Journal of Siberian Federal University. Biology 1 (2015 8) 32-44
УДК 582.282 :576.3+582.661.21
Amaranth Flour as a New Alternative Substrate
for Schizophyllum Commune Fr.: Fr.
and Cordyceps Sinensis (Berk.) Sacc. Growth
Tetiana A. Krupodorova* and Victor Yu. Barshteyn
Institute of Food Biotechnology and Genomics of National Academy of Sciences of Ukraine 2a Оsipovskogo str., Kyiv, 04123, Ukraine
Received 04.08.2014, received in revised form 21.09.2014, accepted 20.12.2014 The possibility of utilization of the waste after CO2-extraction of flour prepared from the Amaranthus hybridus L. grains (amaranth flour), as a medium for Schizophyllum commune Fr.: Fr. and Cordyceps sinensis (Berk.) Sacc. biomass production was explored. Biochemical analysis of amaranth flour was carried out. Basic components (moisture, protein, fat, ash, carbohydrates) of fungi mycelium were studied. Our results showed high biological efficiency of substrate utilization: 45 % for Sch. commune and 29 % for C. sinensis. We obtained 27.0 g/L and 17.4 g/L of mycelium of Sch. commune and C. sinensis, respectively, after 14 days of cultivation on amaranth flour. The fungal biomass of Sch. commune and C. sinensis can be consumed in food industry as a good source of main components: carbohydrates, dietary fiber, essential amino acids and unsaturated fatty acids.
Keywords: amaranth flour, fungi, mycelium, Schizophyllum commune, Cordyceps sinensis.
© Siberian Federal University. All rights reserved
* Corresponding author E-mail address: [email protected]
Шрот амаранта - альтернативный субстрат
для культивирования Schizophyllum commune Fr.: Fr.
и Cordyceps sinensis (Berk.) Sacc.
Т.А. Круподерова, В.Ю. Барштейн
Институт пищевой биотехнологии и геномики Национальной академии наук Украины Украина, 04123, Киев, ул. Осиповского, 2а
Изучена возможность использования шрота амаранта (амарантовой муки) - побочного продукта СО2-экстракции семян Amaranthus hybridus L. - в качестве питательной среды для культивирования Schizophyllum commune Fr.: Fr. и Cordyceps sinensis (Berk.) Sacc. Проанализирован состав амарантовой муки, определены основные характеристики (влажность, белок, жир, зола, углеводы) мицелия грибов. Установлена высокая биологическая эффективность усваивания субстрата: 45 % для Sch. commune и 29 % для C. sinensis. На 14-е сутки поверхностного культивирования получено 27,0 и 17,4 г/л биомассы Sch. commune и C. sinensis соответственно. Биомасса грибов Sch. commune и C. sinensis может быть использована в пищевой промышленности в качестве хорошего источника углеводов, пищевых волокон, незаменимых аминокислот и ненасыщенных жирных кислот.
Ключевые слова: амарантовая мука, грибы, мицелий, Schizophyllum commune, Cordyceps sinensis.
Introduction
Cordyceps sinensis (Berk.) Sacc. is an entomopathogenic fungus subphylum Ascomycotina, phylum Ascomycetes, class Pyrenomycetes, order Clavicipitales, and family Claviupitaceae (Kirk et al., 2008). It can be found in nature only at alpine pastures in north-west and central Himalayan region. Schizophyllum commune Fr.: Fr. belongs to the subphylum Basidiomycotina, phylum Basidiomycetes, class Basidiomycetes, order Agaricales, family Schizophyllaceae (Kirk et al., 2008) and is one of the most common bracket fungi with worldwide distribution. Both Sch. commune and C. sinensis are rich in biologically active compounds with potential therapeutic action and widely used as the components of
nutraceuticals and functional foods. Thus, these fungi are important objects of biomedical research and trials: morphology, physiology, chemistry (Mizuno, 1999; Hsu et al., 2002; Chang, Miles, 2004; Chau, Wu, 2006; Cheung, 2008; Wasser, 2010). However, the knowledge of the nutritional value of the mycelium of these species is limited in comparison to composition of their fruit bodies. Qualitative and quantitative analysis of medicinal and edible fungi for the estimation of nutritional quality and biological activity is very important when they are used as foods or nutraceuticals (Cheung, 2008; Wasser, 2010). Besides this, the production of mycelium by solid-state or submerged fermentation is viewed as a promising alternative to fruit bodies. Biomass production by submerged
fermentation has a number of advantages such as shorter period of cultivation and less chance of contamination. Usually, the culture medium for the higher fungi growth is mostly synthetic and semi-synthetic. The maximum values ofbiomass production and secondary metabolites of these fungi are presented in various reports (Jonathan, Fasidi, 2001b; Dong, Yao, 2005; Kumari et al., 2008; Smirnov et al., 2011). In addition, the reports describe natural monosubstrates for the mycelial cultivation. For example, a water-soluble homopolysaccharide can be produced by fermentation of Sch. commune on coconut water waste in submerged culture (Reyes et al., 2009). Amaranth flour is a waste after carbon dioxide extraction of Amananthus grains for oils and squalene (Matusova, 2008). The amaranth oil is used in cosmetic products for skin and hair (e.g. face cream, shampoo, balsams). Amaranthus L. is a fast-growing agricultural culture, cultivated mainly on the American continent, many countries of Europe, Asia and Africa (Svirskis, 2003). Its unique composition attracts increasing attention of the world food industry: meat and dairy products, bakery, confectionary, instant food and noodles, sauce and mayonnaise, oils, children nutrition, biologically active additives etc.
