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A continuous spectrophotometric assay for inorganic phosphate and for measuring phosphate release kinetics in biological systems.

机译:连续分光光度法测定无机磷酸盐并测量生物系统中磷酸盐的释放动力学。

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摘要

A spectrophotometric method for the measurement of inorganic phosphate (P(i)) has been developed by using 2-amino-6-mercapto-7-methylpurine ribonucleoside and purine-nucleoside phosphorylase (purine-nucleoside:orthophosphate ribosyltransferase, EC 2.4.2.1). This substrate gives an absorbance increase at 360 nm on phosphorolysis at pH 6.5-8.5, and at pH 7.6 the change in extinction coefficient is 11,000 M-1.cm-1. The Michaelis-Menten constants of the two substrates with the enzyme are 70 microM for the nucleoside and 26 microM for P(i); the kcat is 40 s-1 (25 degrees C). The assay was shown to quantitate P(i) in solution at concentrations at least down to 2 microM. It can be used to measure the kinetics of P(i) release from phosphatases, such as GTPases and ATPases, by coupling the two enzymic reactions. The utility of this assay was shown by three test systems: glycerol kinase plus D-glyceraldehyde acting as an ATPase and actin-activated myosin ATPase, and myosin subfragment 1, hydrolyzing a single turnover of ATP, releasing P(i) with a rate constant the same as the steady-state ATPase activity.
机译:通过使用2-氨基-6-巯基-7-甲基嘌呤核糖核苷和嘌呤核苷磷酸化酶(嘌呤核苷:正磷酸核糖核苷转移酶,EC 2.4.2.1),开发了一种用于测定无机磷酸盐(P(i))的分光光度法。 。该底物在pH 6.5-8.5下进行磷解后,在360 nm处的吸光度增加,在pH 7.6下,消光系数的变化为11,000 M-1.cm-1。酶的两个底物的米氏常数为核苷为70 microM,P(i)为26 microM。 kcat为40 s-1(25摄氏度)。实验表明,该试剂盒可对溶液中的P(i)进行定量,其浓度至少应低至2 microM。通过偶联两个酶促反应,可用于测量从磷酸酶(例如GTPases和ATPase)释放P(i)的动力学。三种测试系统显示了该测定法的实用性:甘油激酶加D-甘油醛(充当ATPase和肌动蛋白激活的肌球蛋白ATPase),以及肌球蛋白亚片段1,水解一次ATP转换,以恒定的速率释放P(i)与稳态ATPase活性相同。

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