, S.; Miller, E. L.; van Wezel, G. P.; Rozen, D. E.; Proc. Natl. Acad. Sci. U. S. A. 2015, 112, 11054.

[5] ⁵
de Weert, S.; Kuiper, I.; Lagendijk, E. L.; Lamers, G. E. M.; Lugtenberg, B. J. J.; Mol. Plant-Microbe Interact. 2004, 17, 1185.

[6] ⁶
Bertrand, S.; Bohni, N.; Schnee, S.; Schumpp, O.; Gindro, K.; Wolfender, J.-L.; Biotechnol. Adv. 2014, 32, 1180.

[7] ⁷
Cueto, M.; Jensen, P. R.; Kauffman, C.; Fenical, W.; Lobkovsky, E.; Clardy, J.; J. Nat. Prod. 2001, 64, 1444.

[8] ⁸
Dashti, Y.; Grkovic, T.; Abdelmohsen, U.; Hentschel, U.; Quinn, R.; Mar. Drugs 2014, 12, 3046.

[9] ⁹
Patin, N. V.; Floros, D. J.; Hughes, C. C.; Dorrestein, P. C.; Jensen, P. R.; Microbiology 2018, 164, 946.

[10] ¹⁰
Adnani, N.; Chevrette, M. G.; Adibhatla, S. N.; Zhang, F.; Yu, Q.; Braun, D. R.; Nelson, J.; Simpkins, S. W.; McDonald, B. R.; Myers, C. L.; Piotrowski, J. S.; Thompson, C. J.; Currie, C. R.; Li, L.; Rajski, S. R.; Bugni, T. S.; ACS Chem. Biol. 2017, 12, 3093.

[11] ¹¹
Bertrand, S.; Schumpp, O.; Bohni, N.; Monod, M.; Gindro, K.; Wolfender, J.-L.; J. Nat. Prod. 2013, 76, 1157.

[12] ¹²
Bohni, N.; Hofstetter, V.; Gindro, K.; Buyck, B.; Schumpp, O.; Bertrand, S.; Monod, M.; Wolfender, J.-L.; Molecules 2016, 21, 370.

[13] ¹³
Serrano, R.; González-Menéndez, V.; Rodríguez, L.; Martín, J.; Tormo, J. R.; Genilloud, O.; Front. Microbiol. 2017, 8, 649.

[14] ¹⁴
Yu, L.; Ding, W.; Wang, Q.; Ma, Z.; Xu, X.; Zhao, X.; Chen, Z.; Tetrahedron 2017, 73, 907.

[15] ¹⁵
Wakefield, J.; Hassan, H. M.; Jaspars, M.; Ebel, R.; Rateb, M. E.; Front. Microbiol. 2017, 8, 1284.

[16] ¹⁶
Wu, C.; Zacchetti, B.; Ram, A. F. J.; van Wezel, G. P.; Claessen, D.; Hae Choi, Y.; Sci. Rep. 2015, 5, 10868.

[17] ¹⁷
Pettit, R. K.; Appl. Microbiol. Biotechnol. 2009, 83, 19.

[18] ¹⁸
Onaka, H.; Mori, Y.; Igarashi, Y.; Furumai, T.; Appl. Environ. Microbiol. 2011, 77, 400.

[19] ¹⁹
Rateb, M. E.; Hallyburton, I.; Houssen, W. E.; Bull, A. T.; Goodfellow, M.; Santhanam, R.; Jaspars, M.; Ebel, R.; RSC Adv. 2013, 3, 14444.

[20] ²⁰
Burgess, J. G.; Jordan, E. M.; Bregu, M.; Mearns-Spragg, A.; Boyd, K. G.; J. Biotechnol. 1999, 70, 27.

[21] ²¹
Ueda, K.; Kawai, S.; Ogawa, H.; Kiyama, A.; Kubota, T.; Kawanobe, H.; Beppu, T.; J. Antibiot. (Tokyo) 2000, 53, 979.

[22] ²²
Carlson, S.; Tanouye, U.; Omarsdottir, S.; Murphy, B. T.; J. Nat. Prod. 2015, 78, 381.

