CN100447235C - Anti-locust bacillus thuringiensis and preparation method for Bt locust killing agent - Google Patents
Anti-locust bacillus thuringiensis and preparation method for Bt locust killing agent Download PDFInfo
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Abstract
The present invention discloses a bacillus thuringiensis BTH-13 (CCTCC No. M206061) for preventing grasshoppers. The insecticide is prepared by the following steps: firstly, shaking a flask for fermentation, proportionally adding starch, bean cake powder, cotton cake powder, peptone, yeast powder, corn steep liquor, magnesium sulfate, potassium dihydrogen phosphate, dipotassium hydrogen phosphate, calcium carbonate and alpha-amylase in culture medium with 100 unit volume, and supplying water; secondly, 100 ml of culture medium in a triangular flask, inoculating BTH-13 after sterilization, and breeding to spore abscission under the certain temperature; thirdly, using the selected culture medium, fermenting in a full automatic fermenting tank, acidifying fermenting liquid after fermentation, adding emulsifiers, and preparing wettable powder after fermenting liquid concentration by directly spraying and drying. The present invention has the characteristics of strong specificity, no damage to natural enemy of insects, no poison for human and livestock, no environment pollution and crop yield increase, and has good application perspective.
Description
Technical field
The present invention relates to the bacillus thuringiensis of a kind of anti-locust, also relate to the preparation method of locust agent extremely simultaneously.It is insecticidal crystal protein matter that the bacillus thuringiensis of the anti-locust of this strain has active toxicity, its active substance to Asiatic migrotory locust of Orthoptera etc.With the control that the locust agent can be used for orthoptera pest such as locust etc. of killing of this bacterial strain preparation, the insecticidal crystal protein plasmagene can be used for the research of the structure and the insect-resistant transgenic plants of efficient engineering bacteria.
Background technology
Characteristics such as bacillus thuringiensis (Bacillus thuringiensis, be called for short Bt) is owing to have good disinsection effect, and high specificity is produced and easy to use, and is free from environmental pollution and in biological control of insect pests, brought into play vital role.Different Bt bacterial strains produces different insecticidal crystal protein matter (Insecticidal Crystal Proteins is called for short ICPs), makes that there is notable difference in insecticidal spectrum and the insecticidal activity between bacterial strain.Report that now bacillus thuringiensis has the specificity insecticidal activity to 9 purpose insects such as lepidopteran, Coleoptera, Diptera and mite class, Plant nematode, protozoon, platyhelminth etc.At present, screen efficient specific b t bacterial strain, excavate new ICP gene, bacterial strain is carried out genetic improvement or makes up the high-efficiency broad spectrum genetic engineering bacterium is global problem, it also is the development trend of Bt research, it is reported that tens thousand of bacillus thuringiensis strains of 86 subspecies of 71 H serotype have been isolated in the whole world, have filtered out many strains have toxic effect to insects such as lepidopteran and Coleopteras bacterial strain from strain separated.Aspect the isolation identification of bacillus thuringiensis bacterial strain, screening, document " form, delta-endotoxin proteins matter and the virulence characteristic thereof of the bacillus thuringiensis in soil source (microorganism journal; 1992; 32 (6): 387-393) ", " from the evaluation (Hua Zhong Agriculture University's journal; 1994; second phase) of isolating 410 bacillus thuringiensis strains of soil, " distribution and the insecticidal properties of bacillus thuringiensis in the southern and northern soil of China " (microorganism journal, 1996,36 (4); 295-302), and " the evaluation of five bacillus thuringiensis new subspecieses