1. Introduction
Coumarin
1 Figure 1 is a natural compound of great relevance in the flavour and fragrance industry [
1]. This lactone is one of the first flavours produced by chemical synthesis; it possesses a hay-like, sweet aromatic creamy odour that makes it a suitable ingredient both for food and perfume formulations. Coumarin of natural origin is easily available from the Tonka beans (
Dipteryx odorata Willd.) extract, where it is present as the main odorous component [
2]. Unfortunately, due to its inherent toxicity, this compound has been banned as a food additive and the growing safety concerns have led the European authority to restrict even the use of natural extracts in which it is present, assessing the tolerable daily intake (TDI) to 0.1 mg/Kg [
3]. Consequently, the identification and the production of natural flavours possessing coumarin like odour, which are considered as safe for human health, have become highly desirable. In this context, the use of dihydrocoumarin
2 as a food-flavouring ingredient has taken a primary role during the last twenty years.
The aforementioned lactone has a pleasant sweet, herbaceous, coumarin and coconut-like odor and it has been recognized as safe, being included in the list of the substances Generally Recognized As Safe from the Flavor & Extract Manufacturers Association (FEMA-GRAS), under the number 2381. Although dihydrocoumarin is easily synthesizable by metal-catalyzed hydrogenation of coumarin itself, its availability in natural form is rather limited. In fact, even if this chromanone is a minority component of the Tonka beans extract [
2] and has been identified in different vegetal species including sweet clover blossom (
Melilotus officinalis) [
4], its amount from these sources is largely insufficient to justify an extractive process that could satisfy the growing market request of this natural flavour.
Since the flavours possessing the ‘natural’ status are usually hundreds times as expensive as their synthetic counterparts, any new procedure that provide these compounds in their high value form can be very profitable. According to the European [
5] and USA [
6] legislation, the biotransformation of a natural precursor is a ‘natural method’ of synthesis [
7]. Considering that coumarin of natural origin is a quite cheap commodity, the most suitable procedure to synthesize dihydrocoumarin consists in the biocatalyzed reduction of the 3,4 double bond of natural coumarin [
8,
9]. Several studies have highlighted that this reaction is one of the intermediate steps in the coumarins biodegradation, carried out by filamentous fungi and yeasts [
10,
11,
12,
13,
14].
In nature, the ‘biohydrogenation’ of the α,β-unsaturated esters is performed by ene-reductases, a class of enzymes able to catalyze the asymmetric reduction of the activated C–C double bonds [
15]. Different microorganisms can perform this process, in particulars yeasts proved to be the most versatile ones as they can reduce α,β-unsaturated aldehydes [
16,
17,
18], ketones and esters [
19], including lactones.
Some years ago, during a pioneering study on the stable isotope characterization of
ortho-oxygenated phenylpropanoids [
8], we prepared dihydrocoumarin through the baker’s yeast mediated reduction of coumarin. Since the aim of our work wasn’t the large scale preparation of compound
2, we didn’t improve our synthetic procedure. Few years later, a research group from Degussa and Technical University of Munich published a relevant paper on the biotechnological production of dihydrocoumarin [
9]. According to the reported findings, the latter chromanone was obtained by microbial reduction of natural coumarin using different
Saccharomyces cerevisiae strains. Melilotic acid (
3) was the main product of the biotransformation that was converted into dihydrocoumarin by simple distillation in the presence of a catalytic amount of citric acid (
Figure 2). The same study also underlined the main drawback of the claimed process, namely the high toxicity of coumarin that significantly decreased the yields at a concentration superior to 0.5 g/L.
As we recently set up a research program aimed at the biotechnological production of natural flavours [
20,
21,
22,
23,
24,
25,
26], we decided to design a new process for the preparation of natural dihydrocoumarin based on the microbial reduction of coumarin. To this end, we undertook a comprehensive study intended to select microbial strains showing good tolerance to relatively high coumarin concentrations and that could efficiently perform the reduction of its conjugated double bond.
Herein, we describe the results obtained by our work that, besides confirming and extending those described by previous researches, suggested the prospective utility of the yeasts Torulaspora delbrueckii, Kluyveromyces marxianus and of the fungus Penicillium camemberti for natural dihydrocoumarin production.
2. Results and Discussion
The main problem related with the microbial transformation of coumarin lies in its cytotoxicity that inhibits cell growth along with the cell metabolic activity. In order to select microorganisms able to efficiently perform the coumarin reduction, we defined the following screening conditions.
