RU2646160C2 - Strain of pseudomonas fluorescens for protecting plants from phytopathogenic fungi and bacteria and stimulating plant growth - Google Patents

Abstract

FIELD: microbiology.

SUBSTANCE: invention relates to microbiology. Strain of bacteria Pseudomonas fluorescens BS1506 is proposed to protect plants from phytopathogenic fungi and bacteria and stimulate plant growth. Strain is isolated from the rhizosphere of wild cereals growing on the territory of treatment plants in the town of Pushchino. Bacterial strain Pseudomonas fluorescens was deposited in the All-Russian Collection of Microorganisms of the IBPM them. G. K. Scriabin RAS under the number VKM B-2955D.

EFFECT: strain is able to suppress development of phytopathogenic fungi and bacteria due to the production of heterocyclic antibiotics phenazine-1-carboxylic acid and phenazine-1-carboxamide and stimulate plant growth by increasing the bioavailability of phosphates.

1 cl, 4 dwg, 5 tbl, 7 ex

Description

The invention relates to the microbiological industry and biotechnology, and relates to a new bacterial strain Pseudomonas fluorescens VKM B-2955D, which has the ability to inhibit the development of phytopathogenic fungi and bacteria due to the production of phenazine antibiotics and stimulate plant growth by dissolving inorganic phosphates. The proposed strain can be used to obtain on its basis a bacterial preparation.

At present, one of the most important global problems remains the provision of agricultural products to a growing population of the planet. A serious problem of crop production is phytopathogenic microorganisms and pests, resulting in 30% losses in global agricultural production annually (Tilman D., Balzer C., Hill J., Beford BL Global food demand and the sustainable intensification of agriculture // Proc. Natl. Acad . Sci. - 2011. - No. 108. - P. 20260-20264). Therefore, increasing crop yields and creating effective and environmentally friendly ways to combat phytopathogenic microorganisms is becoming an increasingly urgent task.

The analysis of world experience shows the growing role of biological plant protection products in the range of environmental measures, which, unlike chemical pesticides, are harmless to the environment and the consumer. The development and production of commercial agricultural biological products based on PGPR Pseudomonas is intensively engaged in almost all developed countries (Lucy M., Reed E., Glick BR Applications of free living plant growth-promoting rhizobacteria // Antonie van Leeuwenhoek. - 2004. - V 86. - P. 1-25).

Biological control of soil-born pathogens by fluorescent pseudomonads // Nat. Rev. Microbiol. - 2005. - V. 3(4). - P. 307-319). Наиболее хорошо изученными антибиотиками, играющими важную роль в подавлении болезней растений, являются гетероциклические феназиновые антибиотики. Известно, что феназин-1-карбоновая кислота является относительно слабыми антибиотиком (Смирнов В.В., Киприанова Е.А. Бактерии рода Pseudomonas. - Киев; Наук. думка, 1990. - 264 с.). Ее антагонистическое действие зависит от кислотности среды и значительно снижается при повышении pH. Феназин-1-карбоксамид менее подвержен влиянию кислотности среды. (Chin-A-Woeng T.F.C., G.V. Bloemberg, A.J. van der Bij, K.M.G.M. van der Drift, J. Schripsema, B. Kroon, et al. Biocontrol by phenazine-1-carboxamide-producing Pseudomonas chlororaphis PCL1391 of tomato root rot caused by Fusarium oxysporum f. sp. radicis-lycopersici // Mol. Plant Microbe Interact. - 1998. - V. 11(11). - P. 1069-1077; Patent US 20140309232). Например, при pH 5.7 феназин-1-карбоксамид был в десять раз активнее в отношении фитопатогена Fusarium oxysporum f. sp. radices-lycopersici по сравнению с феназин-1-карбоновой кислотой. Активность феназин-1-карбоновой кислоты полностью уменьшалась при повышении pH до 5.9-7, в то время как антифунгальная активность феназин-1-карбоксамида сохранялась при всех исследованных значениях pH 3.1-7.Pseudomonas PGPR is known to produce a wide range of antibiotic substances that inhibit the growth and metabolism of other microorganisms at low concentrations (Haas D., and