in soil source (microorganism journal; 1999,39 (2): 154-159) wait separation to China bacillus thuringiensis, evaluation, characteristic distributions, crystal proteins form, insecticidal properties etc. to study.Efficiently, the screening aspect of specific strains, document " to the new strain isolated of Bt of the high virulence of prodenia litura and The Characteristic Study thereof (microbiology circular; 1997; 24 (5): 262-265) ", " to the bacillus thuringiensis bacterial strain and the crystal proteins feature (Chinese biological control; 1997; 13 (2) 82-85) thereof of the high virulence of exigua larvae ", and " bacillus thuringiensis to the toxic screening of beet armyworm (Chinese virusology; 2000; Vol.15:98-101); " research of a strain broad spectrum bacillus thuringiensis and fermentation condition thereof " (Hua Zhong Agriculture University's journal; 2003,22:(5) 462-465) " waited and screened the efficient specific strains of lepidopteran noctuidae pests extremely in many bacillus thuringiensis bacterial strains of comforming respectively; Document " activity of the anti-Asiatic migrotory locust of bacillus thuringiensis (Locust migratoria manilensis) " (uses and the environmental organism journal 2005,11 (5): the activity of 592-594) having reported the anti-locust of bacillus thuringiensis.Aspect the killing gene clone, since first insecticidal crystal protein plasmagene in 1981 is cloned, the insecticidal crystal protein matter Cry gene and the two class Cyt genes of having cloned more than 300 bacillus thuringiensiss of 50 classes in the present whole world
(
http://www.lifesci.sussex.ac.uk/home/Neil?Crickmore/Bt)。Document " structure in anti-Coleoptera delta-endotoxin and toxin gene library (biotechnology journal; 1994; 10 (2): 103-108) ", " promotor of bacillus thuringiensis insecticidal crystal protein gene and transcriptional control thereof (microbiology circular; 1999; 26 (2): 130-134) ", " research of bacillus thuringiensis efficient bacterial strain cry genetic analysis and multivalent genetic combination (Nankai University's journal; 1999; 32 (3): 163-168) " etc. has set up the gene library of anti-Coleoptera delta-endotoxin respectively, cloned the gene that kills lepidoptera pest, the expression and the regulation and control of bacillus thuringiensis insecticidal crystal protein gene have been set forth.Document " efficiently expressing of structure of wide spectrum reorganization Bt bacterium and gene " (" microbial pesticide and industrialization thereof ", explain sub-ox chief editor, Science Press, 2000,55-61) the crystallin plasmagene cry1Ac that will kill lepidoptera pest with electric shock transformation method changes in the Bt bacterial strain of coleopteran pest extremely, has obtained the Bt engineering bacteria that wide spectrum kills lepidopteran and coleopteran pest; " structure of disinsection prophylaxis genetically engineered subtilis " (biotechnology journal,-1999,15 (2): be carrier 215-220) with subtilis-bacillus coli shuttle plasmid vector pHB201 and pRP22, by the competence method for transformation, bacillus thuringiensis HD-1 insecticidal protein gene cry1Ac is imported rice sheath blight disease biocontrol strain subtilis B916.The electrophoretic analysis of engineering strain plasmid enzyme restriction, the nucleic acid marking (Southern) is analyzed and desinsection biological activity determination result has confirmed the importing of cry1Ac gene and the effective expression in B916 thereof.Bacteria inhibition assay has proved that engineering bacteria has kept the good bacteriostatic activity of former wild type strain.Aspect the development of sterilant, document " research of new bacterial strain of Coleoptera bacillus thuringiensis and sterilant thereof extremely " (microorganism journal, 1999.12, Vol.39 (6): 515-520) and " wide spectrum reorganization bacillus thuringiensis process study " (Chinese virusology 2000.Vol.15:192-195) waits respectively fermentation of the bacillus thuringiensis of different desinsection characteristics and the research that aftertreatment technology carries out.
