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Poster presentation 146 FLAVONOIDS FROM THE PLANT GERANIUM SANGUINEUM N.Sh. Berdiev, J.F. Ziyavitdinov, Sh.I. Salikhov Institute of Bioorganic Chemistry named after A.S. Sadykov Academy of Sciences of Uzbekistan. e-mail: nodir2884@mail.ru The plants of Geraniaceae family are widespread in the world, it includes from five to eleven genera and a total of about 750 species. Currently, 18 different species of this family were determined in the flora of Uzbekistan. In folk medicine, aqueous and alcoholic extract of Geranium sanguineum root has been used against cold and infectious diseases since ancient times. Geranium sanguineum has been used to treat inflammation, anemia, diarrhea, respiratory infections, and other ailments. Immunostimulatory and anti-inflammatory properties of flavonoids obtained from the root extract have been detected so far. Taking this into account, we aimed to analyze the flavanoids of the above-ground part of the Geranium sanguineum plant grown in the Tashkent Botanical Garden. For analysis, a 10 g of the ground part of the dried Geranium sanguineum plant was taken and extracted in 100 ml of 40% ethyl alcohol solution for 2 hours. An aliquot of the extract was filtered . Chromatography-mass spectrometry of polyphenols was performed on an Agilent Technologies LC/MS/MS Q- TOF 6420B under the following conditions: samples were dissolved in 0.1% TFA and injected into the mass spectrometer using an Agilent Technologies 1260 pump with a flow rate of 15 μl/min and Agilent Technologies Micro WPS autosampler, 2-5 µl each. Separation was performed using a Zorbax SB C18, 5 µm column (150 µm × 0.5 mm). Mobile phase: A - 0.1% formic acid, B - acetonitrile + 0.1% formic acid. The sorbed polyphenols were desorbed from the column at a flow rate of 15 μl/min with the following mobile phase gradient: concentration of solution B: 5% – 3 minutes, 80% – 25-30 minutes, 5% - 35 minutes. Ionization source – electrosprayer; dryer gas flow rate (N2) – 7 l/min, temperature 300 °С; current strength in the skimmer cone 65 V, in the fragmentator 175 V; mass detection range MS within 100 – 3000 m/z, under conditions MS/MS MS 50 – 2400 m/z . The ionization method is negative. To identify the compounds, they were previously characterized using MS data, along with the interpretation of the MS/MS spectra compared to those found in the literature. The following public databases were searched during the identification process: ChemSpider (http://www.chemspider.com), SciFinderScholar (https://scifinder.cas.org), KeggLigand Database (http://www.genome.jp/kegg/ligand.html) and Phenol-Explorer (www.phenol-explorer.eu). The resulting extract was found to contain the following individual substances: pelargonidin 3- O -(6''-succinyl-glucoside) 533.316 m/z , 5,6,7,4'-tetramethoxyflavone 343.164 m/z , peonidin 3- O -(6''-p-coumaroyl-glucoside) 609.284 m/z , cyanidin 3- O - xylosyl-rutinoside 727.38 m/z , 3,5-di- O -galloyl-4- O -digalloylquinic acid 799.27 m/z , quercetin-3- O -glucoside 448.15 m/z , geraniin 951.08 m/z , kaempferol 3- O -rhamnoside 431.37 m/z , betagarin 328.316 m/z , acanthocarpan 328.316 m/z , 4'-hydroxy-5,6,7- trimethoxyflavone 328.316 m/z , 7-hydroxy-2',4',5'-trimethoxyisoflavone 328.316 m/z , kaempferol 286.236 m/z , luteolin 286.236 m/z , aureusidin 286.236 m/z , syringetin 346.288 m/z , axillarin 3,6-dimethyl ether 346.288 m/z , 3-hydroxyphloretin 2’- O – glucoside 452.25 m/z , kaempferol 3- O -beta- D -xyloside 418.394 m/z , corilagin 634.452 m/z . |