Abstract

Lentinan, 1152 Dalton β-D-glucan found in Shiitake Mushroom (Lentinus edodes), has been claimed to have anticancer and immunomodulatory activity. Several extraction methods have been used by researchers to isolate Lentinan including hot water and alkaline solution (1.25 M NaOH). In this study, hot water and alkaline solution (1.25 M NaOH) were used to extract the Lentinan-like β-D-glucan (1151 Dalton) from Tiger’s Milk Mushroom, Termite Mushroom, and selected local market mushrooms. The isolated Lentinan-like β-D-glucan from both hot water and alkaline solution was analyzed by LCMS-QTOF. Commercial Lentinan standard from Lentinus edodes was used as a reference. The results showed significant differences on chromatogram patterns of Lentinan-like β-D-glucan between both extracts. The peak of Lentinan-like β-D-glucan was only found in isolated polysaccharide glucan of hot water extracts. The isolated polysaccharide glucans from Tiger’s Milk Mushroom and Termite Mushroom were found to have μg/mg and μg/mg Lentinan-like β-D-glucan. Button Mushroom, Shiitake Mushroom, and Oyster Mushroom showed the presence of Lentinan-like β-D-glucan at μg/mg, , and μg/mg, respectively.

1. Introduction

Information on Tiger’s Milk Mushroom and Termite Mushroom is still scanty and poor. Tiger’s Milk Mushroom (Lignosus rhinocerus) has been found by Forest Research Institute of Malaysia (FRIM) as the most important medicinal mushroom used by the native [1]. This mushroom has been claimed to have therapeutic effects such as in treating cough, asthma, cancer, food poisoning, and as a general tonic [2]. While Termite Mushroom (Termitomyces heimii) is a wild seasonal mushroom that grows symbiotically with termite especially in rainy season. This mushroom was claimed to have very delicious taste and has extensively been used as human food [3]. It also has been used to treat lower blood pressure, rheumatism, kwashiorkor, obesity, and diarrhea [4].

A lot of potential bioactive compounds that are very useful for therapeutic purposes have been found in mushrooms including polysaccharides, polysaccharide peptide (protein complexes), proteoglycans, proteins, and triterpenoids [57]. β-D-glucan, a derivative of polysaccharide found in mushroom, has been recognized as a biological response modifier (BRM) since it possesses potent immune modulatory and anticancer activities [8, 9]. The compound also has ability to improve human resistance against bacteria and viruses [10].

Lentinan is one of the most active 1,3/1,6-β-D-glucans found in Shiitake Mushroom (Lentinus edodes) that possesses immune modulator and anticancer activities. It is a branched-type β-D-glucan with molecular weight of 1152 Dalton [10, 11]. Lentinan has been widely used as an alternative medicine for potent anticancer and antiviral treatments and also has been consumed as dietary supplements [8, 12]. Hot water, alkaline solution, and polyethylene glycol were types of solvents that have been used in the isolation of Lentinan from mushrooms [12].

In this study, the isolation of Lentinan-like β-D-glucan from Tiger’s Milk Mushroom (Lignosus rhinocerus), Termite Mushroom (Termitomyces heimii), and selected local market mushrooms, namely, Button Mushroom (Agaricus bisporus), Shiitake Mushroom (Lentinus edodes), and Oyster Mushroom (Pleurotus ostreatus), has been done by using hot water and alkaline solution (1.25 M NaOH). The Lentinan-like β-D-glucan content was analyzed through mass spectrometry approach by using Liquid Chromatography Mass Spectrometry-Quadrupole Time of Flight (LCMS-QTOF).

2. Materials and Methods

2.1. Chemicals

Lentinan standard of Lentinus edodes was purchased from CarboMer Incorporation. Megazyme reagent kit was purchased from Merck. HPLC grade solvents were purchased from Fisher Scientific.

2.2. Plant Materials

Tiger’s Milk Mushroom (Lignosus rhinoceros) and Termite Mushroom (Termitomyces heimii) were collected from Pahang and Negeri Sembilan, respectively. Button Mushroom (Agaricus bisporus), Shiitake Mushroom (Lentinus edodes), and Oyster Mushroom (Pleurotus ostreatus) were obtained from Selangor Hypermarket.

2.3. Samples Preparation

All the collected mushrooms were cleaned under running tap water. The cap area was cut into small pieces and oven-dried at 40°C. The dried samples were homogenized with Cyclone Mill and kept at −20°C until further use.

