CN108396035A - A kind of agriculture bacillus mediated rice transformation method - Google Patents

A kind of agriculture bacillus mediated rice transformation method Download PDF

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CN108396035A
CN108396035A CN201711498703.1A CN201711498703A CN108396035A CN 108396035 A CN108396035 A CN 108396035A CN 201711498703 A CN201711498703 A CN 201711498703A CN 108396035 A CN108396035 A CN 108396035A
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callus
bacillus mediated
agriculture bacillus
transformation method
inoculated
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刘佳音
张国栋
张佩
邹丹丹
吴洁芳
王晶
修旺珊
米铁柱
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Qingdao Yuan Ce Biology Technology Co Ltd
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    • C12N15/8261Phenotypically and genetically modified plants via recombinant DNA technology with agronomic (input) traits, e.g. crop yield
    • C12N15/8271Phenotypically and genetically modified plants via recombinant DNA technology with agronomic (input) traits, e.g. crop yield for stress resistance, e.g. heavy metal resistance
    • C12N15/8279Phenotypically and genetically modified plants via recombinant DNA technology with agronomic (input) traits, e.g. crop yield for stress resistance, e.g. heavy metal resistance for biotic stress resistance, pathogen resistance, disease resistance

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Abstract

This application discloses a kind of agriculture bacillus mediated rice transformation methods, include the following steps:1) it induces:After rice paddy seed decladding disinfection, mature embryo is inoculated in inducing culture, induced embryonic callus;2) it infects:Callus obtained by step 1) is detached with endosperm, bud, is inoculated in agrobacterium suspension and infects, is dried later for use;3) it co-cultures;4) it screens;5) break up;6) it takes root.The agriculture bacillus mediated rice transformation method of the present invention takes low-temperature treatment in the induction of callus stage and shortens incubation time, it is preferable that the healing rate and callus quality of Rice Callus compare conventional method, cultivation temperature is reduced in the stage of co-cultivation, shorten incubation time and obtain the relatively conventional preferable conversion ratio of method, the present invention also improves the inductivity and conversion ratio of callus while shortening agrobacterium mediation converted rice process.

Description

A kind of agriculture bacillus mediated rice transformation method
Technical field
Molecular biology tissue cultures and transgenic technology interleaving techniques of the present invention field, more particularly to a kind of extreme condition Under agriculture bacillus mediated japonica rice rapid genetic transformation method.
Background technology
Rice (Oryza sativa L.) is not only the pattern that main cereal crops are also monocotyledon basic research Plant.With the continuous growth and the improvement of people's living standards of world population, to be proposed to yield and quality of rice Higher requirement.Traditional breeding method has breeding year limit for length, and need to continuously be selfed just, which can select the merits of needs, has been difficult Meet demand is combined with traditional breeding technology by modern biotechnology and is had become from now on to improve the yield and quality of rice Main development trend.
With the development of molecular biology, more and more related genes of plant disease-resistant that participate in are separated, such as anti- The gene for reacting related gene, participating in defense signaling is defended, the gene etc. identified to pathogen is participated in, to identify these bases Effect and status of the cause in disease resistance of plant are dry it is necessary to the binary vector such as overexpression, antisense and RNA for building conversion plant The binary vector conversion plant related to, carrys out clearly effect of the gene in plant disease-resistant.
Common genetic transforming method is divided into DNA direct guiding methods and Agrobacterium-medialed transformation method on rice.DNA is direct Introductory technique mainly include PEG (polyethylene glycol) mediate conversion method, electroporated method, Gene Knock-out Mice and Pollen tube channel conversion method.Wherein PEG methods, electroporation are using protoplast as receptor, due to the dependence to protoplast regeneration And it is above very limited in application.
Particle bombardment advantage is that receptor is extensive, is not limited by host range, and conversion ratio is higher, but direct with other DNA Introductory technique equally haves the shortcomings that common:The Integration Mode of exogenous DNA is complicated, and often multicopy is inserted into, and is easier to occur turning base Because of silencing phenomenon, the foreign gene segment of conversion cannot too greatly (upper limit is 16-20kb), and the separation of transgene is in non-Meng sometimes Dare heredity etc..
