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Entrapment of α-Amylase in Agar Beads for Biocatalysis of Macromolecular Substrate

机译:琼脂微珠中诱集的α-淀粉酶对大分子底物的生物催化

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摘要

Attempts have been made to optimize immobilization parameters, catalytic property, and stability of immobilized α-amylase in agar. The work compares natural entrapment efficiency of agar with the ionotropically cross-linked agar hydrogel, with the advantage of easy scale-up and cost and time effectiveness. Beads prepared with 3% (w/v) agar and 75 mM calcium chloride and hardened for 20 minutes were selected for further studies on the basis of entrapment efficiency (80%) and physical stability. Following entrapment, pH and temperature optima of enzyme were shifted from 6 to 6.5 and 50 to 55°C, respectively. Michaelis constant (K m) for both free and entrapped enzymes remained the same (0.83%) suggesting no change in substrate affinity. However, V max⁡ of entrapped enzyme decreased ~37.5-fold. The midpoint of thermal inactivation for entrapped enzyme increased by 8 ± 1°C implying its higher thermal stability. The entrapped enzyme in calcium agar bead had an Ea value of 27.49 kcal/mol compared to 17.6 kcal/mol for free enzyme indicating increased stability on entrapment. Half-life of enzyme increased ~2.2 times after entrapment in calcium agar at 60°C indicating stabilization of enzyme. The reusability of beads was size dependent. Beads with diameter <710 μm were stable and could be reused for 6 cycles with ~22% loss in activity.
机译:已经尝试优化琼脂中的固定化参数,催化性能和固定化的α-淀粉酶的稳定性。这项工作将琼脂的自然包封效率与离子交联的琼脂水凝胶进行了比较,具有易于放大,成本和时间效益的优势。基于包封率(80%)和物理稳定性,选择了用3%(w / v)琼脂和75μmM氯化钙制备并硬化20分钟的珠子,以进行进一步研究。包封后,酶的最适pH和最适温度分别从6移至6.5和50至55℃。游离酶和截留酶的米氏常数(K m)保持不变(0.83%),表明底物亲和力没有变化。但是,被包埋的酶的V max下降了约37.5倍。被包埋的酶的热失活的中点增加了8±1°C,这表明其具有更高的热稳定性。琼脂糖钙珠中捕获的酶的Ea值为27.49 kcal / mol,而游离酶的Ea值为17.6 kcal / mol,表明包埋时稳定性增加。酶的半衰期在60°C陷于钙琼脂中后增加了约2.2倍,表明酶已稳定。磁珠的可重复使用性取决于尺寸。直径小于710μm的珠子是稳定的,可以重复使用6个循环,活性降低约22%。

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