CN115161230B - Acid-resistant and growth-promoting bacillus - Google Patents

Acid-resistant and growth-promoting bacillus Download PDF

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CN115161230B
CN115161230B CN202210722586.7A CN202210722586A CN115161230B CN 115161230 B CN115161230 B CN 115161230B CN 202210722586 A CN202210722586 A CN 202210722586A CN 115161230 B CN115161230 B CN 115161230B
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丁伟
张淑婷
余佳敏
江其朋
齐琳
邓力元
冯长春
李斌
王勇
张宗锦
余祥文
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Southwest University
China National Tobacco Corp Sichuan Branch
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Abstract

The invention relates to acid-resistant and growth-promoting bacillus DW105, which is classified and named: bacillus pseudomycoides, accession number: cctccc NO: m2022678. The bacterial colony of the bacillus is white, round, flat, smooth and glossy at the edge, moist and opaque; the bacillus strain is in a thin rod shape, has flagellum and has positive gram staining. The DW105 has good acid resistance and aluminum resistance, the growth rate of the DW105 is obviously higher than that of Ralstonia solanacearum at the pH of 4.5 and the concentration of aluminum ions of 2.4mmol/L, the growth of tobacco can be obviously promoted, and the fresh weight of the tobacco treated by the DW105 strain is respectively increased by 128.36 percent, 83.42 percent, 136.77 percent and 97.90 percent on the fresh weight of the root, the fresh weight of the upper part of the root, the dry weight of the root and the dry weight of the upper part of the root, and the obvious growth promoting effect on tobacco plants is realized.

Description

Acid-resistant and growth-promoting bacillus
Technical Field
The invention belongs to the technical field of agricultural microorganism control, and relates to acid-resistant and growth-promoting bacillus and application thereof.
Background
Soil acidification is a major cause of soil degradation worldwide, and is increasingly prominent and serious in intensive agricultural production modes. Currently, soil acidification has become a serious global problem, severely restricting the sustainable development of modern agriculture. In recent decades, the main farmland, grasslands and forests in China also have obvious soil acidification phenomenon, the soil affected by acidification has about 2 hundred million hectares, and the soil accounts for about 23% of the total area of the soil in China, and is mainly distributed in the area of the south of Yangtze river, thereby causing serious influence on the agricultural production in the south of China. Soil acidification is generally classified internationally as follows: slightly acidic (pH 6.0-6.5), moderately acidic (pH 5.5-6.0), strongly acidic (pH 5.0-5.5), very strongly acidic (pH 4.5-5.0) and very acidic (pH < 4.5). When the pH of the soil is lower than 5.5, active aluminum ions in the soil begin to dissolve and release from the soil, and particularly when the pH of the soil is lower than 5.0, the content of the aluminum ions in the soil rises exponentially, so that the normal and healthy growth of plants is affected.
Bacterial wilt is a typical soil-borne disease caused by ralstonia solanacearum (Ralstonia solanacearum), and can cause destructive losses to various commercial crops such as tomatoes, peppers and the like besides tobacco. The field data survey finds that the strong acid soil can aggravate the occurrence of tobacco bacterial wilt, and the occurrence of tobacco bacterial wilt has close relation with community composition of soil microorganisms, and the change of the pH value of the soil can strongly influence the activity and community structure of the soil microorganisms. However, the occurrence of tobacco bacterial wilt at different acidification levels is not systematically studied, and the mechanisms of soil acidification and aluminum ions affecting the occurrence of tobacco bacterial wilt are not systematically and deeply studied. Therefore, the research system evaluates the influence of different soil acidification levels on the occurrence of tobacco bacterial wilt, explores the community characteristics of rhizosphere soil microorganisms under different acidification levels, and analyzes the relationship between the change of rhizosphere microorganisms and the occurrence of tobacco bacterial wilt; then, the relation between aluminum ions and occurrence of tobacco bacterial wilt and the influence of different aluminum stress levels in soil on the composition of tobacco bacterial communities are explored, so that the mechanism of influencing the occurrence of the tobacco bacterial wilt by different acidification levels is broken.
Disclosure of Invention
In view of the above, the invention aims to provide an acid-resistant bacterial wilt-resistant bacillus strain, and also provides related agricultural industrial application of the bacterial wilt-resistant bacillus strain, and especially provides a new idea for preventing and treating bacterial wilt and/or growing tobacco plants in acid soil.
In order to achieve the above purpose, the present invention provides the following technical solutions:
1. acid-resistant and growth-promoting bacillus DW105 is named in a classification way: bacillus pseudomycoides, deposited in China center for type culture Collection, address: martial arts, date of preservation: 2022, 5 months and 19 days, deposit number: cctccc NO: m2022678.
