CN1742565A - Method for culturing transgene aloes - Google Patents
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Abstract
The present invention discloses a method for cultivating transgenic alae. Said method uses sterilized alol stem segment as explant and adopts the following main steps: cutting the stem segment into small blocks, soaking the stem block in bacterial solution of agrobacterium with target gene and steeping said stem block, then utilizing different culture media of restoration culture medium, budding inducing and screening culture medium and comatus bud inducing and screening medium to make different cultures, said invention provides the concrete requirements and steps of every culture, making secondary and screening culture to obtain comatus bud, strengthening seedling and rooting so as to obtain the transgenic aloe.
Description
Technical field
The present invention relates to a kind of method of cultivating transgene aloes.
Background technology
Aloe (Aloe) belongs to the perennial monocotyledon of Liliaceae, has medical treatment, beauty treatment, health care, multiple function such as edible, is described as " the 21 century mankind's optimum medicines " by FAO (Food and Agriculture Organization of the United Nation) (FAO).Can be used for the good aloe kind of commercial cultivation, must possess three conditions simultaneously: 1) active constituent content height; 2) adaptability is strong, is convenient to enlarge cultivated area, and the development intensification is produced; 3) yield per unit area height helps obtaining best business efficiency.Yet aloe is not cold-resistant, though drought-enduring, poor growth in barren, arid soil, and yield poorly; Edible Aloe kind bitter, sense of taste are poor, and these unfavorable factors have hindered the extensive industrialization process of aloe.Though aboundresources (having kind more than 500) in the Aloe, aloe blooms shaky, or ripening rate is extremely low, and seed seedling-raising technical sophistication, planting percent low (Xiong Youqing, Yao Li, aloe, the China Agricultyre University Press, 62-65).In addition, the improvement of Part Traits can not reach by conventional breeding, need be by engineered means.At present people lay particular emphasis on analysis and development and use to its active ingredient to the research of aloe.(red by continuing, the aloe Study on tissue culture is made progress, Chinese wild plant resource, 2001,2:10-11 though aloe tissue culture and fast breeding technique are ripe; Du Yongjun, Li Huizhi, Qi Yunzhi, the fast numerous and test-tube plantlet cultivation domestication research of aloe bud, northwest Botany Gazette, 2003,12 (1): 72-75), but the structure of aloe transformation system and the research of relevant transgenosis aspect thereof are not appeared in the newspapers as yet.
Plant transgene mainly adopts agrobacterium-mediated transformation and particle gun mediated method.Agrobacterium-mediated transformation is simple to operate because of having, cost is low, transformation efficiency is high, good reproducibility, can import large fragment DNA, and the gene that imports is generally single copy or low copy is integrated, can reduce advantages such as the reticent phenomenon of producer, be most widely used, in the improvement of dicotyledonous economic crops such as soybean, applied.Along with people's going deep into to agrobacterium-mediated transformation transformation mechanism understanding, method for transformation also constantly is improved, as select the bacterial strain of high infecting potential, super binary vector, suitable explant, promotor, suitable cotransformation medium, suitable selective agent, the phenolic compound such as the acetosyringone (acetoayringone of higher concentration efficiently for use, AS) processing waits (Kong Yingzhen, Zhou Gongke, Wang Genxuan, Wang Yafu, influence the factor of Agrobacterium tumefaciems conversion and the application on monocot crops thereof, Chinese Journal of Applied Ecology, 2000,11 (5): 791-794).The agrobacterium-mediated transformation that utilizes improvement has also successfully obtained transfer-gen plant in paddy rice, corn, wheat, barley etc. have the monocotyledon of important value, and detailed molecular biology and inheritance evidence (Hiei Y have been obtained, Komari T, Kabo T., Transformation of rice mediated by Agrobacteriumtumefaciens., Plant Mol Biol, 1997,35:205-218; Ishida Y, Saito H, Ohta S.High efficiency transformation of maize (Zea mays L) mediated by Agrobacteriumtumefaciens, Nat Biotech, 