Abstract
Biological control against microbial infections has a great potential as an alternative approach instead of fungicidal chemicals, which can cause environmental pollution. The pigment producer Metschnikowia andauensis belongs to the antagonistic yeasts, but details of the mechanism by which it inhibits growth of other microbes are less known. Our results confirmed its antagonistic capacity on other yeast species isolated from fruits or flowers and demonstrated that the antagonistic capacity was well correlated with the size of the red pigmented zone. We have isolated and characterized its red pigment, which proved to be the iron chelating pulcherrimin. Its production was possible even in the presence of 0.05 mg/ml copper sulphate, which is widely used in organic vineyards because of its antimicrobial properties. Production and localisation of the pulcherrimin strongly depended on composition of the media and other culture factors. Glucose, galactose, disaccharides and the presence of pectin or certain amino acids clearly promoted pigment production. Higher temperatures and iron concentration decreased the diameter of red pigmented zones. The effect of pH on pigment production varied depending of whether it was tested in liquid or solid media. In addition, our results suggest that other mechanisms besides the iron depletion of the culture media may contribute to the antagonistic capacity of M. andauensis.
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Introduction
Species capable of biological control have received particular attention, because they are able to inhibit the growth of other microbes and thereby are able to protect fruits or vegetables against decay1,2,3. Different mechanisms, such as secretion of cell wall-degrading enzymes or other antifungal compounds have been proposed as being responsible for their antagonistic activity1,3,4,5. A further possible method of antagonism is the production of ferric ion-specific chelating agents, which results in iron depletion in the environment and causes growth inhibition of microbes that require iron for their cellular processes6,7.
Several Metschnikowia species, including the well-known M. pulcherrima, are able to produce an iron binding red pigment8,9,10,11, which is probably closely linked to its antagonistic capacity, given that pigmentless M. pulcherrima mutants lack the antifungal activity11,12. The red pigment is called pulcherrimin, which is a water-insoluble complex13. The complex is formed from pulcherriminic acid and ferric ions, after conversion of cyclo-leucyl-leucyl to pulcherriminic acid13,14,15. Although pulcherrimin has long been known and some genes involved in its synthesis have also been revealed, the details and conditions of pigment synthesis, and the role of pigment production are not entirely clear12,16. The pigment might act as a siderophore, although some of its features seem to differ from those of typical siderophores11,16,17. Furthermore, pigment production can depend on culture conditions8 and this can strongly influence the antagonistic ability of a strain. Besides, it cannot be ruled out either that other processes may also be implicated in the antimicrobial capacity of the Metschnikowia species. Specifically, certain Metschnikowia species can also produce extracellular enzymes or volatile componds etc.17.
A promising Metschnikowia species is the less-known Metschnikowia andauensis, which produces pulcherrimin18,19,20,21. This species also has a great potential for biocontrol. Strains of M. andauensis have been evaluated for their biological control activity against the most important postharvest pathogens of fruits, like molds Penicillium expansum, P. digitatum, P. italicum, B. cinerea and Rhizopus stolonifer, R. oryzae, Alternaria alternata and Verticillium cinnabarinum or against fungi involved in crop and/or food spoilage (Saccharomyces cerevisiae, Wickerhamomyces anomalus and Dekkera bruxellensis) and M. andauensis was shown to inhibit growth of these species20,21,22.
In order to expand our knowledge of the antagonistic capacity of Metschnikowia species, we investigated the biocontrol capacity and pigment production of M. andauensis. We hypothesized that these features are similar to the M. pulcherrima’s properties. Based on this, we wanted to determine the most important environmental factors which can contribute to the stronger pigment production of M. andauensis. Besides, we studied the growth inhibitory effect of the precursor molecule of the pigment and the extracellular enzyme production capacity of M. andauensis.
Our results confirmed the biocontrol capacity of M. andauensis and revealed that other yeasts living on fruits or flowers can be inhibited by this species. We demonstrated that the red pigment produced by M. andauensis is indeed the iron-containing pulcherrimin and explored culture factors that can influence the production and the localisation of the pigment. Our data also indicate that mechanisms other than iron depletion of the culture media can also contribute to the antagonistic capacity of M. andauensis.
