1. Introduction
The therapeutic properties of many mushrooms, known to indigenous cultures across the globe, have been traced to their underlying chemical compounds with the advent of chemistry and molecular biology. Although the most well-documented are their use in cancer treatment due to beneficial glucan and proteoglycan synthesis [
1], mushrooms have other therapeutic properties including antioxidant, antihypertensive, hepatoprotective, antifibrotic, anti-inflammatory, antidiabetic, antiviral, antimicrobial, and cholesterol-lowering properties [
2].
Great improvements in biomass yield and bioactive compound production have been achieved with the help of biotechnological cultivation technics and conditions applied to mycology [
3,
4,
5,
6].
I. obliquus, also known as Chaga, is a mushroom that lives in certain parts of Europe and Asia at latitudes of 45–50° N as a parasite of birch trees [
7]. In this environment, the Chaga mushroom grows very slowly and is not a reliable source of pharmaceutical compounds for industrial applications [
8].
Recent studies have shown that the Chaga mushroom can produce polyphenols [
9], flavonoids [
10], melanins [
11], and tannins [
12]. It is also able to synthesize biologically active ergosterol peroxide, with a role in anticancer activity [
13], as well as betulin, which has antiviral and anti-inflammatory properties [
14].
Optimization of the various parameters or products of
I. obliquus culture regularly employs a fractional factorial design, coupled with response surface methodology [
15,
16].
In this study, we attempted to increase the biomass of submerged cultures of Chaga mycelium by using a custom mix-process experimental design capable of predicting an optimum nutrient broth composition. Response surface methodology was used to evaluate the effects of different biotechnological parameters on biomass yield and played a role in the optimization process.
2. Materials and Methods
2.1. Inoculum Preparation
Inonotus obliquus (Ach. ex Pers.) Pilát (CBS 314.39) mycelium was purchased from Westerdijk Fungal Biodiversity Institute and grown on PDA agar (VWR Chemicals, Leuven, Belgium) for 7 days at 23.5 °C. Subsequently, 1 × 1 cm agar sectors were each transferred to 250 mL bottles with PTFE (polytetrafluoroethylene) membrane screw caps, which contained PDB seed culture medium (VWR Chemicals, Leuven, Belgium). The mycelia were incubated at the same temperature, with orbital shaking at 100 rpm until they occupied the entire volume of the culture vessels.
2.2. Optimization Design of the Nutrient Broth Components
Modern experimental designs fall into three main study types: factorial, mixture, or custom. The latter is used when the experiment requires adjustments that cannot be accommodated by a standard mixture design, such as when the differences between the high and low of all the mixture components are not the same, or when mixture and process variables are both used in the same design.
In order to optimize growth media in terms of biomass yield, the effect of six mixture components and one numeric factor was studied. Yeast extract (Merck KGaA, Darmstadt, Germany) and malt extract (Oxoid Ltd., Basingstoke, UK) were used as a protein source, while fructose (Schneekoppe GmbH, Buchholz, Germany) and soluble starch (Carl Roth GmbH, Karlsruhe, Germany) provided the carbohydrate source, and the latter also acted as a glucose substitute. We focused on fructose because it was reported that silver birch sap consists mostly of fructose (5.39%
w/
w) and, to a lesser extent, glucose (4.46%
w/
w) and sucrose (0.58%
w/
w) [
17]. All growth media formulas were supplemented with equal amounts of magnesium sulfate heptahydrate (Merck KGaA, Darmstadt, Germany) and calcium chloride dihydrate (Honeywell GmbH, Seelze, Germany). Sterilization was performed at 121 °C for 15 min. The pH value of the growth media represented the single numeric factor, which was measured and entered into the experimental design after each media variant was sterilized, before being inoculated. The boundary values for each variable were chosen according to relevant literature data regarding submerged mushroom mycelium cultivation (
Table 1).
