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Biochemical and crystallographic analyses of maltohexaose-producing amylase from alkalophilic Bacillus sp 707

机译:嗜碱芽孢杆菌707产生麦芽六糖的淀粉酶的生化和晶体学分析

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摘要

Maltohexaose-producing amylase, called G6-amylase (EC 3.2.1.98), from alkalophilic Bacillus sp.707 predominantly produces maltohexaose (G6) from starch and related alpha-1,4-glucans. To elucidate the reaction mechanism of G6-amylase, the enzyme activities were evaluated and crystal structures were determined for the native enzyme and its complex with pseudo-maltononaose at 2.1 and 1.9 Angstrom resolutions, respectively. The optimal condition for starch-degrading reaction activity was found at 45 degreesC and pH 8.8, and the enzyme produced G6 in a yield of more than 30% of the total products from short-chain amylose (DP = 17). The crystal structures revealed that Asp236 is a nucleophilic catalyst and Glu266 is a proton donor/acceptor. Pseudo-maltononaose occupies subsites -6 to +3 and induces the conformational change of Glu266 and Asp333 to form a salt linkage with the N-glycosidic amino group and a hydrogen bond with secondary hydroxyl groups of the cyclitol residue bound to subsite -1, respectively. The indole moiety of Trp140 is stacked on the cyclitol and 4-amino-6-deoxyglucose residues located at subsites -6 and -5 within a 4 Angstrom distance. Such a face-to-face short contact may regulate the disposition of the glucosyl residue at subsite -6 and would govern the product specificity for G6 production.
机译:嗜碱芽孢杆菌707产生的麦芽六糖淀粉酶,称为G6-淀粉酶(EC 3.2.1.98),主要由淀粉和相关的α-1,4-葡聚糖产生麦芽六糖(G6)。为了阐明G6-淀粉酶的反应机理,评估了酶活性,并分别以2.1和1.9埃的分辨率评估了天然酶及其与假麦芽糖的配合物的晶体结构。发现淀粉降解反应活性的最佳条件是在45℃和pH值为8.8时,该酶以短链直链淀粉(DP = 17)的产率超过总产物的30%。晶体结构表明,Asp236是亲核催化剂,Glu266是质子供体/受体。伪麦芽酮糖占据-6至+3亚位,并诱导Glu266和Asp333的构象变化,分别与N-糖苷氨基形成盐键,并与结合至亚位点-1的环醇残基的仲羟基形成氢键。 。 Trp140的吲哚部分堆积在环糊精和位于4埃距离内位于亚位点-6和-5的4-氨基-6-脱氧葡萄糖残基上。这种面对面的短接触可以调节在位点-6处的葡糖基残基的布置,并且可以控制用于G6生产的产物特异性。

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