生物来源物中利法布汀化学和毒理学分析方法的发展

Konovalova Svetlana S., Illarionova Elena A.
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引用次数: 0

摘要

目的:建立从生物材料中分离鉴定利法布汀的方法,用于化学和毒理学分析。材料和方法。采用利法布汀、利法布汀胶囊、含利法布汀150 mg、乙醇95%、盐酸溶液0.1 M、氢氧化钠溶液0.1 M、纯净水、氨溶液10%、硫酸铵溶液20%、硫酸铵饱和、硫酸钠5%、硫酸钠饱和、氯化钠20%、氯化钠饱和溶液进行分析。有机溶剂:苯、二氯甲烷、乙醚、甲苯、氯仿、乙酸乙酯。pH用通用电离计It-1101测定。采用液液萃取法分离,紫外分光光度法检测定量。光密度用SF-2000分光光度计在层厚为1 cm的比色皿中测量。结果。在研究过程中,研究了利福布汀的光学性质,并在231±2 nm和279±2 nm处有两个吸收谱带,确定了95%的乙醇和0.1 M、浓度0.002%的盐酸溶液为最佳溶剂。实验研究了各种因素对水溶液中提取瑞福汀的影响。在pH值为2的条件下,在氯化钠饱和溶液存在下,用二氯甲烷萃取一次,萃取时间为3分钟。结论。建立了用紫外分光光度法从生物体液和器官提取物中分离和定量测定瑞福布汀的方法。
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Development of methods of chemical and toxicological analysis of Rifabutin in objects of biological origin
Objective: to develop a technique for isolating and identifying rifabutin for chemical and toxicological analysis from biological material. Materials and methods. The substance rifabutin, capsules Farbutin containing rifabutin 150 mg, ethyl alcohol 95%, hydrochloric acid solution 0.1 M, sodium hydroxide solution 0.1 M, purified water, ammonia solution 10%, solutions of ammonium sulfate 20%, ammonium sulfate saturated, sodium sulfate 5%, sodium sulfate saturated, sodium chloride 20%, sodium chloride saturated were used for analysis. Organic solvents: benzene, dichloromethane, diethyl ether, toluene, chloroform, ethyl acetate. The pH was determined using a universal ionometer It-1101. Isolation was carried out by liquid-liquid extraction, detection and quantification by spectrophotometric method in the ultraviolet region. The optical density was measured using a SF-2000 spectrophotometer in cuvettes with a layer thickness of 1 cm. Results. In the course of the study, the optical properties of rifabutin, and absorption spectra characterized by two absorption bands at 231±2 nm and 279±2 nm were studied, ethyl alcohol 95% and hydrochloric acid solution 0.1 M, concentration 0.002% as optimal solvents were determined. The effect of various factors on the extraction of rifabutin from aqueous solutions has been experimentally studied. The highest degree of extraction is achieved by dichloromethane at pH 2, in the presence of sodium chloride saturated solution, once for 3 minutes. Conclusion. Methods of isolation and quantitative determination of rifabutin by UV spectrophotometry in extracts from biological fluids and organs have been developed.
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