The software Design-Expert version 11.1.0.1 (Stat-Ease Inc., Minneapolis, MN, USA) was used to achieve the mathematical modeling and statistical analysis of the experiment. By working with the type of design space described so far and inputting the above constraints, the software generates model points (runs) that are chosen algorithmically, though limited to as few runs as possible. These included five replicate points and five lack-of-fit points, supplementing the 20 required model points (
Table 2).
To determine the appropriateness of a design involving mixture components, prediction-based metrics such as fraction of design space (FDS) statistics are employed. The FDS graph is useful for calculating the volume of the design space with a prediction variance equal to or less than a specified value. This custom volume’s ratio to the total volume is the fraction of the design space. The response surface was drawn by predicting the mean outcome as a function of inputs over the region of experimentation (
Figure 1).
The custom quadratic × linear model in which the terms A, B, C, and D, and interactions: AB, AC, AD, AG, BC, BD, BG, CD, CG, and DG, were evaluated by FDS statistics found that 80% of the design space was below a standard error mean of 2.399.
By plotting the standard error of design and the different model values for the A, B, and G terms, the latter’s effect was shown to be the main source of the standard error mean value (
Figure 2).
If the interactions related to the G term were not evaluated, the standard error mean for the same fraction of design space became 0.489. However, this approach hinders the significance of the model’s prediction power when evaluating the experimental response. Because the values of the single numeric factor were not generated algorithmically but were inputted based on real data, their predictive power is low. As such, the optimization results relating to the effect of pH on the dry weight of mycelium were not considered.
2.3. Broth Variants Cultivation
The experimental broths were prepared at a volume of 500 mL in screw-cap bottles with air exchange provided by PTFE membranes (0.22 µm pores). Each variant was inoculated by transferring 20 mL (a 4% v/v inoculum) of triturated and homogenized mycelium suspension from the fully occupied culture vessels. Sterilized glass beads were added to the screw-cap bottles, and vigorous shaking of the mycelium with the beads was used to achieve trituration. The resulting inoculated broth variants were cultured at 26 °C and agitated at 115 rpm for 21 days.
2.4. Bioreactor Cultivation
A 10 L double wall (jacketed) Biostat B (Sartorius Stedim Biotech, Göttingen, Germany) bioreactor, equipped with a dissolved oxygen and pH sensor, temperature control, stirrer, and ring sparger, was used to ensure replicable, pilot scale cultures of I. obliquus. The submerged, aerobic cultivation lasted 15 days and employed a strategy of specific parameter variation, according to the age of the culture. The stirrer shaft speed was kept at 50 rpm until the 5th day of culture, when it was increased to a final value of 75 rpm. Aeration was provided through the ring sparger at a rate of 2 L/min by adjusting a flowmeter. A solenoid valve further limited the airflow to a chosen percentage of the time. At the moment of inoculation, this value was 1%. On the 8th day of culture, aeration was increased to 8% and then again on the 12th day to the final value of 10%. Airflow entry and exit points were passed through Millex-FG50 (Millipore Co., Billerica, MA, USA) filter units. The temperature was maintained at a constant 24 °C throughout the whole culture period.
All bioreactor batches were loaded with 8 L of nutrient broth, 6 L of which were sterilized in 2 L communicating vessels, while 2 L remained in the culture vessel. The communicating vessels were sterilized separately from the bioreactor, although for the same duration of time. This procedure allows for better sterilization efficiency, especially when dealing with custom nutrient broths with ingredients having a high microbial load. Sterilization time differed: for potato dextrose broth, we used 20 min at 121 °C; for the custom nutrient broth, we used 50 min at the same temperature.
Each batch was inoculated by transferring 250 mL (a 3.125% v/v inoculum) of triturated mycelium suspension from one of the fully occupied culture vessels. The dry weight of this inoculum was calculated to be 1.415 g by averaging the weight of three identical lyophilized cultures. Similarly to the shaken cultures, the bioreactor cultures were not pH corrected throughout the fermentation process. For the optimized broth, the pH value at the start of cultivation was 4.89, whereas for the PDB, this value was 5.4 at the moment of inoculation.
