CN116333912A - Bacillus coagulans with broad-spectrum antibacterial effect and application thereof - Google Patents
Bacillus coagulans with broad-spectrum antibacterial effect and application thereof Download PDFInfo
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- CN116333912A CN116333912A CN202211395783.9A CN202211395783A CN116333912A CN 116333912 A CN116333912 A CN 116333912A CN 202211395783 A CN202211395783 A CN 202211395783A CN 116333912 A CN116333912 A CN 116333912A
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- bacillus coagulans
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Abstract
The invention relates to the technical field of functional microorganism screening and application, in particular to a novel bacillus coagulans strainBacillus coagulans) And applications thereof. The preservation number of the coagulating spore rod is CCTCC NO: m20221235 the strain has broad-spectrum antibacterial capability and good denitrification performance, has remarkable inhibition effect on pathogenic bacteria such as escherichia coli, salmonella, clostridium perfringens, staphylococcus aureus, duck in-service Morganella, vibrio and the like, and has good denitrification effect on pathogenic bacteria such as escherichia coli, salmonella, clostridium perfringens and the likeThe removal rate of ammonia nitrogen and nitrite nitrogen reaches 100%, the zearalenone can be efficiently degraded, the degradation rate reaches 80.5%, and the ammonia nitrogen and nitrite nitrogen can be widely applied to the field of livestock and poultry or aquaculture as feed additives, bacteriostats, water regulators and the like, and the application prospect is wide.
Description
Technical Field
The invention relates to the technical field of functional microorganism screening, in particular to bacillus coagulans with a broad-spectrum antibacterial effect and application thereof.
Background
The microecological preparation is prepared by applying the microecological principle under the guidance of microecological theory and utilizing living microorganisms beneficial to a host or bioactive substances generated by microbial metabolism through a special process so as to achieve the aim of regulating the microecological balance of the organism. Microecologics are currently divided into 3 types, namely probiotics, prebiotics and synbiotics. In the 60 s of the 20 th century, with the gradual appearance of potential hazards to farming due to long-term or irregular use of antibiotics, microecologics have only received sufficient attention in livestock farming. After 90 s, aquaculture rapidly progresses, and aquaculture animal diseases are endangered, and aquatic microecologics gradually become research hotspots.
The microecological preparation is added into the feed, so that the immunity and disease resistance of animals can be improved, the production performance and the cultivation benefit of the animals are improved, the pollution to the environment caused by misuse and abuse of antibiotics and various chemical veterinary medicines can be reduced, and good ecological benefit is brought. In the aspect of aquatic products, besides the microecological preparation for feeding, the microecological preparation for regulating water and improving the bottom has the functions of purifying water quality, improving intestinal microbial communities of aquatic products, improving digestion and absorption capacity, promoting animal growth, improving the expression level of specific immune related genes, enhancing the capability of organisms to resist virus and bacterial infection and the like. Therefore, in recent years, the use of microecologics in animal production has been expanding.
The nutrition value of the feeding microecology is mainly expressed in that: 1) Regulating gastrointestinal microecological balance, and correcting intestinal flora dysfunction, thereby reducing infectious diarrhea and non-infectious diarrhea caused by bacteria, viruses and protozoa, because these diarrhea are all related to intestinal flora dysfunction; 2) Inhibiting the proliferation of pathogenic bacteria including amine-producing spoilage bacteria in the intestine, thereby maintaining optimal combination and stability of intestinal flora; 3) Synthesizing amylase, cellulase, protease and other enzymes and promoting the secretion of host digestive enzymes, thereby promoting the digestion and absorption of feed and reducing diarrhea caused by dyspepsia; 4) The vitamin is synthesized, the absorption of calcium and lactose is promoted, and the constipation and diarrhea of piglets are prevented, so that the health care effect on the piglets is realized; 5) The organic acid produced by metabolism can promote gastrointestinal peristalsis, and the microecology can moisten the stool, so that constipation of sows can be prevented; 6) The microecology can induce effective mucosal immunity and humoral immunity reaction, enhance the immunity of a host, reduce the endotoxin content in blood and reduce the occurrence of diseases.