Results
M. andauensis is able to inhibit growth of different yeast species
To expand the list of the species which can be inhibited by M. andauensis cells, wild yeasts isolated from fruits and flowers were investigated. Their taxonomic positions were determined by PCR and sequencing methods, as detailed in Table 1.
Our data confirmed the antagonistic capacity of M. andauensis, as it was able to inhibit the growth of several Candida species, including Candida butyri and Candida orthopsilosis, as well as Starmerella caucasica, Pichia dorogensis, P. kluyveri, Issatchenkia terricola and Metschnikowia laotica (Table 2, Fig. 1A). During these experiments we also noticed that a red pigmented ring often appeared around M. andauensis cells and that this red ring correlated with the border of the inhibitory zone (Fig. 1A).
The M. andauensis pigment contains iron and shows the same characteristics as the pulcherrimin
Since M. pulcherrrima is able to produce a red colour iron chelated pigment, called pulcherrimin, and this was also assumed for M. andauensis18,19, we decided to examin its pigment. Therefore, the red pigment was isolated from the cell-free supernatant of the M. andauensis’s culture medium and was characterized by its UV–Vis spectroscopy. Its iron content was investigated by Flame Atomic Absorption Spectroscopy (FAAS). The UV–Vis spectrum of the M. andauensis pigment showed two characteristic absorption bands with absorption maxima at 380 and 480 nm, similar to the spectrum of pulcherrimin produced by Candida pulcherrima13(Fig. 1B). FAAS analysis showed that the isolated pigment was an iron containing one with 2.19 mg/g iron content.
Effect of carbon source on pulcherrimin production
Both the localisation and colour intensity of the red pigment varied with different media. To reveal the factors which influence the pigment formation, the M. andauensis cells were cultured on media prepared with different components and supplements. The red pigment was produced even in the absence of other microbes and its colour intensity and localisation were strongly influenced by the composition (Fig. 1C,D) and iron content of the media (Fig. 1E). On PDA media supplemented with iron, the red pigment accumulated around the growth, while the yeast cells remained white (Fig. 1D) (no red ring was visible on PDA without iron supplementation). On YDP agar, the cells were pinkish (compared to the colour of the streak grown on PDA) and a pigmented zone around the cells was not observed (Fig. 1C). Furthermore, the localisation and the intensity of the pigmented zone strongly depended on the concentration of Fe3+ cations. The increasing concentration of iron resulted in a darker and narrower ring (Fig. 1E—the iron concentration increased from left to right).
To clarify the correlation between the compostion of the media, culture conditions and pigment zone formation, M. andauensis cells were grown in media prepared from different carbon sources. Specifically, the mono- and disaccharides used as carbon sources in the media highly influenced the size of the pigmented zone (Fig. 2A). Glucose, galactose and the disaccharides maltose, trehalose, cellobiose and sucrose clearly promoted the appearance of large reddish pigmented zones (Fig. 2A,B). However, in the case of glucose, the red pigmented zone, which had appeared after 3 days, was covered by the cells after a longer incubation time (13 days) (Fig. 2A,B). In addition, mannose, fructose, or sorbose did not favour the development of a wide reddish zone around the cells.
The sugar concentration in the media also affected pigment formation by M. andauensis, as can be seen on Fig. 2D. Higher concentrations of cellobiose and galactose resulted in larger or darker pigmented halos (glucose, maltose, trehalose and sucrose gave similar results). In contrast, fructose promoted prolonged growth of M. andauensis instead of pigment production, as evidenced by the 13-days-old culture covering the reddish halo that had appeared after 3 days (Fig. 2D).
