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Pilot-Scale Production of Chito-Oligosaccharides Using an Innovative Recombinant Chitosanase Preparation Approach

机译:利用创新的重组壳聚糖酶制备方法进行试验规模生产甲基寡糖

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摘要

For pilot-scale production of chito-oligosaccharides, it must be cost-effective to prepare designable recombinant chitosanase. Herein, an efficient method for preparing recombinant Bacillus chitosanase from Escherichia coli by elimination of undesirable substances as a precipitate is proposed. After an optimized culture with IPTG (Isopropyl β-d-1-thiogalactopyranoside) induction, the harvested cells were resuspended, disrupted by sonication, divided by selective precipitation, and stored using the same solution conditions. Several factors involved in these procedures, including ion types, ionic concentration, pH, and bacterial cell density, were examined. The optimal conditions were inferred to be pH = 4.5, 300 mM sodium dihydrogen phosphate, and cell density below 1011 cells/mL. Finally, recombinant chitosanase was purified to >70% homogeneity with an activity recovery and enzyme yield of 90% and 106 mg/L, respectively. When 10 L of 5% chitosan was hydrolyzed with 2500 units of chitosanase at ambient temperature for 72 h, hydrolyzed products having molar masses of 833 ± 222 g/mol with multiple degrees of polymerization (chito-dimer to tetramer) were obtained. This work provided an economical and eco-friendly preparation of recombinant chitosanase to scale up the hydrolysis of chitosan towards tailored oligosaccharides in the near future.
机译:对于甲基寡糖的试验规模生产,必须具有成本效益,可以制备可设计的重组壳聚糖酶。在此,提出了通过消除作为沉淀物作为沉淀物从大肠杆菌中制备重组芽孢杆菌胰蛋白酶的有效方法。在用IPTG(异丙基β-D-1-硫酰键虫酸)诱导的优化培养物之后,将收获的细胞重新悬浮,通过超声处理破坏,除以选择性沉淀,并使用相同的溶液条件储存。研究了这些程序的几个因素,包括离子类型,离子浓度,pH和细菌细胞密度。推断出最佳条件是pH = 4.5,300mM磷酸二氢钠,细胞密度低于1011细胞/ ml。最后,将重组壳聚糖酶纯化至> 70%均匀性,活性回收和酶产率分别为90%和106mg / L.当在环境温度下用2500单位的壳聚糖酶水解10μl5%壳聚糖72小时时,得到具有833±222g / mol的摩尔质量的水解产物,得到多程度的聚合(邻离四聚体)。这项工作提供了重组壳聚糖酶的经济型和环保准备,以扩大壳聚糖在不久的将来朝向定制寡糖的水解。

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