Biological control of soil-born pathogens by fluorescent pseudomonads // Nat. Rev. Microbiol. - 2005. - V. 3 (4). - P. 307-319). The most well-studied antibiotics that play an important role in the suppression of plant diseases are heterocyclic phenazine antibiotics. Phenazin-1-carboxylic acid is known to be a relatively weak antibiotic (Smirnov V.V., Kiprianova E.A. Bacteria of the genus Pseudomonas. - Kiev; Nauk. Dumka, 1990. - 264 p.). Its antagonistic effect depends on the acidity of the medium and decreases significantly with increasing pH. Phenazin-1-carboxamide is less susceptible to acidity. (Chin-A-Woeng TFC, GV Bloemberg, AJ van der Bij, KMGM van der Drift, J. Schripsema, B. Kroon, et al. Biocontrol by phenazine-1-carboxamide-producing Pseudomonas chlororaphis PCL1391 of tomato root rot caused by Fusarium oxysporum f. Sp. Radicis-lycopersici // Mol. Plant Microbe Interact. - 1998.- V. 11 (11) .- P. 1069-1077; Patent US 20140309232). For example, at pH 5.7, phenazine-1-carboxamide was ten times more active against the phytopathogen Fusarium oxysporum f. sp. radices-lycopersici compared to phenazine-1-carboxylic acid. The activity of phenazine-1-carboxylic acid completely decreased with increasing pH to 5.9-7, while the antifungal activity of phenazine-1-carboxamide remained at all studied pH values 3.1-7.

A known strain of bacteria Pseudomonas sp. TsMPM B-348, used to obtain the drug for the protection of cereals from the causative agent of ordinary root rot Helminthosporium sativum (USSR Author's Certificate No. 1464468).

However, this strain is ineffective for suppressing the root rot of cereals caused by a complex of fungi Fusarium spp. and Helminthosporium sativum.

A known bacterial strain Pseudomonas putida BKM B-1743D, inhibiting the growth of fungi of the genus Fusarium, and intended to obtain a drug used to stimulate plant growth and protect plants from fungal pathogens (Patent RU 1805849).

The disadvantage of the strain is a narrow spectrum of antagonistic action.

A known bacterial strain Pseudomonas species B-696, which exhibits antagonistic activity against phytopathogenic fungi Alternaria spp., Bipolaris sorokiniana, Fusarium oxysporum, Fusarium gibbosum, Fusarium sumbucinum, and a drug based on it, used to stimulate growth and protect plants from pathogenic microorganisms (pathogenic microorganisms RU 2130261).

However, there is no information on the effect of this strain on such widespread pathogens of plant diseases as Fusarium culmorum, Fusarium graminearum, Fusarium nivale, Fusarium semitectum, Fusarium solani.

A bacterial strain Pseudomonas aureofaciens IB 51 is known that exhibits antagonistic activity against phytopathogenic fungi Alternaria alternata, Bipolaris sorokiniana, Fusarium oxysporum, Fusarium gibbosum, Fusarium culmorum, Fusarium fiumarium fiumarium fiumarium fiumarium fiumarium fiumarium fiumarium fiumarium fiumarium givumium fiumarium fivarium fivarium givumium fiumarium givumarium graminearum RU 2203945).

However, there is no information on the effect of this strain on such a widespread pathogen of wheat root disease as Gaeumannomyces graminis var. tritici.

A known bacterial strain Pseudomonas aureofaciens Tx-1 (ATCC 55670) and a method for its use to control fungal and bacterial infections of plants. The method is based on the use of culture fluid of the strain Pseudomonas aureofaciens Tx-1 containing bacterial cells of this strain and biologically active metabolites, mainly phenazine-1-carboxylic acid. The method is applicable for processing dicotyledonous, monocotyledonous and coniferous plants, seedlings and seeds (Patent US 6348193).