The effects of some polysaccharides on pigment production were also investigated. First, pectin was chosen, as it is an important cell wall component of fruit, and compared with two concentrations of the agar used for the solidification of the media. As Fig. 3A shows, the presence of pectin favoured the production of a darker red pigmented zone at all temperatures, compared to the control (0% pectin). In contrast, the higher agar concentration (2.5%) reduced the size of the halo (Fig. 3B), but did not influence the colour intensity of the pigment (Fig. 3C1). Similar results were obtained in the case of the M. pulcherrima strains used as a control (Fig. 3C2).
M. chrysoperlae, which was regarded as a non-pigment producing species32 and was used as a negative control in these experiments (Fig. 3C3), was also able to produce a small amount of pigment, especially on medium containing 2 or 4% maltose (Fig. 2C1). However, pink cells could be found mainly on the bottom side of the colony and only after 13 days (Fig. 2C2). Almost similar results were found on 4% glucose, sorbose, fructose, sucrose, galactose containing minimal medium (SMA).
The size of the pigmented halo depends on pH, temperature, the presence of certain amino acids and the cell density
The effect of further parameters on pigment production, such as incubation temperature, pH of the medium, presence of amino acids and cell density were also tested. Experiments carried out with liquid media revealed that a lower pH and a higher temperature favoured accumulation of the red pigment (Fig. 4A), in contrast to the experiments on solid media, which showed that the size of the pigmented area was larger at a higher pH (Fig. 4B).
The media set to pH 7.0 allowed us to test the relationship between cell density and size of the pigmented halo. A larger pigmented zone was achieved when the initial concentration of the cell suspension was higher. A 15 μl inoculum containing 1 × 103 cells/ml produced a 1.2 mm zone on SMA and a 1.6 mm zone on PDA, whereas a 15 μl inoculum with a density of 1 × 107 cells/ml gave rise to a 2.8 mm zone on both SMA and PDA media (the agar plates were incubated for 5 days at 25 °C).
Figure 4C demonstrates that the presence of leucine, glutamic acid and arginine in the media could strongly increase the size of the pigmented zones compared to media prepared without amino acid supplementation (similar results were obtained with lysine, serine, threonine, alanine).
Synthetic cyclo-leucyl-leucyl, which is a precursor of pulcherrimin formation, showed growth inhibition on yeasts
The question arose whether growth inhibition can be caused by depletion of iron from the environment alone or also by the presence of cyclo-leucyl-leucyl, the precursor of pulcherrimin formation. To answer this question, cyclo-leucyl-leucyl was synthesized from leucyl dipeptide and its antifungal capacity was investigated using spot assay tests on lawns of Starmerella caucasica (11-1071), Candida stigmatis (11-465) or Saccharomyces cerevisiae cells (11-481, 11-642) (Table 2). Cyclo-leucyl-leucyl caused growth inhibition at the highest (100 mg/ml) of three concentrations (Fig. 1F1,F2).
The presence of copper ions allows budding and pigment production in M. andauensis
Copper sulphate is extensively employed in agriculture because of its fungicidal and bactericidal properties. Furthermore, application of Cu-based chemical treatments is allowed even in organic wineyards. Thus, we wanted to explore the effect of the copper ion on budding and pigment production of M. andauensis. Experiments carried out on Cu-containing media showed that the presence of 0.05 mg/ml copper sulphate in the media allowed both pigment production and budding in M. andauensis (Fig. 4D), but decreased the size of the inhibitory zone on Botrytis cinerea lawn (Fig. 4E).
M. andauensis cells produces various extracellular enzymes
Given the ability of M andauensis to inhibit different yeast species (Table 2), we wondered if other processes besides pulcherrimin production and iron depletion might also contribute to the antagonistic activity of this species. To this end, the extracellular enzyme production capacity of the cells was investigated. As Fig. 5 demonstrates, the M. andauensis cells have a wide range of extracellular enzyme activity. The cells produced proteases capable of clearing casein (Fig. 5A) and melting gelatin (Fig. 5B) in contrast to S. cerevisiae cells used as control, which did neither. Furthermore, a test carried out from a cell-free supernatant demonstrated the presence of a BSA-degrading enzyme in a chromatographic fraction (sample 3, Fig. 5C). Further tests demonstrated the production of acid (Fig. 5D), amylase (Fig. 5E), β-glucosidase production capacity (Fig. 5F). Besides, the cells were able to reduce the intensity of the Congo red staining reaction applied to a carboxymethyl-cellulase containing medium (Fig. 5G).
