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Isomaltulose Synthase from Klebsiella sp. Strain LX3: Gene Cloning and Characterization and Engineering of Thermostability

机译:克雷伯菌属的异麦芽酮糖合酶。 LX3菌株:基因克隆与鉴定及热稳定性工程

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摘要

The gene (palI) encoding isomaltulose synthase (PalI) from a soil bacterial isolate, Klebsiella sp. strain LX3, was cloned and characterized. PalI converts sucrose into isomaltulose, trehalulose, and trace amounts of glucose and fructose. Sequence domain analysis showed that PalI contains an α-amylase domain and (β/α)8-barrel structures, suggesting that it belongs to the α-amylase family. Sequence alignment indicated that the five amino acid residues of catalytic importance in α-amylases and glucosyltransferases (Asp241, Glu295, Asp369, His145, and His368) are conserved in PalI. Purified recombinant PalI displayed high catalytic efficiency, with a Km of 54.6 ± 1.7 mM for sucrose, and maximum activity (approximately 328.0 ± 2.5 U/mg) at pH 6.0 and 35°C. PalI activity was strongly inhibited by Fe3+ and Hg2+ and was enhanced by Mn2+ and Mg2+. The half-life of PalI was 1.8 min at 50°C. Replacement of selected amino acid residues by proline significantly increased the thermostability of PalI. Simultaneous replacement of Glu498 and Arg310 with proline resulted in an 11-fold increase in the half-life of PalI at 50°C.
机译:来自土壤细菌分离株Klebsiella sp。的异麦芽酮糖合酶(PalI)编码基因(palI)。克隆并鉴定了菌株LX3。 PalI将蔗糖转化为异麦芽酮糖,海藻糖和痕量的葡萄糖和果糖。序列结构域分析表明,PalI包含一个α-淀粉酶结构域和(β/α)8-桶形结构,表明它属于α-淀粉酶家族。序列比对表明在α-淀粉酶和葡糖基转移酶中具有催化重要性的五个氨基酸残基(Asp 241 ,Glu 295 ,Asp 369 ,His 145 和His 368 )在PalI中是保守的。纯化的重组PalI表现出高催化效率,蔗糖Km为54.6±1.7 mM,在pH 6.0和35°C时具有最大活性(约328.0±2.5 U / mg)。 Fe 3 + 和Hg 2 + 强烈抑制PalI活性,而Mn 2 + 和Mg 2 + 增强PalI活性。 sup>。 PalI在50°C的半衰期为1.8分钟。用脯氨酸替代选定的氨基酸残基显着提高了PalI的热稳定性。用脯氨酸同时替换Glu 498 和Arg 310 可使50℃下PalI的半衰期延长11倍。

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