However, there is no information on the content in the culture fluid of the bacterial strain Pseudomonas aureofaciens Tx-1 of other phenazine derivatives, in particular phenazine-1-carboxamide.

Known transgenic fluorescent strain of bacteria Pseudomonas sp. for biocontrol of fungal diseases of plants. This strain contains a locus for the biosynthesis of phenazine-1-carboxylic acid, stably integrated in the genome and its own genes for the production of the antibiotic 2,4-diacetylphloroglucin. Thus, the strain is capable of producing two antibiotics - phenazine-1-carboxylic acid and 2,4-diacetylphloroglucin. The strain suppresses phytopathogenic fungi of the genera Rhizoctonia, Gaeumannomyces graminis and Pythium (Patent US 6277625).

The disadvantage of the strain is that it is obtained as a result of genetic manipulations and is a genetically modified microorganism.

Known bioengineered strain Pseudomonas sp., For the production of a new microbiological fungicide, the main component of which is phenazine-1-carboxamide. This strain was obtained as a result of transformation of the parent producer strain of phenazine-1-carboxylic acid Pseudomonas spp. M18 or M18G recombinant plasmid carrying the phzH gene, as a result of which the bioengineered strain becomes able to produce phenazine-1-carboxamide. The strain suppresses phytopathogenic fungi of the genera Pythium, Phytophthora and Rhizoctonia (Patent US 20140309232).

The disadvantage of the strain is that it is obtained as a result of genetic manipulations and is a genetically modified microorganism.

A feature of the invention is the use as a fungicide of a culture fluid (fermentation broth) containing phenazine-1-carboxamide or an antibiotic isolated from it.

A known strain of Pseudomonas aeruginosa B5 and a method for producing ramolipid B and oxychlororaphine (phenazine-1-carboxamide) from its culture fluid. The strain exhibits antifungal activity against phytopathogenic fungi M. grisea, Alternaria mali, Alternaria panax, Alternaria slani, Botryosphaeria dothidia, Cercospora capsici, Botryosphaeria dothidia, Cercospora capsici, Cercospora kikuchi, Cladosporium, etc. (Patent KR 20010038285).

The disadvantage of the strain is that the bacterial species Pseudomonas aeruginosa belongs to opportunistic microorganisms (pathogenicity group 4).

As a prototype, the strain Pseudomonas chlororaphis NCIMB 40616 was selected, which has the ability to produce biologically active antifungal metabolites that inhibit the growth of phytopathogenic fungi of the genera Drechslera, Microdochium, Tilletia and Ustilago, which cause the most common infectious diseases of crops. The strain may be useful for treating plant seeds, vegetative plants, and plant growth media (Patent US 5,900,236).

However, the patent does not contain information on the chemical nature of the produced antifungal metabolites. It is not clear from the description whether phenazine derivatives, in particular phenazine-1-carboxylic acid and phenazine-1-carboxamide, are present in the culture fluid of the bacterial strain Pseudomonas chlororaphis NCIMB 40616. There is no information on the effect of this strain on such a common wheat pathogen as Gaeumannomyces graminis var. tritici, as well as phytopathogenic fungi of the genera Pythium, Fusarium and Rhizoctonia.

In addition, in all of the listed analogues and prototype there is no information about the ability of strains of antagonists of phytopathogenic fungi to increase the availability of insoluble phosphates.

Phosphorus is known to be the second element after nitrogen in importance in plant nutrition. It is present in the soil in the form of organic (deposits of plant, animal and microbial origin) and inorganic or mineral compounds. However, of this total pool of phosphorus compounds, only 1-5% is available to plants (Molla M., and Chowdhury AA. Microbial mineralization of organic phosphate in soil // Plant Soil. - 1984. - V. 78. - P. 393-399) . Some microorganisms, in particular mycorrhizal fungi and some rhizobacteria belonging to the genera Pseudomonas, Bacillus and Rhizobium, are able to enhance the phosphorus intake in plants (Rodriguez N., Fraga R. Phosphate solubilizing bacteria and their role in plant growth promotion // Biotechnol. Adv. - 1999. - V. 17 (4-5). - P. 319-339). The ability of rhizospheric bacteria to dissolve inorganic soil phosphates is considered one of the most important phytostimulating properties and is taken into account when using such microorganisms to create biological products.