Compared with DNA direct guiding methods, Agrobacterium-medialed transformation method does not need the training of protoplast
Currently, in prior art Rice Callus Fiber differentiation, cultivation temperature is 26 DEG C and cultivates 9-12 days, agriculture The time that bacillus mediated transformation rice co-cultures is 2 days, and low-temperature treatment incubation time is taken in the induction of callus stage Long, the healing rate and callus quality of Rice Callus are poor, and the inductivity and conversion ratio of callus are low.
Invention content
Technical problem to be solved by the present invention lies in provide a kind of agriculture bacillus mediated rice transformation method.This Inventive method shortens the process of agrobacterium mediation converted rice, and improve rice by changing cultivation temperature and incubation time The inductivity and conversion ratio of callus.
In order to solve the above technical problems, the present invention provides a kind of agriculture bacillus mediated rice transformation methods, including with Lower step:
1) it induces:After rice paddy seed decladding disinfection, mature embryo is inoculated in inducing culture, induces embryo callus subculture group It knits;
2) it infects:Callus obtained by step 1) is detached with endosperm, bud, is inoculated in agrobacterium suspension and infects, it After dry it is for use;
3) it co-cultures:The callus dried is gone to and is co-cultured in base, thalline occurs in culture to callus surface;
4) it screens:Resistance screening is carried out by being inoculated into screening and culturing medium after the callus cleaning after co-cultivation, is obtained Resistant calli;
5) break up:The resistant calli of acquisition is inoculated on differential medium and is cultivated to differentiating seedling;
6) it takes root:It will take root on seedling inoculation to root media, and carry out PCR detections, select the plant of test positive The rice plant that strain is obtained as conversion.
The inducing culture preferably includes:NB;2,4-D 1.8-2.0mg/mL;6-BA;Agar powder 10-15g/L.
The co-cultivation base preferably includes:NB;AS 100-200umol/L.
The screening and culturing medium preferably includes:NB;2,4-D 1.8-2.0mg/mL;6-BA0.1-0.2mg/mL;Hyg 20- 25mg/L, Timentin 200-400mg/L, agar powder 10-15g/L.
The differential medium preferably includes:NB;Pro 0.3-0.5g/L;CH 0.2-0.3g/L;6-BA1.8-2.0mg/ mL;KT 0.8-1.0mg/mL;NAA 0.3-0.5mg/mL, IAA 0.4-0.5mg/mL; Hyg 20-25mg/L;Timentin 200-400mg/L;Sucrose 25-30g/L;Agar powder 10-15g/L.
The root media preferably includes:NB;NAA 0.4-0.7mg/L;Sucrose 25-30g/L;Agar powder 10-15g/ L。
Step 1) the induction, may further include:After rice paddy seed decladding disinfection, mature embryo is inoculated in induction training It supports in base, 20 DEG C of constant temperature incubations, 7 days induced embryonic callus.
The step 3) co-cultures, and may further include:It is 20 DEG C to co-culture temperature, and incubation time is 24 hours.
The step 3) co-cultures, and may further include:By the Agrobacterium EHA105 containing target gene carrier containing There are the flat lining outs of YEB of 50mg/L Kan and 50mg/L Rif, 26~30 DEG C of dark culturing 2d, with oese picking Agrobacterium Single bacterium colony is inoculated in fresh YEB fluid nutrient mediums, 28 DEG C, 220rpm 46~50h of shaking table culture, then by agriculture bar Bacterium is added in the co-cultivation base of the AS containing 100umol/L, and adjustment cell concentration OD600 to 0.1-0.2 or so obtains co-cultivation and turns The agrobacterium suspension of change.
The YEB culture mediums preferably include:Yeast extract 0.8-1.2g/L;Peptone 4.5-5.0g/L;Beef extract 4.5-5.0g/L;Sucrose 4.0-6.0g/L;Magnesium sulfate 0.3-0.5g/L;Agar 12-15g/L;pH 6.8-7.2.
