Selection of purification condition for recombinant endoglucanase originated from goat rumen bacteria in Escherichia coli

TAP CHI SINH HOC Pub Date : 2020-03-19 DOI:10.15625/0866-7160/v42n1.14455

N. Quy, N. Dương, Dao Trong Khoa, N. Việt, Nguyen Khanh Hai, T. N. Hải, Do Thi Thanh Huyen

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Abstract

Cellulase is an important enzyme that plays a role in cleaving β-1,4 glucoside on cellulose to release glucose, which is of economic value and can be applied in many different fields. The 1545 bp endoglucanase gene mined from goat rumen's bacterial metagenomic data was expressed in Escherichia coli Rosetta2. In this study, the recombinant endoglucanase was purified by his-tag affinity chromatography with differrent processes, such as using phosphate buffer with or without sodium cloride, pretreatment of samples with ammonium sulphate before supplying into affinity column, using various concentration of imidazole for washing... Finally the endoglucanse was sucessfully purified by his-tag affinity column using sodium chloride-free phosphate buffer of which 150 mM and 400 mM imidazole were used for washing and enzyme elution, respectively. The resulting enzyme showed its high purity of 99%. CMC plate assay confirmed that although less active than commercial cellulase (Sigma), the recombinant cellulase hydrolyzed CMC to form a clear zone (halo) around the well. The purified enzyme is capable of using as material for further analysis.

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山羊瘤胃大肠杆菌源重组内切葡聚糖酶纯化条件的选择

纤维素酶是将纤维素上的β-1,4糖苷分解为葡萄糖的一种重要酶，具有经济价值，可应用于许多不同的领域。从山羊瘤胃细菌宏基因组数据中提取的1545 bp内切葡聚糖酶基因在大肠杆菌Rosetta2中表达。本研究采用his-tag亲和层析法纯化重组内切葡聚糖酶，采用含氯化钠或不含氯化钠的磷酸盐缓冲液、硫酸铵预处理后送入亲和柱、不同浓度咪唑洗涤等不同工艺。最后用无氯化钠磷酸盐缓冲液对his-tag亲和柱纯化内切葡聚糖，缓冲液分别用150 mM和400 mM咪唑进行洗涤和酶洗脱。所得酶纯度高达99%。CMC平板实验证实，重组纤维素酶水解CMC，在井周围形成一个清晰的区域(光晕)，虽然活性低于商业纤维素酶(Sigma)。纯化后的酶可作为进一步分析的材料。

本文章由计算机程序翻译，如有差异，请以英文原文为准。

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