The objective of the invention is the selection of a new natural strain of bacteria used to protect plants from phytopathogenic fungi and bacteria by synthesizing heterocyclic antibiotics phenazine-1-carboxylic acid and phenazine-1-carboxamide and stimulating plant growth by dissolving inorganic phosphates.

The technical effect that can be obtained by using the proposed strain is to improve the yield of crops and the quality of agricultural products by suppressing fungal and bacterial infections of plants and increasing the bioavailability of phosphates.

The task is achieved by identifying and using the bacterial strain Pseudomonas fluorescens O9-10, isolated from the rhizosphere of wild cereals growing in the territory of sewage treatment plants in Pushchino (Moscow region).

The strain Pseudomonas fluorescens O9-10 has laboratory number BS1506 and is deposited in the All-Russian collection of microorganisms IBPM them. T.K. Scriabin RAS under the number VKM V-2955D.

The strain Pseudomonas fluorescens VKM B-2955D is characterized by the following features.

Cultivation media

The strain grows well on the following media (g / l, ml / l): LB (bacto-tryptone - 10, yeast extract - 5, sodium chloride - 10, pH 7.2); King B (peptone - 20, K ₂ HPO ₄ - 1.5, MgSO ₄ × 7H ₂ O - 1.5, glycerol - 10); tryptose-soybean agar (tryptose-soybean extract - 30); mineral synthetic medium M9 (Na ₂ HPO ₄ - 6, KH ₂ PO ₄ - 3, NH ₄ Cl - 1, NaCl - 0.5, 1M MgSO ₄ - 2,1M CaCl ₂ - 1, glucose - 2).

Colony morphology

The colony morphology on nutrient media was determined after 4-5 days of growth at 28 ° C.

Colonies on LB medium are round with smooth edges, smooth, slightly convex, opaque, beige, not mucous, diameter 5-6 mm, pigment is not pronounced.

On King B medium, the colonies are green, the pigment is intensely green fluorescent, diffuses into the medium.

Cultural and morphological features

The cells are mobile, rod-shaped, with polar flagella, gram-negative, do not form a spore.

Physiological and biochemical characteristics

Obligate aerob, temperature optimum of growth of 24-30 ° C, grows at 4 ° C, grows within the pH range from 5.2 to 8.0; pH optimum for growth is 6.8-7.4.

It does not need additional growth factors (prototroph).

As a carbon source, it uses glucose, trehalose, glycerin, succinic acid, benzoic acid, anthranilate, meso-inositol.

Thins gelatin

Proven unused carbon sources: xylose, sucrose, hippuric acid, phenylacetic acid, adipic acid, salicylic acid, naphthalene, phenanthrene, camphor, hexadecane, caprolactam.

Antibiotic resistance

The strain is resistant to carbenicillin (1000 μg / ml), ceftazidime (20 μg / ml), cefepime (20 μg / ml), meropenem (20 μg / ml), gentamicin (20 μg / ml), amikacin (30 μg / ml ), tobramycin (50 μg / ml), streptomycin (50 μg / ml), tetracycline (30 μg / ml), chloramphenicol (100 μg / ml). Sensitive to kanamycin (50 mcg / ml). The maximum concentration of the antibiotic in μg / ml in LB agar medium at which bacteria growth is observed is indicated in parentheses.

Chromosomal resistance to heavy metals

The strain has an initial level of chromosomal resistance to zinc and copper. The maximum tolerated concentration (MTK) of zinc is 2.0 mM, copper - 1.5 mM.

The strain is capable of growth at elevated concentrations (5%) of sodium chloride in the growing medium.

Principal physiological properties

The strain has fungicidal and bactericidal properties.

Principal specific products.

