PL241535B1 - 6-Methyl-4'-O-β-D-(4"-O-methylglucopyranosyl)-flavanone and method of producing 6-methyl-4'-O-β-D-(4"-O-methylglucopyranosyl)-flavanone - Google Patents

Abstract

The invention consists in introducing the Isaria fumosorosea KCH J2 strain into a medium suitable for filamentous fungi. After at least 72 hours, the substrate is introduced into the culture, which is 6-methylflavanone of the formula I, dissolved in a water-miscible organic solvent. The transformation is carried out at a temperature of 20 to 30 degrees Celsius with continuous shaking for at least 96 hours. The product 6-methyl-4'-O-β-D- (4 "-O-methylglucopyranosyl) -flavanone of formula II is then extracted with a water-immiscible organic solvent and purified by chromatography.

Description

PL 241 535 B1

Description of the invention

The subject of the invention is 6-methyl-4'-O-/AD-(4"-O-methylglucopyranosyl)-flavanone of the formula 2 shown in the figure.

The subject of the invention is also a method of producing 6-methyl-4'-O-[beta]-D-(4'-O-methylglucopyranosyl)-flavanone.

6-Methyl-4'-O-β-β-(4"-O-methylglucopyranosyl)-flavanone can be used as an antioxidant and antimicrobial compound in pharmaceutical and cosmetic preparations and food products.

Natural flavonoids with one or more methyl groups occur sporadically in plants. C- and O-methylated chalcones were isolated from the Asian tree Syzygium nervosum (Cleistocalyx operculatus): (E)-4,2',4'-trihydroxy-6'-methoxy-3',5'-dimethylchalcone, (E)-2 ',4'-dihydroxy-6'-methoxy-3',5'-dimethylchalcone, (E)-2',4'-dihydroxy-6'-methoxy-3'-methylchalcone, (E)-2,2' ,4'-trihydroxy-6'-methoxy-3',5'-dimethylchalcone. These compounds showed strong inhibition against enzymes derived from two influenza virus strains: H1N1 and H9N2. They blocked the action of neuraminidases, which allow viruses to leave infected cells by breaking down their cell membranes (Dao T. T., Tung B. T., Nguyen P. H., Thuong P. T., Yoo S. S., Kim E. H., Kim S. K., Oh W. K. C-methylated flavonoids form Cleistocalyx operculatus and their inhibitory effects on novel influenza A (H1N1) neuraminidase. Journal of Natural Products 2010, 73, 1636-1642).

Similarly, (2S)-5,7,2'-trihydroxy-8-methylflavanone isolated from the Pisonia aculeate bush showed antimicrobial activity when tested in vitro with the strain Mycobacterium tuberculosis H37Rv. This compound inhibited bacterial growth at a minimum inhibitory concentration of 50 μg/cm ³ (Wu MC, Peng CF, Chen IS, Tsai IL Antitubercular chromones and flavanoids from Pisonia aculeata. Journal of Natural Products 2011, 74, 976-982).

Antibacterial and antifungal activity was also confirmed for flavonoids extracted from above-ground parts of the Eysenhardtia texana plant: (2S)-4',5,7-trihydroxy-8-methyl-6-prenylflavanone and (2S)-4,,5,7-trihydroxy- 6-methyl-8-prenylflavanone. It was proven that at a concentration of 0.1 mg/cm ³ they inhibited the growth of Staphylococcus aureus. (2S)-4',5,7-trihydroxy-8-methyl-6-prenylflavanone also slowed the growth of Candida albicans (Wachter GA, Hoffmann JJ, Furbacher TT, Blake ME, Timmermann BN Antibacterial and antifungal flavanones from Eysenhardtia texana. Phytochemistry 1999 , 52, 1469-1471).

Most flavonoids, apart from catechins, are present in plants in combination with sugars as β-glycosides. Glycosylation results in: increased solubility in water and stability of the flavonoid molecule as well as bioavailability of flavonoid compounds ingested with food. Basically, glucosides are the only glycosides that can be absorbed in the small intestine. On the other hand, flavonoids not absorbed in the small intestine and absorbed flavonoids secreted with bile are degraded along with the disruption of the ring structure by microorganisms (Hollman, P. C. Absorption, bioavailability, and metabolism of flavonoids. Pharmaceutical Biology, 2004, 42, 74-83, Plaza, M.; Pozzo, T.; Liu, J.; Gulshan Ara, K. Z.; Turner, C.; Nordberg Karlsson, E. Substituent effects on in vitro antioxidizing properties, stability, and solubility in flavonoids. Journal of Agricultural Food Chemistry, 2014, 62, 3321-3333).

Hollman et al. showed that a glucose molecule attached to the 3-position of quercetin (3,3',4',5,7-pentahydroxyflavone) increased the absorption of this compound in the small intestine to 52%, compared to 24% absorption of quercetin aglycone and 17% quercetin rutinoside (Hollman, P. C.; Bijsman, M. N. C. R; van Gameren, Y.; Cnossen, E. P. J.; de Vries, J. H.; Katan, M. B. The sugar moiety is a major determinant of the absorption of dietary flavonoid glycosides in man. Free Radical Research, 1999, 31,569-573).

The Isaria fumosorosea strain KCH J2 disclosed in patent application number P416996 is known.

