Introduction

Mushrooms have become attractive as a functional food and as a source for the development of drugs and nutraceuticals [1]. Edible mushrooms are the fleshy and edible fruit bodies of several species of macrofungi. Edibility may be defined by criteria that include absence of poisonous effects on humans and desirable taste and aroma [2,3]. Edible mushrooms are consumed by humans as comestibles for their nutritional value and they are occasionally consumed for their supposed medicinal value. Mushrooms consumed by those practicing folk medicine are known as medicinal mushrooms [4].

Medicinal mushrooms are thought to be treatments for diseases, yet remain unconfirmed in mainstream science and medicine, and so are not approved as drugs or medical treatments [5].

Preliminary research has shown some medicinal mushroom isolates to have cardiovascular, anticancer, antiviral, antibacterial, antiparasitic, anti-inflammatory, and antidiabetic properties [6,7]. Currently, several extracts have widespread use in Japan, Korea and China, as potential adjuvants to radiation treatments and chemotherapy [5,8]. Major medicinal properties attributed to mushrooms include anticancer, antibiotic, antiviral activities, immune response stimulating effects and blood lipid lowering effects [9]. Both fruiting body and mycelium of different mushrooms contain different compounds such as terpenoids, steroids, polyphenol, polyketides, polyglucan, flavonoids, alkaloids, polysaccharides and dietary fibers which exert several pharmacological activities [10]. They are the rich source of antioxidants, antibiotics and antineoplastic activity [11].

The history of mushroom cultivation is not so long in Bangladesh; however, mushroom consumption is increasing rapidly in this country due to cheap source of dietary protein, carbohydrate, vitamins and minerals. For the medicinal and nutritional value, several species of mushroom are being cultivated in Bangladesh [12]. These are reishi, enoki, oyster, shiitake, shimeji, milky, beech and nameko etc. [13].

Hypsizygus tessulatus which is commonly known as Shimeji mushroom contains glucans, niacin, vitamin B and D. Vitamin B aids in immunity and weight loss, while vitamin D is deemed to be effective against osteoporosis and anti-aging [14]. The previous name of this mushroom was Hypsizygus marmoreus and it also contain different biologically active compounds like polysaccharides, l-ergothioneine, sterols, ergosterol - provitamin D2 which have different medicinal uses [15-17].

Pleurotus ostreatus, the oyster mushroom, is a common edible mushroom. The oyster mushroom may be considered a medicinal mushroom, since it contains statins such as lovastatin which work to reduce cholesterol [18].

Lentinula edodes known as Shiitake is an edible mushroom native to East Asia, which is cultivated and consumed in many Asian countries. It is considered a medicinal mushroom in some forms of traditional medicine [19]. Studies there indicate prolonged survival and improved quality of life when gastric cancer patients with unrespectable or recurrent diseases are treated with lentinan in combination with other chemotherapies [20].

The aim of this study was to evaluate the antibacterial, cytotoxic and antioxidant properties of Hypsizygus tessulatus, Lentinula edodes and Pleurotus ostreatus different extract both from submerged culture and mycelia mat.

Materials and method

Mushroom samples

Samples of P. ostreatus, Hypsizygus tessulatus, Lentinula edodes were collected which were cultivated and sold as edible mushrooms from Chittagong, Bangladesh. Identification was done by comparing their morphological, anatomical and physiological characteristics and monographs with descriptions given in the manual [21]. Then mushrooms were air-dried in a liophylizator before analysis. All the specimens were deposited at the herbarium of mycology laboratory, Department of Microbiology, University of Chittagong, Chittagong, Bangladesh. The fruiting bodies, carefully removed from the hyphae were weighed then dried at 40°C for 24 h. The dried fruiting body samples were weighed and ground into powder prior to extraction.

Preparation of methanolic extracts

Preparation of methanolic extracts of mushrooms was done based on procedures described by Barros et al. [22] with some modifications. A fine-dried mushroom powder sample (100 g) was extracted by stirring with 100 ml of methanol at 25°C at 150 rpm for 24 hours and filtered through Whatman no. 4 paper. The residue was then extracted with two additional 100-ml portions of methanol. The combined methanolic extracts were evaporated at 40°C to dryness. The organic solvent in the extracts was removed by a rotary evaporator. For the entire analysis, compounds of extract were dissolved in dimethylsulfoxide (DMSO), and filter-sterilization was done through a 0.22-μm membrane filter. Extracts were kept in the dark at 4°C for not more than 1 week prior to use.

Determination of bioactive components

Phenolic compounds in the mushroom methanolic extracts were measured by a colorimetric assay, wherein 1 ml of sample was mixed with 1 ml of Folin and Ciocalteu’s phenol reagent. After 3 minutes, 1 ml of saturated sodium carbonate solution was added to the mixture and adjusted to 10 ml with distilled water [22]. The reaction was kept in the dark for 90 minutes, after which the absorbance was measured spectrophotometrically at 765 nm. Gallic acid was used to calculate the standard curve (0.01-0.4 mM). The mean values of results were expressed as milligrams of gallic acid equivalents (GAEs) per gram of extract.

