Proximate Analysis and Mineral Content of Laetiporus sulphureus Strain MFLUCC from Northern Thailand

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1 Chiang Mai J. Sci. 2014; 41(4) 765 Chiang Mai J. Sci. 2014; 41(4) : Contributed Paper Proximate Analysis and Mineral Content of Laetiporus sulphureus Strain MFLUCC from Northern Thailand Thatsanee Luangharn [a,b], Kevin D. Hyde [a,b] and Ekachai Chukeatirote * [a,b] [a] School of Science, Mae Fah Luang University, Chiang Rai 57100, Thailand. [b] Institute of Excellence in Fungal Research Mae Fah Luang University, Chiang Rai 57100, Thailand. *Author for correspondence; ekachai@mfu.ac.th Received: 16 January 2014 Accepted: 21 February 2014 ABSTRACT Laetiporus sulphureus, a member of the fungal class Aphyllophorales (Polypores) of the Basidiomycota, is widely distributed in tropical countries. In this article, chemical composition and nutritional quality of the Thai L. sulphureus mushroom were investigated. Protein, fat, crude fibre and carbohydrate concentrations were 6.91, 1.70, 6.43, and 71.74% dry weight, respectively. Mineral contents were determined as mg/kg dry weight for Fe (2.28), Zn (1.20), Mn (0.35), Cu (0.14), Na (11.01), Ca (2.59), and Mg (1.09). Keywords: Laetiporus sulphureus, edible mushroom, nutritional data, element composition 1. INTRODUCTION The genus Laetiporus was introduced by Murrill 1904 and is typified by Boletus sulphureus Bull. [1]. L. sulphureus (Bull.:Fr.) Murrill 1904 is among the most readily recognized of all macrofungi due to its striking orangecoloured, bracket-like fruit-bodies. Some variation is recognized in the bright orange color, fleshy basidiocarps, and imbricate fruiting bodies. This fungus appears to be a cosmopolitan species; its presence is wide from cool temperate to tropical zones. It also has a wide host range, from hardwoods to conifers [2]. L. sulphureus is a wood-rotting basidiomycete and can cause red-brown cubical heart rot in many trees [3]. The species also has a long history of consumption especially in North America [4], Japan [5], and Thailand. In addition, this mushroom was found to medically active in several therapies, such as antitumor, antiviral, antimicrobial, and immunomodulating treatments [6]. Previous studies on this species have revealed many interesting metabolites that can be applied in the medicine and food industries. These compounds include laetiporic acids [7], polysaccharides and alkali-soluble polysaccharides [8], fatty acid and amino acid [9], and α-(1 3)-glucans[10]. In this study, we aim to determine the nutritional value and essential elements of L. sulphureus collected from Northern Thailand. Such data are absent from the literature although the species has been used as food. Therefore, our results obtained are expected to be used as a reference for food composition and nutritional value of this mushroom.

2 766 Chiang Mai J. Sci. 2014; 41(4) 2. MATERIALS AND METHODS 2.1 Mushroom Sample L. sulphureus specimen was collected from a field trip at Doi Mae Salong, Chiang Rai, Thailand. The sample was initially characterized based on its distinct morphology. The mushroom was brought to the laboratory and examined under the compound microscope. Detailed morphology was recorded based on macrocharacters. The sample was subsequently dried at 40 o C for 24hr, wrapped with stencil paper and kept in a polyethylene bag. This dried specimen is deposited at Mae Fah Luang University (voucher specimen no. MFLUCC ). 2.2 Proximate Analysis In general, proximate analysis was carried out based on the standard procedure of the AOAC [11]: moisture content by drying g test sample at 105 o C in a hot air oven (UM500, Memmert); ash content by igniting g sample in an electric furnace (Eurotherm 2416CG, Lento) at 600 o C; and crude fibre by acid treatment and subsequent heating g at 600 o C in the Fibertec System M1020 Extractor (Foss Tecator). The Kjeldahl method was performed to analyse nitrogen-free extract in which the protein content was estimated by multiplying with a conversion factor of 5.99 [12]. Fat content was determined by the Soxtec 2055 Extraction Unit (Foss Tecator) with petroleum ether. All the analyses were carried out in triplicate. 2.3 Mineral Content Analysis Minerals (Fe, Zn, Mn, Cu, Na, Ca, Mg, and K) were analysed based on an atomic absorption spectrophotometric (AAS) technique. Dried mushroom sample (2.000g) was placed in a crucible and burned at 550 o C for 8 h [13]. After cooling down at room temperature, the sample was digested with 50ml of 0.1N HCl and the solution was filtered with 20μm filter papers. The filtrate was passed through the AAS system (Z-5000 Polarized Zeeman AAS, HITACHI, Japan) using different lamps, and calibrated with standard minerals. Stock standard solutions of each element were prepared from commercially available mineral standard solution (1000 ppm, Merck, Germany). Each standard solution was adjusted to 50 ml with 0.1 N HCl. Every sample solution was directly analyzed, except for the Na solution, which was diluted five-fold before analysis. Detection limit is defined as the concentrations corresponding to three times the standard deviation of ten blanks. Detection limit values of elements as milligrams per kilogram (mg/kg) in AAS were for Fe, for Zn, for Mn, for Cu, for Na, for Ca, for Mg, respectively. 3. RESULTS AND DISCUSSION 3.1 Morphology of L. sulphureus Strain MFLUCC In this study, the L. sulphureus samples were collected based on their distinct morphology. This mushroom sample collected from a dead log of Castanopsis was used in morphological study. Fresh fruiting bodies of the mushrooms were conspicuous with bright orange to yellow colored pileus; their textures were soft and fleshy (Figure 1a). Basidiocarps occur in large imbricate clusters and vary considerably in size (7 14cm wide and 12 30cm long) (Figure 1b). Fresh mushroom samples were dried and prepared as powder form for further analysis (Figure 1c). For microscopic analysis, the inner tissue of fresh mushroom was transferred on to potato dextrose agar (PDA) plate and incubated at 30 o C for 14 days. The pure mycelium culture was then obtained by