At present, 2 main feeding micro-ecologies widely applied in animal production in China are bacillus and lactobacillus. In practical application, the 2-size feeding strain is found to have obvious advantages and has the defect of being yet to be improved when being added as an exogenous beneficial bacterium in animal intestinal tracts. The bacillus has the greatest advantages of being resistant to bile salts, gastric acids and alkali, particularly high temperature and extrusion, and can survive in granulated feed. In addition, the microbial enzyme has good enzyme production capacity and broad-spectrum antibacterial capacity. However, bacillus does not produce lactic acid, and can not grow well in anaerobic environment such as intestinal canal, so that the bacillus can not play a direct role in intestinal canal micro-ecological system, and the effect of adding probiotics as feed in feed is limited. Bacillus subtilis and Bacillus licheniformis are the main strains for producing feed bacillus preparations at present. For example, zhang Bingsheng and the like screen a bacillus subtilis SD-KC-001, which has stronger acid resistance, salt resistance and heat resistance, strong growth capacity, can produce enzymes such as amylase, protease and the like with good antibacterial capacity. Through feeding animals, the strain can improve the weight gain, reduce the drug cost, reduce the death rate and the like after being added into the feed. Zhou Yi and the like screen a bacillus licheniformis DN01 strain, have strong inhibition effects on aquatic pathogenic bacteria aeromonas hydrophila, pseudomonas fluorescens and Edwardsiella, can obviously promote the growth of crucian, and greatly improve the survival rate after toxicity attack.
At present, development of a feeding microecological strain with multiple functions, strong stability and excellent effect is still an important research and development point in the field.
Disclosure of Invention
The invention aims to provide a novel bacillus coagulansBacillus coagulans) And applications thereof. The bacillus coagulans has broad-spectrum antibacterial capability, has remarkable inhibition effect on pathogenic bacteria such as escherichia coli, salmonella, clostridium perfringens, staphylococcus aureus, duck in-service bacillus, vibrio and the like, and can be widely applied to the field of cultivation.
The bacillus coagulans provided by the invention is bacillus coagulans NR 372%Bacillus coagulans NR 372) strain which has been preserved in China center for type culture collection (CCTCC NO) of university of Wuhan in China, 8 th month of 2022: m20221235.
The bacillus coagulans NR372 strain provided by the invention has a MALDI-TOF-MS protein fingerprint shown in figure 2 and a rRNA gene fingerprint shown in figure 3.
The 16s rRNA sequence of the bacillus coagulans NR372 strain provided by the invention is SEQ ID NO:1.
the invention provides application of bacillus coagulans NR372 strain in preparation of a bacteriostat.
The bacillus coagulans NR372 strain provided by the invention is applied to water quality purification.
The bacillus coagulans NR372 strain provided by the invention is applied to feed production.
The invention also provides a feed additive, which comprises the bacillus coagulans NR372 strain.
The live bacterial amount of the bacillus coagulans NR372 strain in the feed additive is not less than 10 8 CFU/g。
The bacillus coagulans NR372 obtained by screening has strong comprehensive antibacterial effect, and has remarkable inhibitory effect on pathogenic bacteria such as escherichia coli, salmonella, clostridium perfringens, staphylococcus aureus, duck in-service Morganella, vibrio and the like, wherein the bacillus coagulans has the strongest antibacterial effect on salmonella pullorum, vibrio eurovirens and vibrio alginolyticus, and the diameter of a bacteriostasis zone reaches 2.8-3.5cm.
The bacillus coagulans NR372 has strong gastric acid tolerance, and the survival rate can reach 50% after 4 hours; the strain is completely tolerant to artificial intestinal juice, and the survival rate is up to 100% after 12 hours; the highest tolerance concentration of the strain to bile salts is 1%, and the survival rate after 4 hours is up to more than 90%.
The bacillus coagulans NR372 has strong comprehensive acid production and enzyme production capability, at least can produce 8 organic acids and 4 enzymes, and the content of lactic acid and acetic acid in fermentation liquor is highest and reaches 7309.23 ug/mL and 5501.28 ug/mL respectively; the strain has good denitrification performance, the removal rate of ammonia nitrogen and nitrite nitrogen reaches 100%, and the degradation rate of zearalenone can be efficiently degraded to 80.5%.
The bacillus coagulans NR372 can effectively improve the production performance of weaned pigs, obviously reduce the diarrhea rate of the weaned pigs and has obviously better effect than antibiotics. Compared with the treatment group 1 fed with antibiotics, the diarrhea index of piglets in the treatment group fed with bacillus coagulans is reduced by 20-40%, and the effect is very remarkable.