The purpose of this work was to study Sch. commune and C. sinensis biomass production on amaranth flour in liquid culture under static condition and to investigate the chemical composition of the fungal mycelium.
Materials and methods
Fungi species
Schizophyllum commune Fr.: Fr. (Strain 1768) and Cordyceps sinensis (Berk.) Sacc. (Strain 1928) were obtained from the Culture Collection of Mushrooms (IBK) of the M.G. Kholodny Institute of Botany of the National Academy of Sciences of Ukraine (Buchalo et al., 2011).
Cultivation medium basis
The basis of cultivation medium was the waste after CO2-extraction of flour prepared from the Amaranthus hybridus L. grains (hereinafter referred to as amaranth flour). A. hybridus species was a variety «Ultra» (Mykolaiv Oblast, Ukraine, 2011). CO2-extraction conditions: pressure -7.2 MPa; temperature - 24 °C; duration of extraction - 2 hours.
Growth Conditions
Mycelial cultures were initially grown in Petri dishes (90 mm in diameter) on culture medium, composed of (in g/L): glucose - 20, yeast extract - 3.0, peptone - 2.0, K2HPO4 -1.0, KH2PO4 - 1.0, MgSO4-7H 2O - 0.25, pH 6.0 and then the mycelium was transferred to liquid cultivation medium contained 60 g of amaranth flour per 1L of distilled water. The culture medium was sterilized by autoclaving for 20 min at 121°C. Mycelium was grown as static cultures in 250-mL flasks for 14 days at 26±2°C.
Separation
Mycelium was separated from the medium by filtration through Whatman's filter paper № 4 and washed with distilled water. Then, it was high-vacuum freeze dried with a Cryodos-50 freeze dryer (Terrasa, Spain) and ground using a blade grinder.
Macronutrients
Dry samples were analyzed for chemical composition (moisture, crude protein, crude fat, ash) according to AOAC methods (AOAC, 1990). Total nitrogen was determined with the Kjeldahl's method (Pleshkov, 1976). The crude protein was calculated using the conversion factor 4.38 (Crisan, Sands, 1978). The content of amino acids was estimated with a T-339 amino acid analyzer ("Mikrotechna", Prague, Czech Republic) (Krischenko, 1983).
Lipids were extracted by Folch's method (Folch et al., 1957), and fatty acids were estimated using a "Crystal Lux" chromatograph ("BIOMASHPRIBOR", Yoshkar-Ola, Russia) with flame-ionization detector on the capillary column SP-2560 (Supelco, USA). Fatty acids were presented as percentages of the total sum with precision up to 0.01 %.
Crude fibre was determined according to patent (Osadchenko, Gorlov, 2002).
Carbohydrates (%) were calculated as follows (Grangeria et al., 2011):
Carbohydrates = 100 - ( protein + fat + ash)
The energy content was calculated with the following factors: protein 4.0 kcal/g; fat 8.37 kcal/g and carbohydrates 3.48 kcal/g (Crisan, Sands, 1978).
Biological efficiency (%) was calculated using the following equation (Jwanny et al., 1995):
A
Biological efficiency = (—)-100,
where A is weight of mycelium, B is weight of amaranth flour in the medium.
Vitamins
Determination of vitamin B1 was based on the oxidation of thiaminum to the thiochrome, extraction of residuum with an organic solvent and measuring of intensity of fluorescence (Ostrovsky, 1975).
Detection of vitamin B2 was carried out using riboflavin-binding apoprotein from egg albumin in accordance with method of Kondentsova (1994).
