Wielgus-Kutrowska B, Antosiewicz J M, Długosz M, Holý A, Bzowska A
Department of Biophysics, Warsaw University, Poland.
Biophys Chem. 2007 Feb;125(2-3):260-8. doi: 10.1016/j.bpc.2006.08.008. Epub 2006 Sep 1.
The binding of multisubstrate analogue inhibitor - 2-amino-9-[2-(phosphonomethoxy)ethyl]-6-sulfanylpurine (PME-6-thio-Gua) to purine nucleoside phosphorylase from Cellulomonas sp. at 20 degrees C, in 20 mM Hepes buffer with ionic strength adjusted to 50 mM using KCl, at several pH values between 6.5 and 8.2, was investigated using a stopped-flow spectrofluorimeter. The kinetic transients registered after mixing a protein solution with ligand solutions of different concentrations were simultaneously fitted by several association reaction models using nonlinear least-squares procedure based on numerical integration of the chemical kinetic equations appropriate for given model. It is concluded that binding of a PME-6-thio-Gua molecule by each of the binding sites is sufficiently well described by one-step process, with a model assuming interacting binding sites being more probable than a model assuming independent sites. The association rate constants derived from experimental data, assuming one step binding and independent sites, are decreasing with an increase in pH, changing from 30 to 6 microM(-1)s(-1) per binding site. The dissociation rate constants are in the range of 1-3 s(-1), and they are rather insensitive of changes in pH. Interestingly, for each pH value, the one-step binding model with interacting sites results in the association rate constant per site 1.5-4 times smaller for the binding of the first ligand molecule than that for the binding of the second one. Decrease of association constants with pH indicate that the enzyme does not prefer binding of the naturally occurring anionic form of the 6-thioguanine ring (pK(a) 8.7) resulting from a dissociation of N(1)-H. This finding supports the mechanism in which hydrogen bond interaction of N(1)-H with Glu204 (Glu 201 in mammalian PNPs) is crucial in the catalytic process. Results obtained also indicate that, in contrast to transition-state analogues, for which binding is followed by a conformational change, binding of multisubstrate analogue inhibitors to trimeric PNPs is a one-step process.
在20℃下,于20 mM Hepes缓冲液中(使用KCl将离子强度调节至50 mM),在6.5至8.2的几个pH值条件下,使用停流荧光分光光度计研究了多底物类似物抑制剂——2-氨基-9-[2-(膦酰甲氧基)乙基]-6-硫代嘌呤(PME-6-硫代鸟嘌呤,PME-6-thio-Gua)与纤维单胞菌属嘌呤核苷磷酸化酶的结合情况。将蛋白质溶液与不同浓度的配体溶液混合后记录的动力学瞬变,通过基于适用于给定模型的化学动力学方程数值积分的非线性最小二乘法程序,同时用几种缔合反应模型进行拟合。得出的结论是,每个结合位点与PME-6-硫代鸟嘌呤分子的结合通过一步过程能得到充分描述,与假设独立位点的模型相比,假设相互作用结合位点的模型更有可能。假设一步结合和独立位点,从实验数据得出的缔合速率常数随pH升高而降低,每个结合位点从30降至6 μM⁻¹s⁻¹。解离速率常数在1 - 3 s⁻¹范围内,对pH变化相当不敏感。有趣的是,对于每个pH值,具有相互作用位点的一步结合模型导致第一个配体分子结合的每个位点缔合速率常数比第二个配体分子结合时小1.5 - 4倍。缔合常数随pH降低表明该酶不倾向于结合由N(1)-H解离产生的天然存在的6-硫鸟嘌呤环阴离子形式(pK(a) 8.7)。这一发现支持了N(1)-H与Glu204(哺乳动物PNP中的Glu 201)的氢键相互作用在催化过程中至关重要的机制。所得结果还表明,与结合后会发生构象变化的过渡态类似物不同,多底物类似物抑制剂与三聚体PNP的结合是一个一步过程。
Zotero 插件