Each microbial strain of yeasts or filamentous fungi was grown in liquid media, using the universal Medium for Yeasts (YM) or Malt Extract Medium (MEA), respectively. At the end of the exponential growth phase or after complete formation of the filamentous fungi colonies, the cultures were inoculated with the suitable amount of the coumarin, dissolved in dimethyl sulfoxide. The experiments were performed in aerobic conditions, sealing the flasks with cellulose plugs.
To accomplish our study we singled out eighteen different microbial strains. Since we were interested in developing a reliable process for the production of a natural flavour to be used in food, we limited our study to microorganisms belonging to biosafety level 1, with a strong preference with those recognized with technological beneficial use in foods [
27]. Accordingly, we preferentially chose microbial species that are currently used as probiotics [
28] or for food and flavour processing [
29]. We selected
Saccharomyces cerevisiae (Type II, from Aldrich),
Saccharomyces boulardii (probiotic strain),
Komagataella pastoris,
Torulaspora delbrueckii,
Debaryomyces hansenii and
Kluyveromyces marxianus because these yeasts possess the GRAS status and have been already used as whole-cell biocatalysts in a number of studies [
30,
31,
32,
33]. The yeasts
Yarrowia lipolytica,
Candida boidinii,
Starmerella bombicola and the basidiomycota
Xanthophyllomyces dendrorhous,
Cryptococcus curvatus and
Sporidiobolus johnsonii are oleaginous fungi, industrially used for their ability to degrade/accumulate lipids and have been employed in different flavour production processes [
34,
35,
36,
37].
Concerning the filamentous fungi, we included in our screening the Ascomycota
Aspergillus niger,
Geotrichum candidum,
Penicillium adametzii,
Penicillium corylophilum,
Penicillium camemberti and
Penicillium roqueforti. The biocatalytic activity of
Aspergillus niger was investigated because it has been demonstrated that this microorganism can degrade coumarin and dihydrocoumarin as well as substituted coumarins [
10,
11,
14]. Similarly, we singled out
Geotrichum candidum,
Penicillium adametzii and
Penicillium corylophilum since these species are able to reduce the conjugated double bond of different α,β-unsaturated ketones and lactones [
25,
38,
39]. Finally, we selected two specific strains of
Penicillium camemberti and
Penicillium roqueforti, which are currently used in the dairy industry. The latter microorganisms, besides possessing the GRAS status, have been already employed for the biotechnological production of flavours [
40,
41].
Preliminary experiments, in which the transformation of the substrate was checked by sampling the fermentation flasks every 24 h, showed that the reduction of the conjugated double bond did not proceed further after 5–7 days since the substrate addition. From that time onward, the melilotic acid/coumarin ratio kept a constant value. In addition, the Thin Layer Chromatography (TLC) analysis showed only the presence of the melilotic acid and/or of coumarin whereas the concentration of dihydrocoumarin and/or of other metabolites was insignificant, with the single exception of the Aspergillus niger-mediated biotransformation (see below). The Gas Chromatographic analyses using a Mass detector (GC-MS) confirmed these observations although the results were given as a dihydrocoumarin/coumarin ratio, since the melilotic acid is transformed quantitatively into dihydrocoumarin in the GC injector (see experimental).
According to these initial results, we decided to stop all the biotransformation experiments seven days after the coumarin addition and to evaluate the melilotic acid/coumarin ratio using the GC-MS analysis. Since the only biotechnological method of dihydrocoumarin production [
9] indicated microbial activity inhibition with a coumarin concentration superior to 0.5 g/L, we settled a first set of experiments using a starting coumarin concentration of 0.6 g/L. Depending on the results of the latter screening we decided whether or not the activity of the selected microorganisms should be further studied. Accordingly, microorganisms producing a biotransformation mixture with a melilotic acid/coumarin ratio superior to 40/60 were studied also using a starting substrate concentration of 1.2 g/L and 1.8 g/L.
The microbial strains affording a melilotic acid/coumarin ratio ranging between 40/60 and 5/95, perform the reduction with unsatisfactory efficiency and thus were not investigated further. Lastly, the microbial strains producing only a trace of compound 3 (melilotic acid/coumarin ratio inferior to 5/95) were employed using a starting coumarin concentration of 0.3 g/L. The latter biotransformations were executed in order to better understand the reason for the lack of reactivity. In fact, the latter experiments can show whether the strains are unable to perform the reduction or if they gave unsatisfactory results because they were completely inhibited by the substrate toxicity.
