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Farnesyl diphosphate synthase. Altering the catalytic site to select for geranyl diphosphate activity

机译:法呢基二磷酸合酶。改变催化部位以选择二磷酸香叶酯活性

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摘要

Farnesyl diphosphate synthase (FPPase) catalyzes chain elongation of the C-5 substrate dimethylallyl diphosphate (DMAPP) to the C-15 product farnesyl diphosphate (FPP) by addition of two molecules of isopentenyl diphosphate (IPP). The synthesis of FPP proceeds in two steps, where the C-10 product of the first addition, geranyl diphosphate (GPP), is the substrate for the second addition. The product selectivity of avian FPPase was altered to favor synthesis of GPP by site-directed mutagenesis of residues that form the binding pocket for the hydrocarbon residue of the allylic substrate. Amino acid substitutions that reduced the size of the binding pocket were identified by molecular modeling. FPPase mutants containing seven promising modifications were constructed. Initial screens using DMAPP and GPP as substrates indicated that two of the substitutions, A116W and N144'W, strongly discriminated against binding of GPP to the allylic site. These observations were confirmed by an analysis of the products from reactions with DMAPP in the presence of excess IPP and by comparing the steady-state kinetic constants for the wild-type enzyme and the A116W and N114W mutants. [References: 20]
机译:法呢基二磷酸合酶(FPPase)通过添加两个分子异戊烯基二磷酸(IPP)来催化C-5底物二甲基烯丙基二磷酸(DMAPP)与C-15产品法呢基二磷酸(FPP)的链延长。 FPP的合成分两个步骤进行,其中第一次添加的C-10产物香叶基二磷酸酯(GPP)是第二次添加的底物。通过对残基进行定点诱变形成禽类FPPase的产物选择性,以促进GPP的合成,这些残基形成了烯丙基底物烃残基的结合口袋。通过分子模型鉴定了减少结合口袋大小的氨基酸取代。构建了包含七个有希望的修饰的FPPase突变体。使用DMAPP和GPP作为底物的初步筛选表明,两个取代A116W和N144'W强烈区分GPP与烯丙基位点的结合。通过对在过量IPP存在下与DMAPP反应的产物进行分析,并比较野生型酶与A116W和N114W突变体的稳态动力学常数,证实了这些观察结果。 [参考:20]

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