Advantageous effect of the present invention includes:The agriculture bacillus mediated rice transformation method of the present invention is in induction of callus Stage takes low-temperature treatment and shortens incubation time, and the healing rate and callus quality of Rice Callus compare conventional method Preferably, cultivation temperature is reduced in the stage of co-cultivation, shortens incubation time and obtains the relatively conventional preferable conversion ratio of method, the present invention The inductivity and conversion ratio of callus are also improved while shortening agrobacterium mediation converted rice process.
Description of the drawings
The induction situation photo of Rice Callus when Fig. 1 is 20 DEG C of cultures described in the embodiment of the present invention;
The induction situation photo of Rice Callus when Fig. 2 is 26 DEG C of cultures described in the embodiment of the present invention;
Growing state photo when Fig. 3 is experimental group resistance seedling rooting 2 days described in the embodiment of the present invention;
Fig. 4 is PCR product agarose gel electrophoresis figure described in the embodiment of the present invention.
Specific implementation mode
The present invention is described in detail with reference to embodiment.To keep the objectives, technical solutions, and advantages of the present invention clearer, bright Really, developing simultaneously referring to the drawings, the present invention is described in more detail for embodiment, but the invention is not limited in these embodiments.
Unless otherwise instructed, the raw material in the embodiment of the present invention and catalyst are bought by commercial sources.The present invention Selection rice varieties Nipponbare is experiment material, and agrobacterium strains are the Agrobacterium EHA105 of the carrier containing target gene.Such as 1 institute of table Show, is reagent explanation of the present invention:
1 reagent explanation of the present invention of table
In an embodiment of the present invention, a kind of agriculture bacillus mediated rice transformation method, experimental implementation step are provided Suddenly it is:
1) it induces:After rice paddy seed decladding disinfection, mature embryo is inoculated in inducing culture, induces embryo callus subculture group It knits;
2) it infects:Callus obtained by step 1) is detached with endosperm, bud, is inoculated in agrobacterium suspension and infects, it After dry it is for use;
3) it co-cultures:The callus dried is gone to and is co-cultured in base, thalline occurs in culture to callus surface;
4) it screens:Resistance screening is carried out by being inoculated into screening and culturing medium after the callus cleaning after co-cultivation, is obtained Resistant calli;
5) break up:The resistant calli of acquisition is inoculated on differential medium and is cultivated to differentiating seedling;
6) it takes root:It will take root on seedling inoculation to root media, and carry out PCR detections, select the plant of test positive The japonica rice plant that strain is obtained as conversion;
The specific formula of involved culture medium is as follows:
YEB culture mediums:Yeast extract 0.8-1.2g/L;Peptone 4.5-5.0g/L;Beef extract 4.5-5.0g/L;Sugarcane Sugared 4.0-6.0g/L;Magnesium sulfate 0.3-0.5g/L;Agar 12-15g/L;pH 6.8-7.2;
Inducing culture:NB;2,4-D 1.8-2.0mg/mL;6-BA 0.1-0.2mg/mL;Agar powder 10-15g/L;
Subculture medium:NB;2,4-D1.8-2.0mg/mL;CH 0.2-0.3g/L;Sucrose 28-30g/L;Agar powder 10- 15g/L;
Co-culture culture medium:NB;AS 100-200umol/L;
Screening and culturing medium:NB;2,4-D1.8-2.0mg/mL;6-BA 0.1-0.2mg/mL;Hyg 20-25mg/L, Timentin 200-400mg/L, agar powder 10-15g/L;
Differential medium:NB;Pro 0.3-0.5g/L;CH 0.2-0.3g/L;6-BA 1.8-2.0mg/mL; KT 0.8- 1.0mg/mL;NAA 0.3-0.5mg/mL, IAA 0.4-0.5mg/mL;Hyg 20-25mg/L; Timentin 200-400mg/ L;Sucrose 25-30g/L;Agar powder 10-15g/L;
Root media:NB;NAA 0.4-0.7mg/L;Sucrose 25-30g/L;Agar powder 10-15g/L
In another embodiment of the invention, the method for the present invention Mature Embryos of Rice callus under condition of different temperatures is provided Tissue induction situation.
