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土壤嗜热菌葡萄糖氧化酶基因的分子克隆、表达及酶活性

Molecular Cloning, Expression, and Enzyme Activity of Glucose Oxidase Gene from Soil Thermophilic .

作者信息

Karimiabar Mahsa, Ahari Hamed, Amini Kumarss

机构信息

Department of Food Science and Technology, Science and Research Branch, Islamic Azad University, Tehran, Iran.

Department of Microbiology, Faculty of Basic Science, Saveh Branch, Islamic Azad University, Saveh, Iran.

出版信息

Iran J Biotechnol. 2022 Jan 1;20(1):e2979. doi: 10.30498/ijb.2021.272122.2979. eCollection 2022 Jan.

Abstract

BACKGROUND

Glucose oxidase is an oxidoreductase that depletes oxygen in food processing and is used in biosensors, glucose diagnostic kits, food processing, cosmetics, and chemical industries. This enzyme is often isolated from fungi, such as Penicillium and .

OBJECTIVES

The objective of this study was to clone and express a full-length GOX gene from soil thermophilic streptomyces for bioinformatic and enzyme activity evaluations.

MATERIALS AND METHODS

After collecting samples from the Gandom Beryan area of Kerman province, Iran, Streptomyces strains were identified with specific biochemical and molecular tests. Streptomyces strains with glucose oxidase gene were detected by PCR, and the amplified gene fragment was cloned into host bacterium using TA cloning technique. The expression of the cloned GOX gene in the host bacterium was measured using real-time PCR, and the recombinant plasmids were sequenced. The enzymatic activity was measured in the extracts of cells carrying the plasmids.

RESULTS

After screening the samples, 12 strains of were identified, 4 of which carried the GOX gene. The GOX open reading frame, obtained by PCR, was cloned into a vector and transformed into Escherichia coli origami to generate GOX-producing bacteria. Enzyme activity was confirmed and a phylogenetic tree showed the degree of kinship between Streptomyces species and other species, including Streptomyces SP MI02-7b. The expression levels of GOX genes mRNA were found to be approximately 4-fold higher in transformed than in soil thermophilic Streptomyces (P <0.001).

CONCLUSION

This study showed that natural thermostable streptomyces producing glucose oxidase enzyme could be found in Iran. The enzyme gene was successfully transformed into generating a recombinant host with high yield capability that can be a major step towards the production of this enzyme from indigenous strains. It should be emphasized that the GOX enzyme produced by these strains is profitable due to high production levels correlated to the optimum condition in cheap culture media, short fermentation cycles, high expression capability, and ease of growth.

摘要

背景

葡萄糖氧化酶是一种氧化还原酶,在食品加工过程中消耗氧气,用于生物传感器、葡萄糖诊断试剂盒、食品加工、化妆品和化学工业。这种酶通常从真菌中分离出来,如青霉属和……

目的

本研究的目的是从土壤嗜热链霉菌中克隆并表达全长GOX基因,用于生物信息学和酶活性评估。

材料与方法

从伊朗克尔曼省甘多姆贝里安地区采集样本后,通过特定的生化和分子测试鉴定链霉菌菌株。通过PCR检测带有葡萄糖氧化酶基因的链霉菌菌株,并使用TA克隆技术将扩增的基因片段克隆到宿主细菌中。使用实时PCR测量克隆的GOX基因在宿主细菌中的表达,并对重组质粒进行测序。在携带质粒的细胞提取物中测量酶活性。

结果

筛选样本后,鉴定出12株链霉菌,其中4株携带GOX基因。通过PCR获得的GOX开放阅读框被克隆到载体中,并转化到大肠杆菌Origami中以产生产生GOX的细菌。酶活性得到证实,系统发育树显示了链霉菌物种与其他物种(包括链霉菌SP MI02 - 7b)之间的亲缘关系程度。发现转化后的大肠杆菌中GOX基因mRNA的表达水平比土壤嗜热链霉菌高约4倍(P <0.001)。

结论

本研究表明,在伊朗可以找到产生葡萄糖氧化酶的天然耐热链霉菌。该酶基因成功转化到大肠杆菌中,产生了具有高产能力的重组宿主,这可能是朝着从本土菌株生产这种酶迈出的重要一步。应该强调的是,这些菌株产生的GOX酶由于在廉价培养基中与最佳条件相关的高产量、短发酵周期、高表达能力和易于生长而具有经济效益。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/866d/9284247/1ea97eb1ee77/IJB-20-e2979-g001.jpg

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