In recent years, in the treatment of various diseases and their prevention, compounds of natural origin and their equivalents considered natural, obtained by microbiological transformations, are gaining more and more importance. Therefore, it is important to develop new methods for the production of biologically active compounds by biotransformation, useful for the pharmaceutical, cosmetic and food industries.

In the available literature, there is no information on the preparation of 6-methyl-4'-O-e-D-(4-O-methylglucopyranosyl)-flavanone.

The essence of the invention is 6-methyl-4'-O-e-D-(4'-O-methylglucopyranosyl)-flavanone.

PL 241 535 B1

The essence of the method consists in introducing the strain Isaria fumosorosea KCH J2 into a substrate suitable for filamentous fungi. After at least 72 hours, the substrate, 6-methylflavanone, dissolved in a water-miscible organic solvent, is introduced into the culture. The transformation is carried out at a temperature of 20 to 30 degrees Celsius, with continuous shaking, for at least 96 hours. The product is then extracted with a water-immiscible organic solvent and purified by chromatography. 6-Methyl-4'-O-e-D-(4-O-methylglucopyranosyl)-flavanone is found in the fraction of intermediate polarity, in the seventh band from the starting line.

Preferably, the ratio of the mass of added substrate to the volume of the culture is 0.1 mg:1 cm ³ .

It is also preferred that the process is carried out at a temperature of 25 degrees Celsius.

Additionally, it is preferred that the transformation is carried out for 12 days.

It is also preferred that the purification is carried out using preparative thin-layer chromatography in a system eluting with chloroform and methanol in a 9:1 volume ratio.

Following the invention, the enzyme system contained in the cells of the strain Isaria fumosorosea KCH J2 results in hydroxylation and attachment of 4-methoxy-β-D-glucose at C-4'. The product thus obtained is separated from the aqueous culture of the micro-organism in a known manner by extraction with a water-immiscible organic solvent (ethyl acetate).

The main advantage of the invention is to obtain 6-methyl-4'-O-e-D-(4"-O-methylglucopyranosyl)flavanone at room temperature and pH natural for the strain and using a non-human pathogen microorganism.

The use of biotransformation, instead of chemical synthesis, enables, in an environmentally friendly way, to obtain compounds with greater bioavailability and biological activity than the substrates used.

The invention is explained in more detail by means of an embodiment.

Example d Isaria fumosorosea KCH J2 strain is introduced into a 2000 cm 3 conical flask containing 500 cm ³ of sterile medium containing 10 g of aminobac and 30 g of glucose. After 72 hours of growth, 50 mg of 6-methylflavanone of the formula I, dissolved in 1 cm ³ of tetrahydrofuran, are added. The transformation is carried out at 25 degrees Celsius with continuous shaking for 12 days. The reaction mixture is then extracted twice with ethyl acetate, dried over anhydrous magnesium sulfate, and the solvent is evaporated. The extract obtained is purified by chromatography using a 9:1 mixture of chloroform and methanol as eluent. The product is in the intermediate polar fraction, in the seventh band from the starting line.

In this way, 20.0 mg of 6-methyl-4'-O-e-D-(4'-O-methylglucopyranosyl)-flavanone is obtained (yield 22.1%). HPLC substrate conversion >99%.

The resulting product has the following spectral data.

Claims (4)

PL 241 535 B1 Description of the signals derived from the ¹ H NMR spectrum (601 MHz, Acetone-ds). Signals derived from the flavonoid backbone Signals from sugar unit δ [ppm] J[Hz] h δ [ppm] J[Hz] h 5.53 (dd) 12.9; 2.9 2 4.97(d) 7.8 1 3.12 (dd) 16.7; 12.9 3ax 3.48 (ddd) 9.8; 5.0; 2.0 2” 2.79 (dd) 16.8; 2.9 3eq 3.63(t) 9.0 3 7.62(d) 1.5 5 3.21 (dd) 9.6; 9.1 4” 7.39(m) 7 3.48 (ddd) 9.8; 5.0; 2.0 5” 6.95(d) 8.4 8 3.83(d) 3.69(m) 12.2 6” 7.49 (m) 2' 3.56 (s) C4" oh ₃ 7.12(m) 3' 7.12(m) 5' 7.49 (m) 6' 2.31 (s) C6- CH3 Patent claims 1. 6-Methyl-4'-O-^-D-(4"-O-methylglucopyranosyl)-flavanone of formula 2. 2. A method for the production of 6-methyl-4'-O-^-D-(4'-O-methylglucopyranosyl)-flavanone, characterized in that the strain Isaria fumosorosea KCH J2 is introduced into the medium suitable for filamentous fungi, then, after for at least 72 hours, the substrate, which is 6-methylflavanone of the formula 1, dissolved in an organic solvent miscible with water, is introduced into the culture, the transformation is carried out at a temperature of 20 to 30 degrees Celsius, with continuous shaking, for at least 96 hours, then the product is extracted with a water-immiscible organic solvent and purified by chromatography, the 6-methyl-4'-O-[beta]-D-(4'-O-methylglucopyranosyl)-flavanone of formula 2 being in the intermediate polarity fraction, in the seventh lane from the starting line. 3. The method of claim The method according to claim 2, characterized in that the ratio of the mass of the added substrate to the volume of the culture is 0.1 mg:1 cm ³ . 4. The method of claim 2, characterized in that the process is carried out at a temperature of 25 degrees Celsius.