Every group of each 20 ware, 600 Mature Embryos of Rice of inoculation, totally six groups.Each group is respectively placed in 18 DEG C, 20 DEG C, 22 DEG C, 24 DEG C, 26 DEG C, in 28 DEG C of constant temperature incubation room, wherein 26 DEG C of groups, which are callus, induces normal temperature, and as a control group, culture 7 Callus induction number is counted after it.The results are shown in Table 2, cultivation temperature be 18 DEG C, 20 DEG C, 22 DEG C, 24 DEG C, 26 DEG C, 28 DEG C when, the inductivity of callus is respectively 57.67%, 91.17%, 85.67%, 86.67%, 87.33%, 84.67%. Wherein when cultivation temperature is 18 DEG C, the inductivity of callus is minimum, and only 57.67%, when cultivation temperature is 20 DEG C, Tissue inductivity highest is met, it is higher than control group by 3.84% up to 91.17%.According to research reports, when cultivation temperature be 26 DEG C, training When the foster time is 10 days, the callus induction rate of Nipponbare is 85%-88%, as shown in Table 3, as a result reports phase with research Symbol, this research not only shorten the inductivity that incubation time also improves callus.
2 experimental group of table, callus induction situation when incubation time is 7 days under difference cultivation temperature
3 control group of table, callus induction situation under difference cultivation temperature when incubation time is 10 days
Cultivation temperature 18℃ 20℃ 22℃ 24℃ 26℃ 28℃
Callus induces number 336 447 464 512 504 498
Callus induction rate 56% 74.5% 77.3% 85.33% 84% 83%
The stage is co-cultured in agrobacterium mediation converted rice, with 20 DEG C of cultivation temperature for experimental group, 26 DEG C of cultivation temperature is Control group, two groups co-culture 12h respectively, and for 24 hours, then 36h, 48h carry out kanamycin-resistant callus tissue screening, resistant calli differentiation training It supports, Transformation of Callus situation is observed in PCR detections.Such as table 4, shown in table 5, when cultivation temperature is 20 DEG C, conversion ratio is with training The extension of time is supported in downward trend after first increasing, most suitable incubation time is that for 24 hours, conversion ratio is converted up to 42.3% when cultivating 48h Rate is 39.2%;When cultivation temperature is 26 DEG C, conversion ratio shows a rising trend also with the extension of incubation time, when most suitable culture Between be 48h, conversion ratio 39%.When agrobacterium mediation converted rice co-cultures, cultivation temperature and incubation time influence callus group The transformation efficiency knitted, by table 4 and table 5 it is found that it is 20 DEG C to co-culture temperature, when incubation time is for 24 hours, the conversion effect of callus Rate is higher.
4 experimental group of table, temperature are 20 DEG C, the conversion situation of callus
5 experimental group of table, when temperature is 26 DEG C, the conversion situation of callus
Incubation time 12h 24h 36h 48h
It is inoculated with callus block number 600 600 600 600
Convert number 165 195 208 234
Conversion ratio 27.5% 32.5% 34.7% 39%
In one more embodiment of the present invention, configuration rice callus inducing culture, subculture medium, differentiation training are provided Base is supported, culture medium prescription is as follows:
YEB culture mediums:Yeast extract 0.8-1.2g/L;Peptone 4.5-5.0g/L;Beef extract 4.5-5.0g/L;Sugarcane Sugared 4.0-6.0g/L;Magnesium sulfate 0.3-0.5g/L;Agar 12-15g/L;pH 6.8-7.2;
Inducing culture:NB;2,4-D1.8-2.0mg/mL;6-BA 0.1-0.2mg/mL;Agar powder 10-15g/L;
Subculture medium:NB;2,4-D 1.8-2.0mg/mL;CH 0.2-0.3g/L;Sucrose 28-30g/L;Agar powder 10- 15g/L;
