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Phosphatase-Coupled Universal Kinase Assay and Kinetics for First-Order-Rate Coupling Reaction

机译:磷酸酶偶联通用激酶测定及一级速率偶联反应动力学

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摘要

Kinases use adenosine-5′-triphosphate (ATP) as the donor substrate and generate adenosine-5′-diphosphate (ADP) as a product. An ADP-based phosphatase-coupled kinase assay is described here. In this assay, CD39L2, a nucleotidase, is added into a kinase reaction to hydrolyze ADP to AMP and phosphate. The phosphate is subsequently detected using malachite green phosphate-detection reagents. As ADP hydrolysis by CD39L2 displays a first-order rate constant, relatively simple equations are derived to calculate the coupling rate and the lagging time of the coupling reaction, allowing one to obtain kinase kinetic parameters without the completion of the coupling reaction. ATP inhibition of CD39L2-catalyzed ADP hydrolysis is also determined for correction of the kinetic data. As examples, human glucokinase, P. chrysogenum APS kinase and human ERK1, kinases specific for sugar, nucleotide and protein respectively, are assayed. To assess the compatibility of the method for high-throughput assays, Z′ factors >0.5 are also obtained for the three kinases.
机译:激酶使用5'-三磷酸腺苷(ATP)作为供体底物,并生成5'-二磷酸腺苷(ADP)作为产物。本文介绍了一种基于ADP的磷酸酶偶联激酶测定法。在该测定中,将核苷酸酶CD39L2添加到激酶反应中,以将ADP水解为AMP和磷酸盐。随后使用孔雀石绿磷酸盐检测试剂检测磷酸盐。由于通过CD39L2进行的ADP水解显示一级速率常数,因此导出了相对简单的方程式,以计算偶联速率和偶联反应的滞后时间,从而使人们无需完成偶联反应即可获得激酶动力学参数。还确定了CD39L2催化的ADP水解的ATP抑制作用,以校正动力学数据。作为实例,测定了人葡萄糖激酶,产黄青霉APS激酶和分别对糖,核苷酸和蛋白质特异的激酶人ERK1。为了评估高通量分析方法的兼容性,对于三种激酶,Z'因子均> 0.5。

著录项

  • 期刊名称 PLoS Clinical Trials
  • 作者

    Zhengliang L. Wu;

  • 作者单位
  • 年(卷),期 2008(6),8
  • 年度 2008
  • 页码 e23172
  • 总页数 9
  • 原文格式 PDF
  • 正文语种
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