1996,14:745-750; Cheng Ming, E.F.Joyce, PangShengzhi et al., Genetic transformation of wheat mediated by Agrobacteriumtumefaciens, Plant Physiol, 1997,115:971-980).At present, people are devoted to widen the raising of monocotyledonous host range of Agrobacterium-mediated Transformation and transformation efficiency, set up agriculture bacillus mediated transgenosis scheme (the CHAI Bao-Feng of unifacial leaf annual bluegrass after deliberation as Chai Baofeng etc., LIANG Ai-Hua, WANG Wei, Hu Wei, Agrobacterium-mediated Transformation of Kentucky Bliuegrass, Acta BotanicaSinica, 2003,45 (8): 966-973), find that the principal element that influences transgene efficiency has: the embryo of callus, light application time, the cotransformation time, antibiotic concentration and selection pressure.The monocotyledonous example that successfully transforms that has obtained shows, the embryo callus that rataria and maturation or immature embryo produce through inducing is the basis (Yin Liqing that Agrobacterium-mediated Transformation and regeneration are succeedd, Zhang Jianjun, Wang Huimei, Cheng Lei, Wang Xinqi, Shen Gezhi improves the research that Agrobacterium tumefaciens mediated rice genetic transforms transformation frequency, Shanghai Communications University's journal (agricultural science), 2003,21 (supplementary issues): 43-47), in addition, condition of culture comprises temperature altogether, time, medium component also is the principal element (Li Wei that influences Agrobacterium-mediated Transformation efficient, Guo Guangqin, Zheng state Chang, some new developments (commentary) of Agrobacterium tumefaciens mediated Study on Genetic Transformation, Science Bulletin, 2000,45 (8): 798-807).How to induce the non-embryonal connective tissue that produces suitable Agrobacterium-mediated Transformation, the suitable common condition of culture of development is one of task of at present agriculture bacillus mediated monocotyledon genetic transformation.
Summary of the invention
The purpose of this invention is to provide a kind of method of utilizing agrobacterium-mediated transformation to cultivate transgene aloes.
The method of cultivation transgene aloes provided by the present invention can may further comprise the steps:
1) be explant with stem section through sterilization, after being cut into fritter, under 23-27 ℃, soaking 20-40min with the bacterium liquid of cultivating the Agrobacterium that carries genes of interest made from liquid nutrient medium (ACC) suspension through the aloe Agrobacterium altogether infects, take out the stem piece, under the condition of 22-26 ℃, illumination 8-12 hour/day, further infected 2-4 days again; It is to have added 6-benzyladenine (6-BA) on the basis of 1/8-1/12MS minimal medium that described aloe Agrobacterium is cultivated altogether with liquid nutrient medium, α-Nai Yisuan (NAA), and acetosyringone (acetoayringone, AS), glucose, glutamate and casein hydrolysate;
2) the Caulis Aloe piece that infects through Agrobacterium is placed on the recovery media (ARC) that does not add selective agent, under the condition of 22-26 ℃, illumination 8-12 hour/day, recover to cultivate 6-14 days; The described recovery media that does not add selective agent is the antibiotic that has added 6-benzyladenine and α-Nai Yisuan and Agrobacterium is had lethal effect on the basis of MS minimal medium;
3) the Caulis Aloe piece through recover cultivating is placed on inducing clumping bud and the screening culture medium (ASC), cultivation is 18-22 days under the condition of 22-26 ℃, illumination 8-12 hour/day, the inducing and screening of the bud of growing thickly; Described inducing clumping bud and screening culture medium are to have added 6-benzyladenine on the basis of MS minimal medium, α-Nai Yisuan, glufosinate-ammonium (commercial by name Liberty, French Aventis crop science company) and the antibiotic that Agrobacterium is had lethal effect;
4) callus that will grow on inducing clumping bud and screening culture medium or the tender bud of growing thickly of children move to and carry out subculture and screening and culturing on new inducing clumping bud and the screening culture medium under the conditions identical with step 3), the acquisition bud of growing thickly;
5) will grow thickly after bud carries out strong sprout, takes root, obtain transgene aloes.
The carry out disinfection method of sterilization of Caulis Aloe section be can be: the Caulis Aloe section is earlier soaked 20-30min in 20% NaClO solution, in 0.1% mercuric chloride (HgCl) solution, soak 6-8min again.
