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Cloning of Escherichia coli K12 xylose isomerase (glucose isomerase) gene and studying the enzymatic properties of its expression product

机译:大肠杆菌K12木糖异构酶(葡萄糖异构酶)基因的克隆及其表达产物的酶学性质

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摘要

The coding region of Escherichia coli K12 xylose (glucose) isomerase gene was inserted into the pRAC expression vector and cloned in E. coli BL21(DE3) cells. After induction of expression of the cloned gene, the proportion of recombinant xylose isomerase accounted for 40% of the total protein content. As a result of one-stage purification by affinity chromatography, a protein preparation of 90% purity was obtained. The recombinant enzyme catalyzed the isomerization of glucose to fructose and exhibited maximum activity (0.8 U/mg) at 45° C and pH 6.8. The enzyme required Mg2+ ions as a cofactor. When Mg2+ and Co2+ ions were simultaneously present in the reaction medium, the enzyme activity increased by 15-20%. Complete replacement of Mg2+ with Co2+ decreased the enzyme activity. In the presence of Ca2+ at concentrations comparable to the concentration of Mg2+, the enzyme was not inhibited, although published data reported inhibition of similar enzymes by Ca2+. The recombinant enzyme exhibited a very low thermostability: it underwent a slow inactivation when incubated at 45° C and was completely inactivated after incubation at 65° C for 1 h. (PUBLICATION ABSTRACT)
机译:将大肠杆菌K12木糖(葡萄糖)异构酶基因的编码区插入pRAC表达载体,并克隆到大肠杆菌BL21(DE3)细胞中。诱导克隆基因表达后,重组木糖异构酶的比例占总蛋白质含量的40%。通过亲和色谱法进行一级纯化的结果,获得了纯度为90%的蛋白质制品。重组酶催化葡萄糖异构化为果糖,并在45°C和pH 6.8下显示最大活性(0.8 U / mg)。该酶需要Mg2 +离子作为辅助因子。当反应介质中同时存在Mg2 +和Co2 +离子时,酶活性增加15-20%。用Co2 +完全替代Mg2 +会降低酶的活性。在存在与Mg2 +浓度相当的浓度的Ca2 +的情况下,虽然已发表的数据报道了Ca2 +对类似酶的抑制作用,但该酶并未受到抑制。重组酶表现出非常低的热稳定性:在45°C孵育时,其缓慢失活,在65°C孵育1小时后,其完全失活。 (出版物摘要)

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