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CN106831015A - A kind of bacillus laterosporus microbial manure and its production and use - Google Patents

A kind of bacillus laterosporus microbial manure and its production and use Download PDF

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CN106831015A
CN106831015A CN201710098364.1A CN201710098364A CN106831015A CN 106831015 A CN106831015 A CN 106831015A CN 201710098364 A CN201710098364 A CN 201710098364A CN 106831015 A CN106831015 A CN 106831015A
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fermentation
bacillus laterosporus
amplification cultivation
nutrient solution
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麻林涛
王莉
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    • CCHEMISTRY; METALLURGY
    • C05FERTILISERS; MANUFACTURE THEREOF
    • C05FORGANIC FERTILISERS NOT COVERED BY SUBCLASSES C05B, C05C, e.g. FERTILISERS FROM WASTE OR REFUSE
    • C05F11/00Other organic fertilisers
    • C05F11/08Organic fertilisers containing added bacterial cultures, mycelia or the like
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    • C12BIOCHEMISTRY; BEER; SPIRITS; WINE; VINEGAR; MICROBIOLOGY; ENZYMOLOGY; MUTATION OR GENETIC ENGINEERING
    • C12NMICROORGANISMS OR ENZYMES; COMPOSITIONS THEREOF; PROPAGATING, PRESERVING, OR MAINTAINING MICROORGANISMS; MUTATION OR GENETIC ENGINEERING; CULTURE MEDIA
    • C12N1/00Microorganisms, e.g. protozoa; Compositions thereof; Processes of propagating, maintaining or preserving microorganisms or compositions thereof; Processes of preparing or isolating a composition containing a microorganism; Culture media therefor
    • C12N1/20Bacteria; Culture media therefor

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Abstract

The present invention relates to a kind of preparation method of bacillus laterosporus microbial manure, comprise the following steps:S1:Bacillus laterosporus bacterial strain is activated, and aseptic water washing obtains seed liquor;S2:Amplification cultivation is carried out to seed liquor using the first nutrient solution, the first amplification cultivation liquid is obtained;S3:The first amplification cultivation liquid is cultivated using the second nutrient solution, obtains the second amplification cultivation liquid;S4:Second amplification cultivation liquid carries out liquid fermentation and culture, obtains zymotic fluid;S5:Zymotic fluid is drenched carries out solid fermentation in solid medium, and is post-processed, and obtains fermenting agent;S6:Fermenting agent and organic matter mixture are carried out into compost fermentation treatment, the microbial manure is obtained.Methods described is by being mutually combined between unique multiple technical characteristic and cooperates with, so as to obtain the fermenting agent of the final bacillus laterosporus with excellent technique effect, the widespread demand of multiple fields is disclosure satisfy that, is had a good application prospect and industrial production potential.

Description

A kind of bacillus laterosporus microbial manure and its production and use
Technical field
The present invention relates to a kind of microbial manure and its production and use, more specifically, it is related to a kind of side spore bud Spore bacillus microorganisms fertilizer and its production and use, belongs to microculture and microbial manure applied technical field.
Background technology
Bacillus laterosporus (Bacilluslaterosporus) be gram-positive bacteria, its gemma for ellipse, side life, Middle life is near middle raw, and sporangiocyst expands, and the gemma that dissociates is while, presentation canoe shape thicker than another side.
Bacillus laterosporus has important application in multiple fields, for example:1st, it can secrete substantial amounts of chitinase, suppression Fungus disease processed;2nd, there can be very strong inhibitory action to harmful bacterias such as vibrios, Escherichia coli and baculovirals;3rd, can subtract Few fish, shrimp disease occur, and improve yield;4th, residual bait, excrement, organic matter etc. in decomposable asymmetric choice net pond, eliminate blue-green algae, purify water;5、 Promote plant root growth, strengthen Root Absorption ability, so as to improve crop yield;6th, pathogen inside and outside plant processed is faced upward numerous Grow, mitigate pest and disease damage, reduce residues of pesticides;7th, chesson is improved, soil compaction phenomenon is solved, so that activating soil, improves Utilization rate of fertilizer;8th, strengthen plant metabolism, promote photosynthesis and reinforcing blade protection film, resist pathogen;9th, strengthen Photosynthesis, improves chemical fertilizer utilization ratio, reduces nitrate content;10th, solidify some heavy metals, reduce heavy metal in plant and contain Amount.
Just because of above-mentioned all multipurposes of bacillus laterosporus, so as in animal husbandry, feed industry, agricultural chemicals, fertilizer, kill All had a wide range of applications in the multiple fields such as bacterium, gardens industry, aquaculture, proportion of crop planting, cultivating seedlings, and its application field With new purposes also always in research and expansion.
Also just because of bacillus laterosporus so important effect, people for various bacillus laterosporus products and Cultural method and culture medium of bacillus laterosporus etc. have carried out substantial amounts of further investigation, achieve many achievements in research, example Such as:
CN102399710A discloses a kind of new bacillus laterosporus, and preserving number is CGMCC No.5090 and by the bacterium Microorganism fungus kind agent and microbial manure and their preparation method prepared by strain.The microorganism fungus kind produced using the strain Agent has effective bacterium number and the shelf-life more long higher.
CN103289937A discloses a kind of method that high density solid fermentation produces bacillus laterosporus viable bacteria, and it includes Following steps:Strain selection, inclined-plane seed culture, one-level solid seed culture, two grades of solid seed cultures, solid fermentation trainings Support, tunning drying and tunning are flashed.The culture medium raw material for being used all is to use agricultural byproducts, low cost, formula Rationally, culture propagation nutritional need is disclosure satisfy that, the pH value change of culture medium in calcium carbonate buffering incubation is particularly added, The bacillus laterosporus viable bacteria content of solid fermentation can be substantially increased, experiment and production prove what is prepared using the inventive method The living bacteria count of bacillus laterosporus up to 50,000,000,000/gram, product miscellaneous bacteria rate is less than 5%, and gemma rate is up to more than 90%, The production cost of enterprise can be substantially reduced, the need for meeting microbial bacterial agent production.
CN103416321A discloses a kind of bacillus laterosporus fermentation bed and preparation method thereof.Under shown fermentation bed passes through State method making:By bedding and padding raw material and chicken manure 3-5 by volume:1 is well mixed, and is inoculated with bacillus laterosporus preparation, water content It is 40-60%, carries out piling up pre fermentation 5-7 days;Pre fermentation bedding and padding are laid in hen house, the bedding and padding of same thickness are laid thereon Raw material, is mixed evenly to prepare fermentation bed, and the fermentation bed water content is 30-60%, and the gross thickness of the fermentation bed is 8-25cm;Institute It is 2-5 that bedding and padding raw material is stated by volume ratio:Husk and the sawdust composition of 5-8.The bacillus laterosporus fermenting bed padding thickness is small, The usage amount of bedding and padding is few, is significantly reduced the work workload of raiser, cost-effective;Effect is still fine at high temperature, can To suppress and kill mosquito, improve birds function of intestinal canal, efficient degradation albumen, starch, fat, fecaluria, and ammonia taste, stink compared with It is few;Use and expand column convenient, can Continuous disinfection.