The preparation method of bacterium liquid who carries the Agrobacterium of genes of interest in the step 1) can be: with OD
650Value is cultivated altogether with in the liquid nutrient medium and is got final product for the thalline in the Agrobacterium bacterium liquid that carries genes of interest of 0.6-0.8 is suspended in the long-pending aloe Agrobacterium of 0.6-1 times of bacteria liquid.The Caulis Aloe piece can be placed on the filter paper of sterilization, under 22-26 ℃, illumination 8-12 hour/day condition, infect further.
For determining sterilization effect, before infecting with Agrobacterium, can earlier the Caulis Aloe piece through sterilization be placed on the inducing clumping bud medium (AC), the pre-cultivation 5-6 days under the condition of 22-26 ℃, illumination 8-12 hour/day, preferred pre-condition of culture is: 24 ℃ of temperature, illumination 10 hours/day; Described inducing clumping bud medium is to have added 6-benzyladenine and α-Nai Yisuan on the basis of MS minimal medium.
The Agrobacterium that is used to infect in the described step 1) can be any one Agrobacterium tumefaciems, as EHA101, C58c1 or LBA4404 etc., is preferably EHA101; The aloe Agrobacterium is cultivated altogether to be preferably on the basis of 1/10MS minimal medium with liquid nutrient medium and has added 6-benzyladenine, α-Nai Yisuan, acetosyringone (acetoayringone, AS), glucose, glutamate and casein hydrolysate; Antibiotic in step 3) inducing clumping bud and the screening culture medium can be any one antibiotic that Agrobacterium is had lethal effect, as cephalosporin, vancomycin or carbenicillin etc.
The concentration of used culture medium additive is in above-mentioned breeding method: the concentration of 6-BA was 2.5-4mg/L during the aloe Agrobacterium was cultivated with liquid nutrient medium altogether, be preferably 3mg/L, the concentration of NAA is 0.15-0.2mg/L, be preferably 0.18mg/L, the concentration of AS is 180-220 μ M, be preferably 200 μ M, the mass percentage concentration of glucose is 0.8-1.2%, be preferably 1%, the concentration of glutamate is 0.3-0.7g/L, be preferably 0.5g/L, the concentration of casein hydrolysate is 0.08-0.12g/L, is preferably 0.1g/L; The concentration of not adding 6-BA in the recovery media of selective agent is 2.5-4mg/L, is preferably 3mg/L, and the concentration of NAA is 0.15-0.2mg/L, is preferably 0.18mg/L; The concentration of 6-BA is 2.5-4mg/L in inducing clumping bud and the screening culture medium, be preferably 3mg/L, the concentration of NAA is 0.15-0.2mg/L, be preferably 0.18mg/L, the concentration of glufosinate-ammonium is 2-3mg/L, is preferably 2.5mg/L, antibiotic kind difference is the concentration difference then, as when selecting carbenicillin for use, concentration is 200-300mg/L, is preferably 250mg/L; The concentration of 6-BA is 2.5-4mg/L in the inducing clumping bud medium, is preferably 3mg/L, and the concentration of NAA is 0.15-0.2mg/L, is preferably 0.18mg/L.
The method that in the step 1) Caulis Aloe piece is infected is preferably: after will being cut into small pieces through the Caulis Aloe section of sterilization, earlier under 25 ℃, carry in the bacterium liquid of Agrobacterium of genes of interest and soak 30min, take out the stem piece, again at 24 ℃, under 10 hours/day the condition of illumination, on the filter paper of sterilization, cultivated 3 days; Step 2) recovering culture condition on the recovery media that does not add selective agent through Caulis Aloe piece that Agrobacterium is infected in is preferably: cultivated 7 days under 24 ℃, 10 hours/day condition of illumination; Caulis Aloe piece through recover cultivating in the step 3) is preferably at the condition of culture on inducing clumping bud and the screening culture medium: cultivation is 20 days under 24 ℃, 10 hours/day condition of illumination.