Further, the bacillus colony is white, round, flat, smooth and glossy in edge, moist and opaque; the bacillus strain is in a thin rod shape, has flagellum and has positive gram staining.
Further, the bacillus has higher growth rate than bacterial wilt at pH4.5-6, and has acid resistance and aluminum resistance.
2. The use of the bacillus according to any one of the above technical schemes as a microbial agent for promoting the growth of tobacco plants.
Further, the soil environment in the application is acid soil with pH of 4.5-6.0.
Further, the concentration of Bacillus in the microbial agent was 1X 10 6 cfu/mL-1×10 12 cfu/mL。
Further, the concentration of Bacillus in the microbial agent was 1X 10 8 cfu/mL。
3. The microbial agent also provides a microbial agent, and the active ingredient of the microbial agent comprises bacillus DW105.
Further, the microbial agent further comprises a strain of bacillus pseudomycosis A44 and/or Bacillus panaciterrae A68, wherein the preservation number of the bacillus pseudomycosis A44 is CCTCC NO: m2022676; the preservation number of Bacillus panaciterrae A is CCTCC NO: m2022677.
Further, in the microbial agent, bacillus is cultured to be DW105, so that bacterial suspension is obtained, and the microbial agent is in a liquid state.
The invention has the beneficial effects that: according to the invention, 110 strains are separated from tobacco rhizosphere soil under high aluminum stress conditions, DNA of the separated bacteria is extracted and sequenced, then the bacterial community composition of the tobacco rhizosphere soil is analyzed in combination with the earlier stage, finally 7 aluminum-resistant bacillus strains are selected, aluminum-resistant acid-resistant activity and antagonistic activity evaluation of the 7 strains and prevention and control effects of tobacco bacterial wilt are further researched, two strains which are strong in acid resistance and aluminum-resistant activity and have good prevention and control effects of the tobacco bacterial wilt are screened, and the separated and identified pseudomycobacillus strain is researched and researched for the first time to find out a certain antagonistic effect on the bacterial wilt. The growth rate of the bacillus pseudomycosis DW44 and Bacillus panaciterrae DW is obviously higher than that of the ralstonia solanacearum at the pH value of 4.5-6.0 and the aluminum ion concentration of 2.4mmol/L, the diameter of a bacteriostasis circle of the ralstonia solanacearum is respectively 10.72mm and 13.12mm, and the highest prevention effect on tobacco bacterial wilt in acid soil can respectively reach 75.00% and 83.33%. The bacillus pseudomycoides DW44 and Bacillus panaciterrae DW strain can effectively proliferate in an acidification environment, and provides a new biological material for improving the biological prevention and control effect in acid soil; it also has growth promoting effect on tobacco. The invention also screens an aluminum-resistant strain bacillus pseudomycosis DW105, which has remarkable growth promotion effect on tobacco growth and a certain prevention effect on tobacco bacterial wilt, and compared with a blank control, the fresh weight of tobacco roots, fresh weight of upper parts of the roots, dry weight of the roots and dry weight of upper parts of the roots treated by the DW105 are respectively increased by 128.36 percent, 83.42 percent, 136.77 percent and 97.90 percent. The three bacterial strains can be combined to prepare the composite microbial inoculum for cooperative use, so that the combined community has the comprehensive characteristics of acid resistance, aluminum resistance, disease resistance and growth promotion, and a new idea is provided for the prevention and treatment of acid soil bacterial wilt and/or the growth of tobacco plants.
Preservation information
Strain name: DW44, class naming: bacillus pseudomycoides, deposited in China center for type culture Collection, address: martial arts, date of preservation: 2022, 5 months and 19 days, deposit number: cctccc NO: m2022676.
Strain name: DW68, class naming: bacillus panaciterrae, deposited in China center for type culture Collection, address: martial arts, date of preservation: 2022, 5 months and 19 days, deposit number: cctccc NO: m2022677.
Strain name: DW105, class naming: bacillus pseudomycoides, deposited in China center for type culture Collection, address: martial arts, date of preservation: 2022, 5 months and 19 days, deposit number: cctccc NO: m2022678.
Drawings
In order to make the objects, technical solutions and advantageous effects of the present invention more clear, the present invention provides the following drawings for description:
FIG. 1 is a schematic illustration of a test process flow.
FIG. 2 shows the effect of different aluminum ion concentrations on the occurrence of bacterial wilt in tobacco.
FIG. 3 shows the incidence of bacterial wilt under treatment with different concentrations of aluminium ions.
FIG. 4 shows the content of ralstonia solanacearum in tobacco rhizosphere soil under treatment with different aluminum ion concentrations.