Overall, all the results obtained with the above described experiments are collected in
Table 1 and allow a number of considerations. First, we can observe that all the selected strains possess the ene-reductase activity, even if its biocatalytic efficiency changes dramatically depending on the microbial strain used and on the coumarin concentration.
The yeasts Komagataella pastoris, Starmerella bombicola and the basidiomycota Xanthophyllomyces dendrorhous are completely inactive with a substrate concentration of 0.6 g/L. Nevertheless, small amounts of the melilotic acid (1%, 1% and 4%, respectively) were detected in the biotransformation mixtures produced with the same strains, using a coumarin concentration of 0.3 g/L. Similarly, the microorganisms Debaryomyces hansenii, Candida boidinii and Geotrichum candidum increased their biocatalytic activity using the latter substrate concentration. The results obtained with Geotrichum candidum are especially amazing as the melilotic acid/coumarin ratio measured in the fermentation broth increased from 3/97 to 37/63 by simply halving the substrate concentration. These data underlined the impact of the coumarin toxicity on the biotransformation process.
Moreover, using a starting substrate concentration of 0.6 g/L, the investigated microbial strains showed biocatalytic activities very different from each other. It is worth noting that our
Saccharomyces species (
cerevisiae and
boulardii) gave the disappointing conversion ratio of 17/83 and 9/91, respectively. These results are in sharp contrast with those reported for other
Saccharomyces cerevisiae strains [
9], pointing at the possible biocatalytic activity differences among strains of the same species.
In addition, all experiments afforded the melilotic acid and coumarin as main metabolites, except for Aspergillus niger. In this case, the microbial transformation gave the usual melilotic acid/coumarin mixture (16/84 ratio) close to a plethora of unidentified compounds. The GC-MS analysis indicated that only the 38% of the produced metabolites corresponded to the melilotic acid/coumarin mixture whereas the main part of the formed products are most likely deriving by coumarin oxidation.
Overall, using a substrate concentration of 0.6 g/L, all the tested microorganisms afforded a melilotic acid/coumarin ratio inferior of 40/60 with the exception of the yeasts Torulaspora delbrueckii, Kluyveromyces marxianus and of the filamentous fungi Penicillium camemberti and Penicillium roqueforti. Thus, we decided to employ only the latter four microorganisms for further biotrasformations, performed using increasing concentration of the substrate. Accordingly, we run two sets of four experiments in which the coumarin concentration was doubled and tripled, to a value of 1.2 g/L and 1.8 g/L, respectively.
The results allowed differentiating the fungal strains based on their biotransformation performances. The yeasts Torulaspora delbrueckii and Kluyveromyces marxianus possess comparable activity at 0.6 g/L affording a melilotic acid/coumarin ratio value of 70/30 and 74/26, respectively. However, when the coumarin concentration increases, Torulaspora delbrueckii decreases its biocatalytic efficiency whereas Kluyveromyces marxianus proves to be much less affected by the substrate toxicity. On the contrary, the high level of coumarin strongly inhibited both growth and activity of the Penicillium strains. Penicillium camemberti seems to be the strain most sensitive to coumarin as it completely transformed the substrate at 0.6 g/L concentration whereas at 1.2 and 1.8 g/L the formation of the melilotic acid was almost completely blocked, respectively. Even less remarkably, Penicillium roqueforti showed the same behavior and the biotransformation experiments led to biotransformation mixtures with a melilotic acid/coumarin ratio that ranged from 41/59 to 2/98 by increasing the coumarin concentration from 0.6 g/L to 1.8 g/L.
Another relevant problem that we faced during our study concerns the evaluation of the actual yields of the biotransformation process. Indeed, the melilotic acid/coumarin ratio indicates the progress of the ‘biohydrogenation’ reaction but doesn’t give the concentration value of the two latter compounds in the fermentation broths. In different experiments, we observed that the extraction/distillation procedure, afforded an amount of the dihydrocoumarin/coumarin mixture noticeably inferior to the amount of the starting substrate.
