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阴离子受体大环在涉及核苷酸作为底物、产物和辅因子的酶的超分子串联测定中的应用。

Implementation of anion-receptor macrocycles in supramolecular tandem assays for enzymes involving nucleotides as substrates, products, and cofactors.

机构信息

School of Engineering and Science, Jacobs University Bremen, Campus Ring 1, D-28759, Bremen, Germany.

出版信息

Org Biomol Chem. 2010 Mar 7;8(5):1033-9. doi: 10.1039/b925192h. Epub 2010 Jan 7.

DOI:10.1039/b925192h
PMID:20165793
Abstract

A supramolecular tandem assay for direct continuous monitoring of nucleotide triphosphate-dependent enzymes such as potato apyrase is described. The underlying principle of the assay relies on the use of anion-receptor macrocycles in combination with fluorescent dyes as reporter pairs. A combinatorial approach was used to identify two complementary reporter pairs, i.e. an amino-gamma-cyclodextrin with 2-anilinonaphtalene-6-sulfonate (ANS) as dye (fluorescence enhancement factor of 17 upon complexation) and a polycationic cyclophane with 8-hydroxy-1,3,6-pyrene trisulfonate (HPTS) as dye (fluorescence decrease by a factor of more than 2000), which allow the kinetic monitoring of potato apyrase activity at different ATP concentration ranges (microM and mM) with different types of photophysical responses (switch-ON and switch-OFF). Competitive fluorescence titrations revealed a differential binding of ATP (strongest competitor) versus ADP and AMP, which constitutes the prerequisite for monitoring enzymatic conversions (dephosphorylation or phosphorylation) involving nucleotides. The assay was tested for different enzyme and substrate concentrations and exploited for the screening of activating additives, namely divalent transition metal ions (Ni(2+), Mg(2+), Mn(2+), and Ca(2+)). The transferability of the assay could be demonstrated by monitoring the dephosphorylation of other nucleotide triphosphates (GTP, TTP, and CTP).

摘要

描述了一种用于直接连续监测核苷酸三磷酸依赖酶(如马铃薯脱氨酶)的超分子串联测定法。该测定法的基本原理依赖于阴离子受体大环化合物与荧光染料作为报告对的组合使用。采用组合方法来鉴定两种互补的报告对,即氨基-γ-环糊精与 2-苯胺萘-6-磺酸盐(ANS)作为染料(络合后荧光增强因子为 17)和多阳离子环番与 8-羟基-1,3,6-三磺酸芘(HPTS)作为染料(荧光降低 2000 多倍),这允许在不同的 ATP 浓度范围内(微摩尔和毫摩尔)以不同的光物理响应(开和关)对马铃薯脱氨酶活性进行动力学监测。竞争性荧光滴定显示出 ATP(最强的竞争物)与 ADP 和 AMP 的不同结合,这是监测涉及核苷酸的酶转化(去磷酸化或磷酸化)的前提条件。该测定法已针对不同的酶和底物浓度进行了测试,并用于筛选激活添加剂,即二价过渡金属离子(Ni(2+)、Mg(2+)、Mn(2+)和 Ca(2+))。通过监测其他核苷酸三磷酸(GTP、TTP 和 CTP)的去磷酸化,可以证明该测定法的可转移性。

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