UA139909U - PENICILLIUM RESTRICTUM STRAIN - PRODUCER OF EXTRACELLULAR <font face = "Symbol"> a </font> -L-RAMNOSIDASE - Google Patents

Abstract

The strain Penicillium restrictum - producer of extracellular -L-rhamnosidase is registered in the Depository of the Institute of Microbiology and Virology. D.K. Zabolotny National Academy of Sciences of Ukraine under the number 1MB F-100139.

Description

A useful model belongs to the biotechnological industry, namely to the production of a new strain, a producer of the c-I -rhamnosidase enzyme. a-I-Rhamnosidase |KF 3.2.1.40) - a reagent that cleaves terminal unreduced residues

Y-rhamnose, present in both synthetic and natural glycosides, oligo- and polysaccharides, various glycoconjugates, derivatives of flavonoids - rutin, neohesperidin, hesperidin, naringin, quercitrin, saponins - sginsenosides; terpene glycosides - asiaticosides.

Deramnosylation of natural glycosides can lead to an increase in their biological activity and positively affect the quality of consumer products. Thanks to these properties, o-II-rhamnosidases are used in food technologies and technologies for the creation of drugs for the treatment of cardiovascular diseases, drugs with antiviral and immunotropic effects. By hydrolyzing terpene glycosides, the enzyme promotes the release of aromatic compounds that enhance the aroma of grape juices and wines, and the hydrolysis of naringin, hesperidin, and narirutin improves the quality of citrus juices, which explains the need for the enzyme in the food industry.

It is known that a-I-rhamnosidase is able to be synthesized by some mammals (1|, plants |2), as well as microorganisms - representatives of various taxonomic groups, first of all, these are micromycetes, among which the largest number of producers of IZ glycosidases). However, the most studied to date are the bacterial producers of c-I-rhamnosidases, which were found among Vasiegoide5, Rizorasiegisht K-60,

Zrpipdotopa5 raiysiptorbiiih, Vasiyshe vr., Sioviiditst 5iegsogagisht (4, 5). But bacterial producers synthesize intracellular α-I-rhamnosidases, which greatly complicates their isolation, and is therefore economically unprofitable.

Today, enzyme preparations RepisShit desitrbeps and

AzregoiPiv podeg, which synthesize naringinase and hesperidinase, respectively (Zidta-Aiagisn, OA).

Since most microbial producers have a number of serious drawbacks, the search for new, more efficient producers continues to be an urgent issue, given that in

There are no producers of c-I -rhamnosidases in Ukraine at all.

The proposed strain Repisiint gevigisiisht (Zayo) 1MV E-100139 - a producer of extracellular α-Y -rhamnosidase - was isolated from the soil, which was selected in the territory of the exclusion zone of the Chernobyl nuclear power plant, near the village of Novoshepelichi. It is in the collection of living cultures of the Institute of Microbiology and Virology named after

From D.K. Zabolotny National Academy of Sciences of Ukraine.

The closest analog in terms of technical essence and the result that is achieved is a strain

Repisiysht 5 years IZI, with deep cultivation of which, under certain conditions, it is possible to obtain an enzyme preparation of a-I -rhamnosidase. The activity of the commercial drug was 0.5 Units/mg of protein (p-nitrophenyl substrate) (Zidta, Aiagisp).

Cultural-morphological and physiological-biochemical features.

The strain of the microscopic fungus RepisyShit gevigistsht 1MV E-100139 grows well on natural (wort-agar, potato-glucose agar), artificial (Sabureau agarized medium) and synthetic (Capek agarized medium) media.

On Capek medium, it grows slowly, limitedly, the colonies are folded, the edges are uneven, on the 10-14th day of growth, the diameter reaches 2.5-3.0 cm. The basal mycelium is felty, dense, airy, thin, at first white, then greenish-gray, later darkens to gray-green. Ripe - dull gray. Conidia formation is a little late (on the 10th day) and limited. The exudate is abundant: at first light yellow, then dark red. The smell is weak, indistinct. The reverse is light yellow to red-brown in color.

Conidiophores 20.0-25.0x1.5-1.8 microns, smooth. The panicles are single-lobed, often irregularly branched, the conidiophores have 1-2 branches bearing secondary panicles. Sterigmas are narrowed with a pointed neck, 5.0-5.2x1.5 microns, 6-8 pcs. Conidia globose or slightly elongated, distinctly rough in short chains, 2.0 to 3.0 µm.

