Vallmitjana M, Ferrer-Navarro M, Planell R, Abel M, Ausín C, Querol E, Planas A, Pérez-Pons J A
Institut de Biologia Fonamental "Vicent Villar i Palasí" and Dept Bioquímica i Biologia Molecular, Universitat Autònoma de Barcelona, 08193 Barcelona, Spain.
Biochemistry. 2001 May 22;40(20):5975-82. doi: 10.1021/bi002947j.
The Streptomyces sp. beta-glucosidase (Bgl3) is a retaining glycosidase that belongs to family 1 glycosyl hydrolases. Steady-state kinetics with p-nitrophenyl beta-D-glycosides revealed that the highest k(cat)/K(M) values are obtained with glucoside (with strong substrate inhibition) and fucoside (with no substrate inhibition) substrates and that Bgl3 has 10-fold glucosidase over galactosidase activity. Reactivity studies by means of a Hammett analysis using a series of substituted aryl beta-glucosides gave a biphasic plot log k(cat) vs pK(a) of the phenol aglycon: a linear region with a slope of beta(lg) = -0.8 for the less reactive substrates (pK(a) > 8) and no significant dependence for activated substrates (pK(a) < 8). Thus, according to the two-step mechanism of retaining glycosidases, formation of the glycosyl-enzyme intermediate is rate limiting for the former substrates, while hydrolysis of the intermediate is for the latter. To identify key catalytic residues and on the basis of sequence similarity to other family 1 beta-glucosidases, glutamic acids 178 and 383 were changed to glutamine and alanine by site-directed mutagenesis. Mutation of Glu178 to Gln and Ala yielded enzymes with 250- and 3500-fold reduction in their catalytic efficiencies, whereas larger reduction (10(5)-10(6)-fold) were obtained for mutants at Glu383. The functional role of both residues was probed by a chemical rescue methodology based on activation of the inactive Ala mutants by azide as exogenous nucleophile. The E178A mutant yielded the beta-glucosyl azide adduct (by (1)H NMR) with a 200-fold increase on k(cat) for the 2,4-dinitrophenyl glucoside but constant k(cat)/K(M) on azide concentration. On the other hand, the E383A mutant with the same substrate gave the alpha-glucosyl azide product and a 100-fold increase in k(cat) at 1 M azide. In conclusion, Glu178 is the general acid/base catalyst and Glu383 the catalytic nucleophile. The results presented here indicate that Bgl3 beta-glucosidase displays kinetic and mechanistic properties similar to other family 1 enzymes analyzed so far. Subtle differences in behavior would lie in the fine and specific architecture of their respective active sites.
链霉菌属β-葡萄糖苷酶(Bgl3)是一种保留型糖苷酶,属于1型糖基水解酶家族。对对硝基苯基β-D-糖苷进行的稳态动力学研究表明,对于葡萄糖苷(有强烈底物抑制作用)和岩藻糖苷(无底物抑制作用)底物,可获得最高的k(cat)/K(M)值,且Bgl3的葡萄糖苷酶活性是半乳糖苷酶活性的10倍。通过使用一系列取代芳基β-葡萄糖苷进行哈米特分析的反应性研究,得到了苯酚苷元的log k(cat)与pK(a)的双相图:对于反应性较低的底物(pK(a) > 8),有一个斜率为β(lg) = -0.8的线性区域,而对于活化底物(pK(a) < 8)则没有显著依赖性。因此,根据保留型糖苷酶的两步机制,对于前一种底物,糖基-酶中间体的形成是限速步骤,而对于后一种底物,中间体的水解是限速步骤。为了鉴定关键催化残基,并基于与其他1型β-葡萄糖苷酶的序列相似性,通过定点诱变将谷氨酸178和383分别替换为谷氨酰胺和丙氨酸。将Glu178突变为Gln和Ala后,酶的催化效率分别降低了250倍和3500倍,而Glu383突变体的催化效率降低幅度更大(10^5 - 10^6倍)。通过基于叠氮化物作为外源亲核试剂激活无活性的Ala突变体的化学拯救方法,探究了这两个残基的功能作用。E178A突变体产生了β-葡萄糖基叠氮加合物(通过^1H NMR),对于2,4-二硝基苯基葡萄糖苷,k(cat)增加了200倍,但k(cat)/K(M)对叠氮化物浓度不变。另一方面,对于相同底物,E383A突变体产生了α-葡萄糖基叠氮产物,在1 M叠氮化物存在下k(cat)增加了100倍。总之,Glu178是通用酸/碱催化剂,Glu383是催化亲核试剂。此处给出的结果表明,Bgl3β-葡萄糖苷酶表现出与目前分析的其他1型酶相似的动力学和机制特性。行为上的细微差异可能在于它们各自活性位点的精细和特定结构。
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