FIG. 5 shows the effect of each Bacillus on bacterial growth.
FIG. 6 shows the aluminium resistance activity of each of the isolated bacillus strains.
FIG. 7 shows the acid resistance of each of the isolated Bacillus strains.
FIG. 8 shows the growth promoting ability of each of the isolated Bacillus strains to tobacco.
FIG. 9 is an effect of isolated Bacillus strains on tobacco bacterial wilt.
FIG. 10 is a 16S rDNA evolutionary tree for each strain.
FIG. 11 shows colony morphology and cell morphology of strain A44.
FIG. 12 shows colony morphology and cell morphology of strain A68.
FIG. 13 shows colony morphology and cell morphology of strain A105.
Detailed Description
Preferred embodiments of the present invention will be described in detail below with reference to the accompanying drawings. The experimental methods for which specific conditions are not specified in the examples are generally conducted under conventional conditions or under conditions recommended by the manufacturer.
Example 1
1. The tested soil is collected from soil which is continuously planted for more than 5 years and does not generate bacterial wilt in cherry well village (longitude: 107 DEG 57.913', latitude: 29 DEG 10.008', altitude: 1315 m) of Runxi village, county, miao nationality, peng Shui Miao nationality, in 2019, and the soil type is silt loam. Collecting soil in a soil layer of 10-20 cm, filtering a soil sample through a screen of 2mm, removing large soil particles, plant root tissues and other impurities, and storing the sieved soil in a refrigerator at 4 ℃ for subsequent experiments.
2. Test strain and tobacco variety: the test used a CQPS-1 strain of Ralstonia solanacearum (R.solanacearum) isolated from the Tataricum disease tobacco strain of Chongqing city Peng Shui county, which is a strongly pathogenic strain. The tobacco tested was Benshi tobacco (Nicotiana benthamiana).
3. Test medium:
S-LB medium: the method is used for separating and culturing strains, peptone is 0.5g/L, yeast powder is 0.2g/L, sodium chloride is 10g/L, the strains are added into soil leaching solution with pH of 7.0, the pH is adjusted to 4.5, and the strains are sterilized for standby.
Preparing soil leaching liquid: 200g of neutral soil collected in a plant protection garden of southwest university is taken and added into 1000mL of distilled water, 150rpm is oscillated for 30min,10000rpm is centrifuged for 10min, and the supernatant is taken to pass through a filter membrane of 0.45 mu m.
Liquid medium B: 10g/L bactopeptone, 1g/L yeast powder, 1g/L casein hydrolysate, and sterilizing at 121deg.C for 20 min.
B solid medium: 10g/L of bactopeptone, 1g/L of yeast powder, 1g/L of casein hydrolysate and 15g/L of agar powder, and sterilizing at 121 ℃ for 20min for later use.
The collected Peng Shui healthy soil for planting cigarettes is divided into 4 parts, 10kg of each part is added with 1L of 2.5mmol/L, 5mmol/L and 10mmol/L aluminum sulfate solution respectively, so that the concentration of aluminum ions in the soil is LAl of low aluminum ion concentration, MAl of medium aluminum ion concentration and HAl of high aluminum ion concentration, 30mmol/L sodium sulfate solution is used as a reference, the water holding capacity of the soil is kept at about 60% by adding deionized water, the soil is treated once every month, and after 6 continuous treatments, 500g of soil is air-dried and stored for physical and chemical property detection of the soil.
Transplanting the root matrixes of the Benshi cigarettes which are cultivated in the seedling raising tray for 1 month into the treated soil respectively, wherein each treatment is repeated for 4 times, 8 plants of cigarettes are repeated each, and the seedlings are placed in a greenhouse at 25+/-2 ℃ and with 75% humidity for 14 hours for illumination and 10 hours for dark cultivation. After 14 days of culture, the tobacco plants were pulled out to obtain tobacco plant rhizosphere soil, each treatment was repeated 4 times, and the collected soil was stored at-20 ℃ until used for soil microbial DNA extraction, and the soil bacterial wilt content was detected.
Transplanting the rest soil into tobacco seedling, each treatment is repeated for 3 times, each repeated for 8 plants, and each plant is inoculated with 10mL and 1×10 after 7d 8 CFU/mL of bacterial wilt was investigated after 14d for the occurrence of bacterial wilt in different treatments of tobacco. The test process flow is shown in FIG. 1. As shown in FIG. 2, the effect of different aluminum ion concentrations on the occurrence of tobacco bacterial wilt is that high aluminum stress has no significant effect on the growth of tobacco, the incidence rate of tobacco bacterial wilt treated by medium aluminum concentration stress (MAl) is highest, and is significantly higher than other treatments, and compared with control, LAl and HAl, the incidence rate of tobacco bacterial wilt is divided69.80%, 77.95% and 52.15% (shown in fig. 3) are added respectively. Consistent with the incidence rate change rule of bacterial wilt, the content of bacterial wilt in the rhizosphere soil of the MAl treated tobacco is obviously higher than that of a control (P<0.001 LAl (p=0.0005) and HAl (P)<0.001 The average content of ralstonia in the MAl treated tobacco rhizosphere soil was 1.15, 1.11 and 1.14 times that of the control, LAl and HAl, respectively (fig. 4).