Bacillus coagulans NR372 can obviously reduce the death rate of Litopenaeus vannamei infected with vibrio parahaemolyticus. Compared with the toxicity attacking group, the death rate of the prawns in the probiotics treatment group fed with the bacillus coagulans NR372 is reduced by 80.1 percent, and unexpected technical effects are achieved.
The bacillus coagulans NR372 provided by the invention is widely applied to the field of livestock and poultry or aquaculture as a feed additive, a bacteriostatic agent, a water regulating agent and the like, and has a wide application prospect.
Drawings
FIG. 1 is a colony morphology of NR372 strain;
FIG. 2 is a protein mass spectrum peak diagram of NR372 strain;
FIG. 3 is a rRNA gene fingerprint.
Detailed Description
The bacillus coagulans NR372 provided by the invention meets the regulation requirement, and is identified by multiphase taxonomy, and the bacillus coagulans NR372 is a newly discovered strain. The bacillus coagulans NR372 provided by the invention has remarkable antibacterial effect on various common pathogenic bacteria and has important application value.
The applicant uses bacillus coagulans NR372 @ 4 days of 2022Bacillus coagulans NR 372) strain is preserved in China center for type culture collection (CCTCC NO) of university of Wuhan, china: m20221235.
The screening method of the present invention is not limited to the examples, but known screening methods can be used to achieve the screening purpose, and the screening description of the examples is only illustrative of the present invention and is not intended to limit the scope of the present invention. Modifications and substitutions to methods, procedures, or conditions of the present invention without departing from the spirit and nature of the invention are intended to be within the scope of the present invention.
The present invention will be described in detail with reference to specific examples.
EXAMPLE 1 isolation and screening of strains
1. Sample source:
and 20 parts of compost fermented feed.
2. Bacterial strain primary screening
1g of the sample is weighed and placed in 9 mL sterile normal saline, and evenly mixed for 10min at 200rpm to obtain bacterial suspension; placing the bacterial suspension in a water bath kettle at 80 ℃ for 10min to remove non-spore bacteria; inoculating 1% of the strain into a modified LB culture medium, culturing at 37 ℃ for 20 hours, and performing dilution coating on a modified calcium carbonate identification plate; selecting single colonies which are provided with a calcium dissolving ring and well grown, and respectively carrying out gram staining, spore staining and contact enzyme tests; and selecting 4 strains which are positive in gram staining, spore-producing and positive in contact enzyme, wherein the strains are YB95, YB115, YB202 and YB266 respectively.
3. Bacterial strain re-screening
Selecting more than 20 pathogenic bacteria which often cause animal diseases in the industries of livestock, poultry, aquatic products and pets: and performing bacteriostasis tests on escherichia coli, salmonella, clostridium perfringens, staphylococcus aureus, duck in-service bacillus, vibrio and the like, and evaluating the bacteriostasis capacity of 4 strains of YB95, YB115, YB202 and YB266 obtained through primary screening according to the diameter of a bacteriostasis ring.
The operation flow is as follows: and taking a sterile plate, pouring 18-20 mL of sterile nutrient agar culture medium, uniformly spreading the culture medium in the plate, placing the culture medium on a horizontal table top to solidify, taking the plate as a bottom layer, inverting the plate to evenly divide the region, and marking the to-be-added substance. And (3) taking a proper amount of sterile semi-solid nutrient agar culture medium (the agar content is 1%), cooling to 48-50 ℃, adding 1-2 mL of pathogenic bacteria suspension into each 50-100 mL of culture medium, and respectively adding 5mL of semi-solid nutrient agar culture medium into each plate to uniformly spread on a bottom layer to serve as a bacterial layer. And after being placed on a horizontal table for cooling, 4-6 oxford cups are uniformly arranged in each 1 plate at equal distance. The diameters of the bacteriostasis circles are measured after 0.2mL of the strain bacterial liquid which is cultured by expanding is respectively dripped into oxford cups in each double-layer plate and is cultured for 24 hours at 37 ℃, and the specific results are shown in Table 1.
TABLE 1 antibacterial Effect of strains
As shown in the results of Table 1, the YB202 strain obtained by screening has the best comprehensive antibacterial effect, and has remarkable inhibitory effect on pathogenic bacteria such as escherichia coli, salmonella, clostridium perfringens, staphylococcus aureus, morganella anatipestifer, vibrio and the like, wherein the antibacterial effect on salmonella pullorum, vibrio eurovirens and vibrio alginolyticus is strongest, and the diameter of a bacteriostasis ring reaches 2.8-3.5cm. The applicant designated this strain as NR372 and further identified and functionally evaluated.