3 Chiang Mai J. Sci. 2014; 41(4) 767 Figure 1. Laetiporus sulphureus strain MFLUCC a. Fruiting bodies on the Castanopsis sp. Host. b. Basidiocarps characteristic. c. L. sulphureus powder prepared from dried mushroom. Scale bar: a b =5 cm). subculturing the hyphal tip to new PDA plates, and kept as a stock culture (Figure 2a). When observed under the microscope, pore thama are generative and skeleton hyphae (Figures 2b 2c), the hyphae are dimitic and lack cystidia and clamp connections [14]. Hymenium of basidia are thin wall (Figure 2d). 3.2 Proximate Analysis L. sulphureus, commonly known as a wild edible mushroom, was selected to determine its nutritional value. In this study, a wild strain of L. sulphureus (MFLUCC ) was collected in northern Thailand and the data of chemical composition of this mushroom are shown in Table 1. Thai L. sulphureus is a good source of carbohydrate (71.74%), protein (6.91%), and fibre (6.43%). This Thai strain is also low in fat content (1.70%). In general, wild mushrooms are protein-rich and low in fat content compared to cultivated mushrooms. Cultivated mushrooms generally contain 19-35% protein [15]. According to Sanmee et al. [16], the protein content of some Thai wild mushrooms was between 14 and 24.2%. The protein content of other wild mushrooms also varied ranging from % for European [17] and % for Mexican mushrooms [18]. It is understood that the protein content (as well as other nutritional values) are affected by a number of factors, such as the type of mushrooms, the stage of development, the part sampled, level of nitrogen available and the location [17, 19, 20]. Figure 2. Microscopic features of L. sulphureus strain MFLUCC a. Mycelium appearance culture on PDA media was incubated at 30 o C for 14days. b. Thamal generative hyphae. c. Thamal skeletal hyphae. d. Hymenium of basidia. Scale bar: a =1 cm, b =10 μm, c d =5 μm.

4 768 Chiang Mai J. Sci. 2014; 41(4) Table 1. Chemical composition (% dried weight) of L. sulphureus strain MFLUCC Chemical compositions Amount Ash 2.06 ± 0.81 Moisture ± 0.08 Fat 1.70 ± 0.12 Protein 6.91 ± 0.43 Fibre 6.43 ± 0.19 Carbohydrate ± 0.77 Data shown are means and standard deviations of triplicate determinations. 3.3 Mineral Content Mineral concentrations of wild L. sulphureus were investigated and the data are given in Table 2. For Thai L. sulphureus, the most abundant element was found to be Na, followed by Ca, Fe, Zn, and Mg. Manganese and copper were found at low concentrations whereas potassium is not found in this mushroom sample (Table 2). Table 2. Total elemental compositions (mg/kg dw) of L. sulphureus strain MFLUCC Minerals Concentrations Fe 2.28 ± 0.03 Zn 1.20 Mn 0.35 ± 0.02 Cu 0.14± 0.01 Na ± 0.12 Ca 2.59 ± 0.01 Mg 1.09 K ND Data shown are mean values of triplicate determinations; dw, dry weight; ND, Not detectable. Several publications deal with trace element contents in wild mushrooms [16, 21, 22]. The mineral profiles of mushrooms vary and, similar to the proximate analysis data, this variation can be caused by various environmental factors including soil content, growth substrate, and climate [19, 20]. In general, the mean element content across all fungi were in the order Fe>Zn>Mn>Cu>B>Se [16]. A 20- fold difference in Fe and Se concentrations has been reported in some wild edible fungi [16, 23]. In Thailand, the mineral content of some Thai wild mushrooms is reported [16]. Of all elements determined in this study, there are only Ca and Mg that are found in similar content. 3. CONCLUSIONS Proximate and mineral contents of mushrooms are important and useful in food industry as they can be used as a reference for food compositional data [17]. Our study reveals the proximate and mineral content of Thai L. sulphureus for which there has been no report. This mushroom is edible, and thus this data is important and can be used to indicate its nutritive quality. ACKNOWLEDGEMENTS This work was financially supported by the Thailand Research Fund grant (No. BRG ), and Mae Fah Luang University. REFERENCES [1] Ryvarden L. and Gilbertson R.L., European polypores. Part 1, Syn. Fung., 1993; 6: [2] Banik, M.T., Burdsall H.H. and Volk T.J., Identification of groups within Laetiporus sulphureus in the United States based on RFLP analysis of the nuclear ribosomal, Folia Cryptog. Estonica, fasc., 1998; 33: [3] Banik, M.T., Lindner D.L., Ota Y. and Hattori T., Relationships among North America and Japanese Laetiporus isolates inferred from molecular phylogenetics