The optimal temperature for growth is 24-26 "C, it can grow at temperatures from 5 to 33 "C.

On natural environments, R. gevigisishyt 1MV E-100139 grows faster. On potato-glucose agar, Saburo and wort-agar, sporulation begins on the 7-8th day of cultivation.

On a potato-glucose agar medium at a temperature of 25 "C, colonies are from white to light pink, then gray-blue to dull gray. Colonies from 3.0 to 5.0 cm in diameter, folded. Sporulation is quite limited. Exudate is abundant, first light yellow, then to dark red.The reverse is colored, from yellow to red-brown.

Conidiophores are small, up to 25.0 μmx1.8-2.0 μm, smooth, single-celled with an irregularly branched tassel, forming 1-2 branches. Sterigmas are 5.0x1.5 μm, narrowed, the neck is pointed.

Conidia from 2 to 3 μm, spherical, distinctly rough. Sometimes in short chains.

On wort-agar and agarized Saburo medium, the morphological features are the same as on potato-glucose agar, the vegetative mycelium is more developed.

Fermentation of carbon sources: absent.

Assimilation of carbon sources: assimilates - monosaccharides (arabinose, galactose, glucose, xylose, mannose, rhamnose, sorbose); disaccharides (maltose, lactose, sucrose); trisaccharides (raffinose), polyhydric alcohols (mannitol, sorbitol, dulcitol), as well as soy and corn flour.

The strain reduces nitrates to nitrites.

Physiological and biochemical properties.

Relation to carbon nutrition: the culture well assimilates monosaccharides - arabinose, galactose, glucose, xylose, I-rhamnose, disaccharides - lactose, maltose, sucrose, alcohols - dulcitol, mannitol, inositol, sorbitol, as well as soy flour. Only I -rhamnose ensures the ability of the culture to synthesize α-Й -rhamnosidase.

Relation to nitrogen nutrition: assimilates nitrate and ammonium nitrogen equally well. It assimilates peptone, glycine, urea, yeast autolysate from organic sources of nitrogen. Ammonium sulfate provides the greatest biosynthetic activity.

The strain is stored on wort agar at 5 76.

The identification was carried out according to the identifier: N.M. Pydoplychko. Penicillin / K:. Nauk, dumka, 1972. - 150 p

The strain belongs to the group of avirulent microorganisms I6-9|, incapable of invasion and changes in the internal organs of the studied warm-blooded animals - outbred white mice.

The average effective dose exceeds the recommended maximum threshold value for low-pathogenic strains of mushroom cultures: EDvoregoye"81, EDzvo vch212 million spores/mouse (71

Relationship to oxygen: obligate aerobic.

Relation to temperature: mesophyll, optimal temperature for growth and enzyme biosynthesis 20-25 76.

Relation to the acidity of the nutrient medium: the culture grows in the pH range from 5.0 to 8.0. The optimal initial pH value of the medium for enzyme synthesis is 5.0, in the process of growth and fermentation, an increase in pH to 7.0 is observed.

The nutrient medium for fermentation is a medium with the following composition, (g/l): rhamnose 8.0 (MHg)2504 2.0

КНгРОХ 1.0

M9azOxh7NgO 0.5

KSI 0.5

Ee5Og«x7NgO 0.015 initial pH value 5.0.

Cultivation of mushroom culture is carried out in deep conditions in Erlenmeyer flasks (750 ml) on a rocker, 242 rpm (aeration level 16.76 mg Og/lh.) at 20-25 "C for 5 days. Sowing

From the nutrient medium, 10 95th three-day inoculum is used. Biomass is separated by filtration, enzymatic activity is determined in the supernatant of the culture liquid. p-nitrophenyl-c-I -rhamnopyranoside is used as a substrate for determining activity.

To determine the activity of the enzyme, 0.2 ml of 01 M phosphate-citrate buffer (FCE) pH 5.0 and 0.1 ml of a 0.01 M substrate solution in FCB are added to 0.1 ml of its solution.

The reaction mixture is incubated for 10 min at a temperature of 37 "C. The reaction is stopped by adding 2 ml of a 1 M sodium bicarbonate solution. The same components are added to the control, but in the reverse order. The amount of p-nitrophenol, which was separated as a result of hydrolysis, is determined by the colorimetric method on a SF-26 spectrophotometer by absorption at 400 nm.