Vitamin B12 was determined with the microbiological method (Bilay, 1982) by means of indicatory culture of Escherichia coli 113-2, which has a sensitiveness 0.005-5.0 ^g/ml.
Vitamin A and carotenoids were determined with the colorimetric method based on reaction of antimony trichloride and trifluoroacetic acid (Ostrovsky, 1979).
Measuring of vitamin C (ascorbic acid) was based on its reductive properties in particular, the ability to recover potassium iodate to free iodine, which amount is determined by reaction with starch (Pleshkov, 1976).
Chemical elements
Chemical elements (Na, P, K, Ca, Ti, V, Cr, Mn, Fe, Co, Cu, Zn, As, Zr, Mo, Cd, Ba, La, Hg, Ti, Pb, Ce) were determined using the Thermo Scientific "Element-2" HP-ICP-MS ("Thermo Finnigan", Bremen, Germany) (Chudinov, 1990).
Statistical analysis
All experiments were carried out in triplicate. The data were analyzed by Excel statistical functions using Microsoft Office XP software the Statistical Package for Social Sciences, Program 11.5 Version (SPSS, Inc., 2002). Values are presented as means ± standard error of the mean (SEM). Differences at P < 0.05 were considered to be significant.
Results and discussion
The feasibility of using the agricultural waste, amaranth flour, as an alternative substrate for the cultivation of mycelium was investigated. The growth of fungi depends on the presence of a number of important nutrient substances in a substrate: carbon and nitrogen sources, protein, vitamins, macro- and microelements. Therefore, we investigated our potential substrate for the levels of biologically active constituents.
Amaranth flour used in this study contained 15.4 % protein, 1.5 % fat, 3 % ash, 4 % dietary fiber and 3.7 % moisture (we have obtained these data for A. hybridus for the first time). The content of protein, fat and ash in amaranth flour 35 -
Glutamic acid Glycine Aspartic acid Argenine Serine Lysine* Leucine* Alanine Phenylalanine* Threonine* Tyrosine Proline Histidine Valine* Isoleucine* Cystine Methionine*
4,5 4,3 ^■4 H
■3,7 H 3,51-1
2,5 ■2,3 H 2,1 H ■2 1,4-1
10
15
20
%
25
5
0
5
Fig. 1. Content of amino acids in amaranth flour ( % of the total), *essential amino acids, bars represent standard errors (n = 3)
Table 1. Vitamin content in amaranth flour
Vitamins
Thiamine (VBj), mg/g dw 0.5±0.1
Riboflavin (VB2), mg/g dw not detected
Cyanocobalamin (VBn), ^g/g dw 0.1±0.0
Vitamin A, mg/g dw trace
Carotenoids, mg/g dw trace
Ascorbic acid, mg/g dw 0.5±0.2
Each value is expressed as mean ± SE (n = 3).
from Amaranthus cruenthus L. (Shmalko, 2005) hardly differed from our data, in contrast to fiber and moisture content.
Amaranth flour is rich in amino acids (Fig. 1). Amaranth flour contains a high amount of essential amino acids, such as lysine and leucine, and nonessential amino acids - glutamic acid, aspartic acid and glycine. This is important, given the results of numerous studies (Fasidi, Olorunmaiye, 1994; Jonathan, 2002; Gbolagade
et al., 2006; Johnsy, Kaviyarasan, 2013; Neelam et al., 2013) that have shown that the addition of various amino acids promoted growth of higher fungi.
Five vitamins, mainly ascorbic acid, were found in amaranth flour (Table 1). A number of researchers have shown that vitamins contributed to the increased growth of mycelium. Addition of thiamine increased growth of C. sinensis mycelium by 1.2 times (Dong, Yao, 2005) and
Sch. commune mycelium by 1.8 times (Jonathan, Fasidi, 2001b), addition of ascorbic acid increased growth of Sch. commune mycelium by 1.4 times (Jonathan, Fasidi, 2001b). Thiamine was the best stimulator of mycelial growth of Pleurotusflorida (Adenipekun and Gbolagade, 2006). Effect of thiamine addition on biomass augmentation can be explained by its role as co-enzyme for several enzymes of intermediary metabolism. According to Adejoye et al. (2007), vitamin addition was not absolutely required for Sch. commune growth, since this fungus is able to produce the vitamins necessary for its growth. A similar conclusion was reached as a result of studies of Pleurotus tuber-regium growth (Fasidi, Olorunmaiye, 1994).
