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泡盛曲霉糖化酶的蛋白质工程改造以提高其最适pH值。

Protein engineering of Aspergillus awamori glucoamylase to increase its pH optimum.

作者信息

Fang T Y, Ford C

机构信息

Department of Food Science and Human Nutrition, Iowa State University, Ames 50011, USA.

出版信息

Protein Eng. 1998 May;11(5):383-8. doi: 10.1093/protein/11.5.383.

Abstract

To increase the pH optimum of glucoamylase (GA), five mutations-S411G, S411A, S411C, S411H and S411D--were designed to destabilize the carboxylate ion form of Glu400, the catalytic base, by removing or weakening the hydrogen bond between Ser411 and Glu400, and thereby raising its pK. The substitution of alanine, histidine and aspartate were also designed to study the additional effects of polarity and both positive and negative charges, respectively. S411G GA had catalytic efficiencies like those of wild-type GA for isomaltose, maltose and maltoheptaose hydrolysis at pH 4.4, while S411A and S411C GAs had 54-74% and S411H and S411D GAs had only about 6-12% of wild-type catalytic efficiencies. All five mutations increased the pH optimum in the enzyme-substrate complex, mainly by raising pK1 values. S411A is the best performing and most industrially promising of the pH mutants isolated to date. S411A GA increased the pH optimum by 0.8 units for both maltose and maltoheptaose hydrolysis while maintaining a high level of activity and catalytic efficiency. In hydrolysis of 28% DE 10 maltodextrin, S411A GA had a pH optimum of 7 compared with pH 5.6 for wild-type GA, and had higher initial rates of glucose production than wild-type GA at all pH values tested above pH 6.6.

摘要

为提高葡糖淀粉酶(GA)的最适pH值,设计了5种突变——S411G、S411A、S411C、S411H和S411D,通过去除或削弱Ser411与Glu400之间的氢键来破坏催化碱基Glu400的羧酸根离子形式,从而提高其pK值。还设计了丙氨酸、组氨酸和天冬氨酸的取代,分别研究极性以及正电荷和负电荷的额外影响。S411G GA在pH 4.4时对异麦芽糖、麦芽糖和麦芽七糖水解的催化效率与野生型GA相似,而S411A和S411C GA的催化效率分别为野生型的54 - 74%,S411H和S411D GA仅为野生型的约6 - 12%。所有5种突变均提高了酶 - 底物复合物中的最适pH值,主要是通过提高pK1值。S411A是迄今为止分离出的pH突变体中性能最佳且最具工业前景的。S411A GA对麦芽糖和麦芽七糖水解的最适pH值提高了0.8个单位,同时保持了较高的活性和催化效率。在水解28% DE 10的麦芽糊精时,S411A GA的最适pH值为7,而野生型GA为pH 5.6,并且在pH 6.6以上测试的所有pH值下,S411A GA的葡萄糖生成初始速率均高于野生型GA。

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