Flavonoid concentrations were estimated [23], where in methanolic extract solution (1 ml) was diluted with 4.3 ml of 80% aqueous ethanol, and 0.1 ml of 10% aluminum nitrate and 0.1 ml of 1 M aqueous potassium acetate were added. After 40 minutes at room temperature, the solution was mixed well, and the intensity of the pink color was measured spectrophotometrically (Model - UV-1601 SHIMADZU) at 415 nm. Quercetin was used to calculate the standard curve of total flavonoid concentration absorbance = 0.002108 μg quercetin – 0.01089 (R2: 0.9999).

Ascorbic acid was determined [22], where in methanolic extract (100 mg) was extracted with 10 ml of 1% metaphosphoric acid for 45 minutes at room temperature and filtered through Whatman no, 4 filter paper. The filtrate (1 ml) was mixed with 9 ml of 2, 6-dichloroindophenol (0.025%), and the absorbance was measured within 30 minutes at 515 nm against a blank. Content of ascorbic acid was calculated on the basis of the calibration curve of authentic L-ascorbic acid (0.020-0.12 mg/mL). The results were expressed as milligrams of ascorbic acid per milliliter of extract. All the above estimations of bioactive compounds were carried out in triplicate and means were plotted.

Scavenging activity on DPPH for antioxidant assay

The antioxidant activity of the extracts on the stable radical 1, 1-diphenyl;-2-picrylhydrazyl (DPPH) was determined by the method developed by Feresin et al. (2002) [24]. The 0.1 ml of mushroom ethanol extract, at various concentrations was added to 3 ml of a 0.004% methanol solution of DPPH and was allowed to stand for 30 min for the reaction to occur. The absorbance of the resulting solution was measured at 517 nm from this values the corresponding percentage of inhibitions were calculated by using the following equation:

$$ \mathrm{I}\ \%=\left[\left({\mathrm{A}}_{\mathrm{Blank}}-{\mathrm{A}}_{\mathrm{sample}}\right)/{\mathrm{A}}_{\mathrm{Blank}}\right]\times 100, $$

Where, Ablank is the absorbance of the control reaction (containing all reagents except the test sample) and Asample is the absorbance of sample/standard.

Extract concentration providing 50% inhibition (IC50) was calculated from the graph plotted I% versus concentration curve. The free radical scavenging activity was measured for different concentrations of sample and compared with standard (Ascorbic acid).

Determination of antimicrobial efficacy

Microbial test organisms

The bacterial test organisms used were Staphylococcus aureus (ATCC 25923), Bacillus subtilis (ATCC 6633) as gram-positive species and Escherichia coli (ATCC 25922), Klebsiella pneumonia (ATCC 13883), Pseudomonas aeruginosa (ATCC 27853) and Salmonella typhi (ATCC 33459) as gram-negative species grown in Mueller Hinton agar at 37°C for 24 hours (Merck). Fungal species was unicellular Candida albicans (ATCC 60192) and Saccharomyces cerevisiae (ATCC 9763) grown in potato dextrose agar (Hi Media) at ambient temperature for 72 hours. The bacterial isolates were multidrug resistant determined by disc diffusion assay according to Iwalokun et al. [25].

Antibacterial and antifungal screening

Antimicrobial activity of methanolic extract of mushrooms was determined by the agar well diffusion method [26], with slight modification to suit the conditions of this experiment. Briefly, the methanol extracts were dissolved in 3% dimethylsulfoxide (DMSO) to a final concentration of 10 mg/ml, and filter sterilized through 0.45-μm membrane filter. Small wells (6 mm in diameter) were made in the agar plates by sterile cork borer. One hundred microliters of the extract of each isolate of mushrooms was loaded into the different wells. An overnight culture of each microbial isolate was emulsified with nutrient broth to a turbidity that was equivalent to 0.5 McFarland (108 cfu/ml). In order to determine the antimicrobial efficacy of the fractions, aliquot of test culture (100 μl) was evenly spread over the surface of the solidified agar. Bacteria were cultured on Mueller Hinton agar; and fungi on potato dextrose agar. Ciprofloxacin (5 μg/well) for bacteria, fluconazole (5 μg/well) for fungi were used as positive control and DMSO was used as negative control for test microorganisms. All the preloaded plates with respective extract and test organism were incubated at 37°C, for 24 hours for bacteria and at 27°C. 48 hours for fungi. After incubation period, zone of inhibition was measured in millimeters. All the tests were carried out in triplicate and their means recorded.

Minimum inhibitory concentration (MIC)

The standard agar dilution protocol with doubling dilution was used. The extract was incorporated into nutrient agar at concentrations ranging from 0.39 mg/ml to 25 mg/ml. A control without the extract was also prepared. 10 μL of each test organisms, previously diluted to 10 CFU/ml, were used to inoculate the plates. These were incubated at 37°C for 24 h in the first instance and for another 24 h before the growth was observed and recorded. The minimum inhibitory concentrations (MICs) of the extract for each test microorganism were considered the agar plate with the lowest concentrations without growth [27].