Collecting HAl, treating rhizosphere soil of healthy tobacco plants planted in soil, and preserving at a low temperature of 4 ℃ until the strain separation is completed. Adding 1g rhizosphere soil into 50mL of S-LB liquid medium to obtain suspension, adding 0.5mL of 0.1mol/L aluminum sulfate mother liquor to obtain final concentration of 1mmol/L, shake culturing at 180rpm and 28deg.C for 12 hr, standing for 30min, and diluting 1mL of the bacteria-containing supernatant to 10 -3 、10 -4 The solution was spread on a B solid medium containing 1mmol/L aluminum sulfate at a final concentration, and incubated at 28℃for 3 to 7 days until a significant colony was formed. Single colonies were picked, separated and purified by plate streaking, and after 4 times of separation streaking, the separated strains were stored at-80℃in 25% glycerol.
110 strains are separated from healthy tobacco strain rhizosphere soil treated by high aluminum stress, bacterial DNA is extracted and separated by using a bacterial genome extraction kit, bacterial 16S rRNA genes are amplified by using 27F (AGAGTTTGATCCTGGCTCAG) and 1492R (CTACGGCTACCTTGTTACGA), and PCR amplification conditions are 94 ℃ for 5min; denaturation at 94℃for 1min, annealing at 51℃for 1min, extension at 72℃for 3min,30 cycles; extending at 72℃for 10min. The PCR product was sent to the large gene sequencing company for sequencing. The sequencing results were compared for homology to sequences in the GenBank database using BLAST software. The bacterial community composition of tobacco plant rhizosphere soil is analyzed in the early stage, and the bacillus plays an important role in controlling the occurrence of tobacco bacterial wilt, and the bacillus is remarkably enriched in the tobacco rhizosphere soil subjected to high aluminum stress.
Example 2 molecular characterization of isolated strains
And selecting a 16S rRNA gene sequence of a related strain, performing systematic evolution relation analysis by adopting MEGA4.0 software, and constructing a systematic evolution tree according to a Neighbor-joining method.
The genome DNA of the strain isolated from the healthy tobacco strain rhizosphere soil sample treated with high aluminum concentration is used as a template to amplify 16SrDNA fragments, the amplified PCR fragments are sequenced, the sequencing result is subjected to Blast comparison with sequences in GenBank in NCBI, 7 bacillus strains with different colony morphologies are obtained, the comparison results are shown in table 1, the 16S rDNA sequence comparison homology of A44, A68 and A73 reaches 100%, the homology of A64 is 99.72%, the homology of A75, A97 and A105 is 99.93%, and the 16S rDNA sequence comparison homology of all the strains reaches more than 99%. In conjunction with phylogenetic tree analysis of FIG. 10, A44, A64, A97 and A105 were ultimately identified as Bacillus pseudomycoides (Bacillus pseudomycoides), A68 as Bacillus panaciterrae, A73 as Bacillus proteolyticus and A75 as Bacillus mycoides (Bacillus mycoides).
TABLE 1 alignment of isolated strain 16S rDNA sequences
Figure BDA0003712127980000051
Figure BDA0003712127980000061
FIG. 11 shows colony morphology and cell morphology of strain A44. On solid B medium, colony of strain A44 is white, round, smooth and convex with glossy, moist and semitransparent. The strain A44 is observed by a scanning electron microscope to be in a short rod shape, has flagella and is positive in gram staining.
FIG. 12 shows colony morphology and cell morphology of strain A68. As can be seen from FIG. 12, the colony of strain A68 is white, round, smooth and convex at the edge, moist and opaque on solid B medium. The strain A68 is observed by a scanning electron microscope to be in a thin rod shape, has flagellum and is positive in gram staining.
FIG. 13 shows colony morphology and cell morphology of strain A105. As can be seen from FIG. 13, the colony of strain A105 was white, round, flat, smooth and glossy at the edge, moist and opaque on solid B medium. The strain A105 is observed by a scanning electron microscope to be in a thin rod shape, has flagellum and is positive in gram staining.
Strain A44 was designated DW44, classified under the name: bacillus pseudomycoides, deposited in China center for type culture Collection, address: martial arts, date of preservation: 2022, 5 months and 19 days, deposit number: cctccc NO: m2022676.