Aiming to quantify the loss of the substrate, we specially designed a suitable internal standard to be employed for the GC analyses of the biotransformation reactions. This compound should possess chemical/physical characteristics very similar to those of the melilotic acid. In fact, it must have similar solubility in the fermentation broths, it must be extractable using the same solvent and it must give similar response in the GC-MS detector. Therefore, we selected 3-(2-hydroxy-5-methylphenyl)propanoic acid (=6-methyl-melilotic acid) as the most suitable internal standard. The GC-MS analysis of this compound in the mixture with the melilotic acid show two well-resolved peaks corresponding to dihydrocoumarin and 6-methyldihydrocoumarin. In addition, the synthesis of compound
7 can be easily performed starting from the commercially available 6-methyl-coumarin (
4) (
Figure 3). Accordingly, the chemical hydrogenation of
4 with hydrogen and palladium on charcoal as catalyst afforded the 6-methyl-dihydrocoumarin (
5) that was transformed into sodium salt
6 by treatment with sodium hydroxide in ethanol.
Since compound
5 was obtained in high purity by crystallization and the following transformation into salt
6 is quantitative, we use a standard solution of the latter salt in ethanol as internal standard. All the sample were then acidified, were extracted and then were analyzed by GC-MS. The most relevant data resulting from this study are collected in
Figure 4. We can observe that different strains, besides performing biohydrogenation of the conjugated double bond, further degraded the coumarin/melilotic acid.
Despite this fact, only Aspergillus niger afforded a number of detectable metabolites, whereas the analysis of the biotransformation mixtures obtained using the other strains allowed to detect only the presence of the melilotic acid and coumarin. Therefore, it is reasonable to assume that some species can completely degrade the studied phenylpropanoids through different metabolic pathways. This is the case of the fermentation experiment performed with Sporidiobolus johnsonii and Penicillium adametzii, where more than half of the starting coumarin was completely consumed after seven days. Though in a less pronounced way, also Penicillium camemberti, Torulaspora delbrueckii and Penicillium roqueforti were able to degrade coumarin whereas we didn’t observe these side reactions employing Kluyveromyces marxianus and Saccharomyces cerevisiae.
It is worth noting that the kinetics of the double bond saturation, of the dihydrocoumarin hydrolysis and of the phenylpropanoids degradation can be different from one microorganism to another. In order to acquire comparable data, we selected uniform conditions and a specific transformation time of seven days. Therefore, these results suggest the possibility to improve the biotransformation process by the optimization of the experimental conditions, based on the characteristics of the used strain.
3. Materials and Methods
3.1. Materials and General Methods
All air and moisture sensitive reactions were carried out using dry solvents and under a static atmosphere of nitrogen. All solvents and reagents were of commercial quality and were purchased from Sigma-Aldrich (St. Louis, MO, USA).
Coumarin and 6-methyl-coumarin were purchased from Sigma-Aldrich.
The following reference standard compounds were synthesized in our laboratory and were used either for the unambiguous identification of the compounds formed in the biotransformation experiments or as an internal standard for the determination of the transformation yields.
Dihydrocoumarin (
2) was prepared by the hydrogenation of coumarin at atmospheric pressure, using the acetic acid as a solvent and Pd/C as a catalyst [
42]. After the work up procedure, the crude product was purified by the bulb-to-bulb distillation. The obtained colourless oil showed the following analytic data:
Dihydrocoumarin (2) = (Chroman-2-one)
1H NMR (400 MHz, CDCl3): δ = 7.28-7.16 (m, 2H), 7.13-7.01 (m, 2H), 3.00 (br t, J = 7.3 Hz, 2H), 2.78 (br t, J = 7.3 Hz, 2H).
13C NMR (100 MHz, CDCl3): δ = 168.4 (C), 151.9 (C), 128.2 (CH), 127.9 (CH), 124.3 (CH), 122.6 (C), 116.8 (CH), 29.1 (CH2), 23.6 (CH2).
GC-MS (EI): m/z (%) = 148 [M+] (100), 120 (84), 106 (10), 91 (75), 78 (47), 63 (12), 51 (15).
Melilotic acid (3) was prepared by the treatment of dihydrocoumarin with NaOH in ethanol at a reflux for one hour. The main part of the solvent was removed by evaporation under reduced pressure and the residue was cooled at 0 °C. Diluted HCl aq. (3% w/v) was added dropwise until the pH of the mixture was comprised between the values of 5 and 6. The reaction was then extracted with ethyl acetate and the organic phase was concentrated under reduced pressure. The residue was purified by chromatography using the n-hexane/AcOEt mixture as an eluent to afford a pale yellow thick oil consisting of a 92:8 mixture (by NMR analysis) of melilotic acid and dihydrocoumarin, respectively.