Our study has shown that amaranth flour contains 4 macroelements and 14 microelements (Table 2). Potassium, calcium and phosphorus are necessary components for biosynthetic activity of mycelium. Neelam et al. (2013) indicated the importance of calcium, magnesium and potassium for the growth of Pleurotus ostreatus and P. eryngii. The same behavior was noted for P. tuber-regium (Fasidi, Olorunmaiye, 1994), Sch. commune (Jonathan, Fasidi, 2001b) and P. florida (Adenipekun, Gbolagade, 2006). Calcium and magnesium also provided the best growth of Psathyerella atroumbonata (Pegler) (Jonathan, Fasidi, 2001a). However, calcium had little effect on the growth of C. sinensis (Dong, Yao, 2005). Researchers attach great importance to such essential microelements as Zn, Mn and Cu: zinc is a functional component of enzymes (Garraway, Evans, 1984; Dong, Yao, 2005; Jonathan, Fasidi, 2001b), manganese plays important role in TCA cycle, in ATP metabolism, and nucleic acid synthesis (Garraway, Evans, 1984) and copper is the complement of copper-containing proteins and enzymes, mainly redox ones. It should be noted that the harmful and dangerous ions of Cd, Hg, Pb and As were not present in amaranth flour.
We obtained 27.0±0.2 g/L of mycelial biomass of Sch. commune and 17.4±0.1 g/L of C. sinensis after 14 days of static cultivation on amaranth flour. Maximum biomass of these fungal species varies with fungal strains and with cultivation conditions (medium, temperature, pH, phase of growth, culture duration). However, the biomass of Sch. commune in our experiment was higher than that reported earlier by other researchers who used different mediums: glucose-peptone (Maziero et al., 1999; Bolla et al., 2008), glucose-bacto yeast extract (Shu et al., 2005), optimized medium with sucrose (Kumari et al., 2008; Smirnov et al., 2011; Kumar, Singhal, 2011), glucose-yeast extract (Adejoye et al., 2009), glucose-based medium (Yogita et al., 2011). C. sinensis accumulated higher biomass values compared to those reported by Liang et al. (2009) at solid state cultivation on fermented rice and was identical to the results by Smirnov et al. (2009) in a shorter period of submerged cultivation on molasses-based medium. Biomass obtained in this study in static culture was lower than that obtained by other researchers (Dong, Yao, 2005; Kim, Yun, 2005; Cha et al., 2007) with submerged cultivation on rotary shaker.
Biological efficiency is one of the significant calculated indices for understanding the extent of substrate utilization by growing fungal cultures. Taking into account that we worked with vegetative mycelium of fungi, but not with their fruit bodies, our results showed high biological efficiency of substrate - 45 % for Sch. commune and 29 % for C. sinensis cultivation.
The evaluation of the nutritional quality of different fungal products for their specific use is necessary and important. The basic compositions of the two fungi were significantly different (Table 3). Carbohydrate, dietary fiber and protein were the main components. Sch. commune mycelium contained higher amount of protein (45.4 %) and dietary fiber (35.7 %), whereas C. sinensis
Table 2. Macro- and microelement content in amaranth flour, (ig/g
Macroelements
P K Ca Na
10000±0.8 558.4±0.5 36.4±0.7 10±0.2
Microelements
Ti Ce Ba La Mn Zr Zn Cu Co Mo Cr V Fe Bi
600±0.5 200±0.6 100±0.7 100±0.2 80±0.4 60±0.3 30±0.1 20±0.5 10±0.2 2±0.1 2±0.0 2±0.0 1.9±0.3 1±0.1
Each value is expressed as mean ± SE (n = 3).
Table 3. Basic composition of fungal mycelium
Chemical component C. sinensis Sch. commune
Moisture, g/lOOg ww 2.4±0.1 2.0±0.1
Protein, g/lOOg dw 28.9±0.1 45.4±0.5
Fat, g/lOOg dw 6.5±0.2 8.4±0.2
Ash, g/lOOg dw 6.3±0.2 4.5±0.3
Dietary fiber, g/lOOg dw 29.6±0.4 35.7±0.6
Carbohydrates, g/lOOg dw 58.3 41.7
Energy, kcal/lOOg 372.9 397.0
Each value is expressed as mean ± SE (n = 3).