CN103725626A discloses a kind of bacillus laterosporus preparation, and its preparation technology is as follows:Bacillus laterosporus bacterium Plant (ampoul tube)-test tube slant Spawn incubation-shaking flask Spawn incubation-seeding tank deep fermentation culture-closed solid hair Ferment case culture-bacillus laterosporus preparation.It uses continuously fermenting for advanced " deep fermentation+closed type solid fermentation " Technique, using totally-enclosed autocontrol solid fermentation apparatus, makes the whole process of solid fermentation all in totally enclosed automatic monitoring Under, automation inspection is carried out to environmental conditions such as the medium component in fermentation process, formula, temperature, humidity, ventilation, pH value Survey, electronical display, automatically control, not only increase substantially yield, and ensure that the microbial foliage prepared by said preparation increases Imitate the quality of agent.
CN105219676A discloses a kind of cultural method of bacillus laterosporus, and the Microbiological Culture Collection number is CGMCC No.5090, the cultural method is as follows:1st, by 1 volume bacteria suspension access 20 times of volume No. 1 culture mediums in, 30-38 DEG C aerobic culture 8 hours;2nd, the nutrient solution that step 1 is obtained is added in about 20 times of No. 2 culture mediums of volume, 30-38 DEG C has Oxygen culture 8 hours;3rd, the nutrient solution that step 2 is obtained is added in about 20 times of No. 3 culture mediums of volume, 35-38 DEG C of culture 8 is small When, obtain final product can production microorganism fungus kind culture.
CN105272406A discloses a kind of microbial manure prepared by bacillus laterosporus and preparation method thereof, the fertilizer Expect that gained culture and turf powder are mixed by preserving number for the microorganism fungus kind of CGMCC No.5090 obtains culture by culture Conjunction obtains microorganism fungus kind agent, and gained microorganism fungus kind agent is mixed with common fertilizer forms again, wherein the microbial bacteria The culture side for planting culture is as follows:1st, by 1 volume bacteria suspension access 20 times of volume No. 1 culture mediums in, 30-38 DEG C of aerobic culture 8 hours;2nd, the nutrient solution that step 1 is obtained is added in about 20 times of No. 2 culture mediums of volume, 30-38 DEG C of aerobic culture 8 is small When;3rd, the nutrient solution that step 2 is obtained is added in about 20 times of No. 3 culture mediums of volume, 35-38 DEG C is cultivated 8 hours, and obtaining final product can The culture of production.
As described above, disclosing the multiple-microorganism fertilizer comprising bacillus laterosporus and side spore gemma in the prior art The cultural method of bacillus, but for new bacillus laterosporus microbial manure and preparation method thereof, still suffer from continuing to study Necessity and demand, this is currently the study hotspot and emphasis in microbial manure field, even more the present invention be accomplished it is dynamic Lean on where power and basis.
The content of the invention
In order to seek bacillus laterosporus microbial manure and its production and use, present inventor has performed substantial amounts of Further investigation, after creative work has been paid, so as to complete the present invention.
Specifically, the present invention relates to following aspects.
One side, the present invention relates to a kind of preparation method of bacillus laterosporus microbial manure, methods described bag Include following steps:
S1:Bacillus laterosporus bacterial strain is activated, and aseptic water washing obtains seed liquor;
S2:Amplification cultivation is carried out to seed liquor using the first nutrient solution, the first amplification cultivation liquid is obtained;
S3:The first amplification cultivation liquid is cultivated using the second nutrient solution, obtains the second amplification cultivation liquid;
S4:Second amplification cultivation liquid carries out liquid fermentation and culture, obtains zymotic fluid;
S5:Zymotic fluid is drenched carries out solid fermentation in solid medium, and is post-processed, and obtains bacillus laterosporus Fermenting agent;
S6:Bacillus laterosporus fermenting agent and organic matter mixture are carried out into compost fermentation treatment, it is described so as to obtain Bacillus laterosporus microbial manure.
In the preparation method of bacillus laterosporus microbial manure of the invention, the step S1 is specific as follows:
S1-1:Selection bacillus laterosporus bacterial strain, and be aseptically inoculated in activation training is carried out on slant medium Support, obtain activated strains;
S1-2:Sterile water wash inclined-plane, obtains the seed liquor.
Wherein, the bacillus laterosporus bacterial strain in step S1 may be selected any of spore Bacillus strain, for example CGMCC No.5090, CGMCC No.1755, spore Bacillus strain BL-11, spore Bacillus strain BL-22, the spore bud known Spore bacillus strain BL-21, spore Bacillus strain 1.864, spore Bacillus strain BL-1, spore Bacillus strain 2-Q-9 etc. Deng these bacterial strains can be obtained by various commercial channel, and this is no longer going to repeat them.
Wherein, in step S1, the composition of slant medium is described in per 100g:Agar 5-6g, peptone 3-4g, yeast leaching Cream 0.02-0.03g, analysis for soybean powder 2-3g, corn flour 0.8-1.4g, beef extract 3-4g, sodium chloride 0.2-0.5g, glucose 0.06- 0.1g, balance of sterilized water, and adjust pH value for 7-7.2 (regulating measure is routine techniques, is repeated no more).
Wherein, analysis for soybean powder and corn flour cross 200 mesh sieves.
Wherein, in step S1, the temperature of the activation culture is 30-34 DEG C, for example, can be 30 DEG C, 32 DEG C or 34 DEG C.
Wherein, in step S1, time of the activation culture is 34-40 hour, for example can be 34 hours, 36 hours, 38 Hour or 40 hours.
Wherein, in step S2, using aseptic water washing inclined-plane, flushing liquor is collected, and it is 1.3 × 10 to adjust bacterial concentration8- 1.4×108Individual/ml, so as to obtain the seed liquor.
In the preparation method of bacillus laterosporus microbial manure of the invention, the step S2 is specific as follows:
S2-1:Prepare the first nutrient solution
Following material is weighed respectively:Metallic element aqueous solution 25ml, vitamin E 1.5g, citric acid 0.15g, L- dried meat ammonia Sour 0.2mg, sucrose 2.5g, agar 8g, peptone 12g, yeast extract 1.4g, ammonium sulfate 1g, sodium phosphate 2.5g, beef extract 3.5g With sodium nitrate 4g;
Above-mentioned substance is added in deionized water, is sufficiently stirred for completely, and 1000ml is settled to deionized water, obtained final product To first nutrient solution.