2.4. Determination of Total β-D-Glucan Content

β-D-Glucan content was detected by measuring the total polysaccharide glucan and α-D-glucan content as per Megazyme assay method (Figure 1). 100 mg of dried powder fruit body of each sample was heated in 1.5 mL of concentrated hydrochloric acid (37%; 10 N) at 30°C for 45 minutes. 10 mL of water was added and the mixture was boiled at 100°C for 2 hours. 10 mL of 2 M potassium hydroxide was added once the mixture cooled, followed by addition of 0.2 M sodium acetate buffer (pH 5.0) up to 100 mL. The solution was centrifuged at 1,500 g for 10 minutes. 0.1 mL of the supernatant was taken out and heated with 0.1 mL of highly purified enzyme A (exo-1,3-β-glucanase + β-glucosidase) at 40°C for 60 minutes to obtain the total polysaccharide glucan. In separated process, α-D-glucan was extracted by soaking the mushroom fruit body for 20 minutes in 2 mL KOH (2 N) located in ice water bath. 8 mL of 1.2 M sodium acetate buffer (pH 3.8) and 0.2 mL of Enzyme B (amyloglucosidase + invertase) were added immediately and incubated at 40°C for 30 minutes. The solution was centrifuged at 1500 g for 10 minutes. 0.1 mL of supernatant was mixed into 0.1 mL of sodium acetate buffer (200 mM, pH 5.0) to obtain α-D-glucan.

Both total polysaccharide glucan and α-D-glucan were heated, respectively, in 3 mL of GOPOD reagent at 40°C for 20 minutes. The concentration of total polysaccharide glucan and α-D-glucan was determined by UV-visible mass spectrometry at 510 nm against reagent blank (0.2 mL of 0.2 M sodium acetate).

*Reagent blank and D-glucose standard (0.1 mL of 1 mg/mL D-glucose standard + 0.1 mL of 0.2 M sodium acetate buffer) were also heated with 3 mL of GOPOD at 40°C for 20 minutes:

2.5. Determination of Lentinan-Like β-D-Glucan
2.5.1. Isolation of Polysaccharide Glucan

Polysaccharide glucan was isolated by hot water and alkaline solution (1.25 M Sodium hydroxide), respectively (Figure 2). 300 mg of dried fruit body powder was extracted twice with 10 mL of distilled water at 100°C for one hour. Separately, the same amount of dried fruit body powder was extracted twice with 10 mL of 1.25 M NaOH at 60°C for one hour. Alkaline extract was then neutralized by hydrochloric acid (HCl). Both hot water and alkaline extracts were centrifuged at 10,000 rpm for 15 minutes. The supernatants from both extracts were dialyzed against distilled water in shaking condition for overnight to remove low molecular weight substances. Two volumes of absolute ethanol were added to the hot water and alkaline extracts. Both extracts were left overnight at 4°C for complete precipitation. The solid fractions known as polysaccharide glucan were collected by centrifugation at 10000 rpm for 15 minutes and oven-dried at 60°C. The weight of dried polysaccharide glucan was recorded.

2.5.2. LCMS-QTOF Analysis of Lentinan-Like β-D-Glucan

Sample Preparation. 5 mg of isolated polysaccharide glucan from hot water and alkaline extracts was dissolved with 0.5 mL and 1.0 mL of distilled water, respectively, for four hours at 90°C. The solutions were centrifuged at 13,000 rpm for 10 minutes. The supernatants were filtered through 0.45 μm syringe filter into separated HPLC vials.

Determination of Lentinan-Like β-D-Glucans. Analysis was performed by using an Agilent 1200 series Rapid Resolution Liquid Chromatography (RRLC) equipped with autosampler and diode array detection (DAD) system. An Agilent 6530 Accurate Mass QTOF was used to obtain the MS and MS/MS data. The mobile phases used were highly purified water + 0.1% formic acid (A) and acetonitrile+0.1% formic acid (B). Column used was 4.6 mm × 100 mm Thermo-Carbon column. The flow rate was set up at 0.6 mL/min with 22 minutes total run time. The column temperature was at 40°C. The prepared samples were placed into the LCMS autosampler. The injection volume of sample was 10 μL. The samples were run at gradient 5% B (0−0.5 min); 30% B (0.5−13 min); and 95% B (13–22.0 min). Analysis was performed in negative ion mode with the following settings:- capillary voltage: 3500 V; nozzle voltage: 1000 V; fragmentor voltage: 175 V; nebulizer pressure (N2): 35 psi; drying gas: 5 L/min at 350°C, and sheath gas: 11 L/min at 350°C. The mass range was at 110–2000 m/z.

Lentinan standard was prepared at 1 mg/mL by dissolving in distilled water at 90°C for 4 hours. Fragmentation pattern of molecular mass, elution time, and molecular weight of the Lentinan standard were used to analyze the presence of targeted compound. The profile patterns of total ion chromatogram (TIC) and the extracted ion chromatogram (EIC) of the extracts were recorded. A standard calibration curve of Lentinan was built to determine the Lentinan-like β-D-glucan content in the 5 types of mushrooms.