EXAMPLE 2 identification of NR372 Strain
1. Colony morphology identification
As shown in FIG. 1, NR372 strain forms a round colony with the diameter of 2-3mm after being cultured on MRS culture medium for 24-48 hours, and the colony is white and glossy, and has moist and flat surface and neat edge; the NR372 bacteria form in rod shape, single, paired or chain arrangement, spore end growth.
2. Physiological and biochemical identification
The NR372 strain was subjected to physiological and biochemical identification, and the results are shown in Table 2.
Physiological and biochemical characteristics of NR372 strain and standard bacillus coagulansBacillus coagulans) Substantially identical, initially identified as bacillus coagulans.
TABLE 2 physiological and biochemical tables of strains
| Biochemical characterization | NR372 | Standard Bacillus coagulans |
| Indole test | - | - |
| Starch hydrolysis | + | + |
| Gelatin liquefaction | - | - |
| Yolk reaction | - | - |
| Hydrolysis of amino acids | - | - |
| Anaerobic growth | + | + |
| NaCl 2% | + | + |
| |
+ | + |
| NaCl 7% | - | - |
| |
- | - |
Note that: positive +; + a 90-100% of strains are positive; negative.
3. 16S rRNA identification
The genome of the NR372 strain was extracted using the kit. The genome was then used as a template to amplify its 16S rRNA using specific primers 27F and 1492R.
27F:5’-AGAGTTTGATCATGGCTCAG-3’;
1492R:5’-TAGGGTTACCTTACGACTT-3’。
The PCR system comprises: 0.7. Mu.l 27F, 0.7. Mu.l 14992R, 4. Mu.l template DNA, 17.5. Mu.l SuperMiX and 12.1. Mu.l water. The PCR reaction conditions were set as follows: (1) 94 ℃ for 5min; (2) pre-denaturation at 94℃for 30s; (3) 55 ℃ for 30s; (4) 72 ℃ for 1min; performing the loop of steps (2) to (4) 35; (5) at 72℃for 10min. The amplified PCR product is subjected to 1% agarose gel electrophoresis detection, and the result shows that the size of the PCR product is about 1500bp, thereby meeting the requirements.
The PCR amplified product was sent to sequencing company for sequencing, and the result shows that the 16s rRNA sequence of NR372 strain is SEQ ID NO:1. the sequence was subjected to BLAST alignment in NCBI database, which showed the highest similarity to Bacillus coagulans. Thus, the NR372 strain was preliminarily determined to be Bacillus coagulans.
4. MALDI-TOF-MS profile identification
A small amount of NR372 single colony is coated on a target plate in a film form; adding 1 mu L of lysate in the mass spectrum sample pretreatment kit, and naturally airing at room temperature; adding 1 mu L of matrix solution in the mass spectrum sample pretreatment kit to cover the sample, and naturally airing at room temperature; and (5) placing the sample target into a mass spectrometer for identification. The identification result shows that the NR372 strain is bacillus coagulans, and the protein mass spectrum peak diagram is shown in figure 2.
5. Ribo-Printer full-automatic microorganism gene fingerprint identification
And (3) performing on-machine identification on the NR372 strain according to the operation instruction of a full-automatic microorganism gene fingerprint identification system to obtain an rRNA gene fingerprint diagram of the NR372 strain, wherein the rRNA gene fingerprint diagram is shown in figure 3. By comparison with the fingerprint patterns of known standard strain libraries, the NR372 strain has a similarity with bacillus coagulans of more than 90%, so that the strain is identified as bacillus coagulans.
In summary, the applicant uses three molecular biology methods of 16S rRNA identification, MALDI-TOF-MS protein mass spectrum identification, ribo-Printer full-automatic microorganism gene fingerprint identification to identify NR372 strain, and the identification results are consistent. And then combining colony morphology and physiological and biochemical characteristics of the NR372 strain, the applicant determines that the NR372 strain is bacillus coagulans and names the bacillus coagulans NR 372%Bacillus coagulans NR372)。
The applicant has found that the above Bacillus coagulans NR372 @ 4 of 2022Bacillus coagulans NR 372) is preserved in China center for type culture collection (CCTCC NO) of university of Wuhan in China: m20221235.
EXAMPLE 3 safety evaluation of Bacillus coagulans NR372
1. Hemolysis:
the activated bacillus coagulans NR372 strain is inoculated on a blood plate, and after the blood plate is cultivated for 24 hours at the constant temperature of 37 ℃, whether a transparent hydrolysis ring is generated around a colony is observed.