2.5. Mycelial Biomass Harvesting
All cultures were harvested by separating the mycelium from the broth through a 1 mm sieve, followed by further filtration of the broth through a 250 nm sieve. The mycelia were then washed three times with deionized water and frozen at −50 °C before being lyophilized (Biobase BK-FD12S vacuum freeze dryer). Mycelial biomass was estimated by dry weight and is expressed as g/500 mL for the optimization experiment and as g/L for the bioreactor cultures.
4. Discussion
The submerged optimum broth bioreactor culture of I. obliquus mycelium yielded 93.36% of the dry weight prediction calculated by modeling 29 successful experimental cultures with different broth compositions. We studied the effect of six nutrient components and broth pH in a mixture-process type of experimental design and chose the highest yielding combination of factors using response surface methodology.
By using a stirred and aerated bioreactor, the cultivation period of the I. obliquus mycelium was reduced from 21 days (with static air exchange vessels in an incubator) to 15 days, all while the inoculum volume decreased from 4% to 3.125 % v/v. With these parameters, the mycelium grown in the optimized broth occupied the entire volume of the bioreactor, showing a 24.7-fold increase in dry weight at the end of the culture period.
We also grew I. obliquus mycelium in potato dextrose broth under the same bioreactor conditions to compare growth speed and final yield. Here we found that the culture grew more slowly, with an 11.78-fold increase in dry weight at the end of the cultivation period. We also found differences in the morphology of this mycelium, which accreted in dark-colored globules compared with the one grown in the optimized broth. Here, the color of the broth changed from a pale yellow at the beginning of cultivation to a reddish-brown at the end, indicating the possible release of soluble melanin pigments.
In a study of
I. obliquus optimization, potato dextrose broth was also used in conjunction with submerged culture technics, yielding between 1.65 and 2.36 dry g/L for Difco PDB and fresh potato broth, respectively. The cultivation period lasted 12 days at 26 °C, with 100 mL flasks containing 25 mL of broth being used [
18]. Our findings show similar yields (2.084 g/L) with 8 L of PDB inoculated in a stirred, aerated bioreactor culture.
In another study, shake flask cultures were performed with 250 mL flasks containing 50 mL of glucose, yeast extract, and MgSO
4-based broth. Cultivation lasted 8 days at 25 °C and 150 rpm, and we used an orthogonal design to vary the three broth components. Mycelium dry mass was found to be between 3.6 and 8.11 g/L. Furthermore, a 5 L stirred tank bioreactor was used (3.5 L working volume) at identical temperature and agitation speed for 10 days. This yielded a maximum of 8.24 g/L after 8 days [
14]. Our results confirm high yields when using optimized liquid culture media containing yeast extract, MgSO
4, and a simple monosaccharide. However, we found that after 15 days of bioreactor culture with an optimized liquid medium, the entire 8 L volume was completely occupied by mycelium. The yields reported in the aforementioned study present a 1.88-fold increase in dry mycelium compared with a bioreactor culture that is already fully colonized.
For I. obliquus, we found that the maximum airflow of 0.2 L/min, combined with an agitation value of 75 rpm, was adequate for keeping the broth at an oxygen saturation of 50% for the final 3 days of culture.
In this paper, we provide a low-cost optimized broth formula for the rapid growth of I. obliquus mycelium and present a bioreactor method of culture based on incremental aeration and agitation.
The submerged cultivation of mycelium is well-suited for fast biomass production, and more so when paired with stirred tank bioreactor methods. Fast production of therapeutic metabolites such as betulin and ergosterol peroxide is possible by using this biotechnological approach.
A study of antioxidant constituents identified 22 extracellular and intracellular phenolic compounds in submerged cultures of
I. obliquus grown in different culture media (control, H
2O
2, and arbutin-supplemented broths). The addition of hydrogen peroxide and arbutin increased the total levels of intracellular phenols and decreased these same compounds secreted extracellularly [
8]. By this procedure, the mycelial biomass was enriched in antioxidant compounds. Such methods can easily be coupled with biomass accumulation strategies for a synergistic approach.