The invention provides a kind of method of utilizing agrobacterium-mediated transformation to cultivate transgene aloes, aspect practical application, this method will produce following good effect: (1) quickens the transfer of good foreign gene in aloe; (2) for improving cold-resistant, the salt resistance ability of aloe vegetative stage, the planting range of expansion aloe improves the output of unit are aloe leaf and lays a good foundation; (3) for strengthening the effect and the stability of aloe medical treatment, health product, improve the mouthfeel of aloe food, prolong the aloe food freshness date, improve the aloe cosmetics preserve moisture, prevent many improvement with reality and industrialization meaning such as ultraviolet effect everything goes well with your work realize laying the foundation, thereby quicken the industrialization process of aloe.In addition, the present invention understands fully the principal element that influences agriculture bacillus mediated fleshiness monocotyledon transformation system, excavates and also utilizes agriculture bacillus mediated widely transgene receptor resource also significant.
The present invention will be further described below in conjunction with specific embodiment.
Description of drawings
Fig. 1 is for being induced the bud of growing thickly of generation by the Caulis Aloe section
Figure 1A is the physical map of pPNT289
Figure 1B is the physical map of pPNT290
Fig. 2 is that the coloration result of X-gluc after cultivating 3 days altogether on solid culture medium and the filter paper is respectively infected after the Caulis Aloe section in the combination of different Agrobacteriums-plasmid vector
Fig. 3 is the growing state of Caulis Aloe piece after growing 14 days on the inducing clumping bud solid culture medium that is added with 1mg/L, 3mg/L, 5mg/L glufosinate-ammonium
Fig. 4 for the Caulis Aloe piece at the survival curve figure of growth after 14 days on the inducing clumping bud solid culture medium that is added with variable concentrations (1,2,3,4,5mg/L) glufosinate-ammonium
Fig. 5 is the PCR testing result of transgene aloes
Fig. 6 is the ELISA testing result of transgene aloes
Fig. 7 is the aloe transgenic seedling
Embodiment
Method therefor is conventional method if no special instructions among the following embodiment; Used percentage composition is the quality percentage composition.
Inducing clumping bud medium (AC): on the basis of MS minimal medium, add 2.5mg/L 6-BA and 0.15mg/LNAA.
The aloe Agrobacterium is cultivated altogether with medium (ACC): add 2.5mg/L6-BA on the basis of 1/10 MS medium, 0.15mg/L NAA, 200 μ M AS, 1% glucose, 0.5g/L glutamate, 0.1g/L casein hydrolysate (solid culture medium adds 7-8% agar again).
Aloe recovery media (ARC): on the basis of MS minimal medium, add 2.5mg/L6-BA, 0.15mg/LNAA and 250mg/L carbenicillin.
Aloe inducing clumping bud and screening culture medium (ASC): on the basis of MS minimal medium, add 2.5mg/L6-BA, 0.15mg/L NAA, glufosinate-ammonium 2.5mg/L and 250mg/L carbenicillin.
The optimization of embodiment 1, aloe explant sterilization method
With the Caulis Aloe section is example, sterilizing methods to the aloe explant is optimized, concrete grammar is: the fritter that the Caulis Aloe section is cut into about 1cm * 1cm, after in 70% alcohol, soaking 30s, be divided into four groups, respectively through 0.1% mercuric chloride solution (HgCl) sterilization 8min, 0.1%HgCl solution sterilization 13min, 10% clorox (NaClO) solution sterilization 15min, 20%NaClO solution sterilization 25min, use rinsed with sterile water 3-4 time again, then the Caulis Aloe piece is placed on the inducing clumping bud medium, at 24 ℃, cultivate under 10 hours/day the condition of illumination, statistics explant survival rate and pollution ratio, the result is as shown in table 1, take into account survival rate and sterilizing efficiency, determine the aloe explant is soaked 20-30min earlier in 20%NaClO solution, soaking 6-8min again in 0.1% mercuric chloride (HgCl) solution is preferred aloe explant sterilization method.
The comparative result of the different sterilizing methods effects of table 1 aloe stem explants
| The explant sum | Microbiological contamination explant number not | Not microbiological contamination ratio (%) | Survive the explant number | Survive ratio (%) | |
| 0.1% mercuric chloride soaked 13 minutes | 139 | 121 | 87.1 | 90 | 42.7 |
| 0.1% mercuric chloride soaked 8 minutes | 137 | 90 | 65.7 | ||
| 10% clorox soaked 15 minutes | 59 | 0 | 0.0 | 179 | 82.5 |
| 20% clorox soaked 25 minutes | 289 | 217 | 75.1 |
Embodiment 2, be used for the preferred of aloe explant that Agrobacterium infects
After the aloe sterilization, respectively blade, leaf sheath, stem section are cut into the fritter of 1cm * 1cm, place on the inducing clumping bud medium, under 24 ℃, 10 hours/day condition of illumination, cultivate 4-5 week, observe the regeneration situation of explant, statistics survival number and survival ratio, the result is as shown in table 2, the stem section of determining aloe is to be most appropriate to the explant that Agrobacterium is infected, and grows thickly bud as shown in Figure 1 by it through what induce generation.