The results show that: no hydrolytic circle was produced around the colonies, indicating that the Bacillus coagulans NR372 strain did not possess hemolysis.
2. Drug resistance:
the drug resistance of the strain may cause potential safety hazards in the production and application process. To prevent the presence of drug resistance of bacillus coagulans NR372, its antibiotic susceptibility was studied. The minimum inhibitory concentration (MIC value) of NR372 in 7 common antibiotics was determined according to CLSI antibiotic susceptibility test gradient dilution, the antibiotic used was Sigma standard, and the susceptibility to antibiotics was evaluated with reference to EFSA (2012) standard. See table 3 for specific results.
TABLE 3 minimum inhibitory concentration (MIC value) in antibiotics
| Chloramphenicol | Clindamycin | Gentamicin | Streptomycin | Erythromycin | Vancomycin | Tetracycline |
| 4(S) | 0.08(S) | 1(S) | 2(S) | 1(S) | 2(S) | 1(S) |
Note that: unit ug/ml, S represents sensitivity according to the strain sensitivity to antibiotics evaluation standard EFSA (2012); r represents drug resistance.
From the results in Table 3, it can be seen that the Bacillus coagulans NR372 provided by the invention is sensitive to 7 common antibiotics, and has no drug resistance.
EXAMPLE 4 Bacillus coagulans NR372 test for resistance to Artificial gastrointestinal fluids and bile salts
(1) Test for artificial gastric juice resistance
The bacillus coagulans NR372 bacterial liquid in logarithmic growth phase is prepared according to the following ratio of 1:9 volume ratio is inoculated into artificial gastric juice with pH of 2.0 and artificial intestinal juice with pH of 7.6 respectively, after standing culture is carried out for 4h and 12h respectively at 37 ℃, MRS culture medium is poured for culture, and control group is physiological saline. The viable count was compared before and after plate count, and each sample was repeated 3 times. (2) Test for bile salt resistance
The bacillus coagulans NR372 bacterial liquid in logarithmic growth phase is prepared according to the following ratio of 1:9, respectively inoculating the culture media into MRS liquid culture media with the content of bile salt of 0.1%, 0.2%, 0.3%, 0.5% and 1% by volume, standing at 37 ℃ for 4h, pouring the MRS culture media for culture, taking the culture media which are not subjected to bile salt treatment as a control group, comparing the numbers of viable bacteria before and after the culture media are counted by a flat plate, and repeating each sample for 3 times.
The above results show that: the bacillus coagulans NR372 has strong gastric acid tolerance, and the survival rate can reach 50% after 4 hours; the strain is completely tolerant to artificial intestinal juice, and the survival rate is up to 100% after 12 hours; the highest tolerance concentration of the strain to bile salts is 1%, and the survival rate after 4 hours is up to more than 90%.
EXAMPLE 5 enzymatic Properties of Bacillus coagulans NR372
Inoculating the activated bacillus coagulans NR372 into MRS liquid culture medium, and culturing for 24 hours at 37 ℃ and 220r/min to prepare a bacteria testing solution for later use.
The bacterial solutions are respectively inoculated on a screening culture medium containing amylase, protease, cellulase and lipase, and are cultured for 24 hours at 37 ℃. After the culture of the cellulase screening culture medium is finished, 0.2% Congo red solution is added for dyeing for 30min, and then 1mol/L NaCl is used for washing for 10min, and then the size of an enzyme producing ring is measured. The diameter of the enzyme-producing ring was measured after the amylase screening medium was changed in color by adding a dilute iodine solution, and the results are shown in Table 4.
TABLE 4 evaluation of Bacillus coagulans NR372 enzyme production Effect
| Enzyme species | Protease enzyme | Amylase enzyme | Cellulase enzymes | Lipase enzyme |
| Diameter of enzyme producing ring (mm) | 28 | 25 | 25 | 26 |
As can be seen from the results in Table 4, the Bacillus coagulans NR372 enzyme producing effect provided by the present invention was excellent.
EXAMPLE 6 acid Forming Properties of Bacillus coagulans NR372
6.1 pH change
The activated Bacillus coagulans NR372 was inoculated into 100mL of MRS liquid medium and cultured at 37℃and 200rpm for 24 hours. Samples were taken at 0h, 4h, 8h, 12h, 16h, 18h, 24h, respectively, to determine the pH of the fermentation broth.
