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首页> 外文期刊>Journal of the Serbian Chemical Society >Determination of uric acid in human serum by an enzymatic method using N-methyl-N-(4-aminophenyl)-3-methoxyaniline reagent
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Determination of uric acid in human serum by an enzymatic method using N-methyl-N-(4-aminophenyl)-3-methoxyaniline reagent

机译:N-甲基-N-(4-氨基苯基)-3-甲氧基苯胺试剂酶法测定人血清中的尿酸

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In this work a new enzymatic method for the determination of uric acid in human serum has been developed. The method is based on the oxidative coupling reaction between the N-methyl-N-(4-aminophenyl)-3-methoxyaniline (NCP) reagent and the hydrogen – donor reagent N-ethyl-N-(2-hydroxy-3-sulfopropyl)-3-methylaniline (TOOS), in the system involving three enzymes: uricase, peroxidase and ascorbate oxidase. Using this method uric acid could be determined in concentrations up to 1.428 mmol/L, with a relative standard deviation of up to 1.8 %. The effect of the medium pH and the NCP concentration on the linearity of the chromogen absorbance versus the uric acid concentration curve was investigated. The influence of the uricase activity on the maximum rate of uric acid oxidation was also examined. The use of the NCP reagent demonstrated a more precise and more sensitive determination of the uric acid compared to the determination with 4-aminoantipyrine (4-AA) as the coupling regent. The sensitivity of the method determined from the calibration curve was 0.71 absorbance units per mmol/L of uric acid; the limit of detection was LOD = 0.0035 mmol/L and the limit of quantification was LOQ = 0.015 mmol/L of uric acid.
机译:在这项工作中,开发了一种测定人血清中尿酸的新酶法。该方法基于N-甲基-N-(4-氨基苯基)-3-甲氧基苯胺(NCP)试剂与氢-供体试剂N-乙基-N-(2-羟基-3-磺丙基)之间的氧化偶联反应)-3-甲基苯胺(TOOS),涉及三种酶:尿酸酶,过氧化物酶和抗坏血酸氧化酶。使用这种方法可以测定浓度高达1.428 mmol / L的尿酸,相对标准偏差高达1.8%。研究了介质pH和NCP浓度对发色团吸光度与尿酸浓度曲线的线性关系的影响。还检查了尿酸酶活性对尿酸氧化最大速率的影响。与使用4-氨基安替比林(4-AA)作为偶联剂的测定相比,使用NCP试剂可更准确,更灵敏地测定尿酸。根据校准曲线确定的方法的灵敏度为每mmol / L尿酸0.71个吸光度单位;尿酸的检出限为LOD = 0.0035 mmol / L,定量限为LOQ = 0.015 mmol / L。

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