Discussion
Microbes found on the surface of plants and fruits can be harmless or can cause spoilage of fruits or health problems2,3. To inhibit the growth of these harmful microbes, different approaches can be used, ranging from the application of synthetic chemicals to the use of environment-friendly microorganisms to effect biological control5,24,25. Metschnikowia andauensis belongs to these micoorganisms, as it is able to control growth of different microbes effectively20,22,26.
To expand the list of species whose growth can be inhibited by M. andauensis, wild yeasts isolated from fruit and flowers were investigated for their susceptibility to M. andauensis. The strains were identified in this or previous studies27,28,29,30. The strains included nine Candida species, Pichia dorogensis and P. kluyveri, Issatchenkia terricola and Starmerella caucasica. M. andauensis was able to inhibit the growth of Starmerella caucasica, Pichia dorogensis, Issatchenkia terricola strains and several Candida species, including Candida orthopsilosis and C. butyri, which are of medical importance23,31. We also confirmed the antagonistic effect of M. andauensis against the postharvest pathogen Botrytis cinerea. Taking into account other previously reported susceptible species20,22,26, the M. andauensis emerges as having a wide spectrum of antimicrobial activity.
To elucidate the processes which contribute to its inhibitory capacity, we confirmed that this species produces pulcherrimin, as do M. pulcherrima and, unexpectedly, M. chrysoperlae. The latter species was previously reported not to be capable of pigment production and it was initially used here as a negative control11,12,17,18,21,32. To confirm the identity of the pigment produced by M. andauensis, we isolated and characterized it by UV–Vis spectroscopy and FAAS analyses. The UV–Vis spectrum of the M. andauensis pigment showed the same characteristics as the pulcherrimin made by M. pulcherrima. The visible light absorption spectrum is typical of the presence of metal coordination or a conjugated electron pair system in this compound13. The FAAS analysis demonstrated the presence of iron in the pigment of M. andauensis. It is therefore reasonable to conclude that M. andauensis, like M. pulcherrima and Bacillus subtilis, can produce pulcherrimin and that iron coordination is responsible for the reddish colour13,33.
The production and extent of the pulcherrimin diffusion zone was strongly influenced by the composition of the medium. These data are in good agreement with what has been found for M. pulcherrima8,11,34. The size and colour intensity of the reddish zones were increased by the use of galactose, or disaccharides, such as maltose, trehalose, cellobiose, sucrose as carbon sources, addition of pectin, or higher concentrations of certain sugars. Interestingly, glucose and fructose stimulated growth but not pigment production of M. andauensis after a longer incubation time (13 days), which led to the formation of larger colonies that overran the pigmented zones that had appeared after 3 days.
Supplementation of media with amino acids, such as leucine, glutamic acid, arginine or others also favoured pigment synthesis. Since similar results were obtained with Bacillus subtilis, this data and existence of genes with similar functions found in yeasts and bacteria suggest similar pathway for synthesis of pulcherrimin12,16,17,33. Our further experiments showed that the size of the red zone on agar is pH dependent. The size increased at higher pH (pH 6.0–7.0) at all temperatures (25, 30, 37 °C) and decreased at lower pH (pH 4.0–5.5) or at higher iron concentrations (0.05, 1 mg/ml). As pH influences the ratio of ferric (Fe3+) and ferrous (Fe2+) ions35,36, it also affects the availability and uptake, and is expected to have a strong impact on migration of the precursor and the amount of pulcherrimin produced.