Results

Antimicrobial

The present study has revealed the antibacterial and antifungal activity of mushroom extract. The results of antibacterial activity were presented in Table 1. All the mushrooms also revealed antimicrobial activity showing different MICs for each microorganism (Table 2).

Table 1 Preliminary antimicrobial testing of mushroom extracts through determination of zone of inhibition (mm ± SD)*
Table 2 Minimum inhibitory concentrations determinations of extracts

Antioxidental

In case of antioxidant screening of ethanol extract of Hypsizygus tessulatus powdered mycelium has shown in Table 3. The IC50 value, defined as the concentration of antioxidant required for 50% scavenging of DPPH radicals in this specified time period, is a parameter widely used to measure antioxidant activity; a smaller IC50 value corresponds to a higher antioxidant activity of the plant extract. IC50 value of the ethanol extract was 105.0 μg ml−1. These values state that H. tessulatus has moderate DPPH scavenging activity compared to Ascorbic acid standard.

Table 3 Free radical scavenging activity (IC 50 μg/ml)

Bioactive compounds

Table 4 showed phenol, flavonoid and ascorbic acid concentrations of the isolates; total phenols were the major bioactive component found in extracts of isolates expressed as mg of GAE per gram of fruit body, which ranged from 10.66 ± 0.52 to 5.65 ± 0.05 mg/ml.

Table 4 Bioactive compound contents of the wild edible mushrooms (Mean ± Standard Deviation; n = 3)

Discussion

Antimicrobial assay

All the mushrooms used in this study were found to exhibit various degrees of antimicrobial effects against the tested microorganisms. The zone of inhibition exhibited more than 10 millimeters was considered as highly active for extracts. P. ostreatus has a broad-spectrum antibacterial and antifungal activity. Similar antimicrobial potentials have been observed in the culture extracts of Irpex lacteus (Rosa et al., 2003), Agrocybe sp. (Kavanagh et al., 1950; Mavoungou et al., 1987) [28-30]. The best in-vitro antibacterial activity was by L. edodes (17 ± 0.2mm) followed by Pleurotus ostreatus and Hypsizigus tessulatus against Bacillus subtilis. Lentinula edodes also showed best antimicrobial activity than Pleurotus ostreatus and Hypsizigus tessulatus. This antimicrobial efficacy of Lentinula edodes was similar of the study of Kuznetsov et al., 2005 [31].

Ishikawa et al. (2001), reported data similar to the results obtained in this work, showing antibacterial action of L. edodes against B. cereus, S. aureus and E.coli [32]. Komemushi et al. (1996) also reported that L. edodes inhibited growth of Gram positive and Gram negative bacteria [33]. The revealed information regarding strong antimicrobial activity of Hypsizigus tessulatus against pathogenic isolates has similarity of the study of Hearst et al., 2009 [34].

Candida albicans and Saccharomyces cerevisiae was found to be very susceptible when compared to positive controls. Pseudomonas aeruginosa showed more resistant to mushrooms extract comparatively than other isolates.

Among the bacterial isolates, The MIC of all mushrooms extract was high for Pseudomonas aeruginosa. The MICs of Lentinula edodes against all isolates were low comparatively others. The Lowest MIC was observed for Candida albicans and Saccharomyces cerevisiae against Lentinula edodes. This quite similar result was also observed by Barros et al., 2006 [35].

Antioxidantal

In the DPPH assay, the antioxidants are able to reduce the stable DPPH radical (purple) to the non-radical form DPPH-H (yellow). The DPPH scavenging activities of antioxidants are attributed to their hydrogen donating abilities. All the mushroom extract showed the antioxidant activity. But the differentiation between the extract is too close. Lentinula edodes showed the highest antioxidant activity. This result is quite similar by Emanuel Vamanu, 2012 [36].

The result for antioxidant activity of P. ostreatus is also quite similar by Arbaayah HH And Umi Kalsom Y, 2013 [37].

Bioactive components

Flavonoids, which are also phenolic compounds, were not detected in P. ostreatus. Our observation agrees with findings of Mattila et al., 2001 [38] and according to USDA, mushrooms are regarded as non-sources of flavonoids. Higher contents of bioactive compounds were found in Lentinula edodes. This statement is too similar to the experiment by Calhelha et al., 2007 [22]. The amount of phenolic contents and Flavonoids from H. tessulatus was moderate and similar by the study of Monira et al., 2012 [39].

Conclusion

The present investigation can conclude that the methanolic extract of 3 edible mushrooms showed biopharmaceutical potentiality. However whether such extracts will act as effective therapeutic agents remain to be investigated, the identification of the bioactive compounds and study of mechanisms of actions are necessary prior to application.