Strain a68 was designated DW68, classified under the name: bacillus panaciterrae, deposited in China center for type culture Collection, address: martial arts, date of preservation: 2022, 5 months and 19 days, deposit number: cctccc NO: m2022677.
Strain a105 was designated DW105, classified as: bacillus pseudomycoides, deposited in China center for type culture Collection, address: martial arts, date of preservation: 2022, 5 months and 19 days, deposit number: cctccc NO: m2022678.
EXAMPLE 3 Effect of Bacillus strains on growth inhibition of ralstonia solanacearum
The influence of the aluminum-resistant bacillus on the growth inhibition of the bacterial wilt is evaluated by adopting a plate antagonizing method: diluting ralstonia solanacearum to 1×10 7 CFU/mL was uniformly spread on a B solid medium plate by 200. Mu.L, then 2. Mu.L of different bacillus bacteria were dropped in the center of the plate, sterile water was used as a negative control, gentamicin (GM) at 0.5mg/mL was used as a positive control, each treatment was repeated 3 times, and the plate was placed in a constant temperature incubator at 30℃for 24 hours, and the sizes of the inhibition zones of the different treatments were observed.
The results of analyzing the influence of bacillus on the growth of the bacterial wilt by using a plate antagonism method are shown in table 2 and fig. 5, and the results show that the isolated 7 strains of bacillus have a certain inhibition effect on the growth of the bacterial wilt, the diameter of the inhibition zone of the strain A73 is 16.24mm, and the diameter of the inhibition zone of the strain A68 (13.12 mm) is obviously higher than that of the strains A44, A64, A75 and A105.
TABLE 2 bacteriostatic Effect of Bacillus on bacterial wilt CQPS-1
Figure BDA0003712127980000071
EXAMPLE 4 evaluation of aluminum-resistant Activity and acid-resistant Activity of Bacillus
Respectively adding bacillus strain and bacterial wilt CQPS-1 strain into aluminum sulfate with final concentration of 1.2mmol/L and sodium sulfate B liquid culture medium with final concentration of 3.6mmol/L, treating each with sterile water as negative control, shake culturing at 30deg.C at 180rpm, taking 1mL of mixed bacterial liquid every 2h, and detecting OD 600 nm Absorbance values were measured for 24h and growth curves were plotted for different strains at different aluminium concentrations.
The aluminium resistance of the different bacillus strains isolated is shown in fig. 6 and table 3, and in both clean water Control 1 (Control 1) and sodium sulfate Control 2 (Control 2), the time for the isolated bacillus to enter the log phase is earlier than that of the bacterial wilt, indicating that the adaptation period of the isolated bacillus in the culture medium is earlier than that of the bacterial wilt. In the treatment of 2.4mmol/L aluminum ions (2.4 mmol/L Al) 3+ ) The growth of the bacterial wilt is obviously inhibited, and the aluminum resistance of the separated bacillus is higher than that of the bacterial wilt, wherein the aluminum resistance of the A73 bacteria is strongest, and the bacterial wilt is the A64 bacteria and the A105 bacteria and the bacterial wilt is the A68 bacteria.
TABLE 3 aluminium-resistant Activity of different strains in liquid B Medium for 24h
Figure BDA0003712127980000072
Respectively regulating pH value of the liquid culture medium B to 4.5, 5.0 and 6.0 with hydrochloric acid, sterilizing, respectively inoculating into separated bacillus strain and bacterial wilt CQPS-1 strain, performing shake culture at 30deg.C and 180rpm for 3 times each time, and detecting OD by taking 1mL of mixed bacterial liquid every 2 hours 600nm Absorbance values were measured for 24h and growth curves were plotted for different strains at different pH.
The acid resistance of the isolated different bacillus strains is shown in fig. 7 and table 4, the growth rates of a44, a64, a73 and a75 are faster than that of the bacterial wilt under the condition of pH6.0, the growth rates of a97 are consistent, and the time for a68 to enter the logarithmic phase is 4 hours later than that of the bacterial wilt; under the condition of pH5.0, the growth rate of bacillus is faster than that of bacterial wilt, and the final biomass A68 and A73 strains have no obvious difference with the bacterial wilt; under the condition of pH4.5, the growth of the bacteria except the bacteria A73 is completely inhibited, which shows that the acid resistance of the bacteria A73 is worst, and the growth rate bacteria of other spore strains under the environment of pH4.5 are obviously higher than those of bacterial wilt, and the bacterial wilt has certain acid resistance. The pH of the acidified soil is generally 5.0-5.5, and the strain selected in the study can survive under the condition of pH4.5-6.0, can colonize in the acidified soil and exert biological effects.