16
1G
14
12
10
C. i/rttftsii ■ Sch. commune
////'/W////S/
Fig. 2. Content of amino acids of fungal mycelia ( % of the total), *essential amino acids, bars represent standard errors (n = 3)
mycelium was enriched with carbohydrate (58.3 %). The carbohydrate and dietary fiber content in mycelium of both fungi and protein content in Sch. commune mycelium were higher as compared to those reported by other researchers (Mizuno, 1999; Chang et al., 2001; Hsu et al., 2002; Tseng et al., 2005). The amount of protein in C. sinensis mycelium in our work is similar to that reported
by Smirnov et al. (2009) and Mizuno (1999), but higher than the results of Hsu et al. (2002).
Fungal proteins of our species consisted of 17 amino acids, with glutamic acid predominating for both fungi (Fig. 2). Aspartic acid was high for Sch. commune, that's typical for other species of higher Basidiomycetes (Scherba et al., 1999; Babitskaya et al., 2003). Different numbers of 39 -
Table 4. Content of fatty acids in fungal mycelium ( % of the total)
Constituent C. sinensis Sch. commune
C14:0 0.4±0.1 0.6±0.1
C15:0 1.5±0.3 1.3±0.2
C16:0 16.4±0.2 17.6±0.3
C17:0 0.5±0.2 0.6±0.3
C18:0 2.9±0.3 1.4±0.1
Saturated fatty acids 21.7 21.5
C16:1 0.3±0.1 0.2±0.1
C17:1 0.4±0.1 0.3±0.1
C18:1<o 9 24.2±0.3 21.1±0.5
Monounsaturated fatty acids 24.9 21.6
C18:2ro6 52.3±0.4 55.8±0.4
C18:3ro3 1.1±0.3 1.2±0.1
Polyunsaturated fatty acids 53.4 57.0
Unsaturated fatty acids 78.3 78.6
Unsaturated fatty acids/ Saturated
fatty acids
Each value is expressed as mean ± SE (n = 3).
amino acids in C. sinensis mycelium are reported: 16 by Hsu et al. (2002), 17 by Smirnov et al. (2009), and 18 by Mizuno (1999).
The quantitative analysis of amino acids in both fungal mycelia showed differences in their content (Fig. 2). Seven essential amino acids were presented, but their amount were higher in C. sinensis mycelium. The predominant essential amino acid in this fungus was lysine, and threonine was the second. Leucine and threonine were the major constituents of the essential amino acids in the Sch. commune mycelium. The level of nonessential amino acids in Sch. commune was higher compared to C. sinensis. Glutamic acid, alanine, lysine and proline were maximal in C. sinensis mycelium. The predominance of lysine and alanine in C. sinensis mycelium was in agreement with the results reported by Hsu et al. (2002) and Liang et al. (2009). In contrast, Mizuno (1999) noted the predominance of isoleucine in C. sinensis mycelium.
The lipids content of both fungi was low, less than 10 % of dry weight, which is confirmed by other reports (Mizuno, 1999; Liang et al., 2009; Smirnov et al., 2009). Ten fatty acids were detected (Table 4). Smirnov et al. (2009) reported 9 fatty acids (heptadecenoic acid was absent) in C. sinensis mycelium grown in a fermenter on the molasses-based medium. There were few significant differences in content of individual fatty acids between fungi species. Palmitic acid (16:0) had the highest content among saturated fatty acids in mycelium of both fungi. Polyunsaturated fatty acids (PUFAs) of ra6 and ra3 families were revealed in mycelium. PUFAs are a vital source of energy in our diet. The major fatty acids found were polyunsaturated linoleic acid (18:2ra6) and monounsaturated oleic acid (18:1<»9). We would like to emphasize that the finding of a high content of unsaturated fatty acids and a high percentage of linoleic acid
in these fungal mycelia is a significant factor which defines these fungi as a health food and useful constituent of our diet.
Thus, amaranth flour meets all the required criteria of the substrate: a readily available free waste product (the waste of CO2-extraction), microbiological purity (Pekhov et al., 1992), high nutritional value and good biological efficiency.
Conclusion
Amaranth flour contains amino acids, vitamins, microelements for mycelial growth and can be used for cultivation of fungi as an alternative free substrate. This substrate should be consider as a natural, complete medium which could contribute to reducing the cost of
biomass production not only for Sch. commune and C. sinensis, but for other fungi species. The biomass of Sch. commune and C. sinensis, obtained on this substrate, can be consumed in food industry as a good source of carbohydrates, dietary fiber, nonessential amino and fatty acids. Subsequent research must be devoted to the amaranth flour utilization in submerged culture and to the process of mycelium growing on this substrate for the production of fungal metabolites. The use of amaranth flour expands the boundaries of a waste utilization.
Acknowledgements
The authors would like to thank Professor A.S. Buchalo for cultures of fungi from IBK Collection.
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