S2-2:According to 1:The volume ratio of 40-50, the seed liquor is inoculated in first nutrient solution, at 34-36 DEG C Lower ventilation shaken cultivation 20-24 hours, so as to obtain the first amplification cultivation liquid.
Wherein, in step S2-1, the metallic element aqueous solution be by 2.5g manganese sulfates, 3g zinc chloride, 4g magnesium sulfate, 1.5g cobalt chlorides, 2g copper nitrates, 3g calcium chloride, 4g frerrous chlorides, 3g iron chloride are completely dissolved in 1000ml distilled water and obtain Arrive;Then 20-30ml therein is measured, the 20-30ml metallic element aqueous solution used in as above-mentioned steps S2-1.
Wherein, in step S2-2, it is 1 that the seed liquor is connect with the volume ratio of first nutrient solution:40-50, for example may be used It is 1:40、1:45 or 1:50.
Wherein, in step S2-2, the ventilating ratio of the ventilation is 1:0.8-1, for example, can be 1:0.8、1:0.9 or 1:1.
Wherein, in step S2-2, in the be passed through gas of the ventilation, oxygen volume content is 14-20%, for example, can be 14%th, 16%, 18% or 20%, preferably 16-18%, most preferably 17%.
Inventor has found that the oxygen content in the ventilation has significant impact for final result, in suitable body Best technique effect can be obtained under product content.
Wherein, in step S2-2, the rotating speed of the shaken cultivation is 150-170 revs/min.
In the preparation method of bacillus laterosporus microbial manure of the invention, the step S3 is specific as follows:
S3-1:Yeast extract consumption in first nutrient solution is halved (be reduced to 0.7g), and the metallic element aqueous solution Consumption increase be twice (increase to 50ml), other are constant, so as to obtain second nutrient solution (namely according to first The same procedure of nutrient solution is prepared, be nothing but yeast extract consumption halve with metallic element amount of aqueous solution used increase be twice and );
S3-2:According to 1:The volume ratio of 30-35, the first amplification cultivation liquid is connect and is added to second nutrient solution In, air surge culture is passed through at 34-36 DEG C 14-16 hours, so as to obtain the second amplification cultivation liquid.
Wherein, in step S3-1, the consumption of the metallic element aqueous solution is increased by reducing the consumption of yeast extract, is sent out Superior technique effect can now be obtained, it should be now to have been obtained for sufficient amount and activity in the first amplification cultivation liquid Activation flora, so that the consumption but the demand to metallic element that can reduce yeast extract rise (if yeast extract consumption It is constant, excessively fast passage, but viable count can be caused to reduce on the contrary, instead result in last effect reduction).
Wherein, normal air is passed through in step S3-2, during shaken cultivation, without as wanted in step S2-3 The content for seeking oxygen is 14-20%.
Wherein, in step S3-2, the ventilating ratio for being passed through air is 1:1.
Wherein, in step S3-2, the rotating speed of the shaken cultivation is 150-170 revs/min.
In the preparation method of bacillus laterosporus microbial manure of the invention, the step S4 is specific as follows:
The second amplification cultivation liquid is added in the liquid fermentation medium for 20-30 times of its volume carries out two-part Fermentation at elevated temperatures culture, fermented and cultured total time is 10-12 hours, and period is passed through air always, and the ventilating ratio for being passed through air is 1: 0.6-1, for example, can be 1:0.6、1:0.8 or 1:1, so as to obtain the zymotic fluid.
Wherein, the liquid fermentation medium is with every liter (L) (the 1L compounds for finally giving, namely 1L liquid fermentations Culture medium) meter, comprising yeast extract 0.5g, peptone 2g, maltose 4g, glucose 1g, manganese sulfate 0.6g, sodium chloride 3.8g, Analysis for soybean powder 7g, boric acid 1.5g, potassium nitrate 2.5g, urea 6g, lysine 0.7g and ammonium sulfate 1.5g, balance of sterilized water.
Wherein, analysis for soybean powder crosses 200 mesh sieves.
Wherein, the two-part fermentation at elevated temperatures culture refers to (to start meter in the first half time of fermented and cultured total time 5-6 hours for rising) in, fermentation temperature is 32-34 DEG C, and temperature then is increased into 38-40 DEG C in 10 minutes, and in the temperature The lower fermentation for completing follow-up remaining time.
Inventor's discovery, by two-part fermentation at elevated temperatures culture so, can obtain best technique effect, it should be By after Preliminary fermentation, continuing to heat up, can further improve fermentation efficiency, improve viable count.
In the preparation method of bacillus laterosporus microbial manure of the invention, the step S5 is specific as follows:
According to mass ratio 1:The ratio of 10-14, the zymotic fluid is drenched in solid medium, adds appropriate deionization Water, makes overall biodiversity content for 32-36%, then fully turn it is uniform, load length be 3 meters, width be 1.5 meters and During depth is 1.5 meters of fermentation tank, natural packing ferments 60-70 hours, and period remains that overall biodiversity content is 32-36%, and be passed through sterile wind to keep the central temperature inside fermentation tank is 56-60 DEG C;After fermentation ends, lead to heated-air drying, Until biodiversity content is less than 5%, fermenting agent is obtained.
Wherein, during fermentation, if interval of the biodiversity content of entirety less than 32-36%, by drenching into going The method of ionized water is held it in the range of this, and this is the routine that those skilled in the art should possess after the present invention is read Ability, is no longer described in detail herein.
Wherein, the solid medium is obtained as follows:By 3 weight portion cotton dregs, 4 weight portion peanut shells Powder, 2 weight portion wheat bran, 0.2 weight portion molasses, 2 weight portion peanut cakes, 2.5 weight portion dry silkworm excrements, the dry corn of 10 weight portions Powder of straw, 0.8 weight portion plant ash, 2 weight portion fishbone dusts, the dry bagasse of 4 weight portions, 0.008 part by weight of cellulose enzyme, 1.8 weight portion Dry chick faeces, 0.1 weight portion ammonium chloride, crushed 50 mesh sieves, then 130-140 DEG C of high temperature after being well mixed Vapor fully sterilizes, that is, obtain the solid medium.
In the preparation method of bacillus laterosporus microbial manure of the invention, the step S6 is specially:According to 1: The mass ratio of 40-50, the bacillus laterosporus fermenting agent and organic matter mixture is sufficiently mixed, and carry out compost Fermentation process, obtains final product the bacillus laterosporus microbial manure after post processing.