Locust (Locust) is global great Agricultural pests.The plague of locusts and floods, drought are normal alternate or follow and form agriculture in history three the Nature disasters into the mankind.From the eighties, the locust disaster in the whole world enters the stage of taking place frequently, and except that the South Pole, each continent all has the plague of locusts to take place, and area takes place throughout the year reach 4,680 ten thousand square kilometres, has eighth population to be subjected to the harassment of the plague of locusts throughout the year.The plague of locusts of China also increases the weight of thereupon, and from 1997, China is the big area outburst plague of locusts for successive years, and the highest population density can reach 3000-10000 head/m
2Asiatic migrotory locust in the locust (Locust migratoria manilensis) mainly is distributed in East Asia, south east asia, as in, day, luxuriant and rich with fragrance, safe, state such as get over, in China distribution range the widest, cause disaster the most frequent, the most serious.The plague of locusts China frequently mainly contain three aspect reason: the one,, China's weather drought and waterlogging alternately, the waterlogging back drought omen that takes place of the plague of locusts often earlier; Secondly, the existing locust district 80% of China all is indefinite Bin Hu of weedy river shoal, saltings, coastal waters and water surface fluctuation and reservoir basin etc., and the breeding place of transforming these locusts is quite difficult; In addition, the measure of eliminating locusts is single, mainly adopts broad spectrum chemical pesticides such as organophosphorus, chrysanthemum ester class, and the locust natural enemy is is also killed and wounded, and locust more becomes rampant because of the control of avoiding natural enemy.Taking place frequently of the plague of locusts not only caused heavy losses to agriculture production, and in order to administer the plague of locusts, spend great amount of manpower and material resources and financial resources.At present, control for locust, still mainly be to adopt aircraft big area sprinkling chemical pesticide or manually use the atomizers spray chemical pesticide, still, this big area uses the controlling mode of chemical pesticide when containing locust disaster quickly and effectively, also killed the natural enemy of large number of grasshoppers, destroy the eubiosis, locust is developed immunity to drugs, caused the vicious cycle of the plague of locusts, and severe contamination ecotope, threaten to human health.Therefore in chemical prevention, strengthen the biological method dynamics of eliminating locusts, set up with ecological locust friendly, resources and administer system and technical specifications, become the task of top priority of China's locust control work.
Over nearly 50 years, adopt the development of microbial control locust very fast.As far back as late 1960s, the U.S.----nosema locustae control locust that begins one's study and using microbe, to phase early 1980s, this biological control technology is put into the plan of U.S. control locust, nosema locustae is the biotechnological formulation of the control locust of first registration in the world, also is the biotechnological formulation of eliminating locusts of world's widespread use.U.S. Register muscardine be used to prevent and treat the preparation of locust, Britain and Australia register the green muscardine fungus preparation respectively, and carry out field test in a lot of countries.In addition, India, the U.S. have successfully developed plant insecticide-nimbin.China early carries out the country that biology is eliminated locusts, and just have in the period of Ming and Qing and adopt the example of raising chickens, supporting duck control locust, and so far still some local application.Eastern Jin Dynasty period can be traced back in the record of relevant locust natural enemy, has more than 1700 year apart from the present.Yet up to mid-term 80 year 20th century, China just really carries out the research and the application of locust biological control.China Agricultural University has at first introduced nosema locustae from the U.S., through nearly 10 years effort, on the basis of having furtherd investigate microsporidium pathogenesis, pathophoresis approach and regularty of epidemic, field utilisation technology and the supporting technology system thereof of technology, control grassland grasshopper and the Asiatic migrotory locust of large scale artificial breeding's nosema locustae have successfully been developed, cumulative model is used more than 1,000 ten thousand mu times, good economic benefit, social benefit and ecological benefits have been obtained, this technology level that is in a leading position in the world.The development research of unit such as the Chinese Academy of Agricultural Sciences, University Of Chongqing green muscardine fungus (Metarrhizium anisopliae) preparation, through behind the laboratory experiment for many years, also carried out the field test demonstration in recent years comparatively widely.These microbial preparations all can adopt the method for spraying or dusting to use.Simultaneously, domestic also have several producers producing biotechnological formulations such as nimbin, matrine.
Yet up to the present,, bacillus thuringiensis (Bt) specific strains of efficient anti-locust and insecticidal crystal protein plasmagene thereof and Bt yet there are no report about killing the locust agent.
Summary of the invention
The object of the present invention is to provide the bacillus thuringiensis of a kind of anti-locust, this bacterial strain has specific toxic action to locust of Orthoptera etc., but to people, animal and environmental safety.
Another object of the present invention has provided the method that a kind of Bt of preparation kills the locust agent, the control that the locust agent can be used for locusts such as hazard rice, wheat, corn, Chinese sorghum and herbage of killing with this method preparation is characterized in high specificity, does not does not kill and wound the insect natural enemy, nontoxic to people, animal, environmentally safe.
