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Rapid Electrochemical Enzyme Assay with Enzyme-Free Calibration

机译:无酶校准的快速电化学酶测定

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摘要

The internally calibrated electrochemical continuous enzyme assay (ICECEA, patent pending) was developed for the fast determination of enzyme activity unit (U). The assay depends on the integration of enzyme-free preassay calibration with the actual enzyme assay in one continuous experiment. Such integration resulted in a uniquely shaped amperometric trace that allowed for the selective picomolar determination of redox enzymes. The ICECEA worked because the preassay calibration did not interfere with the enzyme assay allowing both measurements to be performed in succession in the same solution and at the same electrode. The method displayed a good accuracy (relative error, <3%) and precision (relative standard deviation (RSD), <3%) when tested with different working electrodes (carbon nanotubes/chitosan, glassy carbon, platinum) and enzymes (alcohol dehydrogenase, ADH; lactate dehydrogenase, LDH; xanthine oxidase, XOx; glucose oxidase, GOx). The limit of detection for the ADH, LDH, XOx, and GOx was equal to 0.18, 0.14, 0.0031, and 0.11 U L~(-1) (or 4.2, 0.72, 89, and 6.0 pM), respectively. The simplicity, reliability, and short analysis time make the ICECEA competitive with the optical enzyme assays currently in use.
机译:开发了内部校准的电化学连续酶测定法(ICECEA,正在申请专利),用于快速测定酶活性单位(U)。该测定取决于一次连续实验中无酶预测定校准与实际酶测定的整合。这种整合导致独特形状的安培曲线,从而可以选择性皮摩尔确定氧化还原酶。 ICECEA之所以起作用,是因为测定前的校准不会干扰酶的测定,从而可以在相同的溶液和相同的电极上连续进行两次测量。当使用不同的工作电极(碳纳米管/壳聚糖,玻璃碳,铂)和酶(酒精脱氢酶)进行测试时,该方法显示出良好的准确度(相对误差,<3%)和精密度(相对标准偏差(RSD),<3%)。 ; ADH;乳酸脱氢酶LDH;黄嘌呤氧化酶XOx;葡萄糖氧化酶GOx)。 ADH,LDH,XOx和GOx的检出限分别等于0.18、0.14、0.0031和0.11 U L〜(-1)(或4.2、0.72、89和6.0 pM)。简单性,可靠性和短分析时间使ICECEA可以与当前使用的光学酶测定法竞争。

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