Wherein, the organic matter mixture is the arbitrary proportion mixing of all any organic matters that can be used to prepare organic fertilizer Thing, for example can be dry maize straw, drying wheat stalk, wheat bran, drying bagasse, vinasse, dregs of beans, cotton dregs, peanut shell powder, Dry rice straw, biogas residue, dry pig manure, Dry chick faeces, various bone meal etc. in any various mixtures with arbitrary proportion, but For comprehensive nutrition meter, it is preferred to use at least 5 kinds therein, and preferably add appropriate corn flour, beancake powder, peanut cake The assisted fermentations such as powder, molasses, cellulase, amylase and decomposition nutrition matter.
Wherein, the compost fermentation treatment can be using the conventional fermentation techniques in compost fermentation field, until it has fermented It is all only, is no longer described one by one herein.
Wherein, after the completion of the post processing refers to compost fermentation, it is dried to biodiversity content less than 5%, obtains final product The bacillus laterosporus microbial manure.
Second aspect, the present invention relates to the bacillus laterosporus microorganism fertilizer according to obtained in above-mentioned preparation method Material.
Preparation method of the invention is by unique multiple technical characteristics synergy each other and mutually promotes, from And good technique effect is achieved, can provide with high activity, highdensity bacillus laterosporus fermenting agent, and then The bacillus laterosporus microbial manure with excellent properties is arrived, so as to industrially have a good application prospect and produce Potentiality.
3rd aspect, the present invention relates to purposes of the bacillus laterosporus microbial manure in agriculture field.
Find that the bacillus laterosporus microbial manure has superperformance by research, thus can in agriculture field, For example in the plantation and/or cultivation of crops, veterinary antibiotics, flowers or nursery stock etc. have a good application prospect and potentiality.
As described above, the invention provides a kind of bacillus laterosporus microbial manure and its production and use, institute Preparation method is stated by being mutually combined between unique multiple technical characteristics and is cooperateed with, so as to obtain imitating with excellent technology The final bacillus laterosporus microbial manure of fruit, disclosure satisfy that the widespread demand of agricultural technology field, with good application Prospect and industrial production potential.
Specific embodiment
Below by specific embodiment, the present invention is described in detail, but the purposes of these exemplary embodiments and Purpose is only used for enumerating the present invention, not constitutes any type of any restriction to real protection scope of the invention, more non-to incite somebody to action Protection scope of the present invention is confined to this.
Preparation example 1:Slant medium
Often the composition of 100g slant mediums is:Agar 5.5g, peptone 3.5g, yeast extract 0.025g, analysis for soybean powder 2.5g, corn flour 1.1g, beef extract 3.5g, sodium chloride 0.35g, glucose 0.08g, balance of sterilized water, its pH value is 7- 7.2。
Wherein, analysis for soybean powder and corn flour cross 200 mesh sieves.
Preparation example 2:The preparation of the metallic element aqueous solution
By 2.5g manganese sulfates, 3g zinc chloride, 4g magnesium sulfate, 1.5g cobalt chlorides, 2g copper nitrates, 3g calcium chloride, 4g protochlorides Iron, 3g iron chloride are completely dissolved in 1000ml distilled water, so as to obtain the metallic element aqueous solution.
Preparation example 3:Liquid fermentation medium
Liquid fermentation medium in terms of every liter (L), comprising yeast extract 0.5g, peptone 2g, maltose 4g, glucose 1g, manganese sulfate 0.6g, sodium chloride 3.8g, analysis for soybean powder 7g, boric acid 1.5g, potassium nitrate 2.5g, urea 6g, lysine 0.7g and sulfuric acid Ammonium 1.5g, balance of sterilized water.
Wherein, analysis for soybean powder crosses 200 mesh sieves.
Preparation example 4:The preparation (i.e. solid medium in step S5) of solid medium
By 3 weight portion cotton dregs, 4 weight portion peanut shell powders, 2 weight portion wheat bran, 0.2 weight portion molasses, 2 weight portion peanuts Cake, 2.5 weight portion dry silkworm excrements, the dry corn stalk powder of 10 weight portions, 0.8 weight portion plant ash, 2 weight portion fishbone dusts, 4 weights The dry bagasse of amount part, 0.008 part by weight of cellulose enzyme, 1.8 weight portion Dry chick faeces, 0.1 weight portion ammonium chloride, mixing are equal 50 mesh sieves were crushed after even, then 130-140 DEG C of high-temperature vapor fully sterilizes, that is, obtained the solid medium.
Unless otherwise stated, following all of slant medium, the metallic element aqueous solution, liquid fermentation medium and Solid medium is the respective substance in corresponding above-mentioned preparation example 1-4.
Embodiment 1
S1:Bacillus laterosporus bacterial strain is activated, and aseptic water washing obtains seed liquor
S1-1:Selection bacillus laterosporus bacterial strain CGMCC No.1755, and aseptically it is inoculated in slant medium On carry out activation culture, the temperature of the activation culture is 32 DEG C, and the time of activation culture is 37 hours, so as to obtain activating bacterium Strain;
S1-2:Sterile water wash inclined-plane, obtains the seed liquor
Using aseptic water washing inclined-plane, flushing liquor is collected, and it is 1.35 × 10 to adjust bacterial concentration8Individual/ml, so as to obtain The seed liquor;
S2:Amplification cultivation is carried out to seed liquor using the first nutrient solution, the first amplification cultivation liquid is obtained
S2-1:Prepare the first nutrient solution
Following material is weighed respectively:Metallic element aqueous solution 25ml, vitamin E 1.5g, citric acid 0.15g, L- dried meat ammonia Sour 0.2mg, sucrose 2.5g, agar 8g, peptone 12g, yeast extract 1.4g, ammonium sulfate 1g, sodium phosphate 2.5g, beef extract 3.5g With sodium nitrate 4g;
Above-mentioned substance is added in deionized water, is sufficiently stirred for completely, and 1000ml is settled to deionized water, obtained final product To the first nutrient solution;
S2-2:According to 1:45 volume ratio, the seed liquor is inoculated in first nutrient solution, at 34-36 DEG C (ventilating ratio is 1 to ventilation shaken cultivation within 22 hours:0.9, oxygen volume content is 17%, and the rotating speed of shaken cultivation is 160 revs/min Clock), so as to obtain the first amplification cultivation liquid;
S3:The first amplification cultivation liquid is cultivated using the second nutrient solution, obtains the second amplification cultivation liquid
S3-1:Yeast extract consumption in first nutrient solution is halved (be reduced to 0.7g), and the metallic element aqueous solution Consumption increase be twice (increase to 50ml), other are constant, so as to obtain the second nutrient solution;
S3-2:According to 1:32.5 volume ratio, the first amplification cultivation liquid is connect and is added in second nutrient solution, Air surge culture is passed through at 34-36 DEG C, and (ventilating ratio is 1 within 15 hours:1, the rotating speed of shaken cultivation is 160 revs/min), from And obtain the second amplification cultivation liquid;