TABLE 4 acid resistance Activity of different strains in liquid B Medium for 24h
Figure BDA0003712127980000081
EXAMPLE 5 Effect of Bacillus strains on tobacco growth
Cleaning root matrix with deionized water, transplanting into soil without bacterial wilt, illuminating at 25deg.C+ -2deg.C for 12 hr, dark at 20deg.C+ -2deg.C for 12 hr, and culturing under 75% humidity greenhouse condition, and respectively inoculating 10mL 1×10 after one week 8 cfu/mL, continuously culturing for 14 days, cleaning root soil, absorbing water by using water absorbing paper, respectively detecting the fresh weight of the root and the fresh weight of the upper part of the root of the tobacco plant subjected to different treatments, drying for 6 hours at 105 ℃ in a constant-temperature drying box, and weighing the dry weight of the root and the dry weight of the upper part of the root of the tobacco plant subjected to different treatments.
The isolated bacillus strain is externally added into soil, whether the isolated bacillus strain has growth promotion effect on tobacco growth or not is evaluated, and the results are shown in table 5 and fig. 8, and show that the A105 strain can significantly increase the fresh weight (A in fig. 8) and dry weight (C in fig. 8) of the root of the tobacco and the fresh weight (B in fig. 8) and dry weight (D in fig. 8) of the upper root of the tobacco compared with a control; the fresh weight and dry weight of the upper part of the root of the tobacco and the dry weight of the root are obviously increased by the A64 bacteria; the A68 strain significantly increases the root dry weight. The comprehensive evaluation can obtain the A105 bacteria which can obviously promote the growth of tobacco. The fresh weight of tobacco root, fresh weight of upper root, dry weight of root and dry weight of upper root treated by strain a105 were increased by 128.36%, 83.42%, 136.77% and 97.90%, respectively, compared to the blank.
TABLE 5 plant biomass after each treatment
Figure BDA0003712127980000091
EXAMPLE 6 Effect of Bacillus strains on the occurrence of bacterial wilt in tobacco
Picking single colony of bacillus activated on solid B culture medium, inoculating into 20mL sterile liquid B culture medium, shake culturing at 30deg.C and 180rpm on constant temperature shake shaker to OD 600nm =1.0(1×10 9 CFU/mL).
Cleaning root matrix with deionized water, transplanting into soil (pH 5.68) without bacterial wilt, illuminating at 25deg.C+ -2deg.C for 12 hr, darkening at 20deg.C+ -2deg.C for 12 hr, and culturing under 75% humidity greenhouse condition, and respectively inoculating 10mL OD after one week 600nm =0.1(1×10 8 CFU/mL) of bacillus suspension, 3 replicates per treatment, 7 cigarettes per replicate, and 10mL OD per cigarette after 24h 600nm =0.01(1×10 7 CFU/mL), then placing the bacterial suspension in a greenhouse with the temperature of 30 ℃ ± 2 ℃ for 12 hours under illumination, the temperature of 25 ℃ ± 2 ℃ for 12 hours under darkness, and the humidity of 80% for continuous culture, investigating the disease condition of bacterial wilt every day, and recording the disease grade investigation, disease index and disease incidence.
Disease investigation was performed with reference to indoor tobacco bacterial wilt disease classification criteria:
level 0: the tobacco plants have no disease symptoms;
stage 1: wilting 1-2 leaves of the tobacco plant, or fading the base part of the stem of the tobacco plant to make the fading streak less than 1/3 of the whole plant;
2 stages: 2-3 leaves of the tobacco plant wilt, or 1/3-1/2 of the leaf spot of the base portion of the stem of the tobacco plant is faded;
3 stages: 1-2 healthy leaves of the tobacco plant or 1/2-2/3 of the fading strip spots at the base of the stem of the tobacco plant;
4 stages: the whole plant withers, or the stem base of the tobacco plant is subjected to fading and streak fading, which is more than 2/3 of the whole plant.