[23] ²³
Goers, L.; Freemont, P.; Polizzi, K. M.; J. R. Soc. Interface 2014, 11, 20140065.

[24] ²⁴
Stubbendieck, R. M.; Vargas-Bautista, C.; Straight, P. D.; Front. Microbiol. 2016, 7, 1234.

[25] ²⁵
Yang, Y.-L.; Xu, Y.; Straight, P.; Dorrestein, P. C.; Nat. Chem. Biol. 2009, 5, 885.

[26] ²⁶
Nai, C.; Meyer, V.; Trends Microbiol. 2018, 26, 538.

[27] ²⁷
Betancur, L. A.; Naranjo-Gaybor, S. J.; Vinchira-Villarraga, D. M.; Moreno-Sarmiento, N. C.; Maldonado, L. A.; Suarez-Moreno, Z. R.; Acosta-González, A.; Padilla-Gonzalez, G. F.; Puyana, M.; Castellanos, L.; Ramos, F. A.; PLoS One 2017, 12, e0170148.

[28] ²⁸
Correa, H.; Haltli, B.; Duque, C.; Kerr, R.; Microb. Ecol. 2013, 66, 972.

[29] ²⁹
Seyedsayamdost, M. R.; Traxler, M. F.; Clardy, J.; Kolter, R.; Methods Enzymol. 2012, 517, 89.

[30] ³⁰
Caraballo-Rodríguez, A. M.; Dorrestein, P. C.; Pupo, M. T.; Sci. Rep. 2017, 7, 5373.

[31] ³¹
Wolfender, J.-L.; Planta Med. 2009, 75, 719.

[32] ³²
Adnani, N.; Rajski, S. R.; Bugni, T. S.; Nat. Prod. Rep. 2017, 34, 784.

[33] ³³
Onaka, H.; Mori, Y.; Igarashi, Y.; Furumai, T.; Appl. Environ. Microbiol. 2011, 77, 400.

[34] ³⁴
Hoshino, S.; Okada, M.; Awakawa, T.; Asamizu, S.; Onaka, H.; Abe, I.; Org. Lett. 2017, 19, 4992.

[35] ³⁵
Hoshino, S.; Onaka, H.; Abe, I.; J. Ind. Microbiol. Biotechnol. 2018, 1.

[36] ³⁶
Liu, G. Y.; Nizet, V.; Trends Microbiol. 2009, 17, 406.

[37] ³⁷
Yang, Y.-L.; Xu, Y.; Kersten, R. D.; Liu, W.-T.; Meehan, M. J.; Moore, B. S.; Bandeira, N.; Dorrestein, P. C.; Angew. Chem., Int. Ed. 2011, 50, 5839.

Strain code	Taxonomic identification of each strain^a a Determined by 16S rRNA gene sequencing for bacteria, and ITSs gene sequencing for fungi.27,28 (% Similarity)	Source	Inclusion criteria^b b The inclusion criteria were: (1) previous information about its metabolic production and/or biological activity, (2) mycolic acid containing bacteria, (3) bacteria belonging to Streptomyces genus and (4) microorganisms that were isolated from the same sample (ecological criteria).
Strain code		Source	1	2	3	4
PNM-9	Streptomyces pratensis (100%)	Alga Dictyota sp.	X		X	X
PNM-25	Gordonia bronchialis (98.41%)	Sponge Xestospongia sp.	X	X
PNM-115	Paenibacillus elgii (99.73%)	Sediment	X
PNM-123	Paenibacillus ehimensis (99.71%)	Alga Codium sp.	X
PNM-157	Brevibacillus brevis (99%)	Octocoral Erythropodium sp.	X
PNM-161a	Streptomyces griseochromogenes (99.86%)	Alga Bryopsis sp.	X		X
PNM-210	Paenibacillus elgii (99.9%)	Octocoral Eunicea fusca	X
PNM-216	Unidentified	Alga Dictyota sp.	X			X
RKHC-9	Bacillus cereus (100%)	Octocoral Antillogorgia elisabethae	X			X
RKHC-26	Rhodococcus baikonurensis (100%)	Octocoral A. elisabethae		X		X
RKHC-28	Jeotgalicoccus halophilus (99.9%)	Octocoral A. elisabethae	X			X
RKHC-59b	Dietzia schimae (100%)	Octocoral A. elisabethae		X		X
RKHC-62b	Oceanobacillus profundus (99.9%)	Octocoral A. elisabethae	X			X
IBUN-5.1.	Streptomyces sioyaensis (98.9%)	Soil from Tolima	X		X
PNM-67	Purpureocillium lilacinum (99%)	Sponge Niphates digitalis	X