S4:Second amplification cultivation liquid carries out liquid fermentation and culture, obtains zymotic fluid
The second amplification cultivation liquid is added in the liquid fermentation medium for 25 times of its volume carries out two-part liter Warm fermented and cultured, fermented and cultured total time is 11 hours, and period is passed through air always, and the ventilating ratio for being passed through air is 1:0.8, from And obtain zymotic fluid;
Wherein, the two-part fermentation at elevated temperatures culture refer to fermented and cultured total time the first half time it is (i.e. preceding 5.5 Hour) in, fermentation temperature is 33 DEG C, and temperature then is increased into 39 DEG C in 10 minutes, and completes follow-up surplus at such a temperature The fermentation of remaining time (5.5 hours after i.e.);
S5:Zymotic fluid is drenched carries out solid fermentation in solid medium, and is post-processed, and obtains bacillus laterosporus Fermenting agent, specially:
According to mass ratio 1:12 ratio, the zymotic fluid is drenched in solid medium, adds appropriate amount of deionized water, Make overall biodiversity content for 32-36%, then fully turn uniformly, load length for 3 meters, width are for 1.5 meters and deep Spend in the fermentation tank for 1.5 meters, natural packing ferments 65 hours, period remains that overall biodiversity content is 32- 36%, and be passed through sterile wind to keep the central temperature inside fermentation tank is 56-60 DEG C;After fermentation ends, lead to heated-air drying, until Biodiversity content is less than 5%, obtains fermenting agent, is named as F1;
S6:Bacillus laterosporus fermenting agent and organic matter mixture are carried out into compost fermentation treatment, so as to obtain side spore Micro-organisms bacillus fertilizer, specially:
According to 1:45 mass ratio, the bacillus laterosporus fermenting agent and organic matter mixture are fully mixed Close, and compost fermentation treatment is carried out according to routine techniques, after the completion of compost fermentation, be dried to biodiversity content and be less than 5%, bacillus laterosporus microbial manure is obtained final product, it is named as C1;
Wherein, the organic matter mixture is mass ratio 1:1:0.1:2:2:1:0.3 1 weight portion dries maize straw, 1 Weight portion wheat bran, 0.1 weight portion dregs of beans, 2 weight portion drying bagasses, 2 weight portion biogas residues, 1 weight portion Dry chick faeces, 0.3 weight Amount part fishbone dust, 0.05 parts by weight Corn powder, 0.01 weight portion molasses, the mixture of 0.005 weight portion.
Embodiment 2
S1:Bacillus laterosporus bacterial strain is activated, and aseptic water washing obtains seed liquor
S1-1:Selection bacillus laterosporus bacterial strain CGMCC No.1755, and aseptically it is inoculated in slant medium On carry out activation culture, the temperature of the activation culture is 30 DEG C, and the time of activation culture is 40 hours, so as to obtain activating bacterium Strain;
S1-2:Sterile water wash inclined-plane, obtains the seed liquor
Using aseptic water washing inclined-plane, flushing liquor is collected, and it is 1.3 × 10 to adjust bacterial concentration8Individual/ml, so as to obtain The seed liquor;
S2:Amplification cultivation is carried out to seed liquor using the first nutrient solution, the first amplification cultivation liquid is obtained
S2-1:Prepare the first nutrient solution
Following material is weighed respectively:Metallic element aqueous solution 25ml, vitamin E 1.5g, citric acid 0.15g, L- dried meat ammonia Sour 0.2mg, sucrose 2.5g, agar 8g, peptone 12g, yeast extract 1.4g, ammonium sulfate 1g, sodium phosphate 2.5g, beef extract 3.5g With sodium nitrate 4g;
Above-mentioned substance is added in deionized water, is sufficiently stirred for completely, and 1000ml is settled to deionized water, obtained final product To the first nutrient solution;
S2-2:According to 1:40 volume ratio, the seed liquor is inoculated in first nutrient solution, at 34-36 DEG C (ventilating ratio is 1 to ventilation shaken cultivation within 20 hours:0.8, oxygen volume content is 17%, and the rotating speed of shaken cultivation is 150 revs/min Clock), so as to obtain the first amplification cultivation liquid;
S3:The first amplification cultivation liquid is cultivated using the second nutrient solution, obtains the second amplification cultivation liquid
S3-1:Yeast extract consumption in first nutrient solution is halved (be reduced to 0.7g), and the metallic element aqueous solution Consumption increase be twice (increase to 50ml), other are constant, so as to obtain the second nutrient solution;
S3-2:According to 1:30 volume ratio, the first amplification cultivation liquid is connect and is added in second nutrient solution, Air surge culture is passed through at 34-36 DEG C, and (ventilating ratio is 1 within 14 hours:1, the rotating speed of shaken cultivation is 150 revs/min) so that Obtain the second amplification cultivation liquid;
S4:Second amplification cultivation liquid carries out liquid fermentation and culture, obtains zymotic fluid
The second amplification cultivation liquid is added in the liquid fermentation medium for 20 times of its volume carries out two-part liter Warm fermented and cultured, fermented and cultured total time is 10 hours, and period is passed through air always, and the ventilating ratio for being passed through air is 1:0.6, from And obtain zymotic fluid;
Wherein, the two-part fermentation at elevated temperatures culture refers to that (i.e. preceding 5 small in the first half time of fermented and cultured total time When) in, fermentation temperature is 32 DEG C, and temperature then is increased into 38 DEG C in 10 minutes, and completes follow-up remaining at such a temperature The fermentation of time (5 hours after i.e.);
S5:Zymotic fluid is drenched carries out solid fermentation in solid medium, and is post-processed, and obtains bacillus laterosporus Fermenting agent, specially:
According to mass ratio 1:10 ratio, the zymotic fluid is drenched in solid medium, adds appropriate amount of deionized water, Make overall biodiversity content for 32-36%, then fully turn uniformly, load length for 3 meters, width are for 1.5 meters and deep Spend in the fermentation tank for 1.5 meters, natural packing ferments 60 hours, period remains that overall biodiversity content is 32- 36%, and be passed through sterile wind to keep the central temperature inside fermentation tank is 56-60 DEG C;After fermentation ends, lead to heated-air drying, until Biodiversity content is less than 5%, obtains fermenting agent, is named as F2;
S6:Bacillus laterosporus fermenting agent and organic matter mixture are carried out into compost fermentation treatment, so as to obtain side spore Micro-organisms bacillus fertilizer, specially:
According to 1:40 mass ratio, the bacillus laterosporus fermenting agent and organic matter mixture are fully mixed Close, and compost fermentation treatment is carried out according to routine techniques, after the completion of compost fermentation, be dried to biodiversity content and be less than 5%, bacillus laterosporus microbial manure is obtained final product, it is named as C2;
Wherein, the organic matter mixture is with the organic matter mixture in embodiment 1.