Table 2 aloe explant upgrowth situation comparative result
| Explant type | The explant number | The survival number | Survival ratio % |
| Blade | 224 | 0 | 0.0 |
| Leaf sheath | 140 | 31 | 22.1 |
| Stem | 148 | 103 | 69.6 |
The comparison that embodiment 3, different Agrobacterium fungus strains infect effect
With plasmid vector pPNT289 (physical map is shown in Figure 1A), pPNT290 (physical map is shown in Figure 1B), transform Agrobacterium EHA101 respectively, carried the recon of pPNT289, pPNT290, called after EHA101/pPNT289 and EHA101/pPNT290 respectively through screening; With plasmid pPNT289, pPNT290 being transformed Agrobacterium C58c1 respectively, carried the recon of pPNT289, pPNT290, called after C58c1/pPNT289, C58c1/pPNT290 respectively through screening with quadrat method.Collect above-mentioned four kinds of OD
650Value is the thalline of 0.8 reorganization Agrobacterium bacterium liquid, thalline is suspended in the long-pending aloe Agrobacterium of 0.8 times of above-mentioned bacteria liquid cultivates altogether with in the liquid nutrient medium (ACC), obtains Agrobacterium bacterium liquid.To infect 30min to the Caulis Aloe section with four kinds of Agrobacterium bacterium liquid that the suspension of ACC liquid nutrient medium is made then, again respectively on ACC solid culture medium and aseptic blank filter paper at 24 ℃, cultivated altogether 3 days under 10 hours/day the condition of illumination, after cultivating end, it is carried out X-Gluc dyeing, coloration result as shown in Figure 2, the transient expression rate of gus gene in the explant of calculating through infecting, and be analyzed, the result is as shown in table 3, the effect that infects of EHA101/pPNT289 obviously is better than other combination, the transient expression rate of gus gene reaches about 80% in the explant after EHA101 infects, and the transient expression rate of gus gene only has an appointment 30% in the explant of C58c1 after infecting, the integral body that shows the EHA101 fungus strain infects effect and is better than the c58c1 fungus strain, and EHA101 is defined as preferably being used to make up the starting strain that the aloe explant infects bacterial strain.
The different Agrobacteriums of table 3-plasmid vector combination is total on solid culture medium and filter paper respectively after infecting the Caulis Aloe section
Cultivate the coloration result of X-gluc after 3 days
| Fungus strain-carrier combinations | Co-culture method | The explant number that X-gluc detects | Express the explant number of GUS gene | Dyeing ratio (%) |
| EHA101/pPNT289 | Filter paper | 30 | 20 | 66.7 |
| Solid culture medium (ACC) | 31 | 8 | 25.8 | |
| EHA101/pPNT290 | Filter paper | 36 | 2 | 5.6 |
| Solid culture medium (ACC) | 33 | 1 | 3.0 | |
| C58c1/pPNT290 | Filter paper | 33 | 0 | 0.0 |
| Solid culture medium (ACC) | 34 | 0 | 0.0 | |
| C58c1/pPNT289 | Filter paper | 29 | 1 | 3.5 |
| Solid culture medium (ACC) | 34 | 0 | 0.0 |
The cultivation of embodiment 4, transgene aloes and detection
One, the cultivation of transgene aloes
With Agrobacterium EHA101 is starting strain, utilizes agrobacterium-mediated transformation to cultivate transgene aloes, and concrete cultivating process may further comprise the steps:
1, Agrobacterium infects
With the Caulis Aloe section is explant, after cleaning, the Caulis Aloe section is soaked 25min earlier in 20%NaClO solution, soaks 8min again and sterilize in 0.1% mercuric chloride solution.Caulis Aloe section after will sterilizing with the 15# scalpel is cut into the fritter of 1cm * 1cm.With OD
650Value is that the thalline that carries among 0.7 the embodiment 3 in the Agrobacterium EHA101/pPNT289 bacterium liquid of genes of interest is suspended in the long-pending ACC liquid nutrient medium of 1 times of bacteria liquid, obtains EHA101/pPNT289 bacterium liquid.Under 25 ℃, the EHA101/pPNT289 bacterium liquid that will place the suspension of ACC liquid nutrient medium to make through the Caulis Aloe piece of sterilization soaks 30min and infects, take out the stem piece, place on the aseptic blank filter paper, under 24 ℃, 10 hours/day condition of illumination, cultivate altogether again and further infected in 3 days.