The results show that: during 0-12h, the pH of the Bacillus coagulans NR372 broth dropped rapidly, and at 24h the pH dropped to 4.3.
6.2 Determination of organic acid content
And (3) centrifuging the bacillus coagulans NR372 fermentation liquor after 24h fermentation for 10min at 5000r/min, filtering the obtained supernatant with a 0.22um filter membrane, and then performing liquid chromatography to analyze the content of organic acids such as lactic acid, acetic acid and the like in the fermentation liquor. The acid standard curve was determined with the standard concentration (. Mu.g/mL) on the abscissa and the peak area on the ordinate. Substituting the peak area of the sample into a standard curve, and calculating the content of acid in the sample. The results are shown in Table 5.
TABLE 5 analysis of organic acid content in Bacillus coagulans NR372 fermentation broth
| Organic acid | Content (ug/mL) |
| Lactic acid | 7309.23 |
| Acetic acid | 5501.28 |
| Citric acid | 1600.98 |
| Succinic acid | 1534.01 |
| Formic acid | 1001.05 |
| Propionic acid | 902.98 |
| Malic acid | 3093.90 |
| Oxalic acid | 1234.20 |
As can be seen from the data in Table 5, the Bacillus coagulans NR372 provided by the invention has strong comprehensive acid production capability, at least 8 organic acids can be produced, and the contents of lactic acid and acetic acid in fermentation liquor are highest and reach 7309.23 ug/mL and 5501.28 ug/mL respectively, so that unexpected technical effects are achieved.
EXAMPLE 7 Bacillus coagulans NR372 Effect on removal of ammoniacal nitrogen and nitrite nitrogen
Bacillus coagulans NR372 was inoculated into MRS liquid medium and activated at 37℃and 200rpm for 24 hours. 1ml of the bacterial liquid was centrifuged at 4000rpm for 5min. The precipitate was washed three times with 0.9% physiological saline and inoculated into 50ml of a complex nitrogen source medium (glucose 0.1g, (NH) 4 ) 2 SO 4 0.01g,NaNO 2 0.01g,K 2 HPO 4 ·3H 2 O 1g,KH 2 PO 4 0.3g,MgSO 4 ·7H 2 O 0.25g,FeSO 4 ·7H 2 O 0.05g,MnSO 4 ·4H 2 O0.01g,NaCl 30g,pH 8.0), the initial concentration of ammoniacal nitrogen and nitrite nitrogen in the composite nitrogen source culture medium is 2mg/L, and the carbon-nitrogen ratio is 10; blank control was not doneAfter 48h of treatment and shaking culture at 37 ℃ and 150rpm, centrifuging at 4500rpm for 5min to obtain a supernatant, and measuring the content of ammonia nitrogen and nitrite nitrogen in the supernatant by referring to the method described in national standard GB 17378.4-2007. The removal rates of Bacillus coagulans NR372 for ammoniacal nitrogen and nitrite nitrogen were calculated according to the following formulas, respectively.
Ammonia nitrogen removal (%) = (X1-X2)/X1X 100%.
Nitrite nitrogen removal (%) = (Y1-Y2)/y1×100%.
X1 is the ammonia nitrogen content in the blank control after 48 hours of culture, and X2 is the ammonia nitrogen content in the test group culture medium after 48 hours of culture; y1 is the nitrite nitrogen content in the blank control after 48h of culture, and Y2 is the nitrite nitrogen content in the test group medium after 48h of culture.
The results show that the bacillus coagulans NR372 provided by the invention has good denitrification performance, and has unexpected technical effects on the removal rate of ammoniacal nitrogen and nitrite nitrogen reaching 100%.
Example 8 degradation Effect of Bacillus coagulans NR372 on zearalenone
40. Mu.L of Bacillus coagulans NR372 fermentation broth was inoculated into 4 mL of MRS liquid medium containing Zearalenone (ZEN) (10. Mu.g/mL), and incubated at 37℃and 200rpm for 48 hours with no inoculation of ZEN (10. Mu.g/mL) of MRS liquid medium as a control. According to the specification of the zearalenone ELISA detection kit, the culture solution is treated, the residual amount of ZEN in the culture solution is detected by an enzyme-labeled instrument, and the degradation rate is calculated.
Degradation rate (%) =
×100%。
The result shows that the bacillus coagulans NR372 provided by the invention can efficiently degrade zearalenone, and the degradation rate reaches 80.5%.