Embodiment 3
S1:Bacillus laterosporus bacterial strain is activated, and aseptic water washing obtains seed liquor
S1-1:Selection bacillus laterosporus bacterial strain CGMCC No.1755, and aseptically it is inoculated in slant medium On carry out activation culture, the temperature of the activation culture is 34 DEG C, and the time of activation culture is 34 hours, so as to obtain activating bacterium Strain;
S1-2:Sterile water wash inclined-plane, obtains the seed liquor
Using aseptic water washing inclined-plane, flushing liquor is collected, and it is 1.4 × 10 to adjust bacterial concentration8Individual/ml, so as to obtain The seed liquor;
S2:Amplification cultivation is carried out to seed liquor using the first nutrient solution, the first amplification cultivation liquid is obtained
S2-1:Prepare the first nutrient solution
Following material is weighed respectively:Metallic element aqueous solution 25ml, vitamin E 1.5g, citric acid 0.15g, L- dried meat ammonia Sour 0.2mg, sucrose 2.5g, agar 8g, peptone 12g, yeast extract 1.4g, ammonium sulfate 1g, sodium phosphate 2.5g, beef extract 3.5g With sodium nitrate 4g;
Above-mentioned substance is added in deionized water, is sufficiently stirred for completely, and 1000ml is settled to deionized water, obtained final product To the first nutrient solution;
S2-2:According to 1:50 volume ratio, the seed liquor is inoculated in first nutrient solution, at 34-36 DEG C (ventilating ratio is 1 to ventilation shaken cultivation within 24 hours:1, oxygen volume content is 17%, and the rotating speed of shaken cultivation is 170 revs/min Clock), so as to obtain the first amplification cultivation liquid;
S3:The first amplification cultivation liquid is cultivated using the second nutrient solution, obtains the second amplification cultivation liquid
S3-1:Yeast extract consumption in first nutrient solution is halved (be reduced to 0.7g), and the metallic element aqueous solution Consumption increase be twice (increase to 50ml), other are constant, so as to obtain the second nutrient solution;
S3-2:According to 1:35 volume ratio, the first amplification cultivation liquid is connect and is added in second nutrient solution, Air surge culture is passed through at 34-36 DEG C, and (ventilating ratio is 1 within 16 hours:1, the rotating speed of shaken cultivation is 170 revs/min) so that Obtain the second amplification cultivation liquid;
S4:Second amplification cultivation liquid carries out liquid fermentation and culture, obtains zymotic fluid
The second amplification cultivation liquid is added in the liquid fermentation medium for 30 times of its volume carries out two-part liter Warm fermented and cultured, fermented and cultured total time is 12 hours, and period is passed through air always, and the ventilating ratio for being passed through air is 1:1, so that Obtain zymotic fluid;
Wherein, the two-part fermentation at elevated temperatures culture refers to that (i.e. preceding 6 small in the first half time of fermented and cultured total time When) in, fermentation temperature is 34 DEG C, and temperature then is increased into 40 DEG C in 10 minutes, and completes follow-up remaining at such a temperature The fermentation of time (6 hours after i.e.);
S5:Zymotic fluid is drenched carries out solid fermentation in solid medium, and is post-processed, and obtains bacillus laterosporus Fermenting agent, specially:
According to mass ratio 1:14 ratio, the zymotic fluid is drenched in solid medium, adds appropriate amount of deionized water, Make overall biodiversity content for 32-36%, then fully turn uniformly, load length for 3 meters, width are for 1.5 meters and deep Spend in the fermentation tank for 1.5 meters, natural packing ferments 70 hours, period remains that overall biodiversity content is 32- 36%, and be passed through sterile wind to keep the central temperature inside fermentation tank is 56-60 DEG C;After fermentation ends, lead to heated-air drying, until Biodiversity content is less than 5%, obtains fermenting agent, is named as F3;
S6:Bacillus laterosporus fermenting agent and organic matter mixture are carried out into compost fermentation treatment, so as to obtain side spore Micro-organisms bacillus fertilizer, specially:
According to 1:50 mass ratio, the bacillus laterosporus fermenting agent and organic matter mixture are fully mixed Close, and compost fermentation treatment is carried out according to routine techniques, after the completion of compost fermentation, be dried to biodiversity content and be less than 5%, bacillus laterosporus microbial manure is obtained final product, it is named as C2;
Wherein, the organic matter mixture is with the organic matter mixture in embodiment 1.
Comparative example 1-6:The investigation of nutrient solution
Comparative example 1-3:In addition to second nutrient solution of S3 replaces with the first nutrient solution the step of respectively by embodiment 1-3 (i.e. First liquid culture medium is used in step S2-S3), other operations are constant, so as to repeat embodiment 1-3, point Comparative example 1-3 is not obtained, and gained bacillus laterosporus fermenting agent is sequentially named as DF1, DF2 and DF3, gained is finally fertile Material is sequentially named as DC1, DC2 and DC3.
Comparative example 4-6:In addition to first nutrient solution of S2 replaces with the second nutrient solution the step of respectively by embodiment 1-3 (i.e. Second liquid culture medium is used in step S2-S3), other operations are constant, so as to repeat embodiment 1-3, point Comparative example 4-6 is not obtained, and gained bacillus laterosporus fermenting agent is sequentially named as DF4, DF5 and DF6, gained is finally fertile Material is sequentially named as DC4, DC5 and DC6.
Comparative example 7-10:The investigation of oxygen content in being divulged information in step S2-2
The oxygen volume content (other operations are constant) in the step S2-2 shown in following table is respectively adopted, institute is accumulated using oxysome Content, correspondence embodiment, the name of gained bacillus laterosporus fermenting agent and final fertilizer see the table below 1.
Table 1
Comparative example 11-16:The investigation that two-part heats up in step S4
Comparative example 11-13:Except respectively by embodiment 1-3 the step of S4 two-part heat up be revised as respective first Whole at a temperature of section to have implemented all of fermentation (the correspondingly warming temperature without 10 minutes), other operations are constant, so that Repeated embodiment 1-3, respectively obtain comparative example 11-13 (i.e. comparative example 11,12,13 the step of S3 in whole fermentation Temperature is respectively 33 DEG C, 32 DEG C, 34 DEG C), by gained bacillus laterosporus fermenting agent be sequentially named as DF11, DF12 and DF13, DC11, DC12 and DC13 are sequentially named as by the final fertilizer of gained.