The strain synthesizes heterocyclic phenazine antibiotics phenazine-1-carboxylic acid and phenazine-1-carboxamide, hydrogen cyanide (HCN), siderophores, indolyl-3-acetic acid.

Biosafety Information

The strain is not pathogenic for warm-blooded animals and humans. It does not have phytopathogenic activity, as evidenced by the absence of maceration on the potato slices when applied to them with an injection of live strain cells.

The bacterial strain Pseudomonas fluorescens VKM B-2955D is stored on plates with LB medium at 4-7 ° C. Reseeding on fresh environments - once a month. It can be stored for at least 1 year in 15% glycerol at -20 ° C, for no more than 10 years under liquid paraffin in a semi-liquid medium of the following composition (g / l): nutrient broth (Difco) - 4, NaCl - 5, agar - 6, pH 6.8.

The bacterial strain Pseudomonas fluorescens VKM B-2955D inhibits the growth of the following phytopathogenic fungi: Gaeumannomyces graminis var. tritici strain Ggt 1818, Gaeumannomyces graminis var. tritici strain 119 (2), Gaeumannomyces graminis var. tritici strain PIT, Fusarium graminearum, Fusarium moniliforme, Fusarium oxysporum, Fusarium geterosporum, Fusarium culmorum, Fusarium sporotrichum, Fusarium solani VKM F-2316, Rhizoctonia solanumllium fibrium albium albium fibrium alba albium albium albium albium alba albium albium alba albom F-4284.

The bacterial strain Pseudomonas fluorescens VKM B-2955D inhibits the growth of phytopathogenic bacteria Pectobacterium carotovorum B15 and Burkholderia caryophylli VKM B-1296.

The bacterial strain Pseudomonas fluorescens VKM B-2955D can be used to protect plants from a wide range of phytopathogenic infections.

The possibility of implementing the proposed objects of the invention is confirmed by the following examples, but is not limited to.

Example 1. Obtaining biomass of the bacterial strain Pseudomonas fluorescens VKM B-2955D.

The strain is grown for 24 hours at 24-30 ° C with aeration to a titer of 10 ⁹ CFU / ml on LB medium of the following composition (g / l): peptone - 10, yeast extract - 5, sodium chloride - 10, tap water - 1 l If necessary, the cell suspension is diluted with water to the desired titer.

Example 2. Antagonistic activity of the strain Pseudomonas fluorescens VKM B-2955D against phytopathogenic fungi of the genera Gaeumannomyces, Fusarium, Rhizoctonia, Verticillium, Sclerotonia, Alternaria.

The bacterial strain Pseudomonas fluorescens VKM B-2955D is grown in LB liquid medium for 18 h. 5 μl of the bacterial strain Pseudomonas fluorescens VKM B-2955D is sown on a Petri dish with agar medium Kanner.

5 mm in diameter at a distance of 3-3.5 cm from the center of the cup) and grown for 2 days to achieve complete synthesis of secondary metabolites. Then, a mycelial segment (5-10 mm in diameter) of the fungal strain is placed in the center of the Petri dish on the surface of the agar. The fungal mycelium is grown in advance on glucose-potato agar at room temperature for 7 days.

Petri dishes are sealed with parafilm to maintain the necessary humidity and incubated at room temperature for 5-10 days, after which the presence of a zone of inhibition of growth of phytopathogens is visually assessed (table 1, Fig. 1).

From table 1 it follows that the bacterial strain Pseudomonas fluorescens VKM B-2955D inhibits, to one degree or another, all phytopathogenic fungi used in this experiment.

In FIG. 1 shows the inhibition of mycelial growth of phytopathogenic fungi Gaeumannomyces graminis var. tritici (strain Ggt 1818) (a) and Fusarium graminearum (b) with the proposed bacterial strain Pseudomonas fluorescens VKM B-2955D (1) and rhizospheric bacterial strains (2, 3), which are not producers of phenazine antibiotics. The growth inhibitory zone of the test fungus is clearly visible near the Pseudomonas fluorescens VKM B-2955D strain (1). Rhizospheric strains (2, 3) do not inhibit the mycelium formation of the studied fungi. There are no suppression zones around them.

