Production, partial purification, and characterization of a glucoamylase from Epicoccum nigrum

Q3 Agricultural and Biological Sciences Acta Scientiarum. Biological Sciences Pub Date : 2023-03-22 DOI:10.4025/actascibiolsci.v45i1.61179
D. B. Martim, F. C. Santos, I. Barbosa-Tessmann
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Abstract

Starch processing industries use amylases, accounting for approximately 30% of the world’s enzyme market. Previously, an amylase-producing strain of Epicoccum nigrum was isolated from maize grains. Although E. nigrum amylase production is already reported in the literature, no published data on production optimization or characterization of the produced enzyme exists. The objectives of this work were to improve the amylase production by the E. nigrum PG 16 strain and to purify and characterize the produced enzyme. The E. nigrum PG 16 amylase production best conditions in submerged culture were: inoculum of 4% (v v-1) of a five-days-old stationary culture homogenate, agitation at 100 rpm, 25°C, natural light, 72 hours of incubation, starch as the carbon source, and an initial medium pH of 7.0. A molecular exclusion chromatography profile has shown the production of only one amylase, which was partially purified with ammonium precipitation and dialysis. The enzyme optima pH and temperature are 6.0 and 50°C, respectively. The partially purified enzyme lost its activity when incubated for 30 min in temperatures above 40°C, presenting a T50 of 46.25°C. The KM and Vmax of the partially purified enzyme are 1.72 mg mL-1 of starch and 0.15 mg min-1 of degraded starch, respectively. The ion Ca2+ slightly activated the studied enzyme. The ions Cu2+, Zn2+, and Fe3+ and the detergents SDS and Tween 80 acted as inhibitors of the studied enzyme. The partially purified enzyme released glucose from p-nitrophenyl α-D-glucopyranoside (p-NPG). Glucose was the enzyme’s main product from starch hydrolysis, as evidenced by thin-layer chromatography. The E. nigrum PG 16 studied enzyme is a glucoamylase and represents an alternative for enzymatic starch hydrolysis.
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一种表麸糖淀粉酶的生产、部分纯化和特性研究
淀粉加工工业使用淀粉酶,约占世界酶市场的30%。以前,从玉米籽粒中分离到一株产生淀粉酶的外表皮菌。虽然文献中已经报道了黑乳杆菌淀粉酶的生产,但没有关于生产优化或所生产酶的表征的公开数据存在。本工作的目的是提高E. nigrum PG 16菌株的淀粉酶产量,并纯化和表征所产生的酶。大肠杆菌PG - 16淀粉酶的最佳培养条件为:接种量为4% (v -1),固定培养5 d的匀浆,搅拌100 rpm, 25°C,自然光,培养72小时,淀粉为碳源,初始培养基pH为7.0。分子排斥层析谱图显示,只有一种淀粉酶的生产,这是部分纯化与铵沉淀和透析。酶的最适pH为6.0℃,最适温度为50℃。部分纯化的酶在40℃以上的温度下培养30 min后失去活性,T50为46.25℃。部分纯化酶的KM和Vmax分别为1.72 mg mL-1淀粉和0.15 mg min-1降解淀粉。Ca2+离子略微激活了所研究的酶。Cu2+、Zn2+和Fe3+离子以及去垢剂SDS和Tween 80均为该酶的抑制剂。部分纯化的酶从对硝基苯α- d -葡萄糖吡喃苷(p-NPG)中释放葡萄糖。薄层色谱法证明,葡萄糖是淀粉水解酶的主要产物。研究的E. nigrum PG 16酶是一种葡萄糖淀粉酶,代表了酶解淀粉的一种替代方法。
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来源期刊
Acta Scientiarum. Biological Sciences
Acta Scientiarum. Biological Sciences Agricultural and Biological Sciences-Agricultural and Biological Sciences (all)
CiteScore
1.00
自引率
0.00%
发文量
45
审稿时长
38 weeks
期刊介绍: The journal publishes original articles in all areas of Biological Sciences, including anatomy, bacteriology, molecular biology, biochemistry, botany, cytology and cell biology, animal behavior, ecology, limnology, embryology, and histology, morpho-physiology, genetics, microbiology, parasitology and zoology.
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