Comparative example 14-16:Except respectively by embodiment 1-3 the step of S4 two-part heat up be revised as respective second Whole at a temperature of section to have implemented all of fermentation (the correspondingly warming temperature without 10 minutes), other operations are constant, so that Repeated embodiment 1-3, respectively obtain comparative example 14-16 (i.e. comparative example 11,12,13 the step of S3 in whole fermentation Temperature is respectively 39 DEG C, 38 DEG C, 40 DEG C), by gained bacillus laterosporus fermenting agent be sequentially named as DF14, DF15 and DF16, DC14, DC15 and DC16 are sequentially named as by the final fertilizer of gained.
Performance
A, the investigation of colony counting
According to the traditional test methods in this area, the different bacillus laterosporuses obtained to each embodiment and comparative example Fermenting agent carries out colony counting investigation at once after preparing, investigated respectively viable count in every gram of fermenting agent and Gemma rate, as a result see the table below 2.
Wherein, multiple fermenting agents of identical group take its average.
Table 2
As can be seen here:1st, the F1-F3 that the inventive method is obtained has viable count very high and gemma rate;2 and ought make always During with the first nutrient solution or the second nutrient solution, viable count and gemma rate are significantly reduced, and especially the second nutrient solution is reduced more It is obvious (see DF4-DF6);3rd, in step S2-2 divulge information oxygen content it is extremely important, when for 17% when can obtain best skill Art effect, it is bigger to deviate the value, then viable count and gemma rate reduction more obvious (see DF7-DF10), and this proves the determination of oxygen content With unobviousness, and effect is unexpected;4th, the two-part fermentation at elevated temperatures in step S4 equally has for final result Significant impact the most, when warming temperature is not carried out, always in the first stage at a temperature of when fermenting, viable count and gemma rate are most Difference is (see DF11-DF13);It is straight in the first stage at a temperature of when fermenting, viable count and gemma rate are also reduced significantly (see DF14- DF16), but it is better than DF11-DF13, this demonstrate that only being heated up using two-part of the invention, best technology could be obtained Effect.
The investigation of B, heat-resisting quantity
Each embodiment and comparative example 40 minutes after different bacillus laterosporus fermenting agents are obtained, respectively in difference Temperature (70 DEG C, 80 DEG C, 90 DEG C and 100 DEG C) under constant temperature keep 20 minutes, its viable count, and and initial live are then measured again Bacterium number is calculated, and so as to obtain the survival rate after high temperature, as a result see the table below 3.
Wherein, multiple fermenting agents of identical group take its average.
Table 3
As can be seen here:1st, the F1-F3 that the inventive method is obtained has excellent high temperature resistant property, and this prepares organic in fermentation There is more preferable high-temperature adaptability when fertile;2 and the resistance to elevated temperatures of the fermenting agent of comparative example, especially when higher than 80 DEG C With obvious reduction, especially DF11-DF13, bacterium colony resistance to elevated temperatures now is significantly reduced.
The investigation of C, storage stability
By each embodiment and comparative example after different bacillus laterosporus fermenting agents are obtained, kept in dark place under normal temperature Regular hour, and viable count when investigating different time respectively, and calculated with initial viable count, so as to obtain different storages The survival rate after the time is deposited, 4 are as a result see the table below.
Wherein, multiple fermenting agents of identical group take its average.
Table 4
As can be seen here:1st, the F1-F3 that the inventive method is obtained has excellent storage stability, and this is in feed and microorganism Fertilizer field has good application value, can store the longer time;2 and the storage stability of the fermenting agent of comparative example Then there is obvious reduction, especially significantly, wherein DF11-DF13 is worst for DF7-DF8, DF11-DF16 reduction, and this proves step Oxygen content in rapid S3 and the two-part fermentation at elevated temperatures in step S4 can unpredictably influence final performance.
The plantation culture Performance of fertilizer
I, corn planting volume increase are investigated
According to every 100 square metres as one piece of sample plot (corn variety be good beautiful 99), be divided into control group, chemical group, Microbial manure group, it is specific as follows:
Control group:Any fertilizer is not used.
Chemical group:Using normal chemical fertilizer, i.e. N, P, K fertilizer, 5kg ammonium chlorides, 5kg potassium sulfates and 3kg phosphorus can be used Sour ammonium is applied fertilizer.
Microbial manure group:Using the microbial manure of the 5kg embodiment of the present invention or comparative example, (each sample plot is only respectively Use a kind of microbial manure), and N, P, K of the same ratio of the amount of additional chemical group 1/4 are fertile.
After normal field management and harvesting, per mu yield yield is converted to, as a result see the table below 5.
Table 5
Wherein, wherein, the data of C1-C3 carry out correspondence, example, " 805,801,799 " meaning in that same order respectively C1 for 805, C2 is that 801 and C3 is 799.Numbered corresponding relation (be also so tool in following all forms Have same implication, no longer list one by one when the time comes), this is no longer going to repeat them.
As can be seen here, microbial manure C1-C3 of the invention has effect of increasing production the most excellent, increases relative to chemical group Produce>10%, although other contrast fertilizer will be significantly below C1-C3, but still chemical group is significantly better than, also achieve good Effect of increasing production.
II, growing tomatoes are investigated
According to every 100 square metres as one piece of sample plot (tomato variety be in miscellaneous 109), be divided into control group, chemistry Group, microbial manure group, it is specific as follows:
Control group:Any fertilizer is not used.
Chemical group:Using normal chemical fertilizer, i.e. N, P, K fertilizer, 8kg ammonium chlorides, 4kg potassium sulfates and 6kg phosphoric acid are used Ammonium is applied fertilizer.
Microbial manure group:Using the microbial manure of the 6kg embodiment of the present invention or comparative example, (each sample plot is only respectively Use a kind of microbial manure), and N, P, K of the same ratio of the amount of additional chemical group 1/4 are fertile.
After normal field management and harvesting, per mu yield yield is converted to, (is as benchmark using the yield of control group 100) fractional yield of chemical group and microbial manure group, is calculated, 6 are as a result see the table below.
Wherein, due to each group in multiple fertilizer corresponding to tomato production deviation less, therefore use each group Average value investigated.
Table 6
As can be seen here, microbial manure C1-C3 of the invention has berry effect of increasing production the most excellent, relative to control Group increases 27.8%, also has relative to chemical group and significantly increases production.And contrast microbial manure then has relative to C1-C3 Significant reduction, especially DC11-DC13, this performance trend also with fermenting agent are consistent.But even significantly reduce, Still it is significantly better than control group and chemical group.
In sum, the invention provides a kind of bacillus laterosporus microbial manure and its production and use, institute Preparation method is stated by being mutually combined between unique multiple technical characteristics and is cooperateed with, so as to obtain imitating with excellent technology The final bacillus laterosporus microbial manure of fruit, disclosure satisfy that the widespread demand of agricultural technology field, with good application Prospect and industrial production potential.
