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Improved RPLC determination of acyclovir using hexylamine as silanol masking agent.

机译:使用己胺作为硅烷醇掩蔽剂改进了RPLC对阿昔洛韦的测定。

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The aim of the present work is to improve the sensitivity in the RPLC determination of acyclovir [9-(2-hydroxy ethoxymethyl) guanine] (ACV) and guanine, the major impurity of the drug synthesis and one of the compounds found in the chemical degradation process of ACV. The method was applied to the quantification of drug in liposomal formulations. The most important problem for RPLC analysis of both compounds are their high pKa values, mainly guanine, and the interaction with reactive silanol groups in the stationary phase. In order to avoid these problems there are four basic strategies: (i) ionic pair reagents, (ii) deactivated silica columns, (iii) polymeric based columns and (iv) silanol masking agents. A validation protocol was followed to develop the analytical method, using a Spherisorb ODS (250 x 4.6 mm i.d.) analytical column, with a mobile phase of 95% aqueous phosphate buffer (pH 3.0) and 5% HPLC methanol pumped isocratically at 1.3 ml/min(-1), with ultraviolet detection at 254 nm. The results showed a high reproducibility in retention time value, with R.S.D. of 2.37% for ACV and 0.32% for guanine. The lowest concentration levels assayed, 0.15 microg/ml(-1) for guanine and 1 microg/ml(-1) for ACV, showed good R.S.D. in the quantification parameter (peak area) 11.0% (guanine) and 9.64% (ACV)
机译:本工作的目的是提高RPLC测定阿昔洛韦[9-(2-羟基乙氧基甲基)鸟嘌呤](ACV)和鸟嘌呤,药物合成的主要杂质以及化学中发现的化合物之一的灵敏度。 ACV的降解过程。该方法用于定量脂质体制剂中的药物。两种化合物的RPLC分析中最重要的问题是它们的高pKa值(主要是鸟嘌呤)以及与固定相中反应性硅烷醇基团的相互作用。为了避免这些问题,有四种基本策略:(i)离子对试剂,(ii)失活的硅胶色谱柱,(iii)聚合物基色谱柱和(iv)硅烷醇掩蔽剂。遵循验证方案来开发分析方法,使用Spherisorb ODS(250 x 4.6毫米内径)分析柱,流动相为95%磷酸盐水溶液(pH 3.0)和5%HPLC甲醇,等度泵入1.3 ml / min(-1),在254 nm处进行紫外线检测。结果显示保留时间值具有很高的重现性,R.S.D。 ACV为2.37%,鸟嘌呤为0.32%。测定的最低浓度水平,鸟嘌呤为0.15 microg / ml(-1),ACV为1 microg / ml(-1),显示出良好的R.S.D.在定量参数(峰面积)中为11.0%(鸟嘌呤)和9.64%(ACV)

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