We do not know whether the larger and mostly lighter red or the narrower, dark red pigmented zones has the stronger antagonistic effect. The darker colour pigment intensity might indicate that a higher amount of iron is bound, which can cause a higher iron depletion from the environment and thereby growth inhibition of the microbes. The larger pigmented zone appears to cause a more extensive inhibition, as evidenced by the observation that borders of the red pigmented and inhibitory zones are often correlated. Since the iron-containing pulcherrimin is regarded as a water-insoluble and non-diffusible complex8,13,14,15, while the precursor molecule is thought to be a diffusible agent37,38, it is possible that the precursor can also have an inhibitory effect. This might be supported by our observation that the synthetic cyclo-leucyl–leucyl could inhibit yeast growth. It is not clear whether cyclo-leucyl-leucyl is found in the extracellular region of M. andauensis in nature, although the closely related M. pulcherrima does secrete cyclo-leucyl–leucyl12. In any case, this result is in good agreement with the findings which show that highly stable cyclic dipeptides can have antifungal, antibacterial effects39,40,41.
Since production of the pulcherrimin occurs even in the presence of 0.05 mg/ml copper sulphate, which is widely used in agriculture because of its fungicidal and bactericidal properties, the red pigment and/or its precursor should function as biocontrol agents in the field, even in the presence of agricultural copper sulphate.
Our results also revealed that the M. andauensis cells could produce proteases, as suggested by the degradation of casein, BSA and gelatin. To demonstrate a relationship between protease production and antifungal capacity requires further studies, but it is plausible, as a positive correlation has been found between protease activity and biocontrol capacity in certain bacterial strains42. Further studies showed that M. andauensis produces acids, and might have amylase and β-glucosidase activities. However, production of certain enzymes may depend on composition of the culture medium, as protease production and starch utilization has not been detected on other media20,21,22,23,24,25,26,27,28,29,30,31,32,33,34,35,36,37,38,39,40,41,42,43. At the same time, its β-glucosidase activity is in good agreement with the previous results22. This latter capacity might also contribute to appearance of the lighter red zone around the cells on the carboxymethyl-cellulose containing medium. All these processes, together or separately, may contribute to the wide-spectrum antifungal ability of M. andauensis.
In conclusion, the present study gives further evidence for the antagonistic capacity of the pigment producer M. andauensis and that this yeast species produces iron-chelate pulcherrimin. We demonstrated that there is a correlation between antagonistic capacity and the size of the red pigmented zone and determined some environmental factors that can increase the amount of pulcherrimin produced. Our results show that this species is able to produce proteases, α-glucosidase and amylase, which may contribute to the antagonistic capacity of M. andauensis. All these data suggest that this species has a great potential as a biocontrol agent. These data can contribute to the process of optimizing its efficacy in field trials and selecting the proper plant material.
Material and methods
Strains, culture media and taxonomic identification
Strains and their origin
The strains used in this study and their origin are listed in Table 1. Three Metschnikowia collection strains—two pigment-producing: M. pulcherrima (11-11, 11-578) and M. crysoperlae (11-1158) strain, which was chosen to be a negative control, but was found in the study to produce a small amount of pigment under certain conditions—and one Saccharomyces cerevisiae (11-642) were used as reference material. The susceptibility of 19 wild yeast strains which were isolated from fruits or flowers was tested to M. andauensis. They were collected in different geographical regions (Table 1). The samples were immersed in sterile water and aliquots were spread onto YDP medium. After 7 days single yeast colonies were isolated.
A B. cinerea strain (1) was also used to test antagonistic activities of the M. andauensis (11-1120) strain.
Identification of wild yeasts
PCR and sequencing methods were applied for determination of taxonomic positions of the collected yeast strains. Sequences of the D1/D2 domains of the large subunit ribosomal RNA gene were amplified by PCR (primers: NL1-5′-GCA TAT CAA TAA GCG GAG GAA AAG-3′ and NL4-5′-GGTCCG TGT TTC AAG ACG G-3′)49. The reaction was subjected to the following program: 94 °C 2 min, 95 °C 1 min, 51 °C 1 min 72 °C 1 min, (30X). The PCR fragments were purified and sequenced using the same primers. The taxonomic positions of the strains were accepted when 100% identity was found in the BLAST analysis to sequences of the type strains (NCBI database-https://blast.ncbi.nlm.nih.gov/Blast).