It should be appreciated that the purposes of these embodiments is merely to illustrate the present invention and is not intended to limit protection model of the invention Enclose.Additionally, it will also be appreciated that after technology contents of the invention have been read, those skilled in the art can make each to the present invention Plant and change, change and/or modification, all these equivalent form of value equally falls within the guarantor that the application appended claims are limited Within the scope of shield.
In sum, the invention provides a kind of Novel culture method of bacillus laterosporus, methods described is by uniqueness Multiple technical characteristics between be mutually combined and cooperate with, so as to obtain the final bacillus laterosporus with excellent technique effect Fermenting agent, disclosure satisfy that the widespread demand of multiple fields, have a good application prospect and industrial production potential.
It should be appreciated that the purposes of these embodiments is merely to illustrate the present invention and is not intended to limit protection model of the invention Enclose.Additionally, it will also be appreciated that after technology contents of the invention have been read, those skilled in the art can make each to the present invention Plant and change, change and/or modification, all these equivalent form of value equally falls within the guarantor that the application appended claims are limited Within the scope of shield.

Claims (10)

1. a kind of preparation method of bacillus laterosporus microbial manure, methods described comprises the following steps:
S1:Bacillus laterosporus bacterial strain is activated, and aseptic water washing obtains seed liquor;
S2:Amplification cultivation is carried out to seed liquor using the first nutrient solution, the first amplification cultivation liquid is obtained;
S3:The first amplification cultivation liquid is cultivated using the second nutrient solution, obtains the second amplification cultivation liquid;
S4:Second amplification cultivation liquid carries out liquid fermentation and culture, obtains zymotic fluid;
S5:Zymotic fluid is drenched carries out solid fermentation in solid medium, and is post-processed, and obtains bacillus laterosporus fermentation Microbial inoculum;
S6:Bacillus laterosporus fermenting agent and organic matter mixture are carried out into compost fermentation treatment, so as to obtain the side spore Micro-organisms bacillus fertilizer.
2. preparation method as claimed in claim 1, it is characterised in that:The step S1 is specific as follows:
S1-1:Selection bacillus laterosporus bacterial strain, and be aseptically inoculated in activation culture is carried out on slant medium, obtain To activated strains;
S1-2:Sterile water wash inclined-plane, obtains the seed liquor;
In step S1-1, the composition of slant medium is described in per 100g:Agar 5-6g, peptone 3-4g, yeast extract 0.02- 0.03g, analysis for soybean powder 2-3g, corn flour 0.8-1.4g, beef extract 3-4g, sodium chloride 0.2-0.5g, glucose 0.06-0.1g, it is remaining It is sterilized water to measure, and adjusts pH value for 7-7.2.
3. the preparation method as described in claim any one of 1-2, it is characterised in that:The step S2 is specific as follows:
S2-1:Prepare the first nutrient solution
Following material is weighed respectively:Metallic element aqueous solution 25ml, vitamin E 1.5g, citric acid 0.15g, L-PROLINE 0.2mg, sucrose 2.5g, agar 8g, peptone 12g, yeast extract 1.4g, ammonium sulfate 1g, sodium phosphate 2.5g, beef extract 3.5g and Sodium nitrate 4g;
Above-mentioned substance is added in deionized water, is sufficiently stirred for completely, and 1000ml is settled to deionized water, that is, obtain institute State the first nutrient solution.
S2-2:According to 1:The volume ratio of 40-50, the seed liquor is inoculated in first nutrient solution, is led at 34-36 DEG C Wind shaken cultivation 20-24 hours, so as to obtain the first amplification cultivation liquid.
4. preparation method as claimed in claim 3, it is characterised in that:In step S2-1, the metallic element aqueous solution be by 2.5g manganese sulfates, 3g zinc chloride, 4g magnesium sulfate, 1.5g cobalt chlorides, 2g copper nitrates, 3g calcium chloride, 4g frerrous chlorides, 3g iron chloride It is completely dissolved in obtained from 1000ml distilled water.
5. the preparation method as described in claim any one of 3-4, it is characterised in that:It is described to be passed through in step S2-2 Gas in, oxygen volume content be 14-20%, preferably 16-18%, most preferably 17%.
6. the preparation method as described in claim any one of 1-5, it is characterised in that:The step S3 is specific as follows:
S3-1:Yeast extract consumption in first nutrient solution is halved, and the consumption increasing of the metallic element aqueous solution is twice, other It is constant, so as to obtain second nutrient solution;
S3-2:According to 1:The volume ratio of 30-35, the first amplification cultivation liquid is connect and is added in second nutrient solution, Air surge culture is passed through at 34-36 DEG C 14-16 hours, so as to obtain the second amplification cultivation liquid.
7. the preparation method as described in claim any one of 1-6, it is characterised in that:The step S4 is specific as follows:
The second amplification cultivation liquid is added in the liquid fermentation medium for 20-30 times of its volume carries out two-part intensification Fermented and cultured, fermented and cultured total time is 10-12 hours, and period is passed through air always, and the ventilating ratio for being passed through air is 1:0.6- 1, so as to obtain the zymotic fluid;
Wherein, the liquid fermentation medium is in terms of every liter (L), comprising yeast extract 0.5g, peptone 2g, maltose 4g, Portugal Grape sugar 1g, manganese sulfate 0.6g, sodium chloride 3.8g, analysis for soybean powder 7g, boric acid 1.5g, potassium nitrate 2.5g, urea 6g, lysine 0.7g and Ammonium sulfate 1.5g, balance of sterilized water;
Wherein, the two-part fermentation at elevated temperatures culture refers to that fermentation temperature is in the first half time of fermented and cultured total time 32-34 DEG C, temperature is then increased to 38-40 DEG C in 10 minutes, and completes the fermentation of follow-up remaining time at such a temperature.
8. the preparation method as described in claim any one of 1-7, it is characterised in that:The step S5 is specific as follows:
According to mass ratio 1:The ratio of 10-14, the zymotic fluid is drenched in solid medium, adds appropriate amount of deionized water, Make overall biodiversity content for 32-36%, then fully turn uniformly, load length for 3 meters, width are for 1.5 meters and deep Spend in the fermentation tank for 1.5 meters, natural packing ferments 60-70 hours, period remains that overall biodiversity content is 32- 36%, and be passed through sterile wind to keep the central temperature inside fermentation tank is 56-60 DEG C;After fermentation ends, lead to heated-air drying, until Biodiversity content is less than 5%, obtains fermenting agent.
9. the bacillus laterosporus microbial manure obtained in preparation method according to claim any one of 1-8.
10. purposes of the bacillus laterosporus microbial manure in agriculture field described in claim 9.
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Application publication date: 20170613