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Cloning, expression and characterization of an aspartate aminotransferase gene from Lactobacillus brevis CGMCC 1306

机译:短乳杆菌CGMCC 1306的天冬氨酸转氨酶基因的克隆,表达和鉴定

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ABSTRACT An aspartate aminotransferase (AATase) gene from Lactobacillus brevis CGMCC 1306 was cloned, which contains a 1182-bp open reading frame coding for 393 amino acids (41.43 kDa). When expressed in Escherichia coli BL21 (DE3), the recombinant AATase was purified and subsequently characterized. The recombinant AATase can catalyse the conversion of L-Asp to L-Glu, and the k cat / K m was determined to be 25.5 (mmol/L) ?¢????1 s ?¢????1 for L-Asp and 207.8 m(mol/L) ?¢????1 s ?¢????1 for ???±-ketoglutarate. With optimum temperature as 25 ????C, the AATase may be a novel and special psychrophilic enzyme which exhibited a good thermal stability below 55 ????C. The conserved active site residue of AATase was identified as Lys237 by phylogenetic analysis. Secondary structure of the enzyme includes ???±-helix (39.2%), ???2-sheet (5.5%), ???2-turn (8.8%), and random coil (36.5%) by circular dichroism spectral analysis. Phase diagram for the fluorescence data analysis showed that guanidinium chloride-induced unfolding of AATase involved at least one intermediate.
机译:摘要克隆了来自短乳杆菌CGMCC 1306的天冬氨酸转氨酶(AATase)基因,该基因包含一个1182 bp的开放阅读框,编码393个氨基酸(41.43 kDa)。当在大肠杆菌BL21(DE3)中表达时,将重组AATase纯化并随后鉴定。重组AATase可催化L-Asp向L-Glu的转化,L的k cat / K m为25.5(mmol / L)。 -Asp和±7.8酮戊二酸的207.8m(mol / L)·············································································在最适温度为25℃的条件下,AAT酶可以是一种新颖而特殊的嗜冷酶,它在55℃以下显示出良好的热稳定性。通过系统进化分析,保守的AATase活性位点残基被鉴定为Lys237。酶的二级结构通过圆二色性光谱包括±螺旋(39.2%),2-折叠(5.5%),2-转(8.8%)和无规卷曲(36.5%)。分析。荧光数据分析的相图表明,氯化胍诱导的AATase折叠涉及至少一种中间体。

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