Brasil

Brasil

BINARY CO-CULTURE SELECTION FROM MARINE-DERIVED MICROORGANISMS FOR DIFFERENTIAL PRODUCTION OF SPECIALIZED METABOLITES

Abstract

INTRODUCTION

EXPERIMENTAL SECTION

General

Microorganism selection

Primary selection of couples to be evaluated

Binary co-cultures

Bacteria-bacteria interactions

Bacteria-fungus interactions

Extraction

Metabolic profiling

RESULTS AND DISCUSSION

Bacteria-bacteria co-cultures

Distance assays

Contact assays

Bacteria-fungus co-cultures

Distance assays

Contact assays

CONCLUSIONS

ACKNOWLEDGMENTS

SUPPLEMENTARY MATERIAL

REFERENCES

Publication Dates

History

Bacteria in co-culture with the fungus PNM-67	PDA			LBG			ISP2			ISP3
	Change			Change			Change			Change
	Phenotypic	HPLC-DAD	¹H NMR	Phenotypic	HPLC-DAD	¹H NMR	Phenotypic	HPLC-DAD	¹H NMR	Phenotypic	HPLC-DAD	¹H NMR
PNM-9	-	-	○	-	-	○	+	+	-	+	-	-
PNM-25	-	-	○	-	-	○	-	-	○	-	-	○
PNM-115	-	-	○	-	-	○	+	-	-	+	+	+
PNM-123	+	+	+	-	-	○	+	-	-	+	+	+
PNM-157	NE	NE	NE	-	-	○	+	+	-	-	-	○
PNM-161a	-	-	○	-	-	○	-	-	○	-	-	○
PNM-210	-	-	○	+	-	○	+	+	-	+	+	+
PNM-216	-	-	○	-	-	○	-	-	○	-	-	○
RKCH-9	NE	NE	NE	-	-	○	NE	NE	NE	-	-	○
RKHC-26	-	-	○	-	-	○	-	-	○	-	-	○
RKHC-28	NE	NE	NE	-	-	○	NE	NE	NE	-	-	○
RKHC-59b	NE	NE	NE	-	-	○	NE	NE	NE	-	-	○
RKHC-62b	NE	NE	NE	-	-	○	NE	NE	NE	NE	NE	NE
IBUN-5.1	-	-	○	+	-	○	NE	NE	NE	+	+	+

Binary co-culture		Type of assay	Change
Strain	Strain	Type of assay	¹H NMR (δ_H ppm, multiplicity)	HPLC-DAD	Probable producer
Streptomyces sp. PNM-161a	Rhodococcus sp. RKHC-26	Contact	1.5-1.7 2.35-2.50 2.95 (bt, J=7.5Hz) 7.15 (m)	Not observed	-
Purpureocillium sp. PNM-67	Paenibacillus sp. PNM-123	Distance	7.6-7.8	2 peaks (λ_max =320nm)	Paenibacillus sp. PNM-123
Purpureocillium sp. PNM-67	Paenibacillus sp. PNM-115, Paenibacillus sp. PNM-123, Paenibacillus sp. PNM-210, Streptomyces sp. IBUN-5.1.	Distance	7.28 (d, J=2.1Hz) 6.70 (d, J=2.6Hz) 6.61 (d, J=2.6Hz) 6.37 (d, J=2.1Hz)	1 peak (λ_max=256, 287, 337 y 298nm)	Purpureocillium sp. PNM-67
Purpureocillium sp. PNM-67	Rhodococcus sp. RKHC-26	Contact	0.84-0.87 4.54 (td, J=11.0; 4.2 Hz) 7.85-7.88	Not observed	-