Example 9 application Effect of Bacillus coagulans NR372 on the prevention of diarrhea in weaned piglets
1. Experiment site:
animal houses of Qingdao university.
2. And (3) test design:
healthy commercial castrated boars 40 with average weight of 7.5 and kg are selected (26+/-1) for weaning at the day, and the average is divided into 4 treatment groups, and 10 piglets in each treatment group are fed into one colony house for 4 colony houses.
Grouping of test treatment groups:
control group: the basic diet group is free from adding any antibiotics and bacillus coagulans;
treatment group 1: basic ration + antibiotics (kitasamycin 50 g/t, oxytetracycline 50 g/t, aureomycin 75 g/t);
treatment group 2: basic ration + Bacillus coagulans NR372 (1X 10) 7 CFU/g);
Treatment group 3: basic ration + Bacillus coagulans NR372 (5X 10) 7 CFU/g)。
The test pigs are fed according to the weaned pig management scheme, basic ration is fed for the first 3 days, free feeding and drinking are carried out, only insect expelling and immunization are carried out on the test pigs, the 4 th morning is subjected to empty stomach weighing, and the test period is 10 days. 3 times daily feeding and free drinking water are carried out in the test period, and the temperature of the pig house is reasonably controlled. Test 10d, all test pigs were tested for body weight, feed intake, and for analysis of growth performance indicators such as average daily gain, average daily feed intake, feed conversion ratio, diarrhea index, etc. The results are shown in Table 6.
The diarrhea index is calculated by taking a cage as a statistical unit as follows:
diarrhea index (%) =number of diarrhea piglets/(number of piglets×days of test) ×100%.
TABLE 6 influence of Bacillus coagulans NR372 on growth performance of weaned piglets
| Index (I) | Control | Treatment group | 1 | Treatment group 2 | Treatment group 3 |
| Initial weight (kg) | 7.52 | 7.53 | 7.51 | 7.50 | |
| Last weight (kg) | 9.21 b | 9.54 a | 9.45 a | 9.56 a | |
| Average daily gain (g/d) | 168 b | 200 a | 193 a | 206 a | |
| Average daily feed intake (g/d) | 216 ab | 242 ab | 240 ab | 258 a | |
| Feed to meat ratio | 1.29 a | 1.21 b | 1.24 ab | 1.25 ab | |
| Diarrhea index (%) | 18 a | 10 b | 8 b | 6 b |
As can be seen from the data in table 6, the average daily gain, daily feed intake, feed conversion ratio and diarrhea index were significantly improved for each treatment group fed with antibiotics and bacillus coagulans, as compared to the control group. Compared with the treatment group 1 fed with antibiotics, the diarrhea index of piglets in the treatment group fed with bacillus coagulans is reduced by 20-40%, and the effect is very remarkable. Therefore, the bacillus coagulans NR372 provided by the invention can effectively improve the production performance of weaned pigs, obviously reduce the diarrhea rate of the weaned pigs, and has obviously better effect than antibiotics.
EXAMPLE 10 protective Effect of Bacillus coagulans NR372 on vannamei
1. Source of vannamei:
some breeding factory in Laiyi city
2. Experiment site:
a blue biological aquaculture room.
3. Experiment design:
healthy, disease-free and close-specification litopenaeus vannamei was selected and randomly divided into 4 groups of 3 replicates, 10 replicates each, and 21d cultivation experiments were performed in a 60L glass aquarium. During the experiment, each day was 8:00 and 16: feeding for two times at 00, wherein the average water temperature is about 25 ℃, the salinity is about 8.0, the pH is about 8.0, the continuous trace aeration is carried out, the dissolved oxygen is kept above 5mg/L, and the test is carried out according to the following groups after 3 days of feeding without any abnormal condition.
(1) Control group: feeding a non-antibiotic basic material, and normally feeding without toxicity attack;
(2) Benefit (benefit)Group of bacteria: feeding antibiotic-free base material and bacillus coagulans NR372 (3×10) 7 CFU/g), normal feeding is carried out without toxicity attack;
(3) Attack the poison group: feeding antibiotic-free base material, intramuscular injection of Vibrio parahaemolyticus culture solution with injection concentration of 1.0X10 6 CFU/mL, injection volume 25. Mu.L;
(4) Probiotic treatment group: feeding antibiotic-free base material and bacillus coagulans NR372 (3×10) 7 CFU/g), after 3 days of continuous feeding, the Vibrio parahaemolyticus culture solution was intramuscular injected at a concentration of 1.0X10 6 CFU/mL, injection volume was 25. Mu.L. The basic material containing bacillus coagulans NR372 is fed once every 3d, and the basic material is normally fed in the rest time.
