A new method for measuring gentamicin in liposomes fluorometrically is described. The assay is based on the reaction between the amino groups in the gentamicin molecule and o-phthaldialdehyde (OPA), under basic pH conditions; the product's fluorescence can be read directly on a simple fluorimeter. The effects of several factors (time of reaction, volume of the OPA reagent, and product stability) were investigated. The standard curve was linear in the concentration range of 0.5-4.0microg, showing an excellent determination coefficient of r(2)=0.99. Additionally, the influence of different liposomal lipids on gentamicin determination was tested. Liposomal lipids containing no free amino groups (PC, Chol, DOTAP) have no influence on the reaction when present in the reaction mixture. In contrast, amino groups containing lipid (SA) showed intense method interference. Therefore, a method of lipid extraction was adapted to remove undesired lipids. The described method was successfully utilised during 2 years of liposomal gentamicin experiments.

译文

:描述了一种通过荧光法测定脂质体中庆大霉素的新方法。该测定基于庆大霉素分子中的氨基与邻苯二甲醛(OPA)在碱性pH条件下的反应;产品的荧光可以在简单的荧光计上直接读取。研究了几个因素的影响(反应时间,OPA试剂的体积和产品稳定性)。标准曲线在0.5-4.0microg的浓度范围内是线性的,显示出极好的测定系数r(2)= 0.99。另外,测试了不同脂质体脂质对庆大霉素测定的影响。当存在于反应混合物中时,不含游离氨基的脂质体脂质(PC,Chol,DOTAP)对反应没有影响。相反,含脂质(SA)的氨基表现出强烈的方法干扰。因此,脂质提取的方法适用于去除不需要的脂质。所描述的方法在庆大霉素脂质体实验中成功使用了2年。

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