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一种快速测定乙二醇的方法。

A rapid method for measurement of ethylene glycol.

作者信息

Blandford D E, Desjardins P R

机构信息

Department of Clinical Chemistry, Health Sciences Centre, Winnipeg, Manitoba, Canada.

出版信息

Clin Biochem. 1994 Feb;27(1):25-30. doi: 10.1016/0009-9120(94)90007-8.

Abstract

It has been reported that ethylene glycol produces a positive interference in the triglyceride assay on the DuPont aca discrete analyzer. The sensitivity of this method for ethylene glycol was exploited to develop a rapid and convenient method for detecting and quantitating ethylene glycol in serum by the use of a "triglyceride gap." This method is based on the difference between two different enzymatic triglyceride measurements; the DuPont aca triglyceride measurement, which uses lipase and glycerol dehydrogenase, and a Boehringer Mannheim method, which uses lipase, glycerol kinase, glycerolphosphate oxidase, and peroxidase. Serum pools were spiked with increasing concentrations of ethylene glycol to construct a standard curve (linear to 25 mmol/L). Patients specimens and control sera were analyzed using a one point calibration. Within-run and between-run coefficients of variation (CV) of 1.5, 2.8, 5.8, and 3.2%; 3.4%; and 12.6% were obtained at ethylene glycol concentrations of 20.13, 8.37, and 2.18 mmol/L, respectively. The sensitivity of this method is 1.0 mmol/L. Methanol, ethanol, n-propanol, isopropanol, and acetone at 100 mmol/L; 20 mmol/L 1,3-propanediol; and 10 mmol/L glycolic acid, oxalic acid, glyoxylic acid, and lactic acid did not interfere in the quantitation of ethylene glycol. High levels (10 mmol/L) of beta-hydroxybutyrate and glycerol showed a slight positive interference on the quantitation of ethylene glycol, whereas 10 mmol/L glycoaldehyde caused a substantial overestimation of serum ethylene glycol. The presence of propylene glycol, at levels ranging from 5 to 50 mmol/L, resulted in an underestimation of serum ethylene glycol.(ABSTRACT TRUNCATED AT 250 WORDS)

摘要

据报道,乙二醇对杜邦aca离散分析仪上的甘油三酯测定产生正干扰。利用该方法对乙二醇的敏感性,开发了一种通过“甘油三酯差值”快速便捷地检测和定量血清中乙二醇的方法。该方法基于两种不同的酶法甘油三酯测量值之间的差异;杜邦aca甘油三酯测量法,使用脂肪酶和甘油脱氢酶,以及勃林格殷格翰法,使用脂肪酶、甘油激酶、甘油磷酸氧化酶和过氧化物酶。向血清样本中加入浓度递增的乙二醇以构建标准曲线(线性范围至25 mmol/L)。患者样本和对照血清采用单点校准进行分析。在乙二醇浓度分别为20.13、8.37和2.18 mmol/L时,批内和批间变异系数(CV)分别为1.5%、2.8%、5.8%和3.2%;3.4%;以及12.6%。该方法的灵敏度为1.0 mmol/L。100 mmol/L的甲醇、乙醇、正丙醇、异丙醇和丙酮;20 mmol/L的1,3 - 丙二醇;以及10 mmol/L的乙醇酸、草酸、乙醛酸和乳酸对乙二醇的定量没有干扰。高水平(10 mmol/L)的β - 羟基丁酸和甘油对乙二醇的定量有轻微正干扰,而10 mmol/L的乙醇醛会导致血清乙二醇的大幅高估。浓度范围为5至50 mmol/L的丙二醇会导致血清乙二醇的低估。(摘要截短至250字)

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