The vitality, ingestion and death of the prawns in each group are recorded every day, and the death rate is counted after 21 d. The specific results are shown in Table 7.
TABLE 7 influence of Bacillus coagulans NR372 on mortality of Vernaeus vannamei
| Grouping | Mortality rate of |
| Control group | 4.95% |
| Probiotics group | 2.35% |
| Toxin eliminating group | 66.7% |
| Probiotic treatment group | 13.3% |
From the results in table 7, the mortality of the probiotics group prawns fed with bacillus coagulans NR372 was reduced by 52.5% compared to the control group. After the prawn of the virus attack group is injected with vibrio parahaemolyticus, the prawn shows reduced ingestion, redness of appendages, empty stomach, hepatopancreatic enlargement, immobility or roaming along the wall of a cultivation barrel, and weak vitality until the prawn dies finally, and the 21d death rate is up to 66.7%; the death rate of the prawns in the probiotics treatment group fed with the bacillus coagulans NR372 before and after the injection of the vibrio parahaemolyticus is only 13.3 percent, which is reduced by 80.1 percent compared with that of the virus attack group.
The result shows that the bacillus coagulans NR372 provided by the invention can effectively improve the immunity of the prawns, inhibit the growth and proliferation of pathogenic bacteria such as vibrio parahaemolyticus and the like, greatly reduce the death rate of the prawns and achieve unexpected technical effects.
Claims (9)
1. The bacillus coagulans is characterized in that the collection number of the bacillus coagulans is CCTCC NO: m20221235.
2. The bacillus coagulans of claim 1, wherein the bacillus coagulans has a MALDI-TOF-MS protein fingerprint as shown in fig. 2 and a rRNA gene fingerprint as shown in fig. 3.
3. The bacillus coagulans of claim 1, wherein the bacillus coagulans has a 16s rRNA sequence of SEQ ID NO:1.
4. the use of bacillus coagulans according to claim 1 for the preparation of a bacteriostatic agent.
5. The use of the bacillus coagulans according to claim 1 for water purification.
6. The use of bacillus coagulans according to claim 1 in feed production.
7. A feed additive comprising the bacillus coagulans of claim 1.
8. The feed additive according to claim 7, wherein the viable bacteria amount of Bacillus coagulans in the feed additive is not less than 10 8 CFU/g。
9. Use of the feed additive according to claim 7 or 8 in feed production.
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| Publication number | Priority date | Publication date | Assignee | Title |
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| CN117143770A (en) * | 2023-08-30 | 2023-12-01 | 广州格拉姆生物科技有限公司 | Wettman coagulans GLM336 and application thereof |
| CN117286079A (en) * | 2023-11-22 | 2023-12-26 | 广东容大生物股份有限公司 | Enteric-derived condensation Wittman's bacterium and application thereof, feeding microecological preparation comprising same and preparation method thereof |
| CN117305160A (en) * | 2023-09-19 | 2023-12-29 | 无锡爱科派生物科技有限公司 | Compound bacillus coagulans microbial inoculum and preparation method and application thereof |
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Cited By (5)
| Publication number | Priority date | Publication date | Assignee | Title |
|---|---|---|---|---|
| CN117143770A (en) * | 2023-08-30 | 2023-12-01 | 广州格拉姆生物科技有限公司 | Wettman coagulans GLM336 and application thereof |
| CN117143770B (en) * | 2023-08-30 | 2024-03-08 | 广州格拉姆生物科技有限公司 | Wettman coagulans GLM336 and application thereof |
| CN117305160A (en) * | 2023-09-19 | 2023-12-29 | 无锡爱科派生物科技有限公司 | Compound bacillus coagulans microbial inoculum and preparation method and application thereof |
| CN117286079A (en) * | 2023-11-22 | 2023-12-26 | 广东容大生物股份有限公司 | Enteric-derived condensation Wittman's bacterium and application thereof, feeding microecological preparation comprising same and preparation method thereof |
| CN117286079B (en) * | 2023-11-22 | 2024-03-15 | 广东容大生物股份有限公司 | Enteric-derived condensation Wittman's bacterium and application thereof, feeding microecological preparation comprising same and preparation method thereof |
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