2, recover to cultivate
The Caulis Aloe piece through Agrobacterium is infected that step 1 is obtained places on the recovery media that does not add the antibiotic-screening agent, under 24 ℃, 10 hours/day condition of illumination, recovers to cultivate 7 days.
3, grow thickly the determining of the inducing of bud, screening and selective agent suitable concentration
1) the determining of selective agent glufosinate-ammonium suitable concentration in inducing clumping bud and the screening culture medium
The Caulis Aloe piece through recovering to cultivate that step 2 is obtained places and is added with variable concentrations (1mg/L, 2mg/L, 3mg/L, 4mg/L, 5mg/L) in the inducing clumping bud solid culture medium of selective agent glufosinate-ammonium, at 24 ℃, cultivate under 10 hours/day the condition of illumination, observe growth of aloe explant and bud and induce situation, the Caulis Aloe piece of cultivating after 14 days is being added with 1mg/L, 3mg/L, growing state on the inducing clumping bud solid culture medium of 5mg/L glufosinate-ammonium as shown in Figure 3, the stem hop count and the survival ratio of statistics survival, statistics is as shown in table 4, be depicted as curve map (Fig. 4 according to statistics, abscissa is a selective agent concentration, ordinate is the survival ratio), selective agent concentration during with survival rate 50% is decided to be its suitable concentration, thus determine aloe transform in the suitable concentration of selective agent glufosinate-ammonium in inducing clumping bud and the screening culture medium (with the bar gene as selected marker) be 2.5mg/L.
Under variable concentrations glufosinate-ammonium selective agent, the survive statistics of ratio of table 4 Caulis Aloe section
| Selective agent concentration (mg/L) | Caulis Aloe section sum | Survival stem hop count | Survival ratio (%) |
| 1 | 43 | 34 | 79.1 |
| 2 | 38 | 24 | 63.2 |
| 3 | 40 | 17 | 42.5 |
| 4 | 39 | 15 | 38.5 |
| 5 | 39 | 11 | 28.2 |
2) grow thickly the inducing, screen of bud
Caulis Aloe piece through recover cultivating is placed on the inducing clumping bud and screening culture medium that contains 2.5mg/L glufosinate-ammonium, and cultivation is 20 days under 24 ℃, 10 hours/day condition of illumination, the inducing and screening of the bud of growing thickly.
4, the grow thickly acquisition of bud
Callus that step 3 is grown on inducing clumping bud and screening culture medium or the tender bud of growing thickly of children move to and carry out subculture and screening and culturing on new inducing clumping bud and the screening culture medium under the conditions identical with step 3, the acquisition bud of growing thickly.
5, the acquisition of transgene aloes
The bud of growing thickly that step 4 is obtained carries out strong sprout, take root after, obtain transgene aloes.
Two, the detection of transgene aloes
1, the PCR of transgene aloes detects
The transgene aloes that step 1 is obtained detects with the method for PCR, designs primer according to NPT II gene order, and primer sequence is as follows:
Primer 1 (upstream primer): 5 '-TGTTCCGGCTGTCAGCGCAG-3 '
Primer 2 (downstream primer): 5 '-TCGGCAAGCAGGCATCGCCA-3 '
Adopt the SDS method extract total DNA of aloe regrowth and with this as template, under the guiding of primer 1 and primer 2, the NPT II gene in the transfer-gen plant is carried out pcr amplification, the PCR reaction condition is: 94 ℃ of 5min earlier; 94 ℃ of 30s then, 58 ℃ of 30s, 72 ℃ of 90s, totally 30 circulations; Last 72 ℃ of 10min.After reaction finishes, the PCR product is carried out 1% agarose gel electrophoresis to be detected, testing result is (swimming lane M:DNA MarkerDL2000 as shown in Figure 5, swimming lane 1-8: different plant to be measured, swimming lane 9: negative control, swimming lane 10: positive control), can amplify size and be the positive transfer-gen plant of 476bp dna fragmentation.