Example 3. The antibacterial activity of the strain Pseudomonas fluorescens VKM B-2955D.

The bacterial strain Pseudomonas fluorescens VKM B-2955D and the test microorganisms shown in Table 2 are grown in LB liquid medium for 18 hours. An undiluted culture of the test microorganisms is used, as well as its dilution 10, 100 and 1000 times. 100 μl of the culture of the test microorganisms is applied to the pre-dried agarized LB medium and evenly distributed with a microbiological spatula. Then, at a distance of 3-3.5 cm from the center of the plate, 3-5 μl of strain culture is applied.

bacteria Pseudomonas fluorescens VKM B-2955D. Cups are incubated for 7 days at 24 ° C. The presence of a zone of inhibition of growth of test microorganisms is determined visually on days 1, 3 and 7 (table 2, Fig. 2). Zones are measured in mm, measured from the edge of the colony of the bacterial strain Pseudomonas fluorescens VKM B-2955D.

From table 2 it follows that the bacterial strain Pseudomonas fluorescens VKM B-2955D inhibits, to one degree or another, all test microorganisms used in this experiment. The strain inhibits the growth of both gram-negative and gram-positive bacteria.

In FIG. Figure 2 shows the inhibition of the growth of the bacterial strain Burkholderia caryophylli VKM B-1296 (0 dilution) with the proposed bacterial strain Pseudomonas fluorescens VKM B-2955D (1) and rhizospheric bacterial strains (2, 3), which are not producers of phenazine antibiotics. The zone of inhibition of growth of the test microorganism is clearly visible near the Pseudomonas fluorescens VKM B-2955D strain (1). Rhizospheric strains (2, 3) do not inhibit the development of the test microorganism. There are no suppression zones around them.

Example 4. The ability of the bacterial strain Pseudomonas fluorescens VKM B-2955D to produce phenazine antibiotics.

Qualitative analysis of phenazine antibiotics (phenazine-1-carboxylic acid and phenazine-1-carboxamide) is carried out using the method of thin-layer chromatography (TLC). To extract phenazines, bacterial cultures were grown for 72 hours at 24 ° C in 10 ml of tryptose-soy broth or King B. After sedimentation of the cells (5 min, 10,000 rpm), the supernatant was acidified with HCl to pH 2 and extracted with an equal volume chloroform. After centrifugation, the chloroform fraction was collected and evaporated.

For TLC, samples were dissolved in 20 μl of acetonitrile. 3-5 μl of the solution is applied to silica gel plates with a fluorescence analyzer (Fluka, Germany) and a chloroform: ethyl acetate solvent system is used:

formic acid (5: 4: 1). Phenazine-1-carboxylic acid and phenazine-1-carboxamide (Sigma, USA) are used as standards.

In FIG. Figure 3 shows thin-layer chromatography of phenazine-1-carboxylic acid (Rf value 0.8) (4), phenazine-1-carboxamide (Rf value 0.7) (5), culture fluid extracts (6, 7) rhizospheric strains that are not antagonists of phytopathogenic fungi and producers of phenazine antibiotics and culture fluid extract (8) of the proposed bacterial strain Pseudomonas fluorescens VKM B-2955D.

TLC shows that a number of compounds accumulate in the culture fluid extract (8) of the proposed bacterial strain Pseudomonas fluorescens VKM B-2955D. The two compounds (Rf values 0.8 and 0.7) are identical in color to visible light, UV fluorescence, and Rf in identical phenazine-1-carboxylic acid (4) and phenazine-1-carboxamide (5). With prolonged cultivation of the proposed bacterial strain Pseudomonas fluorescens VKM B-2955D, phenazine antibiotics may precipitate in the form of blue-green crystals in the culture medium.

The extracts of the culture fluid (6, 7) of rhizospheric strains that are not antagonists of phytopathogenic fungi do not accumulate the indicated phenazine antibiotics. Spots with Rf values of 0.8 and 0.7 are absent on the TLC plate.