Melilotic acid (3) = (3-(2-hydroxyphenyl)propanoic acid)
1H NMR (400 MHz, CDCl3): δ = 9.08 (br s, 2 H), 7.13–7.01 (m, 2H), 6.89–6.77 (m, 2H), 2.92 (br t, J = 7.1 Hz, 2H), 2.74 (br t, J = 7.1 Hz, 2H).
13C NMR (100 MHz, CDCl3): δ = 180.1 (C), 153.8 (C), 130.3 (CH), 127.9 (CH), 126.7 (CH), 120.8 (C), 116.3 (CH), 34.4 (CH2), 24.8 (CH2).
MS (ESI): 189.0 (M+Na+); 164.9 (M−H+).
GC-MS (EI): The GC-MS analysis of the melilotic acid shows a single peak with the retention time and mass spectra identical to those recorded for dihydrocoumarin.
6-Methyl-dihydrocoumarin (5) was prepared by the hydrogenation of 6-methyl-coumarin (4) at an atmospheric pressure, using the acetic acid as a solvent and Pd/C as a catalyst. After the work up procedure, the crude product was purified by chromatography using the n-hexane/AcOEt mixture as an eluent to afford pure 5 as a colorless solid, showing the following analytic data:
6-Methyl-dihydrocoumarin (5) = (6-methylchroman-2-one)
M.p: 78–80 °C
1H NMR (400 MHz, CDCl3): δ = 7.04 (dm, J = 8.2 Hz, 1H), 6.99 (br s, 1H), 6.94 (d, J = 8.2 Hz, 1H), 2.99–2.92 (m, 2H), 2.80–2.73 (m, 2H), 2.32 (s, 3H).
13C NMR (100 MHz, CDCl3): δ = 168.7 (C), 149.9 (C), 134.0 (C), 128.7 (CH), 128.4 (CH), 122.3 (C), 116.6 (CH), 29.3 (CH2), 23.7 (CH2), 20.7 (Me).
GC-MS (EI): m/z (%) = 162 [M+] (100), 134 (83), 120 (23), 105 (13), 91 (77), 77 (17), 65 (13), 51 (16).
3.2. Analytical Methods and Characterization of the Products Deriving from the Biotransformation Experiments
3.2.1. Instruments and Analytic Condition
Nuclear Magnetic Resonance spectroscopy (NMR): 1H and 13C-NMR spectra and DEPT experiments were recorded in CDCl3 solutions at rt using a Bruker-AC-400 spectrometer at 400 MHz, 100 MHz and 100 MHz, respectively; 13C spectra are proton decoupled; chemical shifts are in ppm relative to internal SiMe4 (=0 ppm).
TLC: Merck silica gel 60 F254 plates (Merck Millipore, Milan, Italy). Column chromatography: Silica gel.
Melting points were measured on a Reichert apparatus (Reichert, Vienna, Austria), equipped with a Reichert microscope, and are uncorrected.
Mass spectrum were recorded on a Bruker ESQUIRE 3000 PLUS spectrometer (ESI detector) (Billerica, MA, USA) or by GC-MS analyses.
GC-MS analyses: HP-6890 gas chromatograph equipped with a 5973 mass detector, using a HP-5MS column (30 m ′ 0.25 mm, 0.25 μm film thickness; Hewlett Packard, Palo Alto, CA, USA) with the following temp. program: 38° (9 min) − 3°/min − 90° (1 min) − 6°/min − 180° (1 min) − 15°/min − 280° (5 min); carrier gas, He; constant flow 1ml/min; split ratio, 1/30; tR given in min:
tR(1) 37.78, tR(2) 36.26, tR(5) 39.07.
The biotransformation reactions were analyzed using two different procedures depending on whether the internal standard was used or not.