2, the ELISA of transgene aloes detects
Detect the expression of NPTII albumen in the transfer-gen plant with the ELISA method, adopt the Pathoscreen kit for neomycin phosphotransferase II kit and the reference reagent box specification of agdia company to operate, testing result is the (plant to be measured of the 1-4:PCR positive as shown in Figure 6; 5: negative control; 6-7: do not carry out the plant to be measured that PCR detects; 8: positive control), obtained positive transgene aloes (Fig. 7) through step 1 PCR detection and step 2 ELISA detection.
Claims (10)
1, a kind of method of cultivating transgene aloes may further comprise the steps:
1) be explant with stem section through sterilization, after being cut into fritter, under 23-27 ℃, soaking 20-40min with the bacterium liquid of cultivating the Agrobacterium that carries genes of interest made from the liquid nutrient medium suspension through the aloe Agrobacterium altogether infects, take out the stem piece, under the condition of 22-26 ℃, illumination 8-12 hour/day, further infected 2-4 days again; It is to have added 6-benzyladenine on the basis of 1/8-1/12 MS minimal medium that described aloe Agrobacterium is cultivated altogether with liquid nutrient medium, α-Nai Yisuan, acetosyringone, glucose, glutamate and casein hydrolysate;
2) the Caulis Aloe piece that infects through Agrobacterium is placed on the recovery media that does not add selective agent, under 22-26C, illumination 8-12 hour/day condition, recover to cultivate 6-14 days; The described recovery media that does not add selective agent is the antibiotic that has added 6-benzyladenine, α-Nai Yisuan and Agrobacterium is had lethal effect on the basis of MS minimal medium;
3) the Caulis Aloe piece through recover cultivating is placed on inducing clumping bud and the screening culture medium, cultivation is 18-22 days under the condition of 22-26 ℃, illumination 8-12 hour/day, the inducing and screening of the bud of growing thickly; Described inducing clumping bud and screening culture medium are the antibiotic that has added 6-benzyladenine, α-Nai Yisuan, glufosinate-ammonium and Agrobacterium is had lethal effect on the basis of MS minimal medium;
4) callus that will grow on inducing clumping bud and screening culture medium or the tender bud of growing thickly of children move to and carry out subculture and screening and culturing on new inducing clumping bud and the screening culture medium under the conditions identical with step 3), the acquisition bud of growing thickly;
5) will grow thickly after bud carries out strong sprout, takes root, obtain transgene aloes.
2, method according to claim 1 is characterized in that: in the described step 1) to the carry out disinfection method of sterilization of Caulis Aloe section be: the Caulis Aloe section is earlier soaked 20-30min in 20%NaClO solution, soak 6-8min again in 0.1% mercuric chloride solution.
3, method according to claim 1 is characterized in that: carrying the bacterium liquid of the Agrobacterium of genes of interest in the described step 1), is with OD
650Value is cultivated with making in the liquid nutrient medium altogether for the thalline in the Agrobacterium bacterium liquid that carries genes of interest of 0.6-0.8 is suspended in 0.6-1 times of bacteria liquid long-pending aloe Agrobacterium; The Caulis Aloe piece under 22-26 ℃, illumination 8-12 hour/day condition, is further infected and is to carry out on the filter paper of sterilization.
4, according to claim 1 or 2 or 3 described methods, it is characterized in that: before infecting, will place on the inducing clumping bud medium pre-the cultivation 5-6 days under the condition of 22-26 ℃, illumination 8-12 hour/day earlier through the Caulis Aloe piece of sterilization with Agrobacterium; Described inducing clumping bud medium is that to have added concentration on the basis of MS minimal medium be that 6-benzyladenine and the concentration of 2.5-4mg/L is the α-Nai Yisuan of 0.15-0.2mg/L.
5, method according to claim 4 is characterized in that: describedly the Caulis Aloe piece is carried out pre-incubated condition be: 24 ℃ of temperature, illumination 10 hours/day.
