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用于测定血浆中辅酶Q10的改进型高效液相色谱法。

Improved high-performance liquid chromatographic method for the determination of coenzyme Q10 in plasma.

作者信息

Grossi G, Bargossi A M, Fiorella P L, Piazzi S, Battino M, Bianchi G P

机构信息

Laboratorio Centralizzato, Policlinico S. Orsola, Bologna, Italy.

出版信息

J Chromatogr. 1992 Feb 28;593(1-2):217-26. doi: 10.1016/0021-9673(92)80289-7.

Abstract

Coenzyme (Co) Q10 was dissociated from lipoproteins in plasma by treatment with methanol and extraction with n-hexane. Subsequent clean-up on silica gel and C18 solid-phase extraction cartridges with complete recovery (99 +/- 1.2%) produced a clean extract. High-performance liquid chromatographic (HPLC) separation was performed on a C18 reversed-phase column. Three simple, rapid procedures are presented: HPLC with final UV (275 nm) detection, a microanalysis utilizing a three-electrode electrochemical detector and a microanalysis with column-switching HPLC and electrochemical detection. The methods correlate very well with classical ethanol-n-hexane extraction with UV detection. The identity and purity of the Co Q10 peak were investigated and the resulting methods were concluded to be suitable for total plasma Co Q10 determination. The average level in healthy subjects was 0.80 +/- 0.20 mg/l; the minimum detectable Co Q10 plasma level was 0.05 and 0.005 mg/l for UV and electrochemical detection, respectively. The methods were applied to many samples and the plasma Co Q10 reference values for healthy subjects, athletes, hyperthyroid, hypothyroid and hypercholesterolaemic patients are given.

摘要

通过用甲醇处理并以正己烷萃取,从血浆中的脂蛋白中分离出辅酶(Co)Q10。随后在硅胶和C18固相萃取柱上进行净化,回收率达到100%(99±1.2%),得到了纯净的提取物。在C18反相柱上进行高效液相色谱(HPLC)分离。介绍了三种简单、快速的方法:采用最终紫外(275nm)检测的HPLC法、利用三电极电化学检测器的微量分析法以及采用柱切换HPLC和电化学检测的微量分析法。这些方法与经典的乙醇 - 正己烷萃取并紫外检测法具有很好的相关性。对Co Q10峰的同一性和纯度进行了研究,得出所得到的方法适用于测定血浆中总Co Q10的结论。健康受试者的平均水平为0.80±0.20mg/l;紫外检测和电化学检测的最低可检测血浆Co Q10水平分别为0.05和0.005mg/l。这些方法应用于多个样本,并给出了健康受试者、运动员、甲状腺功能亢进、甲状腺功能减退和高胆固醇血症患者的血浆Co Q10参考值。

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