Co-culture culture medium:NB;AS 100-200umol/L;
Screening and culturing medium:NB;2,4-D 1.8-2.0mg/mL;6-BA 0.1-0.2mg/mL;Hyg 20-25mg/L, Timentin 200-400mg/L, agar powder 10-15g/L;
Differential medium:NB;Pro 0.3-0.5g/L;CH 0.2-0.3g/L;6-BA 1.8-2.0mg/mL; KT0.8- 1.0mg/mL;NAA0.3-0.5mg/mL, IAA 0.4-0.5mg/mL;Hyg 20-25mg/L; Timentin 200-400mg/ L;Sucrose 25-30g/L;Agar powder 10-15g/L;
In another embodiment of the invention, a kind of method for inducing and cultivating of Mature Embryos of Rice callus is provided:
1) choose it is full, without going mouldy ripe rice paddy seed, slough husk (paying attention to keeping embryo complete) by hand;
2) on superclean bench, appropriate amounts of sterilized water (be subject to and do not cross seed, similarly hereinafter) is added and is cleaned;
3) water is abandoned, appropriate 75% alcohol is poured into, shakes stirring, surface sterilization 1-3min;
4) alcohol is abandoned, appropriate amounts of sterilized water is added to be cleaned;
5) water is abandoned, appropriate 2%NaClO is added, shakes stirring, concussion sterilizing 20-30min;
6) 2%NaClO is abandoned, with sterile water wash 4-5 times, is stopped 1-2 minutes every time;
7) sterile water is removed, is blotted the moisture of the surface of the seed with the aseptic filter paper after sterilizing;
8) it uses tweezers, scalpel to take out the mature embryo of sterilizing seed, is inoculated on callus inducing medium (every 30, ware, uniformly puts), this part be divided into two groups of experimental groups be 18 DEG C, 20 DEG C, 22 DEG C, 24 DEG C, 26 DEG C, 28 DEG C of light cultures 7 It;Control group is 18 DEG C, 20 DEG C, 22 DEG C, 24 DEG C, 26 DEG C, 28 DEG C of light cultures 10 days;
9) after cultivating, the callus that mature embryo scultellum is grown is peeled, is transferred on subculture medium, in the same terms Lower squamous subculture.Squamous subculture is primary every two weeks later.Select pale yellow, compact structure callus squamous subculture 6-7d Afterwards, it is used for Agrobacterium-mediated Transformation receptor.
In another embodiment of the present invention, a kind of cultural method of Agrobacterium tumefaciems is provided:
By the Agrobacterium EHA105 containing target gene carrier in the YEB tablets containing 50mg/L Kan and 50mg/L Rif Upper scribing line, 28 DEG C of dark culturing 2d are inoculated in fresh YEB fluid nutrient mediums with oese picking Agrobacterium single bacterium colony In, 28 DEG C, 220rpm shaking table culture 48h, then Agrobacterium is added in the co-cultivation base of the AS containing 100umol/L, adjusts thalline Concentration OD600 to 0.1-0.2 or so as co-cultures the agrobacterium suspension of conversion.
In another embodiment of the invention, a kind of co-culture method of Rice Callus and Agrobacterium is provided:
The callus for carefully choosing sterile, state preferably (pale yellow, compact structure) is put into sterile triangular flask, It is added suitable agrobacterium suspension (guarantee has enough bacterium solutions and material), room temperature infects under the conditions of 120rpm 20min stands 10min after the completion of infecting, is then transferred to callus on sterile filter paper and sucks extra Agrobacterium bacterium Liquid, and 2-3h is blown in superclean bench, until surface is visible by naked eyes thalline, transfers it to and be covered with one layer of sterile filter On the solidified co-cultivation medium of paper (NB+100umol/LAS), experimental group distinguishes dark culturing 12h under the conditions of being 20 DEG C, for 24 hours, 36h, 48h;Control group distinguishes dark culturing 12h, for 24 hours, 36h, 48h under the conditions of being 26 DEG C.