3.2.2. Extraction/Analysis Procedure (without Internal Standard)
The biotransformation broth was treated at 0 °C with a concentrated HCl aq. (37% w/v) in order to bring the pH between 3 and 4. Ethyl acetate (about one fourth of the volume of the broth) was added and the mixture was filtered on a celite pad. The celite-biomass cake was washed with acetate, the phases were separated and the aqueous phase was extracted with further solvent. The combined organic phases were dried (Na
2SO
4) and concentrated under reduced pressure. The residue was analyzed using different methods. The TLC analysis showed the absence of dihydrocoumarin and the presence of the melilotic acid and/or of coumarin the in the crude biotrasformation mixture. The NMR analysis allows measuring the coumarin/melilotic acid ratio in the crude biotrasformation mixture. The GC-MS analysis gave a dihydrocoumarin/coumarin ratio (
Table 1). In these analyses, the dihydrocoumarin and coumarin GC peaks area were directly proportional to the concentration of the melilotic acid and coumarin, respectively. Most likely, when the sample is introduced in the GC injector, melilotic acid is quantitatively transformed into dihydrocoumarin whereas coumarin goes through the column unaffected. The GC-MS results are in good agreements with those obtained by the NMR analysis of the same samples, thus confirming that both analytical methods are suitable for the determination of the melilotic acid and coumarin concentration in the fermentation broths.
3.2.3. Quantitative Analysis Procedure (with Internal Standard)
A solution of disodium salt of 3-(2-hydroxy-5-methylphenyl)propanoic acid in ethanol was prepared by filling a 5 mL volumetric flask contained 100 mg of 6-methyl-dihydrocoumarin with a solution of NaOH (5% w/v) in absolute ethanol. The resulting pale-yellow solution was heated at 60 °C for 10 min and then was stored at 4 °C before the use. The latter solution (500 μL) was added to a 40 mL sample of the biotransformation broth. The mixture was stirred ad rt and acidified (final pH 3-4) by the dropwise addition of a concentrated HCl aq. (37% w/v). Ethyl acetate (10 mL) was added and the mixture was vigorously stirred for half an hour. The mixture was then centrifuged for 5 min, (4 °C, 3220 g) and the organic phase was collected, dried (Na2SO4) and analyzed by GC-MS. The 6-methyl-dihydrocoumarin peak (internal standard) correspond to a concentration of 250 mg/L of the same compound in the fermentation broth.
3.3. Microorganisms and Biotransformation Experiments
3.3.1. Microorganisms and Media
Saccharomyces cerevisiae (Type II YSC2, Lot BCBR1308) was purchased from Sigma-Aldrich (St. Louis, MO, USA).
Saccharomyces boulardii (probiotic strain SB80®, I-3799) was purchased from AR Fitofarma s.r.l (Assago, Italy).
Penicillium camemberti (DSM 1233), Geotrichum candidum (DSM 10452), Komagataella pastoris (DSM 70382), Yarrowia lipolytica (DSM 8218), Torulaspora delbrueckii (DSM 70483), Debaryomyces hansenii (DSM 70590), Candida boidinii (DSM 70026), Starmerella bombicola (DSM 27465), Kluyveromyces marxianus (DSM 70073), Xanthophyllomyces dendrorhous (DMS 5626), Cryptococcus curvatus (DSM 70022) and Sporidiobolus johnsonii (DSM 70580) were purchased from DSMZ GmbH collection (Braunschweig, Germany).
Aspergillus niger (CBS 626.26) was purchased from the CBS-KNAW collection (Utrecht, The Netherlands).
Penicillium adametzii (ATCC 10407) was purchased from the ATCC collection (Mannanas, VA, USA).
Penicillium corylophilum (MUT 5838) and Penicillium roqueforti (MUT 5856) were isolated as axenic cultures in our laboratory, then identified by the Mycotheca Universitatis Taurinensis (MUT) of the University of Turin and finally deposited in the same institution under the collection number given in brackets.
The biotransformation experiments were performed using two different media, namely the universal Medium for Yeasts (YM) and Malt Extract Medium (MEM), depending on the microorganism used.
YM composition: yeast extract (3 g/L), malt extract (3 g/L), peptone from soybeans (5 g/L), glucose (10 g/L).
MEM composition: glucose (20 g/L), malt extract (20 g/L), peptone from soybeans (2 g/L).
YM was used for Saccharomyces cerevisiae, Saccharomyces boulardii, Komagataella pastoris, Torulaspora delbrueckii, Yarrowia lipolytica, Debaryomyces hansenii, Candida boidinii, Starmerella bombicola, Kluyveromyces marxianus, Xanthophyllomyces dendrorhous, Cryptococcus curvatus and Sporidiobolus johnsonii.
MEM was used for Geotrichum candidum, Aspergillus niger, Penicillium camemberti, Penicillium roqueforti, Penicillium adametzii and Penicillium corylophilum.
