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首页> 外文期刊>Applied and Environmental Microbiology >Cloning of the Pseudomonas glumae lipase gene and determination of the active site residues.
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Cloning of the Pseudomonas glumae lipase gene and determination of the active site residues.

机译:假单胞菌脂肪酶基因的克隆和活性位点残基的确定。

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The lipA gene encoding the extracellular lipase produced by Pseudomonas glumae PG1 was cloned and characterized. A sequence analysis revealed an open reading frame of 358 codons encoding the mature lipase (319 amino acids) preceded by a rather long signal sequence of 39 amino acids. As a first step in structure-function analysis, we determined the Ser-Asp-His triad which makes up the catalytic site of this lipase. On the basis of primary sequence homology with other known Pseudomonas lipases, a number of putative active site residues located in conserved areas were found. To determine the residues actually involved in catalysis, we constructed a number of substitution mutants for conserved Ser, Asp, and His residues. These mutant lipases were produced by using P. glumae PG3, from which the wild-type lipase gene was deleted by gene replacement. By following this approach, we showed that Ser-87, Asp-241, and His-285 make up the catalytic triad of the P. glumae lipase. This knowledge, together with information on the catalytic mechanism and on the three-dimensional structure, should facilitate the selection of specific modifications for tailoring this lipase for specific industrial applications.
机译:克隆并鉴定了编码由假单胞菌PG1产生的细胞外脂肪酶的lipA基因。序列分析揭示了一个358个密码子的开放阅读框,该密码子编码成熟的脂肪酶(319个氨基酸),随后是一个较长的39个氨基酸的信号序列。作为结构功能分析的第一步,我们确定了组成该脂肪酶催化位点的Ser-Asp-His三联体。基于与其他已知的假单胞菌脂肪酶的一级序列同源性,发现位于保守区的许多推定的活性位点残基。为了确定实际参与催化的残基,我们为保守的Ser,Asp和His残基构建了许多取代突变体。这些突变型脂肪酶是通过使用P. glumae PG3产生的,通过基因置换从野生型脂肪酶基因中删除了突变型脂肪酶。通过遵循这种方法,我们表明Ser-87,Asp-241和His-285组成了P. glumae脂肪酶的催化三联体。这些知识以及有关催化机理和三维结构的信息,应有助于选择特定的修饰,以针对特定的工业应用定制这种脂肪酶。

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