Abstracts
Aspergillus sp. NR46F13, isolated from soil via sinigrin-barium sulphate agar technique, was tested for myrosinase production. The fungus degraded glucosinate and produced 3.19 U mL-1 of myrosinase after 48h cultivation. due to the high myrosinase production, this new isolate is a potential candidate for industrial applications.
myrosinase; Aspergillus sp.; sinigrin; glucosinolate; allylisothiocyanate
A linhagem Aspergillus sp. NR46FB, isolada de solo através da técnica do ágar sulfato de bário-sinigrina, foi testada quanto à produção de mirosinase. O fungo degradou completamente o glicosinolato e produziu 3,19 U.mL-1 de mirosinase, após 48 h de cultivo. Devido à alta produção de mirosinase, esse novo isolado é um potente candidato para aplicações industriais.
myrosinase; Aspergillus sp.; sinigrin; glucosinolate; allylisothiocyanate
INDUSTRIAL MICROBIOLOGY
Screening of filamentous fungi for production of myrosinase
Seleção de fungos filamentosos para a produção do mirosinase
Nuansri Rakariyatham*; Bordin Butrindr; Hataichanoke Niamsup; Lalida Shank
Department of Chemistry, Faculty of Science, Chiang Mai University, Chiang Mai, Thailand
ABSTRACT
Aspergillus sp. NR46F13, isolated from soil via sinigrin-barium sulphate agar technique, was tested for myrosinase production. The fungus degraded glucosinate and produced 3.19 U mL-1 of myrosinase after 48h cultivation. due to the high myrosinase production, this new isolate is a potential candidate for industrial applications.
Key words: myrosinase, Aspergillus sp., sinigrin, glucosinolate, allylisothiocyanate
RESUMO
A linhagem Aspergillus sp. NR46FB, isolada de solo através da técnica do ágar sulfato de bário-sinigrina, foi testada quanto à produção de mirosinase. O fungo degradou completamente o glicosinolato e produziu 3,19 U.mL-1 de mirosinase, após 48 h de cultivo. Devido à alta produção de mirosinase, esse novo isolado é um potente candidato para aplicações industriais.
Palavras-chaves: myrosinase, Aspergillus sp., sinigrin, glucosinolate, allylisothiocyanate
INTRODUCTION
Glucosinolates are amino acid derived from natural plant products containing thioglucose and sulfate moieties. They are found in Brassicales, mainly in Brassicaceae (Cruciferae), and in several other families of dicotyledonous angiosperms. Upon tissue disruption, glucosinolates are hydrolyzed by myrosinase (b-thioglucoside glucohydrolase EC 3.2.3.1), to unstable intermediates that, as dictated by chemical conditions, spontaneously rearrange to isothiocyanates, thiocyanates or nitriles (1,8). Glucosinolate breakdown products are proposed to act as allelochemicals and play a role in plant defenses against herbivores, pets and pathogens (1,8). As components of food for humans and feed for livestock, the biological activities of glucosinolate hydrolysis products have generated considerable toxicological and pharmacological interest. Natural isothiocyanates derived from aromatic and aliphatic glucosinolates are effective chemoprotective agents that block chemical carcinogenesis and prevent several types of cancer in rodent model (13).
Myrosinase and glucosinolates have been studied extensively. Many reports have described the isolation and characterization of myrosinase, especially from mustard and oilseed rape. A significant effort has been put into the recent cloning of plant myrosinase genes (2). Myrosinase was not only found in plants but also in microorganisms. Over the past 40 years a number of microorganisms including bacteria and fungi have been reported for their glucosinolate-degradation properties. Most works have been concentrated on characterization of glucosinolate degradation by intact microbial cells (3,6,9,12) and several reports described the selection of Aspergillus sp. for myrosinase production (4,10,12). The study of myrosinase, therefore, is significant for both biological and biotechnological aspects of food and feed industries.
Our research unit has been interested in studying myrosinase from Aspergillus sp. in many aspects including biodegradation in liquid and solid cultures (9,10). A new technique for detection of microorganisms that produces myrosinase, using sinigrin-barium agar plates, was developed (11). To our knowledge no investigation has been carried out on screening of microorganisms for improved myrosinase production.
In this paper, we describe the screening and characterization of a new isolate for myrosinase production.
MATERIALS AND METHODS
One hundred fifty soil samples, potentially containing glucosinolate-degrading microorganisms, were collected from Lamphun province, Thailand. Soil samples were bottled in sterile vials. One gram of each sample was suspended in 10 mL sterile distilled water. After shaking at room temperature (25ºC), the samples were let to settle at room temperature for 2-3 hr. Then, 100 µL of the supernatant was spread onto nutrient agar (2 g beef extract, 2 g tryptone and 1.5 g agar in 100 mL distilled water) and potato dextrose agar (3.9 g potato dextrose agar in 100 mL distilled water) plates.
