首页> 外文期刊>Clinical Chemistry: Journal of the American Association for Clinical Chemists >Fully enzymatic method for determining 1,5-anhydro-D-glucitol in serum.
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Fully enzymatic method for determining 1,5-anhydro-D-glucitol in serum.

机译:完全酶法测定血清中1,5-脱水D-葡萄糖醇的方法。

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摘要

We have developed a fully enzymatic method to measure 1,5 anhydro-D-glucitol (1,5-AG) in serum through use of pyranose oxidase (PROD: EC 1.1.3.10), glucokinase (EC 2.7.1.2), and an ATP-regenerating system. In a previous report (Clin Chem 1989;35:2039-43) the glucose interfering with the measurement of 1,5-AG was removed with a minicolumn. In the method used here, glucokinase and an ATP-regenerating system efficiently convert glucose to the unreactive compound, glucose 6-phosphate, making the method selective for 1,5-AG. The hydrogen peroxide produced in the oxidation of 1,5-AG by PROD is detected with a standard enzymatic color-developing system. The within-run and day-to-day precision (CV) of this method was 0.52-1.29% and 1.17-4.48%, respectively. The correlation (r) between the results obtained with our proposed method (y) and those obtained with the mini-column method (x) was 0.998 (y = 1.007x + 0.493 mg/L; n = 100; Sy/x = 0.641 mg/L). This newly developed method allows quicker and easier measurement of serum 1,5-AG than previously described methods.
机译:我们已经开发出一种完全酶促方法,可通过使用吡喃糖氧化酶(PROD:EC 1.1.3.10),葡萄糖激酶(EC 2.7.1.2)和血清中的1,5-脱水D-葡萄糖醇(1,5-AG)来测定血清中ATP再生系统。在以前的报告(Clin Chem 1989; 35:2039-43)中,用小柱去除了干扰1,5-AG测定的葡萄糖。在此处使用的方法中,葡萄糖激酶和ATP再生系统可将葡萄糖有效地转化为非反应性化合物6-磷酸葡萄糖,从而使该方法对1,5-AG具有选择性。用标准酶显色系统检测通过PROD氧化1,5-AG产生的过氧化氢。该方法的内部运行精度和日常精度(CV)分别为0.52-1.29%和1.17-4.48%。用我们提出的方法(y)获得的结果与用小柱方法(x)获得的结果之间的相关性(r)为0.998(y = 1.007x + 0.493 mg / L; n = 100; Sy / x = 0.641毫克/升)。与先前描述的方法相比,这种新开发的方法可以更快,更轻松地测量血清1,5-AG。

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