The severity of the disease is calculated according to the disease classification, and the disease rate is calculated according to the number of disease plants, and the formula is as follows:
Figure BDA0003712127980000092
Figure BDA0003712127980000093
table 6 shows the incidence of bacterial wilt of tobacco, table 7 shows the disease index of bacterial wilt of tobacco, and the influence of different bacillus strains on bacterial wilt of tobacco is shown in FIG. 9, wherein the left graph shows the incidence rate, and the right graph shows the disease index. Research results show that the bacterial wilt of tobacco can be obviously delayed by the bacterial wilt of A68 and the bacterial wilt of A44, and the bacterial wilt of A68 starts to occur on the 25 th day after inoculation, compared with the control, the bacterial wilt is delayed by 12 days; a44 bacteria started to develop on day 26, 13 days later than control bacterial wilt. The A68 bacteria has the best prevention and control effect on tobacco bacterial wilt, and secondly, when the A44 bacteria are regulated and examined for 40 days, the incidence rate of the tobacco bacterial wilt of the A68 bacteria and the A44 bacteria is 6.67 percent and 10.00 percent respectively, and the relative prevention and control effect is 83.33 percent and 75.00 percent respectively. The A105 strain has slightly weaker prevention effect on tobacco bacterial wilt than the A68 strain and the A44 strain, can be independently used as a biological bacterial agent for promoting tobacco growth, and can also be used as a compound bacterial agent with other bacterial strains with inhibition effect on bacterial wilt for promoting tobacco growth and protecting tobacco bacterial wilt.
Table 6 incidence of bacterial wilt in tobacco
Figure BDA0003712127980000101
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Figure BDA0003712127980000111
Table 7 shows the disease index of each strain for the occurrence of bacterial wilt of tobacco
Figure BDA0003712127980000112
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Figure BDA0003712127980000121
Figure BDA0003712127980000131
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The acid-resistant and aluminum-resistant bacillus separated by the invention mainly comprises four types of bacillus pseudomycoides (Bacillus pseudomycoides), bacillus panaciterrae, bacillus proteolyticus and bacillus mycoides (Bacillus mycoides), and researches show that the bacillus pseudomycoides can activate the combined potassium in the soil and can be used as a potassium-decomposing biological fertilizer, and meanwhile, the bacillus pseudomycoides and the mica fertilizer are mixed and applied to replace potassium chloride fertilizer to improve the effectiveness of potassium in the soil and increase the absorption of potassium elements by plants. In addition, the research also shows that the bacillus pseudomycoides (B.pseudomycoides C6) can effectively remove copper ions in water and prevent a large amount of copper from entering plants to cause copper poisoning. The identified strain of bacillus pseudomycosis A105 (Bacillus pseudomycoides A) screened by the invention shows growth promotion effect on tobacco, and can be related to promotion of potassium absorption of tobacco plants. In addition to the growth promoting effect, the study also found that bacillus pseudomycosis (Bacillus pseudomycoides DSM, 12442) has a cluster of genes synthesizing the antibiotic lanthocin, and that the production of an antibacterial substance having activity against gram-positive bacteria was detected in the cell wash extract of this strain, identified as a lanthocin antibacterial peptide. The separated and identified bacillus pseudomycosis strain is firstly found to have a certain antagonism on the bacterial wilt, and the bacillus pseudomycosis A44 strain has a good control effect on the tobacco bacterial wilt, has strong acid and aluminum resistance, and can be used as biocontrol bacteria for the tobacco bacterial wilt for deep research.
The Bacillus panaciterrae A strain analyzed by the research of the invention has a growth rate slower than other bacillus strains under the conditions of acidity (pH 4.5) and aluminum stress, but has good control effect on tobacco bacterial wilt. Research shows that Bacillus proteolyticus GT has phosphate dissolving effect and can promote rice growth.
The development of high-throughput sequencing technology provides a solution for the research of plant and soil microorganism interaction, and according to sequencing data, the community composition of soil microorganisms can be primarily determined, but the microbial community composition achieved by high-throughput sequencing is a relative result, and in order to verify the functions, functional flora needs to be separated, and the functions are verified through interaction with plants. In Liu Y.X., qin Y., bai Y.reduction synthetic community approaches in root microbiome research [ J ]. Current Opinion in Microbiology,2019,49:97-102, it is shown that synthetic community (SynCom) methods can provide functional and mechanistic insights into how plants regulate their microbial communities, and how microbial communities in turn affect plant growth and health, and the reproducibility of synthetic communities makes future bacterial community establishment and functional research possible under laboratory conditions. Berendsen et al (Berendsen R.L., vismanns G, yu K, song Y., de Jonge R., burgman W.P., burmole M., herschend J., bakker Pahm, pietese C.M. J. Disease-induced assemblage of a plant-beneficial bacterial consortium [ J ]. ISME Journal,2018,12 (6): 1496-1507) have found that isolated beneficial microorganisms, individual strains, have no significant effect on plant growth and pathogen numbers, and that plants exhibit significant growth promoting effects when three synergistic strains are mixed. Similarly, lee et al (Lee S.M., kong H.G., song G.C., ryu C.M. dispersion of Firmicutes and Actinobacteria abundance in tomato rhizosphere causes the incidence of bacterial wilt disease [ J ]. ISME Journal,2020,15 (1): 330-347.) isolated strains associated with inhibition of tomato bacterial wilt by high throughput sequencing results, the strains alone were not significant in controlling tomato bacterial wilt, and the synthetic community could significantly reduce tomato bacterial wilt. In summary, the invention researches and screens 7 strains of bacillus, in particular to strains of bacillus pseudomycoides A44 (Bacillus pseudomycoides A) and Bacillus panaciterrae A (68) which have strong acid-resistant and aluminum-resistant activities and good prevention and treatment effects on tobacco bacterial wilt, and an aluminum-resistant strain of bacillus pseudomycoides (Bacillus pseudomycoides A) which has growth promotion effects on tobacco, and the strains can be synthesized according to the characteristics of the strains to prepare a composite bacterial agent for use, so that the synthesized community has the comprehensive characteristics of acid resistance, aluminum resistance, disease resistance and growth promotion, and provides a new idea for preventing and treating the bacterial wilt of acid soil and/or growing tobacco plants.