Culture media
Compositions of the media and culture conditions are listed in Table S1. YDP medium was used for the strain isolation, while YEA was generally used as standard medium.
Antimicrobial activity of M. andauensis against wild yeasts was tested on SMA medium incubated at 25 and 37 °C. Presence of the inhibitory zone was checked daily.
Pigment production and its diffusion were tested on different media, such as the complete medium YDP, Synthetic Minimal Media SML, SMA44 and Edinburgh Minimal Medium (EMMA)45, Potato Dextrose Media (PDA and PDB) and their modified versions (Table S1). To increase the visibility of the pulcherrimin ring the media were generally supplemented with FeCl3. Colour intensity and size of the red pigmented zone were checked daily.
SMG (gelatin-containing medium) was used to evaluate protease activity. SMG media were prepared with different brands of gelatin (Oetker or Lucullus). Since 2 and 4% gelatin plates were softer than 2% agar plates, M. andauensis cells were dropped and not streaked onto the surface of the plates, which were incubated at 24 °C and melting of the medium around the yeast cells was checked daily.
Media for extracellular enzyme activity assays were prepared according to the previous articles using pH5 and 7 values46,47,48 (Table S1). Protease activity was tested on casein-containing medium46, while amylase activity was tested on starch-containing rich medium46. A possible β-glucosidase activity was tested on cellobiose-containing rich medium47. Acid productivity was tested on CaCO3-containing medium48, while cellulose degradation was tested on carboxymethyl-cellulose-containing rich medium46.
Botrytis cinerea cultures were grown on YM medium. Antagonistic capacity of M. andauensis against Botrytis cinerea was tested on SMA and SMA supplemented with different amount of CuSO4. Presence of inhibitory zone was checked daily.
Test for antimicrobial activity against yeasts and Botrytis cinerea
Spot assay to monitor the antimicrobial activity of M. andauensis cells against yeasts
The M. andauensis cells (11-1120) (test-strain) were cultured in a shaker in YEL medium at until OD595 = 1. The cells were harvested, washed with sterile distilled water and a cell suspension was prepared in sterile water. 15 ul of a cell suspension containing 7 × 107 cells/ml was dropped onto the surface of the SMA media (pH5 and pH7) which had earlier been flooded with 400 µl cell suspension of the strain used as lawn (OD595 = 1) and dried in a sterile box. Appearance of the inhibitory zone was checked daily. When the cells of the lawn were able to grow on the medium far from the test-strain, but not around it (that is, a clear inhibitory zone was found), inhibition was recorded as positive (see in the Table 2). In contrast, absence of an inhibitory zone was recorded as a negative (-) result. The results come from three or more separate experiments.
Test for antagonism against Botrytis cinerea
A small piece (5 mm x 5 mm) of a single colony of Botrytis cinerea (1) was cut out and moved into 150 ml YM medium (in a 250 ml Erlenmeyer flask) and incubated on a shaker. After 1 week, mycelia of the mold were ground by hand in a mortar and a weak suspension was made with sterilized water. 400 µl of the cell suspension was spread onto SMA and SMA supplemented with CuSO4. After drying, cells of the M. andauensis test-strain, a 15 μl inoculum containing 7 × 107 cells/ml were dropped onto the agar plates. Growth of Botrytis cinerea around the test strain was checked daily. The results come from three separate experiments.
Isolation and characterisation of the red pigment produced by M. andauensis
Isolation of the red pigment
M. andauensis grown for one week at 30 °C in 50 ml of SML medium containing 0.01 mg/ml FeCl3. The culture was centrifuged at 9000 g at 4 °C for 20 min. The supernatant was collected and concentrated by lyophilization. The dry material was dissolved in 10 ml of 50 mM sodium acetate buffer (pH 5.0), and centrifuged at 13000 g at 4 °C for 40 min. The sample was filter-sterilized by passing through a sterile 0.22 μm membrane disk. The sample was fractionated using size-exclusion chromatography. One ml of the sample was loaded onto a Sephadex G-25 column (10 ml, d:8 mm) that was pre-equilibrated with 50 mM sodium acetate buffer, pH 5.0 and the eluate was collected in 1 ml fractions. All the fractions of the gel-filtered sample were subjected to UV–Vis spectrophotometry, SDS-PAGE analysis and a protease activity test.