5 Chiang Mai J. Sci. 2014; 41(4) 769 and single-spore incompatibility reactions, Mycologia, 2010; 102: [4] Gilbertson R.L. and Ryvarden L., North American Polypores. Fungiflora, Oslo, Norway, [5] Imazeki R., Otani Y. and Hongo T., Fungi in Japan (in Japanese), Tokyo, Yama-kei, [6] Zhang M., Cui S.W., Cheung P.C.K. and Wang Q., Antitumor polysaccharides from mushrooms: A review on their isolation process, structural characterisrics and antitumor activity, Trends Food Sci. Tech., 2007; 18: [7] Davoli P., Mucci A., Schenetti L. and Weber R.W.S., Laetiporic acids, a family of noncarotenoid polyene pigments from fruitbodies and liquid cultures of Laetiporus sulphureus (Polyporales, Fungi), Phytochemistry, 2005; 66: [8] Olennikov D.N., Agafonova S.V., Borovskii G.B., Penzina T.A. and Rokhin A.V., Alkali-soluble polysaccharides of Laetiporus Sulphureus (Bull.: Fr.) Murr fruit bodies, Appl. Biochem. Microbiolol., 2009; 45: [9] Agafonova S.V., Olennikov D.N., Borovskii G.B. and Penzina T.A., Chemical composition of fruiting bodies from two strains of Laetiporus sulphureus, Chem. Natural Comp., 2007; 43: [10] Wiater A., Pleszczynska M., Szczodrak J. and Janusz G., Comparative studies on the induction of Trichoderma harzianum Mutanase by α-(1!3)-glucan-rich fruiting bodies and mycelia of Laetiporus sulphureus, Int. J. Mol. Sci., 2012; 13: [11] AOAC Association of Official Analysis Chemistry, 13 th Ed., Official Methods of Analysis of AOAC international, Washington, DC, [12] Fujihara S., Kasuga A., Aoyagi Y. and Sugahara T., Nitrogen-to-Protein Conversion Factors for Some Common Edible Mushrooms, J. Food Sci., 1995; 60: [13] Handoyo T., Maeda T., Urisu A., Adachi T. and Morita N., Hypoallergenic buckwheat flour preparation by Rhizopus oligosporus and its application to soba noodle, Food Res. Int., 2006; 39: [14] Ota Y., Hattori T., Banik M.T., Hagedorn G., Sotome K., Tokuda S. and Yasuhisa A.B.E., The genus Laetiporus (Basidiomycota, Polyporales) in East Asia, Mycological Res.., 2009; 113: [15] Chang S.T. and Buswell J.A., Mushroom nutriceuticals, World J. Microbiol. Biotechnol., 1996; 12: [16] Sanmee R., Dell B., Lumyong P., Izumori K. and Lumyong S., Nutritive value of popular wild edible mushrooms from northern Thailand, Food Chem., 2003; 82: [17] Kalac P., Chemical composition and nutritional value of European species of wild growing mushroom: A review, Food Chem., 2009; 113: [18] Guzman M.F.L., Silva I. and Lopez M.G., Proximate chemical composition, free amino acid contents, and free fatty acid contents of some wild edible mushrooms from Queretaro, Mexico, Food Chem., 1997; 45: [19] Colak A., Faiz O. and Sesli E., Nutritional composition of some wild edible mushroom, Turk J Biochem., 2009; 34: [20] Ogbe A.O. and Obeka A.D., Proximate, mineral and anti-nutrient composition of wild Ganoderma lucidum: implication on its utilization in poultry production, Iranian J. Appl. Ani. Sci., 2013; 3:

6 770 Chiang Mai J. Sci. 2014; 41(4) [21] Genccelep H., Uzun Y., Tuncturk Y. and Demirel K., Determination of mineral contents of wild-grown edible mushrooms, Food Chem., 2009; 113: [22] Mendil D., Uluozlu O.D., Hasdemir E. and Caglar A., Determination of trace elements on some wild edible mushroom samples from Kastamonu, Turkey, J. Agric. Food Chem., 2004; 88: [23] Quinche J.P., Les teneurs en selenium de 95 especes de champignons superieurs et de quelques terre, Schweiz Landw. For., 1983; 22:

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