Finally, it is noted that the above-mentioned preferred embodiments are only intended to illustrate rather than limit the invention, and that, although the invention has been described in detail by means of the above-mentioned preferred embodiments, it will be understood by those skilled in the art that various changes in form and details may be made therein without departing from the scope of the invention as defined by the appended claims.

Claims (8)

1. An acid-tolerant growth-promoting bacillus pseudomycoides (Bacillus pseudomycoides) DW105 deposited in the chinese collection of typical cultures at the address: martial arts, date of preservation: 2022, 5 months and 19 days, deposit number: cctccc NO: m2022678.
2. Use of the bacillus pseudomycoides of claim 1 as microbial agent for promoting the growth of tobacco plants.
3. The use according to claim 2, wherein the soil environment in use is an acid soil with a ph of 4.5-ph 6.0.
4. The use according to claim 2, wherein the concentration of the pseudomycobacillus in the microbial agent is 1 x 10 6 cfu/mL-1×10 12 cfu/mL。
5. The use according to claim 2, wherein the concentration of the pseudomycobacillus in the microbial agent is 1 x 10 8 cfu/mL。
6. A microbial agent comprising the Bacillus pseudomycoides of claim 1 as an active ingredient.
7. The microbial agent of claim 6, wherein the active ingredient of the microbial agent further comprises a strain of bacillus pseudomycoides DW44 and/or Bacillus panaciterrae DW, said bacillus pseudomycoides DW44 having a accession number cctccc NO: m2022676; the preservation number of Bacillus panaciterrae DW is CCTCC NO: m2022677.
8. The microbial agent according to claim 6, wherein the bacillus pseudomycosis according to claim 1 is cultured to obtain a bacterial suspension, which is a liquid microbial agent.
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Citations (3)

* Cited by examiner, † Cited by third party
Publication number Priority date Publication date Assignee Title
CN106754557A (en) * 2017-01-25 2017-05-31 贵州省烟草公司贵阳市公司 Bacillus subtilis YBM 4 and its application in preventing and treating tobacco black shank and growth promotion
CN113201474A (en) * 2021-04-26 2021-08-03 中国农业科学院烟草研究所 Bacillus subtilis TBWR1, application thereof and obtained control agent
WO2021241759A1 (en) * 2020-05-29 2021-12-02 国立大学法人東海国立大学機構 Bacterial strain belonging to bacillus genus, and microbiological control agent using said bacterial strain

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* Cited by examiner, † Cited by third party
Publication number Priority date Publication date Assignee Title
US20060018883A1 (en) * 2002-12-04 2006-01-26 Yuanguang Li Microbial preparation & method for preventing and curing the bacterial wilt the plant and its use
CN101659932B (en) * 2009-09-18 2010-10-20 南京农业大学资产经营有限公司 Antagonistic bacteria preventing and removing continuous cropping tobacco bacterial wilt and microbial organic fertilizer thereof

Patent Citations (4)

* Cited by examiner, † Cited by third party
Publication number Priority date Publication date Assignee Title
CN106754557A (en) * 2017-01-25 2017-05-31 贵州省烟草公司贵阳市公司 Bacillus subtilis YBM 4 and its application in preventing and treating tobacco black shank and growth promotion
WO2021241759A1 (en) * 2020-05-29 2021-12-02 国立大学法人東海国立大学機構 Bacterial strain belonging to bacillus genus, and microbiological control agent using said bacterial strain
CN115885033A (en) * 2020-05-29 2023-03-31 国立大学法人东海国立大学机构 Bacterial strain belonging to the genus bacillus and microbial control agent using the same
CN113201474A (en) * 2021-04-26 2021-08-03 中国农业科学院烟草研究所 Bacillus subtilis TBWR1, application thereof and obtained control agent

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