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Altered Large-Ring Cyclodextrin Product Profile Due to a Mutation at Tyr-172 in the Amylomaltase of Corynebacterium glutamicum

机译:谷氨酸棒杆菌淀粉酶中Tyr-172突变导致大环环糊精产物改变

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摘要

Corynebacterium glutamicum amylomaltase (CgAM) catalyzes the formation of large-ring cyclodextrins (LR-CDs) with a degree of polymerization of 19 and higher. The cloned CgAM gene was ligated into the pET-17b vector and used to transform Escherichia coli BL21(DE3). Site-directed mutagenesis of Tyr-172 in CgAM to alanine (Y172A) was performed to determine its role in the control of LR-CD production. Both the recombinant wild-type (WT) and Y172A enzymes were purified to apparent homogeneity and characterized. The Y172A enzyme exhibited lower disproportionation, cyclization, and hydrolysis activities than the WT. The kcat/Km of the disproportionation reaction of the Y172A enzyme was 2.8-fold lower than that of the WT enzyme. The LR-CD product profile from enzyme catalysis depended on the incubation time and the enzyme concentration. Interestingly, the Y172A enzyme showed a product pattern different from that of the WT CgAM at a long incubation time. The principal LR-CD products of the Y172A mutated enzyme were a cycloamylose mixture with a degree of polymerization of 28 or 29 (CD28 or CD29), while the principal LR-CD product of the WT enzyme was CD25 at 0.05 U of amylomaltase. These results suggest that Tyr-172 plays an important role in determining the LR-CD product profile of this novel CgAM.
机译:谷氨酸棒杆菌淀粉酶(CgAM)催化聚合度为19或更高的大环环糊精(LR-CD)的形成。将克隆的CgAM基因连接到pET-17b载体中,并用于转化大肠杆菌BL21(DE3)。进行了CgAM中Tyr-172对丙氨酸(Y172A)的定点诱变,以确定其在控制LR-CD产生中的作用。重组野生型(WT)和Y172A酶均被纯化至明显的同质性并进行了表征。与野生型相比,Y172A酶的歧化,环化和水解活性较低。 Y172A酶歧化反应的kcat / Km比WT酶低2.8倍。酶催化产生的LR-CD产物曲线取决于孵育时间和酶浓度。有趣的是,Y172A酶在较长的孵育时间内显示出与WT CgAM不同的产物模式。 Y172A突变酶的主要LR-CD产物是聚合度为28或29(CD28或CD29)的环淀粉混合物,而WT酶的主要LR-CD产物是淀粉酶0.05 U的CD25。这些结果表明,Tyr-172在确定这种新型CgAM的LR-CD产品概况中起着重要作用。

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