首页> 外文期刊>Journal of molecular catalysis, B. Enzymatic >Construction of combinatorial library of starch-binding domain of Rhizopus oryzae glucoamylase and screening of clones with enhanced activity by yeast display method
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Construction of combinatorial library of starch-binding domain of Rhizopus oryzae glucoamylase and screening of clones with enhanced activity by yeast display method

机译:米根霉葡糖淀粉酶淀粉结合域组合文库的构建及酵母展示法筛选活性增强的克隆

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Most of the glucoamylases (GA),which catalyze the hydrolysis of alpha-1,4 and alpha-1,6 glycosidic linkages,have a distinct region called a starch-binding domain (SBD).We have developed a powerful method for screening a library of GA mutants by a combination of GA display and SBD mutagenesis on the yeast-cell surface.In the case of Rhizopus oryzae glucoamylase (RoGA),three amino acids (63S,71T,73S) of the SBD were combinatorially mutated to enhance the degradation activity toward cooked corn starch and the mutated RoGAs were displayed on yeast-cell surface by cell-surface engineering.After the first screening by halo assay using an iodine-starch reaction,about 200 of the 8000 colonies formed clear halos.Incubation of the yeast with the mutated and displayed RoGAs caused direct degradation of cooked corn starch.Repeated screening revealed that some of the mutants produced a degradation rate around approx1.4-fold higher than did wild type.The results obtained from the DNA sequences of the mutated SBDs indicated that amino-acid residues with a carbonyl group (D,E,Q,N) in the SBD enhance the degradation ability of the GA by enhancing the binding activity of the SBD.
机译:大多数催化α-1,4和α-1,6糖苷键水解的葡糖淀粉酶(GA)都有一个独特的区域,称为淀粉结合域(SBD)。我们开发了一种有效的方法来筛选通过将GA展示和SBD诱变结合在酵母细胞表面上的GA突变体文库。在米根霉葡糖淀粉酶(RoGA)的情况下,将SBD的三个氨基酸(63S,71T,73S)组合突变以增强通过细胞表面工程在酵母细胞表面显示出对煮熟的玉米淀粉的降解活性和突变的RoGAs。使用碘-淀粉反应通过光晕试验首次筛选后,8000个菌落中约有200个形成了透明的光晕。带有RoGAs突变和展示的酵母直接导致熟玉米淀粉降解。重复筛选显示,某些突变体的降解率比野生型高约1.4倍。突变的SBDs表明,SBD中具有羰基(D,E,Q,N)的氨基酸残基通过增强SBD的结合活性而增强了GA的降解能力。

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