Stabilization of a truncated Bacillus sp. strain TS-23 α-amylase by replacing histidine-436 with aspartate

被引:0
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作者
Huei-Fen Lo
Ya-Hui Chen
Nai-Wan Hsiao
Hsiang-Ling Chen
Hui-Yu Hu
Wen-Hwei Hsu
Long-Liu Lin
机构
[1] Hungkuang University,Department of Food and Nutrition
[2] Taichung Healthcare and Management University,Graduate Institute of Bioinformatics
[3] National Chung Hsing University,Institute of Molecular Biology
[4] National Chiayi University,Department of Applied Chemistry
关键词
Bacillus sp. strain TS-23; α-amylase; site-directed mutagenesis; histidine; thermostability;
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摘要
Histidine-436 of a truncated Bacillus sp. strain TS-23 α-amylase (His6-tagged ΔNC) has been known to be responsible for thermostability of the enzyme. To understand further the structural role of this residue, site-directed mutagenesis was conducted to replace His-436 of His6-tagged ΔNC with aspartate, lysine, tyrosine or threonine. Starch-plate assay showed that all Escherichia coli M15 transformants conferring the mutated amylase genes retained the amylolytic activity. The over-expressed proteins have been purified to near homogeneity by nickel-chelate chromatography and the molecular mass of the purified enzymes was approximately 54 kDa. The specific activity for H436T was decreased by more than 56%, while H436D, H436K, and H436Y showed a higher activity to that of the wild-type enzyme. Although the mutations did not lead to a significant change in the Km value, more than 66% increase in the value of catalytic efficiency (kcat/Km) was observed in H436D, H436K, and H436Y. At 70 °C, H436D exhibited an increased half-life with respect to the wild-type enzyme.
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页码:411 / 416
页数:5
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