All the UV–Vis spectra were collected on a Specord 210 Plus dual-beam spectrophotometer.
For the protease activity test, 20 μl of the chromatographic fractions was concentrated five times and incubated with 10 μl of a 5 mg/ml BSA solution for 6 h at 37 °C. The incubated solutions were analysed by 12% SDS-PAGE.
Study of the red pigment by Flame Atomic Absorption Spectrometry (FAAS)
The solid red pigment was weighed, and 65% nitric acid was added to produce iron (III) nitrate. After a few hours the supernatant was discarded, and the iron (III) nitrate was dissolved in MilliQ water. The concentration of Fe (III) ion was determined using the FAAS method (UNICAM SP 1900 AAS) with the following parameters: air: 4.6 l/min (3 bar), acetylene: 1.4 l/min, Narva iron hollow cathode lamp, optical slit width: 0.1 mm, lamp current: 15 mA, observation height: 10 mm, burner length slot: 10 cm.
Effect of environmental factors (C-source, presence of amino acid, pH, temperature or cell density) on pigment production and diffusion
Test for the effect of the C-source on pigment production
Different sugar-containing SMA media were prepared using 2% sugar concentration. To test the effect of sugar concentration, the media were prepared with 1, 2, and 4% sugar. All media were supplemented with 0.001 mg/ml FeCl3. The same amount of M. andauensis (11-1120) and M. crysoperlae (11-1158) cells were dropped onto the surface of the media. The plates were incubated at 25 °C and the pigmented zones were checked after 3 and 13 days.
The effect of pectin was investigated on YEA containing 0.5% or 1% pectin. The colour and size of the pigmented zone were compared to those of the agar plates prepared without pectin.
In order to learn the effect of agar concentration on the diameter of the pigmented zone, YDP containing 1 and 2.5% agar were used for culturing. The plates were measured after 2, 4, 6, 10 days.
Test for effect of amino acids on pigment production
A cell suspension was prepared from M. andauensis cells (11-1120) with sterile water. A 15 μl inoculum containing 1 × 106 cells/ml was dropped onto the surface of PDA and SMA media (pH 7.0) supplemented with different amino acids and FeCl3. The results come from three separate experiments.
Relation between cell density and size of the red pigmented zone
Cell suspensions were prepared with sterile water from the M. andauensis (11-1120) cells grown on YEA for 1 day. A 15 μl inoculum containing 1 × 103 or 1 × 107 cells/ml was dropped onto the surface of SMA (pH 7.0) and PDA (pH 7.0) supplemented with 0.01 mg/ml FeCl3. The agar plates were incubated at 25 °C. After 5 days size of the red pigmented zone was measured by ruler. The results come from three separate experiments.
Investigation of extracellular enzyme activity and growth of gelatin medium
Extracellular enzyme activity assays
M. andauensis (11-1120) and M. pulcherrima (11-578) cells were grown on YEA for 3 days at 25 °C. Cell suspensions were preapared with sterile distilled water, whose cell densities were OD595 = 0.1. 15 µl of the cell suspensions were dropped onto the surface of the given media. The agar plates were incubated at 25 °C. The protease activity was tested on casein-containing medium. Production of protease was indicated by the presence of a clear zone around the colony46. Amylase activity was tested on starch-containing rich medium, after washing the plates with lugol solution. A clear zone was observed around the colony when the cells had enzymatic activity46. Cellulose degradation capacity was tested on carboxymethyl-cellulose-containing medium. Activity of the cellulose degrading enzymes is indicated by appearance of a transparent halo around the colony when washed with Congo Red46. a possible β-glucosidase activity was tested on cellobiose-containing rich medium47. Acid productivity was indicated by a clear zone around the cells on CaCO3-containing medium48.