To achieve these goals, the present invention adopts following technical measures:
The purpose of invention is that separation screening has the bacillus thuringiensis of specificity toxic action to the insects such as locust of Orthoptera.Therefore, screen the Bt specific strains of anti-locust, can be development Bt and kill the locust agent and lay the foundation.This is for keeping diversity of organism better, and maintaining ecological balance realizes that the Sustainable development of agricultural has crucial meaning.
This bacterial strain of bacillus thuringiensis (Bacillus thuringiensis is called for short Bt) is deposited in Chinese typical culture collection center (CCTCC), and deposit number is: NO:M206061.BTH-13 is that a strain separates from China's pedotheque and serves as the examination worm with the Asiatic migrotory locust of Orthoptera, through virulence bioassay filters out the insects such as Asiatic migrotory locust of Orthoptera is had the bacterial strain of high virulence; The insecticidal activity of this bacterial strain is that the insecticidal crystal protein matter by the 124kD of its generation is determined.
Basic know-why is: utilize the gemma can anti-80 ℃ of pyritous characteristics, separate bacillus thuringiensis by playing local method under 80 ℃ of high temperature.With 1 age Asiatic migrotory locust serve as the examination worm, carry out virulence bioassay, through virulence median lethal dosage Lc relatively
50, screen this supper toxic strain Bacillus thuringiensisssp.BTH-13.
The preparation method of anti-locust bacillus thuringiensis bacterial strain BTH-13;
Utilize the gemma can anti-80 ℃ of pyritous characteristics, under 80 ℃ of high temperature by playing local method, fall with common solid bacteria substratum dull and stereotyped, at 30 ℃ of cultivations 3 days down, separation of bacterial list bacterium colony.Consisting of of this common solid bacteria substratum: peptone 1%, extractum carnis 0.5%, sodium-chlor 0.5%, agar 1.5%, water replenish volume to 100ml.Random choose list bacterium colony smear is observed under opticmicroscope with PHENOL 99.8 MIN ((CARBOLIC ACID)) azaleine dyeing back, and screening can produce gemma and crystalline bacillus thuringiensis.Its code BTH formed in first letter according to the title (Heilongjiang) in the pedotheque source place of separating this Bt bacterial strain, again because of this bacterial strain from a strain that screens and be numbered 13 in isolating many bacillus thuringiensis strains a collection of pedotheque, therefore with this bacillus thuringiensis called after BTH-13.
With the Asiatic migrotory locust is the examination worm, and the bacillus thuringiensis that filters out is carried out virulence bioassay, through comparing virulence median lethal dosage Lc
50, screen this supper toxic strain Bacillus thuringiensisssp.BTH-13.
The concrete feature of this bacterial strain is as follows:
The essential characteristic of anti-locust bacillus thuringiensis Bacillus thuringiensis ssp.BTH-13:
A. morphological feature: the cellular form of Bacillus thuringiensis ssp.BTH-13 is shaft-like, produces oval row gemma and rhombus parasporal crystal protein matter.
B. cultural characteristic: cultivated 24 hours for 30 ℃ in Bacillus thuringiensis ssp.BTH-13 extractum carnis-peptone Agar Plating, form the light yellow small colonies of needle point size, edge-smoothing, cultivated 72 hours, formation garden plate-like bacterium colony, oyster white, the edge is irregular, there is wrinkle on the surface like obscure glass.
C. physio-biochemical characteristics:
The major physiological biochemical character of bacillus thuringiensis BTH-13 bacterial strain
D. serotype: carry out agglutination reaction and cross absorption agglutination reaction test with the flagellar antigen of BTH-13 and the standard antiserum(antisera) of Bt, the H serotype of BTH-13 is H16, but contain the flagellar antigen composition that is different from the Bt.subsp.indiana subspecies, therefore this bacterial strain may be a new subspecies among the Bt, tentative Bacillusthuringiensis ssp.BTH-13 (Bt.subsp.locustcidus) by name.
E. insecticidal crystal protein matter: analyze through SDS-PAGE, bacterial strain BTH-13 produces the insecticidal crystal protein matter of 128kD.