In another embodiment of the present invention, a kind of screening technique of resistant calli is provided:
Then for the callus after picking mediated transformation in culture dish, callus surface can not if existing without thalline It is rinsed with sterile water, 3-5 times is rinsed under the conditions of 120rpm with sterile water if with the presence of thalline, for the last time with containing The sterile water of 500mg/L Cef stands 1h, is subsequently placed on aseptic filter paper dry 30min, until callus surface is without visible Agrobacterium exists.Then the screening for callus being transferred to 20-25mg/L containing Hyg and 200-400mg/L Timentin is trained Foster base carries out screening kanamycin-resistant callus tissue, and 28 DEG C of light cultures, 15d screenings are primary, screen altogether twice.
In another embodiment of the invention, a kind of differentiation method of resistant calli is provided:
In the resistant calli grown after being screened through two-wheeled, the resistant calli for selecting milk yellow densification goes to and contains On the differential medium for having Hyg 20-25mg/L and 200-400mg/L Timentin, then first light culture 7d goes to 15h/d It is cultivated under illumination condition, generally grows new kanamycin-resistant callus tissue by 15d or so and green point occur.Then milk yellow densification is selected There is the resistant calli of green point to transfer on new differential medium, seedling is further differentiated after 25d.It needs periodically super Net workbench aeration-drying kanamycin-resistant callus tissue, prevents the kanamycin-resistant callus tissue aquation of differentiation.
In another embodiment of the present invention, a kind of PCR Resistance detectings method is provided:
The seedling of step 6 is taken root in root media, each strain takes 3 plants of seedlings, is taken from every young plant after two weeks A little blade extracts DNA, carries out PCR detections, and the seedling of test positive is carried out hardening, is transplanted in soil.
DNA is extracted:3 plants of Nipponbare rice resistant plants and one plant of non-transgenic rice varieties Nipponbare are randomly selected, point Indescribably take genomic DNA.DNA extraction steps are as follows:The rice leaf of about 2cm long is taken to be placed in 2ml centrifuge tubes;Add in mortar Enter 800 μ L 1.5XCTAB, grind blade is to being homogenized and refund in centrifuge tube;65 DEG C of water-bath 20-30min overturn mixing per 5min 1 time;Isometric chloroform/isoamyl alcohol (24 is added:1), turn upside down mixing, continues 10min;10000rpm centrifuges 10min; 400 μ L supernatants are drawn to new centrifuge tube, 95% ethyl alcohol that 2 times of volumes are pre-chilled through ice are added, -20 DEG C of ice set 20min; 12000rpm centrifuges 15min;Supernatant is abandoned, 500 μ L, 75% ethyl alcohol is added, overturns rinsing, 12000rpm centrifuges 5min;It abandons Clearly, it is placed in super-clean bench drying or naturally dry, adds 100 μ L ddH2O dissolving DNAs.
With Hyg gene design primer sequences:F1:5′-GGACTTCGGGGCAGTCCT-3′;R1: 5′- CGATGTAGGAGGGCGTGG-3 ' is primer, respectively with Nipponbare rice resistant plant genomic DNA (sample), used in conversion Plasmid DNA (positive control), non-transgenic Nipponbare genomic DNA (negative control) are template, carry out PCR detections.PCR reacts Program and system are as follows:Program:94 DEG C of pre-degenerations 5min, 94 DEG C of denaturation 45s, 55 DEG C of annealing 45s;72 DEG C of extension 1.5min; 30 A cycle;72 DEG C re-extend 10min;16 DEG C of end.Reaction carries out in 20 μ L systems, including:10×EasyTaq 2 μ L of 2 μ L of Buffer (+Mg2+), 1 μ L, 2mM dNTPs of DNA profiling, the forward direction of 10 μM/L, each 1 μ L, 5U/ μ L of reverse primer Taq DNA polymerases 1 μ L, ddH2O complement to 20 μ L.
The above is only several embodiments of the present invention, not any type of limitation is done to the present invention, although this hair It is bright to be disclosed as above with preferred embodiment, however not to limit the present invention, any person skilled in the art is not taking off In the range of technical solution of the present invention, makes a little variation using the technology contents of the disclosure above or modification is equal to Case study on implementation is imitated, is belonged in technical solution of the present invention protection domain.