Growth on gelatin solidified medium
To obtain further evidence for protease activity, growth on gelatin medium was also tested. M. andauensis (11-1120) and non pigment-producing Saccharomyces cerevisiae (10-642) were cultured in YPL medium at 28 °C in a shaker. After 1 day, a 10 µl cell suspension containing 1.5 × 106 cells/ml was dropped onto the surface of the media solidified with gelatin. The agar plates were incubated at 24 °C and melting of the medium around the M. andauensis cells was investigated.
Preparation and investigation of cyclo-leucyl-leucyl
Preparation of cyclo-leucyl-leucyl
N,N′-Dicyclohexyl-carbodiimide (1.05 g, 4.30 mmol) was added to the solution of Leu-Leu dipeptide (PubChem) in N,N-dimethylformamide (50 ml) and stirred for 30 min, then pyridine (2 ml) was added and the reaction mixture was stirred for 24 h. The reaction mixture was concentrated and co-concentrated with toluene (3 × 20 ml). Column chromatography (hexane:ethyl acetate 7:3) of the residue afforded the capture of the cyclic product (880 mg, 77%). The concentrated cyclic product was dissolved in DMSO (Sigma, final concentration was 100 mg/ml). The cyclic-leucyl-leucyl solution was divided into Eppendorf tubes (100–100 µl) and stored in − 20 °C.
Effect of cyclo-leucyl-leucyl on growth of yeasts
Cell suspensions of Saccharomyces cerevisiae (11-481, 10-462), Candida stigmatis (11-465), or Starmerella caucasica (11-1071) were prepared with sterile water from 1-day-old cells grown on YEA at 25 °C. The final cell density of the cell suspensions was OD595 = 1 and the surface of the YEA plates was flooded with the cell suspensions to form a lawn. After drying under a sterile box, a 15 µl inoculum containing 100 mg/ml cyclo-leucyl-leucyl dissolved in DMSO (Sigma), two dilutions (50 and 33 mg/ml prepared with DMSO or PEG4000) or DMSO and PEG4000 as controls were dropped onto the surface of the media. The agar plates were incubated at 25 °C and growth of the lawn was investigated.
Statistical analysis
Statistical analysis was created using the BoxPlotR program (http://shiny.chemgrid.org/boxplotr/)50.
Data availability
The dataset(s) supporting the conclusions of this article is (are) included within the article.
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Acknowledgements
We thank Ilona Lakatos for technical assistance.
Funding
This research was supported by the European Union and Thematic Excellence Programme of the Ministry for Innovation and Technology in Hungary (FIK 20428-3/2018, TKP2020-IKA-04). EFOP-3.6.1-16-2016-00022 provided funds for purchase of the reagents and paid a scholarship for EH, while FIK 20428-3/2018, TKP2020-IKA-04 projects partly contributed to the purchase of chemicals. The funding bodies were not involved in study design, data collection, analysis and writing of the manuscript.
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E.H.: performed the assays for antimicrobial activity and pigment production, participated in study design. L.D.: tested effect of the amino acids, relation between the cell number and antimicrobial activity. E.Sz. and T.B.: performed the red pigment isolation, SDS-PAGE analysis and protease activity test. J.P.: carried out the FAAS analysis. L.K.: prepared the cyclo-leucil. M.S.: collected the strains, determined the taxonomic position of the strains. H.Cs.: designed and tested the extracellular activity. IM: performed the study design, data analysis and writing the manuscript. All authors read and approved the manuscript.
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Horváth, E., Dályai, L., Szabó, E. et al. The antagonistic Metschnikowia andauensis produces extracellular enzymes and pulcherrimin, whose production can be promoted by the culture factors. Sci Rep 11, 10593 (2021). https://doi.org/10.1038/s41598-021-89982-y
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DOI: https://doi.org/10.1038/s41598-021-89982-y
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