Re-plating was made until pure cultures were obtained. The selected strains were inoculated onto sinigrin-barium agar plates (11), arid incubated at 30ºC. Growth was observed daily, and the strains that grew on sinigrin-barium agar plates were re-plated onto mustard extract agar (10). Incubation was carried out at 30ºC. The plates were observed daily. Each distinct growing colony was picked and then plated onto nutrient agar or potato dextrose agar plates.
Myrosinase production by the selected strains was tested in mustard extract medium in different conditions of pH, incubation time and incubation temperature.
An innoculum, prepared from 1-week-old culture having a concentration of 106 spores mL-1, was transfered to eighteen 125 mL Erlenmeyer flasks containing 25 mL mustard extract medium with different pH values (10 mM glucosinolates in 0.1 M sodium phosphate buffer). Incubation was carried out at 30ºC in a water-bath, shaken at 150 rev min-1. At each time point, a two mycelial samples were harvested and washed. One mycelial sample was used for determination of fungal cell dry weight by washing and drying at 105ºC. A culture filtrate of the other sample was assayed for glucose and glucosinolates contents while fungal cell pellet was disrupted using a mortar. Cell-free extract obtained after centrifugation (12,000 x g, 25 min, 4ºC) was assayed for myrosinase activity. The effect of incubation temperature on myrosinase production was studied at 28 to 40ºC. The myrosinase assay was done according to Sakorn et al., 1999. Protein was determined according to Petroski and Kwolek, 1985. One unit of myrosinase activity was defined as the amount of enzyme that catalyzed the liberation 1 mmol of glucose per minute from sinigrin under the above described conditions.
RESULTS AND DISCUSSION
One hundred fifty soil samples suspected to contain myrosinase-producing microorganisms were collected. One hundred sixty one microorganisms were isolated and tested for myrosinase production. The screening result showed 28 newly isolated strains with positive opaque zone on sinigrin-barium sulphate agar. Myrosinase activity was found in all positive Aspergillus sp. that grew on sinigrin barium sulphate agar.
In this study, most selected strains degraded all glucosinolate in the first 36 h growth period, with more than half of glucosinolate degraded within 18 hr of growth (Fig. 1). On the other hand, Aspergillus sp. NR46F4, NR46F13 and NR46F14 did not completely degrade glucosinolate within the same growth period.
Growth on mustard extracted media was investigated in all selected strains. Aspergilllus sp. grown on mustard extracted medium with no supplement presented relatively high intracellular myrosinase activity. Maximum myrosinase production varied from 3.19 to 1.25 U mL-1,and was higher when to previous reported results: Aspergillus syndowi IFO4284 (0.08 U mL-1) (5), Aspergillus niger AKU3302 (0.088 U mL-1) (4), Aspergillus syndowi QW31c (0.096 U mL-1) (7) and Aspergillus sp. NR-4201 (0.28 U mL-1) (10). Aspergillus sp. NR46F13 presented the highest myrosinase activity (3.19 U mL-1), and cell dry weight (15.67 mg mL-1) within 48 hr of glucosinolate degradation. The highest myrosinase production and the highest fermentation parameters did not coincide with rapid glucosinolate consumption. (Tab. 1)
Optimal conditions for myrosinase production were different in selected strains (pH 6-7, 28-35ºC). Glucosinolate degradation rate was higher than that reported in previous works for Aspergillus sp NR-4201 (9,10) and Aspergillus calvatus (12). The new isolate of Aspergillus sp. presented higher myrosinase production than that reported in previous studies.
A microorganism that presents high myrosinase activity a relatively short time would be more effective for process optimization on an industrial scale, since such organism requires less energy and is less likely to be contaminated. Some of the filamentous fungi tested presented maximum myrosinase activity in 30 to 36 h, however this production was relatively low (Fig. 1). For other strains, (NR46F4, NR46F13 and NR46F14) a long growth period was required for total glucosinolate degradation. Myrosinase production for those strains occurred at 42 hr.
We hereby introduce new myrosinase-overproducing microorganisms, characterized by high levels of enzymatic activity, that also possess ability to grow in the low cost medium. Considering the potential application of these fungi in degradation of glucosinolate-rich wastes from agro industry, and the possibility of producing valuable glucosinolate derived products, further studies are certainly warranted.
In conclusion, a newly isolated myrosinase-overproducing Aspergillus sp. newly has been obtained and characterized as a good enzyme producer, with valuable hydrolysis products. This myrosinase enzyme offers a great potential for industrial applications, such as feed detoxification and enhanced yield of flavor industrial production (allylisothiocyanate production).
ACKNOWLEDGEMENTS
The authors wish to thank the Department of Chemistry, Faculty of Science, Chiang Mai University. This research was financially supported by the Thailand Research Fund (TRF).
Submitted: February 18, 2005; Returned to authors for corrections: May 30, 2005; Approved: July 05, 2005
References
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Publication Dates
-
Publication in this collection
20 Feb 2006 -
Date of issue
Sept 2005
History
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Received
18 Feb 2005 -
Reviewed
30 May 2005 -
Accepted
05 July 2005