6, according to claim 1 or 2 or 3 described methods, it is characterized in that: the Agrobacterium starting strain that is used to infect in the described step 1) is EHA101 or C58c1; The aloe Agrobacterium is cultivated with liquid nutrient medium altogether to have added 6-benzyladenine on the basis of 1/10 MS minimal medium, α-Nai Yisuan, acetosyringone (acetoayringone, AS), glucose, glutamate and casein hydrolysate; Antibiotic in step 3) inducing clumping bud and the screening culture medium is cephalosporin, vancomycin or carbenicillin.
7, method according to claim 6 is characterized in that: the Agrobacterium starting strain that is used to infect in the described step 1) is EHA101.
8, according to claim 1 or 2 or 3 described methods, it is characterized in that: the concentration that described aloe Agrobacterium is cultivated altogether with 6-BA in the liquid nutrient medium is 2.5-4mg/L, the concentration of NAA is 0.15-0.2mg/L, the concentration of AS is 180-220 μ M, the mass percentage concentration of glucose is 0.8-1.2%, the concentration of glutamate is 0.3-0.7g/L, and the concentration of casein hydrolysate is 0.08-0.12g/L; The concentration of not adding 6-BA in the recovery media of selective agent is 2.5-4mg/L, and the concentration of NAA is 0.15-0.2mg/L; The concentration of 6-BA is 2.5-4mg/L in inducing clumping bud and the screening culture medium, and the concentration of NAA is 0.15-0.2mg/L, and the concentration of glufosinate-ammonium is 2-3mg/L.
9, method according to claim 8, it is characterized in that: the concentration that described aloe Agrobacterium is cultivated altogether with 6-BA in the liquid nutrient medium is 3mg/L, the concentration of NAA is for being 0.18mg/L, the concentration of AS is 200 μ M, the mass percentage concentration of glucose is 1%, the concentration of glutamate is 0.5g/L, and the concentration of casein hydrolysate is 0.1g/L; The concentration of not adding 6-BA in the recovery media of selective agent is 3mg/L, and the concentration of NAA is 0.18mg/L; The concentration of 6-BA is 3mg/L in inducing clumping bud and the screening culture medium, and the concentration of NAA is 0.18mg/L, and the concentration of glufosinate-ammonium is 2.5mg/L.
10, according to claim 1 or 2 or 3 described methods, it is characterized in that: the method that in the described step 1) Caulis Aloe piece is infected is: will be first under 25 ℃ through the Caulis Aloe piece of sterilization, soak 30min with the bacterium liquid of cultivating the Agrobacterium that carries genes of interest of making through the aloe Agrobacterium altogether with the liquid nutrient medium suspension, take out the stem piece, again at 24 ℃, under 10 hours/day the condition of illumination, cultivated 3 days; Described step 2) recovering culture condition on the recovery media that does not add selective agent through Caulis Aloe piece that Agrobacterium is infected in is: cultivated 7 days under 24 ℃, 10 hours/day condition of illumination; Caulis Aloe piece through recover cultivating in the described step 3) at the condition of culture on inducing clumping bud and the screening culture medium is: cultivation is 20 days under 24 ℃, 10 hours/day condition of illumination.
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Cited By (2)
| Publication number | Priority date | Publication date | Assignee | Title |
|---|---|---|---|---|
| US8816154B2 (en) | 2005-09-26 | 2014-08-26 | Thegreencell, Inc. | Transgenic aloe plants for production of proteins and related methods |
| CN104805116A (en) * | 2015-02-13 | 2015-07-29 | 夏松 | Fusion expression application method of active protein gene in aloe |
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Cited By (3)
| Publication number | Priority date | Publication date | Assignee | Title |
|---|---|---|---|---|
| US8816154B2 (en) | 2005-09-26 | 2014-08-26 | Thegreencell, Inc. | Transgenic aloe plants for production of proteins and related methods |
| US9267149B2 (en) | 2005-09-26 | 2016-02-23 | Thegreencell, Inc. | Transgenic aloe plants for production of proteins and related methods |
| CN104805116A (en) * | 2015-02-13 | 2015-07-29 | 夏松 | Fusion expression application method of active protein gene in aloe |
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