A validated stability-indicating reversed-phase-UPLC method for simultaneous estimation of promethazine hydrochloride, methylparaben, propylparaben and sodium benzoate assay of cough suppressant and antihistamine liquid oral dosage forms

IF 1.8 4区医学 Q4 BIOCHEMICAL RESEARCH METHODS

Biomedical Chromatography Pub Date : 2024-07-14 DOI:10.1002/bmc.5944

Sreenivas Pippalla, Arjuna Rao Nekkalapudi, Venugopal Reddy Komreddy

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Abstract

A quick, simple, sensitive, efficient and stability-indicating reverse-phase ultraperformance liquid chromatographic method for the estimation of propylparaben, methylparaben and sodium benzoate in a pharmaceutical liquid oral formulation was developed. A Waters Acquity UPLC BEH C₁₈, 50 × 2.1 mm, 1.7 μm i.d. column was used to perform chromatographic separation with a 0.1% perchloric acid mobile phase used as solvent A and a mixture of 0.1 % perchloric acid and methanol in the ratio 20:80 (v/v), respectively, as solvent B. The experiments were carried out at a flow rate of 0.4 ml/min and the detection wavelength was 240 nm. The compartment temperature of the column was set at 40°C and the injection volume was set at 2 μl. The main aim of the research was to develop a single UPLC assay method for promethazine (active ingredient) and preservatives in the oral solution of promethazine HCl and dextromethorphan HBr that contains promethazine (active ingredient) and methylparaben, propylparaben and sodium benzoate (preservatives). An assay of dextromethorphan HBr was developed and validated by another HPLC method. The drug and preservatives were eluted at retention times of 19.3 min for promethazine HCl, 9.3 min for methylparaben, 18.9 min for propylparaben and 8.9 min for sodium benzoate. Validation of the developed method was carried out as stated by the International Conference on Harmonization guidelines ICH Q2B and under USP<1225>. The analytical parameters verified specificity/selectivity, linearity, accuracy, ruggedness and robustness. The linearity ranges of promethazine HCL, methylparaben, propylparaben and sodium benzoate were 10–100, 10–80, 1.0–8.0 and 10–80 μg/ml, respectively, with a correlation coefficient of active ingredients and preservatives of 1.00. Percentage recoveries of promethazine, propylparaben, methylparaben, and sodium benzoate were 100.0–100.2, 99.0–100.3, 99.5–98.0 and 99.0–100.0%. The validated analytical method proves that the method is specific, precise, linear, accurate, sensitive, rugged and stable, indicating the quantification of the active ingredient and all preservatives in liquid oral formulations.

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同时测定镇咳药和抗组胺药口服液剂型中盐酸异丙嗪、对羟基苯甲酸甲酯、对羟基苯甲酸丙酯和苯甲酸钠含量的稳定性指示反相-UPLC方法。

建立了一种快速、简便、灵敏、高效、稳定性好的反相超高效液相色谱法，用于口服液体制剂中苯甲酸丙酯、苯甲酸甲酯和苯甲酸钠的测定。采用Waters Acquity UPLC BEH C18, 50 × 2.1 mm, 1.7 μm i.d.色谱柱进行分离，以0.1%高氯酸为流动相作为溶剂A，以0.1%高氯酸和甲醇按20:80 (v/v) 的比例混合作为溶剂B，流速为0.4 ml/min，检测波长为240 nm。色谱柱的室温为 40°C，进样量为 2 μl。该研究的主要目的是开发一种单一的超高效液相色谱法，用于检测盐酸异丙嗪和右美沙芬口服溶液中的异丙嗪（有效成分）和防腐剂，该溶液中含有异丙嗪（有效成分）和对羟基苯甲酸甲酯、对羟基苯甲酸丙酯和苯甲酸钠（防腐剂）。通过另一种高效液相色谱法开发并验证了右美沙芬 HBr 的检测方法。药物和防腐剂的洗脱保留时间分别为：盐酸异丙嗪 19.3 分钟，对羟基苯甲酸甲酯 9.3 分钟，对羟基苯甲酸丙酯 18.9 分钟，苯甲酸钠 8.9 分钟。根据国际协调会议准则 ICH Q2B 和美国药典的规定，对所开发的方法进行了验证。分析参数验证了特异性/选择性、线性、准确性、坚固性和稳健性。异丙嗪盐酸盐、苯甲酸甲酯、苯甲酸丙酯和苯甲酸钠的线性范围分别为 10-100、10-80、1.0-8.0 和 10-80 μg/ml，活性成分与防腐剂的相关系数为 1.00。异丙嗪、对羟基苯甲酸丙酯、对羟基苯甲酸甲酯和苯甲酸钠的回收率分别为 100.0-100.2、99.0-100.3、99.5-98.0 和 99.0-100.0%。该分析方法具有特异、精密、线性、准确、灵敏、耐用和稳定等特点，可用于口服液体制剂中有效成分和所有防腐剂的定量分析。

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来源期刊

Biomedical Chromatography 生物-分析化学

CiteScore

3.60

自引率

5.60%

发文量

268

审稿时长

2.3 months

期刊介绍： Biomedical Chromatography is devoted to the publication of original papers on the applications of chromatography and allied techniques in the biological and medical sciences. Research papers and review articles cover the methods and techniques relevant to the separation, identification and determination of substances in biochemistry, biotechnology, molecular biology, cell biology, clinical chemistry, pharmacology and related disciplines. These include the analysis of body fluids, cells and tissues, purification of biologically important compounds, pharmaco-kinetics and sequencing methods using HPLC, GC, HPLC-MS, TLC, paper chromatography, affinity chromatography, gel filtration, electrophoresis and related techniques.