首页> 外文期刊>Journal of Planar Chromatography-Modern TLC: JPC >Stability-Indicating Densitometric High-Performance Thin-Layer Chromatographic Method for the Quantitative Analysis of Biomarker Naringin in the Leaves and Stems of Rumex vesicarius L.
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Stability-Indicating Densitometric High-Performance Thin-Layer Chromatographic Method for the Quantitative Analysis of Biomarker Naringin in the Leaves and Stems of Rumex vesicarius L.

机译:稳定性指示光度高效薄层色谱法定量研究酸模(Rumex vesicarius L)叶片和茎中生物标记柚皮苷的含量。

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摘要

A simple, sensitive, and stability-indicating high-performance thin-layer chromatography (HPTLC)-densitometric method was developed for the quantification of biomarker naringin in the methanol extracts of stems and leaves of Rumex vesicarius. Chromatography was performed on glass-backed silica gel 60 F_(254) high-performance thin-layer chromatography (HPTLC) plates with ethyl acetate-glacial acetic acid-MeOH-H_2O (30:10:5:1, vlv) as mobile phase. Scanning and quantification were done at 275 nm. The system was found to give compact spot for naringin at R_F = 0.46 +- 0.001. The linear regression analysis data for the calibration plots showed good linear relationship with r2 = 0.998 with respect to area in the concentration range of 100-1000 ng. The regression equation of standard was found to be Y= 3.438X+ 38.485. Naringin was subjected to acid and alkali hydrolysis, peroxide oxidation, photodegradation, dry heat, moist heat, and ultraviolet (UV) treatment. The drug undergoes complete degradation under acidic treatment and mild degradation under basic and hydrogen peroxide treatment. The degraded products were well-separated from the pure drug. The statistical analysis proves that the developed method for quantification of naringin is reproducible and selective. Due to the ability of the method in separating naringin from other constituents including its degradation products, it can be employed as stability-indicating method for in-process as well as finished products in the market. It is for the first time that authors are reporting a complete stability-indicating densitometric HPTLC method for the estimation of biomarker naringin in the leaves and stems of R. vesicarius L.
机译:建立了一种简单,灵敏,可指示稳定性的高效薄层色谱(HPTLC)-光密度测定法,用于定量胡麻茎和叶甲醇提取物中生物标志物柚皮苷的含量。色谱在玻璃背硅胶60 F_(254)高效薄层色谱(HPTLC)板上进行,乙酸乙酯-冰醋酸-MeOH-H_2O(30:10:5:1,vlv)作为流动相。在275nm处进行扫描和定量。发现该系统在R_F = 0.46±0.001下给出了柚皮素的紧致斑点。校准图的线性回归分析数据显示,相对于100-1000 ng浓度范围内的面积,r2 = 0.998具有良好的线性关系。发现标准回归方程为Y = 3.438X + 38.485。柚皮苷经过酸和碱水解,过氧化物氧化,光降解,干热,湿热和紫外线(UV)处理。该药物在酸性处理下会完全降解,在碱性和过氧化氢处理下会轻微降解。降解产物与纯药物完全分离。统计分析证明,开发的柚皮苷定量方法具有可重复性和选择性。由于该方法具有将柚皮苷与其他成分(包括其降解产物)分离的能力,因此可以用作市场中制成品和成品的稳定性指示方法。这是作者首次报告完整的指示光密度的HPTLC方法,该方法可用于估计罗汉果叶片和茎中生物标记柚皮苷。

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