3. Results and Discussion

3.1. Determination of Total β-D-Glucan Content

The concentration of β-D-glucan in Tiger’s Milk Mushroom (Lignosus rhinoceros), Termite Mushroom (Termitomyces heimii), Button Mushroom (Agaricus bisporus), Shiitake Mushroom (Lentinus edodes), and Oyster Mushroom (Pleurotus ostreatus) was determined by using UV-Visible Spectrophotometer. Figure 3 showed the results of total β-D-glucan contents (% w/w) in the five selected mushrooms: From the graph, it is shown that more than 50% of total polysaccharide glucan content in the mushroom fruit bodies was comprised of β-D-glucan. Oyster Mushroom showed the highest β-D-glucan content with 41.357% w/w as compared to other four mushrooms, followed by Tiger’s Milk Mushroom and Shiitake Mushroom with 33.950% w/w and 24.183% w/w β-D-glucan, respectively. Termite Mushroom was found to have 21.167% w/w β-D-glucan. Button Mushroom showed the least β-D-glucan content with 6.077% w/w.

3.2. LC-QTOF Analysis of Lentinan-Like β-D-Glucan

As shown in Figure 4, more yield of isolated polysaccharide glucan is obtained through 1.25 M NaOH as compared to the hot water extract. Hot water extraction is the normal procedure in the isolation of polysaccharide glucan. However, alkaline solution has been determined to have ability in improving the isolation yields of the compound [1214]. The ratio of polysaccharide glucan in alkaline extract to the hot water extract was 14 : 1 for Tiger’s Milk Mushroom, 11 : 4 for Termite Mushroom, 16 : 6 for Oyster Mushroom, 13 : 8 for Shiitake Mushroom, and 5 : 0.4 for Button Mushroom.

LQMS-TOF was used to detect the presence of Lentinan-like β-D-glucan in the hot water and alkaline extracts. A commercial Lentinan standard isolated from Lentinus edodes was used in this analysis. The data of molecular weight, retention time, and fragmentation pattern of the Lentinan standard obtained by negative mode MSMS were used as reference (Figure 5).

The results of total ion chromatogram (TIC) of polysaccharide glucan isolated by hot water and alkaline solution were totally different (Figure 6). From the extracted ion chromatogram (EIC) data of hot water extract there was a peak eluted at minutes 9. Molecular weight analysis on that peak exposed the presence of 1152 Dalton of β-D-glucan (Figure 7). Comparison of the fragmentation patterns between Lentinan standard (Figure 5) and the 1152 Dalton β-D-glucan (which is not shown here) showed that the Lentinan-like β-D-glucan brought the same ion fragments as Lentinan of Lentinus edodes. These suggested the presence of Lentinan-like β-D-glucan in all the five mushrooms. However, the alkaline solution extract expressed no peak eluted at that specific time. This was due to the structure alteration of β-D-glucan as well as Lentinan in alkaline solution as β-D-glucan structure could undergo conformational change when dissolved in different solvents [7, 12].

3.3. Determination of Lentinan-Like β-D-Glucan Content

The concentrations of Lentinan-like β-D-glucan in the isolated polysaccharide glucan of hot water extracts were determined by using Lentinan standard calibration curve. As shown in Table 1, the isolated polysaccharide glucan of Tiger’s Milk Mushroom and Termite Mushroom was found to have μg/mg and μg/mg Tiger’s Milk Mushroom and Termite Mushroom, respectively. While Button Mushroom contained the highest Lentinan-like β-D-glucan (μg/mg) among the five mushrooms, Shiitake Mushroom and Oyster Mushroom showed μg/mg and μg/mg Lentinan-like β-D-glucan, respectively. By taking into account the total amount of dried isolated polysaccharide glucan obtained (as reported in Figure 1), the Lentinan-like β-D-glucan content in the whole fruit body of Tiger’s Milk Mushroom and Termite Mushroom was   and μg/mg, respectively. Button Mushroom was found to have μg/mg Lentinan-like β-D-glucan in its fruit body. The fruit bodies of Shiitake Mushroom and Oyster Mushroom showed μg/mg and μg/mg Lentinan-like β-D-glucan.

4. Conclusion

Mushroom β-D-glucan has been targeted as an important medicinal agent as it exposes immune modulator and anticancer properties. It has been widely used as alternative medicine and dietary supplement for years. Isolation of this compound by different solutions could affect the yield of the isolated β-D-glucan extract and also its conformational state. Alkaline solution has improved the extract yield of isolated β-D-glucan as compared to the hot water. Nevertheless, it also led to the changes in retention time of the compound as the alteration of conformational state has been occurred. These concluded that different solvents may not only affect the yield of isolated β-D-glucan but also its general structure which might divert their retention time.

Acknowledgments

The authors acknowledge Agro-Biotechnology Institute, Malaysia (ABI), and Ministry of Science, Technology and Innovation (MOSTI), for providing research Grant (08-05-ABI PB030) to support this study. This project was financially supported by ABI R&D Initiative Fund. There is no conflict of interests regarding this study.