Example 5. The ability of the bacterial strain Pseudomonas fluorescens VKM B-2955D to dissolve inorganic phosphates.

The ability to dissolve inorganic phosphates is evaluated by the appearance of transparent zones (halo) during the cultivation of bacteria on a selective mineral medium with calcium hydroxyapatite (Ca ₁₀ (PO ₄ ) ₆ (OH) ₂ ) or calcium phosphate (Ca ₃ (PO ₄ ) ₂ ) as the only source of phosphorus.

A selective medium with calcium hydroxyapatite contains in g / l: MgSO ₄ × 7H ₂ O - 2; NaCl - 1; NH ₄ Cl - 10; tris (tris (hydroxymethyl) aminomethane) -1; glucose - 10, agar - 15, calcium hydroxyapatite solution - 5%. A solution of calcium hydroxyapatite (Ca ₁₀ (PO ₄ ) ₆ (OH) ₂ ) (Calcium phosphate hydroxide, type 3, Sigma, USA) is prepared in advance. For this, 10 g of calcium hydroxyapatite are washed 10-15 times with deionized water. The washed calcium hydroxyapatite is poured into 100 ml of deionized water and sterilized. To the expanded agar medium (20 ml), add 1 ml of the prepared suspension of calcium hydroxyapatite, mix intensively on a shaker and pour into Petri dishes.

Bacterial strains are grown in advance on complete LB medium. Biomass is resuspended in physical. solution (0.85% NaCl) and apply 3-5 μl to plates with agarized selective medium with calcium hydroxyapatite or calcium phosphate. After 5-7 days of cultivation, the appearance of transparent zones (halo) around the bacterial culture is determined.

In FIG. Figure 4 shows that the largest dissolution zone of calcium hydroxyapatite (more than 3 mm) is observed near the colony of the proposed bacterial strain Pseudomonas fluorescens VKM B-2955D (1).

Rhizospheric bacterial strains that are not capable of dissolving phosphates and are not producers of phenazine antibiotics can grow on this selective medium, but enlightenment zones either do not form (2, 3) or form within a radius of 0.5-1 mm from them (9).

Example 6. Determination of phytostimulating ability of the proposed bacterial strain Pseudomonas fluorescens VKM B-2955D.

The ability to stimulate the growth of plant roots (wheat, rye, mung bean (golden beans)) is determined in Petri dishes by comparing the seeds treated with the proposed strain with the control ones. The seeds of plants of the same size (20 pieces) are placed in a test tube with a 100-fold diluted culture of the bacterial strain Pseudomonas fluorescens VKM B-2955D and shake them until completely wetted. Seeds are incubated at room temperature for 2 hours, then evenly laid out in Petri dishes on the surface of a paper filter moistened with a 10 mm solution of magnesium sulfate. As control use seeds placed in a test tube with 10 ml of a solution of 10 mm magnesium sulfate without bacteria. The plates are incubated in a thermostat at 24 ° C in the dark for 3 days. Measure the average and total length of the roots of inoculated seedlings and compare with the control (untreated seedlings). The experiment is repeated 3 times.

From table 3 it can be seen that the length of the roots of seedlings treated with the proposed bacterial strain Pseudomonas fluorescens VKM B-2955D is longer compared to control plants. The average root length in processed mash seedlings increases by 10%, in rye by 45%, in wheat by 54%.

Example 7. The effect of treatment with the strain Pseudomonas fluorescens VKM B-2955D on the development of fungal diseases and yield of winter wheat in field experiments.

The studies were conducted on the experimental field of the municipal budget institution "Accomplishment" of the urban district of Pushchino, Moscow region. Type of soil - gray forest.

The sowing of winter wheat seeds of the Governor of the Don variety was carried out in the first ten days of September with a sowing rate of 2.5 c / ha to a depth of 5-7 cm in black steam.