H. insecticidal properties: through virulence bioassay, bacterial strain BTH-13 has higher insecticidal activity to orthoptera pests such as Asiatic migrotory locusts, its fermented liquid and crystal proteins through alkali and protease treatment after, can obviously improve the activity of anti-locust.
I. leavening property: bacterial strain BTH-13 is easy to cultivate, and leavening property is good, under suitable fermentation condition
Growth is neat, and fermentation period is short.
The preparation of anti-locust Bt sterilant
The preparation of anti-locust Bt bacterial strain BTH-13 sterilant (killing the locust agent):
Shake flask fermentation:
The purpose of shake flask fermentation is to select best fermentating formula, and optimization of fermentation conditions adopts different solid contents to carry out L with different C/N ratios
9(3
4) orthogonal test.
Table 2 L
9(3
4) the orthogonal experiment factor/horizontal percentage composition table
According to orthogonal test, the optimal medium prescription that obtains bacterial strain BTH-13 is: in the substratum of 100 unit volumes, and starch 3.0-4.0%, soybean cake powder 1.8-2.4%, the sub-powder 1.2-1.8% of cottonseed cake, peptone 0.5-0.9%, yeast powder 0.4%, corn steep liquor 2.0%, 7 water magnesium sulfate (MgSO
47H
2O) 0.04%, potassium primary phosphate (KH
2PO
4) 0.2%, dipotassium hydrogen phosphate (K
2HPO
4) 0.2%, lime carbonate (CaCO
3) 0.1%, and α-Dian Fenmei (starch content 1/400), water is supplemented to volume 100.
Utilize above-mentioned culture medium prescription, dress 100ml substratum in the triangular flask of 500ml, inoculation BTH-13 in sterilization back is cultured to 80% bacillus exfoliation with 200 rev/mins in 30 ℃ of shaking tables.Shake flask fermentation liquid carries out virulence bioassay.
Lab scale in automatic fermenter:
The best fermentating formula that employing screens carries out fermentation test in automatic fermenter, the substratum preceding pH7.8 that disappears, and the back pH that disappears is about 7.0.Every jar of inoculation-Zhi is through 60 ℃ of slant strains of handling 30 minutes, 37 ℃ of inoculation temps.Adopt alternating temperature, speed change, transformation (0-11 hour, 0.6 cubic metre/hour of 32 ℃, 500 rev/min, air flow; 12-21 hour, 0.8 cubic metre/hour of 29 ℃, 600 rev/min, air flow; 22-fermentation ends, 0.8 cubic metre/hour of 32 ℃, 600 rev/min, air flow) the fermentation means, determined the best zymotechnique of a cover.Fermentation period is 38 hours, and fermentation ends secondary fermentation liquid is acidified to pH5.0, adds 0.1% emulsifying agent (farming breast 100), makes the outstanding agent of breast.Fermented liquid concentrates the direct spraying drying in back or adds 10% stopping composition (lime carbonate) back spraying drying and prepares wettable powder.
Bt kills the pilot scale and the production of locust agent:
Condition according to the lab scale fermentation is carried out pilot scale in 10 tons fermentor tank, pilot product carries out virulence bioassay.On the pilot scale basis, produce on a large scale.
Advantage and effect
Bacillus thuringiensis BTH-13 has the advantages that to kill orthoptera pests such as Asiatic migrotory locust, the domestic present bacillus thuringiensis commodity preparation that kills orthoptera pests such as Asiatic migrotory locust that still do not have, thereby can utilize BTH-13 to produce novel bacillus thuringiensis (Bt) and kill the locust agent, make the product diversification and the seriation of thuringiensis cladosporioides bacillus insecticide, enlarge the use range of thuringiensis cladosporioides bacillus insecticide, reduce the pesticide control expense, reduce the pollution of chemical pesticide, increase crop yield environment.The genetic improvement that the insecticidal crystal protein plasmagene of BTH-13 can be used for the Bt bacterial strain to be making up the Bt engineering bacteria of efficient anti-locust, and can be used for herbage and the farm crop of research to obtain anti-locust of transgenic plant.Thereby,, suitability for industrialized production technology maturation low, aspects such as people and animals and plants safety, the free from environmental pollution and market requirement are considered that bacillus thuringiensis BTH-13 and killing gene thereof have good popularizing application prospect from superior and unique insecticidal properties, production and use cost.
