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基于流动注射分析的化学偶联分光光度法测定:通过对肌酸、氨、肼、磷酸盐和连二亚硫酸盐的测定来测定固氮酶。

Chemically coupled spectrophotometric assays based on flow injection analysis: determination of nitrogenase by assays for creatine, ammonia, hydrazine, phosphate, and dithionite.

作者信息

Davis L C, Radke G A

出版信息

Anal Biochem. 1984 Aug 1;140(2):434-42. doi: 10.1016/0003-2697(84)90190-8.

DOI:10.1016/0003-2697(84)90190-8
PMID:6592986
Abstract

Micromethods of direct chemical coupling have been developed for several different enzyme reactions, using the principles of flow injection analysis. Samples of 1-25 microliters are injected into a flowing stream of color-forming reagents and the peak of color change is measured after about 1 min. Alternatively, continuous slow infusion of a reacting system (5-100 microliters/min) gives a continuous change of color which can be monitored to derive enzyme reaction rates. These techniques are highly sensitive, requiring a few nanomoles of the substance being detected. Phosphate, ammonia, dithionite, creatine, and hydrazine have been measured. Consumption of reagents is less than 75 ml per hour; typical sample throughout is 30-40 samples per hour by the injection method, and 5 samples per hour by continuous infusion. The procedure has been applied to nitrogenase, continuously monitoring creatine produced from creatine phosphate by creatine kinase which is used to supply a constant level of ATP for nitrogenase. In this way nitrogenase activity can be determined over a wide range of enzyme concentrations. Production of inorganic phosphate directly from ATP, by injection of formaldehyde-quenched samples, was used when coupling to creatine kinase was not possible. Both injection of aliquots and continuous infusion were used for detection of hydrazine during nitrogenase reduction of azide, and the injection method has been used for ammonia assay during dinitrogen reduction. Dithionite oxidation was measured directly from decolorization of iodine, after trapping both dithionite and bisulfite with formaldehyde.

摘要

利用流动注射分析原理,已为几种不同的酶反应开发出直接化学偶联的微量方法。将1 - 25微升的样品注入形成颜色的试剂流中,约1分钟后测量颜色变化的峰值。或者,以连续缓慢注入反应体系(5 - 100微升/分钟)的方式会产生颜色的连续变化,可对其进行监测以得出酶反应速率。这些技术高度灵敏,只需检测几纳摩尔的物质。已对磷酸盐、氨、连二亚硫酸盐、肌酸和肼进行了测量。试剂消耗量每小时少于75毫升;采用注射法时,典型的样本通量为每小时30 - 40个样本,连续注入法为每小时5个样本。该方法已应用于固氮酶,通过连续监测肌酸激酶由磷酸肌酸产生的肌酸,肌酸激酶用于为固氮酶提供恒定水平的ATP。通过这种方式,可以在很宽的酶浓度范围内测定固氮酶活性。当无法与肌酸激酶偶联时,通过注入甲醛淬灭的样品来直接检测由ATP产生的无机磷酸盐。在叠氮化物被固氮酶还原过程中,采用注射等分试样和连续注入两种方法来检测肼,并且在二氮还原过程中采用注射法来测定氨。在用甲醛捕获连二亚硫酸盐和亚硫酸氢盐后,通过碘的脱色直接测量连二亚硫酸盐的氧化。

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