The preparation of a pilot sample of a biological product based on the proposed strain of Pseudomonas fluorescens VKM B-2955D is carried out as follows. The strain is grown for 24 hours at 24-30 ° C with aeration to a titer of 10 ⁹ -10 ¹⁰ CFU / ml in LB medium. The culture is diluted 100 times with tap water to a titer of 10 ⁷ -10 ⁸ CFU / ml Winter wheat plants are sprayed using a knapsack sprayer twice during the growing season: in the tillering phase - the beginning of the exit to the tube (May 5) and on the flag sheet (May 31) in the normal flow rate of a working solution of 300 l / ha. For comparison, a commercial biological product Pseudobacterin-2 based on the bacterial strain Pseudomonas aureofaciens BS1393 is used. Plants without treatment are used as a control. Spraying plants is carried out in the morning with no wind. The plot area is 20 m ² , the repetition is 4-fold.

Observations of affected plants and their accounting are carried out throughout the growing season before treatments and after treatments (on 10-20 days). Accounting for leaf diseases is carried out by sampling and subsequent analysis in the laboratory.

The intensity of the development of the disease is determined by the area of the affected surface of the leaves, covered with spots, plaques, pustules. The development of the disease is taken into account eyeballs, using a special palette that increases the accuracy of the assessment, and determine the percentage of the surface of the affected tissue of the plant.

The prevalence of the disease is established by the generally accepted formula:

P (%) = (n × 100) / N, where

P is the prevalence of the disease;

n is the number of diseased plants in the samples;

N is the total number of plants in the samples.

Accounting for the technical (biological) effectiveness of the protective measure is carried out according to the formula:

B = ((P _to -P _o ) × 100) / P _to , where

B - biological effectiveness in%;

P _to - an indicator of the development of the disease in the control;

P _o - a similar indicator in the experience.

Economic efficiency is determined by the difference in the actual yield on the cultivated and control plots in terms of 1 ha according to the formula:

X = ((AB) × 100) / A, where

X - economic efficiency in%;

A - crop on the cultivated field;

In - harvest in control.

Harvesting grain of winter wheat is carried out on July 7 in the phase of full ripeness using the platform method (4 × 0.25 m ² in plots). A mass of 1000 grains is determined according to GOST 10842-89. Disease and Grain Productivity Data

subjected to mathematical processing by analysis of variance.

The results of treating winter wheat with the proposed bacterial strain Pseudomonas fluorescens VKM B-2955D for infection of plants with fungal pathogens are presented in table 4.

The table shows that the prevalence of fungal diseases on the flag leaf of plants treated with the proposed strain was lower after the first and second treatments (23 and 60%, respectively) compared with the control (47 and 72%, respectively).

The prevalence of fungal diseases on the first leaf in plants treated with the proposed strain, after the first treatment, is also lower (81%) compared with the control (91%).

The biological effectiveness of the proposed bacterial strain Pseudomonas fluorescens VKM B-2955D is comparable to the commercial drug Pseudobacterin-2 (table 4).

The effect of treatments with the proposed strain of Pseudomonas fluorescens VKM B-2955D on winter wheat productivity is presented in table 5. The yield increase during processing of the proposed strain of Pseudomonas fluorescens VKM B-2955D is 2.1 kg / ha (6.9%) compared with the control and higher compared to the commercial biological product Pseudobacterin-2 (1.2 kg / ha, 2.9%). The economic efficiency of the proposed strain in these conditions is 6.4%.

Thus, the proposed bacterial strain Pseudomonas fluorescens VKM B-2955D has the ability to inhibit the growth of a wide range of phytopathogens and dissolve phosphates. The strain is not toxic to plants in concentrations recommended for treatments. It can be used to create on its basis a biological product designed to protect plants from phytopathogenic fungi and bacteria and stimulate plant growth by increasing the bioavailability of phosphates.

Claims (1)

The bacterial strain Pseudomonas fluorescens BS1506, deposited in the All-Russian collection of microorganisms IBPM them. G.K. Scriabin RAS under VKM number B-2955D, for protecting plants from phytopathogenic fungi and bacteria and stimulating plant growth.

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