活性位点配体与大肠杆菌谷氨酰胺合成酶结合的热力学
Thermodynamics of active-site ligand binding to Escherichia coli glutamine synthetase.
作者信息
Ginsburg A, Gorman E G, Neece S H, Blackburn M B
机构信息
Laboratory of Biochemistry, National Heart, Lung, and Blood Institute, Bethesda, Maryland 20892.
出版信息
Biochemistry. 1987 Sep 22;26(19):5989-96. doi: 10.1021/bi00393a007.
Active-site ligand interactions with dodecameric glutamine synthetase from Escherichia coli have been studied by calorimetry and fluorometry using the nonhydrolyzable ATP analogue 5'-adenylyl imidodiphosphate (AMP-PNP), L-glutamate, L-Met-(S)-sulfoximine, and the transition-state analogue L-Met-(S)-sulfoximine phosphate. Measurements were made with the unadenylylated enzyme at pH 7.1 in the presence of 100 mM KCl and 1.0 mM MnCl2, under which conditions the two catalytically essential metal ion sites per subunit are occupied and the stoichiometry of active-site ligand binding is equal to 1.0 equiv/subunit. Thermodynamic linkage functions indicate that there is strong synergism between the binding of AMP-PNP and L-Met-(S)-sulfoximine (delta delta G' = -6.4 kJ/mol). In contrast, there is a small antagonistic effect between the binding of AMP-PNP and L-glutamate (delta delta G' = +1.4 kJ/mol). Proton effects were negligible (less than or equal to 0.2 equiv of H+ release or uptake/mol) for the different binding reactions. The binding of AMP-PNP (or ATP) to the enzyme is entropically controlled at 303 K with delta H = +5.4 kJ/mol and delta S = +150 J/(K.mol). At 303 K, the binding of L-glutamate (delta H = -22.2 kJ/mol) or L-Met-(S)-sulfoximine [delta H = -45.6 kJ/mol with delta Cp approximately equal to -670 +/- 420 J/(K.mol)] to the AMP-PNP.Mn.enzyme complex is enthalpically controlled with opposing delta S values of -29 or -46 J/(K.mol), respectively. The overall enthalpy change is negative and the overall entropy change is positive for the simultaneous binding of AMP-PNP and L-glutamate or of AMP-PNP and L-Met-(S)-sulfoximine to the enzyme. For the binding of the transition-state analogue L-Met-(S)-sulfoximine phosphate (which inactivates the enzyme by blocking active sites), both enthalpic and entropic contributions also are favorable at 303 K [delta G' approximately equal to -109 and delta H = -54.8 kJ/mol of subunit and delta S approximately equal to +180 J/(K.mol)].
已通过量热法和荧光法,使用不可水解的ATP类似物5'-腺苷亚氨基二磷酸(AMP-PNP)、L-谷氨酸、L-蛋氨酸-(S)-亚砜亚胺以及过渡态类似物L-蛋氨酸-(S)-亚砜亚胺磷酸,研究了活性位点配体与来自大肠杆菌的十二聚体谷氨酰胺合成酶的相互作用。在pH 7.1、100 mM KCl和1.0 mM MnCl₂存在的条件下,对未腺苷化的酶进行了测量,在此条件下每个亚基的两个催化必需金属离子位点被占据,且活性位点配体结合的化学计量比等于1.0当量/亚基。热力学连锁函数表明,AMP-PNP与L-蛋氨酸-(S)-亚砜亚胺的结合之间存在强烈的协同作用(ΔΔG' = -6.4 kJ/mol)。相比之下,AMP-PNP与L-谷氨酸的结合之间存在较小的拮抗作用(ΔΔG' = +1.4 kJ/mol)。对于不同的结合反应,质子效应可忽略不计(释放或摄取的H⁺小于或等于0.2当量/摩尔)。在303 K时,AMP-PNP(或ATP)与酶的结合受熵控制,ΔH = +5.4 kJ/mol,ΔS = +150 J/(K·mol)。在303 K时,L-谷氨酸(ΔH = -22.2 kJ/mol)或L-蛋氨酸-(S)-亚砜亚胺[ΔH = -45.6 kJ/mol,ΔCp约等于-670 ± 420 J/(K·mol)]与AMP-PNP·Mn·酶复合物的结合受焓控制,其相反的ΔS值分别为-29或-46 J/(K·mol)。对于AMP-PNP和L-谷氨酸或AMP-PNP和L-蛋氨酸-(S)-亚砜亚胺同时与酶的结合,总的焓变是负的,总的熵变是正的。对于过渡态类似物L-蛋氨酸-(S)-亚砜亚胺磷酸(通过阻断活性位点使酶失活)的结合,在303 K时焓和熵的贡献也都是有利的[ΔG'约等于-109,亚基的ΔH = -54.8 kJ/mol,ΔS约等于+180 J/(K·mol)]。
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