All the biotransformations were carried out in triplicate and the presented results are the media of three experimental data.
The experimental conditions used for the biotransformations are based on the type of microorganism used. We used two main general procedures related to the different morphological features of the active grow mycelia.
3.3.2. General Procedure for the Biotransformation of Coumarin Using Microorganisms with Yeast-Shape Mycelium (Saccharomyces cerevisiae, Saccharomyces boulardii, Komagataella pastoris, Torulaspora delbrueckii, Yarrowia lipolytica, Debaryomyces hansenii, Candida boidinii, Starmerella bombicola, Kluyveromyces marxianus, Xanthophyllomyces dendrorhous, Cryptococcus curvatus, Sporidiobolus johnsonii and Geotrichum candidum)
A small amount of active mycelium was picked-up from a petri dish, was suspended in 1 mL of sterile water and then was inoculated in a 100 mL conical pyrex flask containing 40 mL of the suitable medium. The flask was shaken for three days at 28 °C and 140 rpm (with the exception of Xanthophyllomyces dendrorhous, Geotrichum candidum and Saccharomyces boulardii that were grown at 20 °C, 25 °C and 37 °C, respectively). After this period, the cells were centrifuged for 5 min, (4 °C, 3220 g) and collected, removing the medium. The cells were suspended in 3 mL of sterile water and were inoculated in a 1 L conical biotransformation flask containing 400 mL of fresh medium. In order to ensure aerobic conditions, the flask was sealed with a cellulose plug. The microorganism was grown in the same conditions described before for two days and then was treated with the suitable amount of a 300 g/L solution of coumarin in dry DMSO. The flask was then shaken at the indicated temperature and 140 rpm for seven days before performing the work-up and isolation procedures.
3.3.3. General Procedure for the Biotransformation of Coumarin Using Microorganisms with Spore-Forming Mycelium (Aspergillus niger, Penicillium camemberti, Penicillium roqueforti, Penicillium adametzii and Penicillium corylophilum)
In the case of the spore-forming mycelium, the spores were collected from a fully sporulated surface of a culture grown on a 90 mm in the diameter potato dextrose agar (PDA) plate and were then suspended in 10 mL of sterile water. After that, 1 mL of the same suspension was used to inoculate a 1 L conical biotransformation flask containing 400 mL of the suitable medium. In order to ensure aerobic conditions, the flask was sealed with a cellulose plug. The flask was shaken for three days at 25 °C and 140 rpm and then was treated with the suitable amount of a 300 g/L solution of coumarin in dry DMSO. The biotransformation was performed at 25 °C and 140 rpm for seven days before proceeding with the work-up and isolation procedure.
3.3.4. Isolation of the Dihydrocoumarin from the Fermentation Broth by Steam Distillation
The biotransformation was stopped by cooling the fermentation broth (400 mL) at 0 °C and by the addition of citric acid in order to bring the pH between 3 and 4. The mixture was steam distilled until the coumarin and/or dihydrocoumarin content in the last distillate fraction, were no longer detectable by the TLC analysis. The combined distillate fractions were saturated with NaCl and extracted with CH2Cl2 (3 × 100 mL). The combined organic phases were dried (Na2SO4) and concentrated under reduced pressure. The residue is a brown oil consisting of a nearly pure dihydrocoumarin/coumarin mixture. Pure dihydrocoumarin can be obtained by chromatographic purification of the latter oil, using the n-hexane/Et2O mixture as an eluent.
3.3.5. Isolation of the Dihydrocoumarin from the Fermentation Broth by Extraction-Distillation Procedure
The biotransformation was stopped by cooling the fermentation broth (400 mL) at 0 °C and by treatment with concentrated HCl aq. (37% w/v) in order to bring the pH between 3 and 4. Ethyl acetate (100 mL) was added and the mixture was filtered on a celite pad. The celite-biomass cake was washed with acetate, the phases were separated and the aqueous phase was extracted with further solvent. The combined organic phases were dried (Na2SO4) and concentrated under reduced pressure. The residue was treated with a catalytic amount of citric acid (20 mg) and the mixture was distilled under reduced pressure. The obtained pale yellow oil consists of a nearly pure dihydrocoumarin/coumarin mixture. Pure dihydrocoumarin can be obtained by chromatographic purification of the latter oil, using the n-hexane/Et2O mixture as an eluent.