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Isomaltose Production by Modification of the Fructose-Binding Site on the Basis of the Predicted Structure of Sucrose Isomerase from Protaminobacter rubrum

机译:通过基于红曲霉的蔗糖异构酶的预测结构通过修饰果糖结合位点生产异麦芽糖

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摘要

“Protaminobacter rubrum” sucrose isomerase (SI) catalyzes the isomerization of sucrose to isomaltulose and trehalulose. SI catalyzes the hydrolysis of the glycosidic bond with retention of the anomeric configuration via a mechanism that involves a covalent glycosyl enzyme intermediate. It possesses a 325RLDRD329 motif, which is highly conserved and plays an important role in fructose binding. The predicted three-dimensional active-site structure of SI was superimposed on and compared with those of other α-glucosidases in family 13. We identified two Arg residues that may play important roles in SI-substrate binding with weak ionic strength. Mutations at Arg325 and Arg328 in the fructose-binding site reduced isomaltulose production and slightly increased trehalulose production. In addition, the perturbed interactions between the mutated residues and fructose at the fructose-binding site seemed to have altered the binding affinity of the site, where glucose could now bind and be utilized as a second substrate for isomaltose production. From eight mutant enzymes designed based on structural analysis, the R325Q mutant enzyme exhibiting high relative activity for isomaltose production was selected. We recorded 40.0% relative activity at 15% (wt/vol) additive glucose with no temperature shift; the maximum isomaltose concentration and production yield were 57.9 g liter−1 and 0.55 g of isomaltose/g of sucrose, respectively. Furthermore, isomaltose production increased with temperature but decreased at a temperature of >35°C. Maximum isomaltose production (75.7 g liter−1) was recorded at 35°C, and its yield for the consumed sucrose was 0.61 g g−1 with the addition of 15% (wt/vol) glucose. The relative activity for isomaltose production increased progressively with temperature and reached 45.9% under the same conditions.
机译:“ Protaminobacter rubrum”蔗糖异构酶(SI)催化蔗糖异构化为异麦芽酮糖和海藻糖。 SI通过涉及共价糖基酶中间体的机制催化糖苷键的水解并保持异头构型。它具有 325 RLDRD 329 基序,该基序高度保守,在果糖结合中起重要作用。 SI的预测的三维活性位点结构被叠加在家族13中的其他α-葡萄糖苷酶上,并与之比较。我们确定了两个Arg残基,它们在弱离子强度的SI底物结合中可能起重要作用。果糖结合位点的Arg 325 和Arg 328 处的突变减少了异麦芽酮糖的产生,并略微增加了海藻糖的产生。另外,在果糖结合位点处的突变残基和果糖之间的扰动相互作用似乎已经改变了该位点的结合亲和力,其中葡萄糖现在可以结合并用作异麦芽糖生产的第二种底物。从结构分析设计的八种突变酶中,选择对异麦芽糖生产具有较高相对活性的R 325 Q突变酶。在没有温度变化的情况下,我们在15%(wt / vol)的添加葡萄糖下记录了40.0%的相对活性;最高异麦芽糖浓度和产量分别为57.9 g升 -1 和0.55 g异麦芽糖/ g蔗糖。此外,异麦芽糖的产生随温度增加而在> 35℃的温度下减少。在35°C时记录到最大异麦芽糖产量(75.7 g升 -1 ),消耗的蔗糖产量为0.61 gg -1 ,添加15%( wt / vol)葡萄糖。异麦芽糖生产的相对活性随温度逐渐增加,在相同条件下达到45.9%。

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