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Optimal Immobilization of β-Galactosidase onto κ-Carrageenan Gel Beads Using Response Surface Methodology and Its Applications

机译:响应面法优化β-半乳糖苷酶在κ-角叉菜胶凝胶珠上的固定及其应用

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摘要

β-Galactosidase (β-gal) was immobilized by covalent binding on novel κ-carrageenan gel beads activated by two-step method; the gel beads were soaked in polyethyleneimine followed by glutaraldehyde. 22 full-factorial central composite experiment designs were employed to optimize the conditions for the maximum enzyme loading efficiency. 11.443 U of enzyme/g gel beads was achieved by soaking 40 units of enzyme with the gel beads for eight hours. Immobilization process increased the pH from 4.5 to 5.5 and operational temperature from 50 to 55°C compared to the free enzyme. The apparent K m after immobilization was 61.6 mM compared to 22.9 mM for free enzyme. Maximum velocity V max was 131.2 μmol·min−1 while it was 177.1 μmol·min−1 for free enzyme. The full conversion experiment showed that the immobilized enzyme form is active as that of the free enzyme as both of them reached their maximum 100% relative hydrolysis at 4 h. The reusability test proved the durability of the κ-carrageenan beads loaded with β-galactosidase for 20 cycles with retention of 60% of the immobilized enzyme activity to be more convenient for industrial uses.
机译:β-半乳糖苷酶(β-gal)通过共价结合固定在通过两步法激活的新型κ-角叉菜胶凝胶珠上;将凝胶珠粒先浸入聚乙烯亚胺,再浸入戊二醛。采用2 2 全因子中心复合实验设计优化了最大酶负载效率的条件。通过将40个单位的酶用凝胶珠浸泡8小时可以达到11.443 U的酶/克凝胶珠。与游离酶相比,固定过程将pH从4.5提高到5.5,操作温度从50提高到55°C。固定后的表观K m为61.6μmM,而游离酶为22.9μmM。游离酶的最大速度V max为131.2μmol·min -1 ,而最大速度为177.1μmol·min -1 。完全转化实验表明,固定化酶形式与游离酶一样具有活性,因为它们都在4?h达到最大100%相对水解。可重用性测试证明了装载有 β -半乳糖苷酶的κ-角叉菜胶珠的耐久性为20个循环,保留了固定化酶的60%活动更便于工业使用。

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