Claims (10)

1. a kind of agriculture bacillus mediated rice transformation method, which is characterized in that include the following steps:
1) it induces:After rice paddy seed decladding disinfection, mature embryo is inoculated in inducing culture, induced embryonic callus;
2) it infects:Callus obtained by step 1) is detached with endosperm, bud, is inoculated in agrobacterium suspension and infects, dry in the air later It is dry for use;
3) it co-cultures:The callus dried is gone to and is co-cultured in base, thalline occurs in culture to callus surface;
4) it screens:Resistance screening is carried out by being inoculated into screening and culturing medium after the callus cleaning after co-cultivation, obtains resistance Callus;
5) break up:The resistant calli of acquisition is inoculated on differential medium and is cultivated to differentiating seedling;
6) it takes root:It will take root on seedling inoculation to root media, and carry out PCR detections, the plant of test positive is selected to make To convert obtained rice plant.
2. agriculture bacillus mediated rice transformation method according to claim 1, which is characterized in that the inducing culture packet It includes:NB;2,4-D 1.8-2.0mg/mL;6-BA 0.1-0.2mg/mL;Agar powder 10-15g/L.
3. agriculture bacillus mediated rice transformation method according to claim 1, which is characterized in that the co-cultivation Ji Bao It includes:NB;AS 100-200umol/L.
4. agriculture bacillus mediated rice transformation method according to claim 1, which is characterized in that the screening and culturing medium packet It includes:NB;2,4-D 1.8-2.0mg/mL;6-BA 0.1-0.2mg/mL;Hyg 20-25mg/L, Timentin 200-400mg/ L, agar powder 10-15g/L.
5. agriculture bacillus mediated rice transformation method according to claim 1, which is characterized in that the differential medium packet It includes:NB;Pro 0.3-0.5g/L;CH 0.2-0.3g/L;6-BA 1.8-2.0mg/mL;KT 0.8-1.0mg/mL;NAA 0.3- 0.5mg/mL, IAA 0.4-0.5mg/mL;Hyg 20-25mg/L;Timentin 200-400mg/L;Sucrose 25-30g/L;Fine jade Cosmetics 10-15g/L.
6. agriculture bacillus mediated rice transformation method according to claim 1, which is characterized in that the root media packet It includes:NB;NAA 0.4-0.7mg/L;Sucrose 25-30g/L;Agar powder 10-15g/L.
7. agriculture bacillus mediated rice transformation method according to claim 1, which is characterized in that the step 1) induction, Further comprise:After rice paddy seed decladding disinfection, mature embryo is inoculated in inducing culture, 20 DEG C of constant temperature incubations induce for 7 days Embryo callus.
8. agriculture bacillus mediated rice transformation method according to claim 1, which is characterized in that the step 3) is trained altogether It supports, further comprises:It is 20 DEG C to co-culture temperature, and incubation time is 24 hours.
9. agriculture bacillus mediated rice transformation method according to claim 1, which is characterized in that the step 3) is trained altogether It supports, further comprises:Agrobacterium EHA105 containing target gene carrier is being contained 50mg/L Kan and 50mg/L Rif's The flat lining outs of YEB, 26~30 DEG C of dark culturing 2d are inoculated in fresh YEB with oese picking Agrobacterium single bacterium colony In fluid nutrient medium, 28 DEG C, 220rpm 46~50h of shaking table culture, then Agrobacterium is added to the total training of the AS containing 100umol/L It supports in base, adjustment cell concentration OD600 to 0.1-0.2 or so obtains the agrobacterium suspension for co-culturing conversion.
10. agriculture bacillus mediated rice transformation method according to claim 9, which is characterized in that the YEB culture mediums packet It includes:Yeast extract 0.8-1.2g/L;Peptone 4.5-5.0g/L;Beef extract 4.5-5.0g/L;Sucrose 4.0-6.0g/L;Sulfuric acid Magnesium 0.3-0.5g/L;Agar 12-15g/L;pH 6.8-7.2.
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