The virulence of the anti-Asiatic migrotory locust of Bt bacterial strain BTH-13
Embodiment
1. the preparation method of anti-locust bacillus thuringiensis bacterial strain BTH-13:
Utilize the gemma can anti-80 ℃ of pyritous characteristics, under 80 ℃ of high temperature by playing local method, fall with common solid bacteria substratum dull and stereotyped, at 30 ℃ of cultivations 3 days down, separation of bacterial list bacterium colony.Consisting of of this common solid bacteria substratum: peptone 1%, extractum carnis 0.5%, sodium-chlor 0.5%, agar 1.5%, water replenish volume to 100ml.Random choose list bacterium colony smear is observed under opticmicroscope with PHENOL 99.8 MIN ((CARBOLIC ACID)) azaleine dyeing back, and screening can produce gemma and crystalline bacillus thuringiensis.Its code BTH formed in first letter according to the title (Heilongjiang) in the pedotheque source place of separating this Bt bacterial strain, again because of this bacterial strain from a strain that screens and be numbered 13 in isolating many bacillus thuringiensis strains a collection of pedotheque, therefore with this bacillus thuringiensis called after BTH-13.
With the Asiatic migrotory locust is the examination worm, and the bacillus thuringiensis that filters out is carried out virulence bioassay, through comparing virulence median lethal dosage Lc
50, screen this supper toxic strain Bacillus thuringiensisssp.BTH-13.
2. the preparation of anti-locust Bt sterilant
The preparation of anti-locust Bt bacterial strain BTH-13 sterilant (killing the locust agent):
Shake flask fermentation:
The purpose of shake flask fermentation is to select best fermentating formula, and optimization of fermentation conditions adopts different solid contents to carry out L with different C/N ratios
9(3
4) orthogonal test.
Table 2 L
9(3
4) the orthogonal experiment factor/horizontal percentage composition table
According to orthogonal test, the optimal medium prescription that obtains bacterial strain BTH-13 is: in the substratum of 100 unit volumes, and starch 4.0%, soybean cake powder 2.4%, the sub-powder 1.5% of cottonseed cake, peptone 0.5%, yeast powder 0.4%, corn steep liquor 2.0%, magnesium sulfate heptahydrate (MgSO
47H
2O) 0.04%, potassium primary phosphate (KH
2PO
4) 0.2%, dipotassium hydrogen phosphate (K
2HPO
4) 0.2%, lime carbonate (CaCO
3) 0.1%, and α-Dian Fenmei (starch content 1/400), water is supplemented to volume 100.
Utilize above-mentioned culture medium prescription, dress 100ml substratum in the triangular flask of 500ml, inoculation BTH-13 in sterilization back is cultured to 80% bacillus exfoliation with 200 rev/mins in 30 ℃ of shaking tables.Shake flask fermentation liquid carries out virulence bioassay.
Lab scale in automatic fermenter:
The best fermentating formula that employing screens carries out fermentation test in automatic fermenter, the substratum preceding pH7.8 that disappears, and the back pH that disappears is about 7.0.Inoculate one through 60 ℃ of slant strains of handling 30 minutes, 37 ℃ of inoculation temps for every jar.Adopt alternating temperature, speed change, transformation (0-11 hour, 0.6 cubic metre/hour of 32 ℃, 500 rev/min, air flow; 12-21 hour, 0.8 cubic metre/hour of 29 ℃, 600 rev/min, air flow; 22-fermentation ends, 0.8 cubic metre/hour of 32 ℃, 600 rev/min, air flow) the fermentation means, determined the best zymotechnique of a cover.Fermentation period is 38 hours, and fermentation ends secondary fermentation liquid is acidified to pH5.0.Add 0.1% emulsifying agent (farming breast 100), make the outstanding agent of breast.Fermented liquid concentrates the direct spraying drying in back or adds 10% stopping composition (lime carbonate) back spraying drying and prepares wettable powder.
