Isolation, identification and quantification of flavonoids from the flowers of Staphylea pinnata L.

A. Y. Sokolova, A. Poluyanov, A. Bardakov, S. Sologova, N. V. Bobkova
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Abstract

Introduction. Search for new plant species containing biologically active substances (hereinafter – BAS) is one of the leading tasks of pharmacognosy as a science. The search for flavonoid glycosides in plant raw materials is especially relevant, since they have anti-inflammatory, antioxidant, immunostimulating, as well as weak fungicidal and bacteriostatic action. Staphylea pinnata L. is an endemic plant of the Caucasus, cultivated not only in Georgia, but also in the Russian Federation in the Northern and Northwestern Caucasus. In foreign literature there are studies of antioxidant, antiproliferative and cytotoxic activity of leaf extracts of several species of S. pinnata L., as well as inhibitory activity of COX-1, COX-2 and LTB4 formation. Meanwhile, no serious Russian-language scientific studies on either the chemical composition or pharmacological action of generative organs of S. pinnata were found in the literature. This work is part of a comprehensive phytochemical study of S. pinnata. The aim of the work is to study the qualitative and quantitative composition of flavonoids in the studied object.Aim. To isolate, identify and quantify flavonoids in flowers and buds of Staphylea pinnata L.Materials and methods. Alcohol-water extracts from dried generative organs of the studied plant were used as analyzed solutions. Solutions were analyzed on a spectrophotometer SF-2000 (LLC "OKB Spectr", Russia) after sample preparation with aluminum chloride and on an HPLC Nexera-i LC-2040 (Shimadzu Corporation, Japan) equipped with a column and sample thermostat, degasser and autosampler using an individually selected elution gradient of the mobile phase (0.1 % orthophosphoric acid/acetonitrile solution). The primary data were processed using LabSolutions Single LC software (Shimadzu Corporation, Japan). Compounds from the flavonoid group were identified by retention times. Detection was carried out using a UV detector with an absorption wavelength of 365 ± 2 nm.Result and discussion. Alcohol-water extracts from flowers and buds of S. pinnata L. were obtained. Quantitative evaluation by spectrophotometry for flavonoid content was carried out. A gradient elution mode for HPLC was selected for simultaneous determination of 7 flavonoid glycosides. These chromatographic conditions allowed the identification and quantification of astragaline, cynaroside, cosmosiin, narcissin and rutin in flowers and buds of Staphylea pinnata L. Flavonoid glycosides: raponticin and kaempferol were not detected.Conclusion. Flavonoid glycosides were isolated from the generative organs of S. pinnata L., a technique for quantitative determination of flavonoid glycosides in alcohol-water extracts was developed, astragalin, cynaroside, cosmosiin, narcissin and rutin were detected and quantified.
从羽扇豆花中分离、鉴定和量化黄酮类化合物
导言。寻找含有生物活性物质(以下简称 "BAS")的植物新品种是药用植物学的主要任务之一。寻找植物原料中的黄酮苷具有特别重要的意义,因为它们具有抗炎、抗氧化、免疫刺激以及微弱的杀菌和抑菌作用。Staphylea pinnata L. 是高加索地区的一种特有植物,不仅在格鲁吉亚种植,在俄罗斯联邦的北高加索和西北高加索地区也有种植。国外文献研究了几种羽扇豆叶提取物的抗氧化、抗增殖和细胞毒性活性,以及对 COX-1、COX-2 和 LTB4 形成的抑制活性。同时,在俄语文献中还没有发现关于羽扇豆生成器官的化学成分或药理作用的严肃科学研究。这项工作是对羽扇豆进行全面植物化学研究的一部分。这项工作的目的是研究研究对象中黄酮类化合物的定性和定量组成。分离、鉴定和定量分析羽扇豆花和花蕾中的黄酮类化合物。从所研究植物的干燥生成器官中提取酒精-水提取物作为分析溶液。使用氯化铝进行样品制备后,在分光光度计 SF-2000 (LLC "OKB Spectr",俄罗斯)上对溶液进行分析;使用单独选择的洗脱梯度流动相(0.1 % 正磷酸/乙腈溶液),在配备有色谱柱和样品恒温器、脱气器和自动进样器的 HPLC Nexera-i LC-2040 (岛津公司,日本)上对溶液进行分析。使用 LabSolutions Single LC 软件(日本岛津公司)处理原始数据。根据保留时间对黄酮类化合物进行鉴定。使用吸收波长为 365 ± 2 nm 的紫外检测器进行检测。从羽扇豆花和芽中获得了水醇提取物。采用分光光度法对黄酮含量进行定量评估。采用高效液相色谱的梯度洗脱模式同时测定了 7 种黄酮苷。在这种色谱条件下,可以鉴定并定量检测出黄芪苷、蛇床子苷、波斯菊苷、水仙苷和芦丁。从羽扇豆的生成器官中分离出了黄酮苷,建立了水醇提取物中黄酮苷的定量测定技术,检测并定量了黄芪苷、蛇床子苷、波斯菊苷、水仙苷和芦丁。
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