A unit of enzyme activity is taken as its amount, which hydrolyzes 1 μmol of substrate in 1 minute under the conditions of the experiment (101.

It was established that the level of enzymatic activity in R. hevigistitis strain 1MV E-100139 does not decrease during storage and reseeding for 1 year.

The activity of c-I-rhamnosidase, which is synthesized by the strain R. gevzigisht 1MV BE-100139, under optimal conditions in the culture liquid is equal to 4.5 units/mg of protein.

The advantage of the proposed producer is its ability to synthesize highly active and thermostable α-I-rhamnosidase, lack of seasonality and toxicity, which is technologically efficient. The enzyme preparation obtained from this culture by precipitation with ammonium sulfate (90 9o saturation) is able to work effectively at physiological pH values of the environment (3.0-7.0) with a noticeable peak of activity at pH 5.0. The enzyme is stable at the above pH values throughout the day.

The enzyme preparation is active at 4-80°C, with maximum activity at 60°C.

The thermostability of the drug at 25 "C is completely preserved throughout the day; at 60 "C - 120 min.

The proposed enzyme can find use in the food industry and medical-technological processes.

Thus, a new strain was isolated, which, in comparison with the known ones, has different cultural characteristics and is a new culture with stable biochemical properties.

Sources of information: 1. Oiap 5., Mi N., Oiap 5. Ryniisayop apa sNagasiyegigayop oi aiozsip-o-I -- natpovzidaze that kind

Imeg // Snet. apa RNagt. Viiiep. - 2005. - Mine. 53, Mo 8. -R. 911-914. 2. I osaiviii M., Eriiapo E., Sbepomese 5. Apipgadtsipope rgoiiye, apiokhidapi apa apiitisgoria ryuorepiez oi Bak ehigasiye oi RPatpib5 saiShanpisiye apa A. obishiatsv5 | Maishga! Rhodisi

Sottipisaiiopv - 2011. - Mine. b, Me9. - R. 1275-1280. 3. Madam MU., Madam R. K., Madam 5., Madam K. 0. 5. a-I-Apatpovzidave: A hemiem // Rgosev5

Viospetiviga. - 2010. - Mine. 45, Mo. 8. - R. 1226-1235. 4. Varbanets L. D., Borzova N. V. - Glycosidases of microorganisms and methods of their research /

Kyiv: Nauk. Dumka, 2010.-437 p. 5. Maplapagez R., MaiIe5 5., Katop 0., Oge)a5 M. a-Yi-Apatpovzidavze: od apa pem ipvidniv //

Ipdivipa! Epgutezvz, Zrhipdeg, 2007. - R.I 17-140. b. Medical-biological studies of production strains of microorganisms and toxic-hygienic evaluation of microbial preparations, determination of their safety and justification of hygienic standards and regulations. Methodological guidelines of the Ministry of Health of Ukraine. Kyiv, 2004. 7. Methodological recommendations "Establishment of criteria for the assessment of the pathogenicity of mycelial fungi-producers and the admissibility of their application in industry",

Angarsk, 1986. 8. Research method in veterinary mycology. Kurasova V.V. et al., M. "Kolos", 1971. 9. Handbook of microbiological research methods. Ed. Birger M., M. "Medicine", 1983. 10. Kotego S, Mapiop A., Vaziida 9. A teinoa og azzauipd patpovzidaze asiimiu oi pagipdipase /

Apa/uiisa! Viospetiviga. 1985. - Mine. 149, Me2, R.566-571.

Claims (1)

FORMULA OF USEFUL MODEL Zo Strain Repisiyisht gevigisisht - producer of extracellular so-I-rhamnosidase, registered in the Depository of the Institute of Microbiology and Virology named after D.K. Zabolotny National Academy of Sciences of Ukraine under number 1MV B-100139. 000 KomputernaverstkaL.Tsikhanovska.dD (00000000 77777 Ministry of Economic Development, Trade and Agriculture of Ukraine, (00000 12/2 M. Hrushevsky St., Kyiv, 01008, Ukraine SE "Ukrainian Institute of Intellectual Property", Glazunova St., 1 , Kyiv - 42, 01601