Bt kills the pilot scale and the production of locust agent:
Condition according to the lab scale fermentation is carried out pilot scale in 10 tons fermentor tank, pilot product carries out virulence bioassay.On the pilot scale basis, produce on a large scale.
The enzymolysis of fermented liquid: in the BTH-13 fermented liquid, add 10M potassium hydroxide (NaOH), transfer about the pH value to 11.0 of fermented liquid.37 ℃ of incubation 3h, microscopy is observed, and dissolves fully up to crystal.Add trypsinase, making its final concentration is 25mg/ml, 37 ℃ of incubation 2-4h.
The enzymolysis of crystallin
5mg/ml crystal parent toxin protein is dissolved in 0.05M yellow soda ash-sodium bicarbonate (Na
2CO
3-NaHCO
3) 37 ℃ of incubation 3h in (pH10) the damping fluid, microscopy is observed, and dissolves fully up to crystal.Add trypsinase dry powder, make wherein that concentration is 25mg/ml, 37 ℃ are incubated overnight, and the centrifugal 5min of 5000rpm discards precipitation, stays supernatant liquor, adds phenylmethylsulfonyl fluoride (PMSF) and stops enzyme reaction, does further purification and electrophoretic analysis and uses.
Claims (2)
1, the bacillus thuringiensis of a kind of anti-locust is characterized in that, it is bacillus thuringiensis (Bacillusthuringiensis) bacterial strain BTH-13, and its deposit number at China typical culture collection center (CCTCC) is NO:M206061.
2, a kind of method for producing insecticide by bacillus thuringiensis BTH-13 preparation is characterized in that it comprises the following steps:
A, shake flask fermentation:
The culture medium prescription that obtains bacterial strain BTH-13 is: in the substratum of 100 unit volumes, starch 3.0-4.0%, soybean cake powder 1.8-2.4%, the sub-powder 1.2-1.8% of cottonseed cake, peptone 0.5-0.9%, yeast powder 0.4%, corn steep liquor 2.0%, magnesium sulfate heptahydrate 0.04%, potassium primary phosphate 0.2%, dipotassium hydrogen phosphate 0.2%, lime carbonate 0.1%, 1/400 α-Dian Fenmei of starch content, water is supplemented to volume 100, utilize the basal culture medium prescription, dress 100ml substratum in the triangular flask of 500ml, inoculation BTH-13 in sterilization back is cultured to 80% bacillus exfoliation with 200 rev/mins in 30 ℃ of shaking tables;
The substratum that screens in B, the employing A step, in automatic fermenter, carry out fermentation test, the substratum preceding pH7.8 that disappears, pH was 7.0 after substratum disappeared, inoculate one through 60 ℃ of slant strains of handling 30 minutes, 37 ℃ of inoculation temps, the fermentation process of employing temperature-speed-changing transformation, 0-the 11st hour, under the condition of 0.6 cubic metre/hour of 32 ℃, 500 rev/min, air flow, cultivate; At 12-21 hour, under the condition of 0.8 cubic metre/hour of 29 ℃, 600 rev/min, air flow, cultivate; The 22nd hour-fermentation ends, under the condition of 0.8 cubic metre/hour of 32 ℃, 600 rev/min, air flow, cultivate, fermentation period is 38 hours, fermentation ends secondary fermentation liquid is acidified to pH5.0, add 0.1% emulsifying agent, make the outstanding agent of breast, spraying drying prepared wettable powder after ferment liquid concentrated the direct spraying drying in back or adds 10% lime carbonate.
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| CN112514916A (en) * | 2020-11-30 | 2021-03-19 | 云南省微生物发酵工程研究中心有限公司 | Suspending agent for controlling locusta migratoria manilensis |
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| Title |
|---|
| 1株广谱苏云金芽孢杆菌及其发酵条件的研究. 蔡亚君,彭可凡,戴顺英,高梅影.华中农业大学学报,,第22卷第5期. 2003 * |
| 苏云金芽孢杆菌WB9的研究. 黄志鹏,99-107,福建农林大学. 2005 * |
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