CN1806529A - Method for in-vitro breeding indirect regenerated plant of watermelon cotyledon - Google Patents
Method for in-vitro breeding indirect regenerated plant of watermelon cotyledon Download PDFInfo
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- 241000219109 Citrullus Species 0.000 title claims abstract description 56
- 235000012828 Citrullus lanatus var citroides Nutrition 0.000 title claims abstract description 55
- 241000196324 Embryophyta Species 0.000 title claims abstract description 25
- 238000000034 method Methods 0.000 title claims abstract description 15
- 238000000338 in vitro Methods 0.000 title claims description 14
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- SEOVTRFCIGRIMH-UHFFFAOYSA-N indole-3-acetic acid Chemical compound C1=CC=C2C(CC(=O)O)=CNC2=C1 SEOVTRFCIGRIMH-UHFFFAOYSA-N 0.000 claims description 2
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Abstract
The invention discloses a method for secondhand regenerating watermelon plant through isolated culture of cotyledon, comprising the following steps: (1) seed germinating: employing Jingxin or Yixuan watermelon cultivating seed for seed germinating; (2) callus inducing: employing part between hypocotyls and cotyledon of four-day seedling as aexplant and inoculating it to inducing culture medium to culture under 25 Deg. C in dark for 20 days, and getting callus; (3) differentiating callus for adventitious bud: transporting callus to differentiation culture medium, culturing under light for 30 days and getting secondhand regenerating adventitious bud; (4) extending and root culturing the regenerating adventitious bud and getting secondhand regenerating plant. The integral plant of watermelon can be got by using the method in this invention.
Description
Technical field
The present invention relates to the method for a kind of method for tissue culture, particularly in-vitro breeding indirect regenerated plant of watermelon cotyledon.
Background technology
Watermelon is fragrant and sweet delicious, and contains higher vitamin and tomatin, therefore is subjected to liking of consumers in general.Watermelon is as a kind of important vegetable crop, and annual production is above 8,100 ten thousand tons in the world.The influence of various natural calamities such as but watermelon suffers disease easily, damage to plants caused by sudden drop in temperature causes its cultivation to be very restricted.Meanwhile, along with the raising of socio-economic development and living standards of the people, people are more and more higher to the requirement of watermelon kind and quality, wish constantly to have throughout the year watermelon launch high-quality, different cultivars.The genetic character of watermelon can be improved by cultured in vitro, improvement of genes and somaclone screening mutant, thereby many anti-, high-quality variety of watermelon can be obtained for cultivation.The watermelon cultured in vitro has had the history of decades, and from various approach such as Shoot Tip Culture, adventitious bud inducing and somatic embryo generations the watermelon cultured in vitro is studied.But, watermelon tissue culture in the past or the approach acquisition plant of adopting directly regeneration; After inducing the complete dedifferentiation callus of watermelon, further do not carry out dedifferentiation and obtain regeneration plant.Michact E.Compton and D.J.Gray use the cotyledon of watermelon immature embryo as explant, through the somatic embryo that inducing culture obtains directly and indirect (callus approach) regenerates; This method not only frequency ratio is low, and the somatic embryo germination rate of gained is very low.Yet, in plant tissue culture course,, obtain the somaclone mutant that hereditary shape obtains improveing thereby be beneficial to by easier the undergoing mutation of the direct regeneration of the indirect reproduction ratio of explant.If carry out genetic transformation as material, then might increase the chance of carrying the foreign gene microbial infection, thereby improve the frequency of genetic transformation with callus.And cultivate and somatic hybridization when obtaining regeneration plant by anther culture, protoplast, must just can obtain plant by indirect regeneration approach again.
Summary of the invention
At the deficiencies in the prior art part, the invention provides a kind of method of in-vitro breeding indirect regenerated plant of watermelon cotyledon.
The present invention is to realize by such technical scheme: a kind of method of in-vitro breeding indirect regenerated plant of watermelon cotyledon is provided, may further comprise the steps for reaching above purpose:
1), seed sprouting: selecting Jing Xin or Yi Xuan class cultivating watermelon kind for use is that material carries out seed sprouting;
2), callus induction:
Choose between the plumular axis of above-mentioned 4 age in days seedling aseptic seedling and the cotyledon position as explant;
When the cultivating watermelon kind is that the capital is when glad, above-mentioned explant is inoculated on the inducing culture A, and inducing culture A is according to the ratio that adds 20 gram sucrose, 7 gram agar, 1.0 milligrams of methyls (NAA), 0.5 milligram of six benzyladenine (BA) and 2.0 milligrams of 6-chaff aminopurines (KT) in every liter of MS minimal medium and to regulate the pH value be 5.8 made;
When the cultivating watermelon kind is Yi Xuanshi, above-mentioned explant is inoculated on the inducing culture B, and inducing culture B is according to the ratio that adds 20 gram sucrose, 7 gram agar, 1.0 milligrams of NAA, 2.0 milligrams of BA and 1.0 milligrams of KT in every liter of MS minimal medium and to regulate the pH value be 5.8 made;
With the above-mentioned explant that is inoculated on the inducing culture, cultivated 20 days down in 25 ℃ dark conditions, induce the acquisition callus;
3), callus differentiation indefinite bud:
According to adding the ratio of 0.1 milligram of heteroauxin (IAA), 2.0 milligrams of BA and 2.0 milligrams of KT in every liter of MS minimal medium and regulating the pH value is 5.8, has made differential medium;
Above-mentioned callus is forwarded on the differential medium, and move on under the light and to continue to cultivate 30 days, obtain indirect regenerated adventitious bud;
4), with above-mentioned indirect regenerated adventitious bud extend, culture of rootage, obtain indirect regenerated plant.
A kind of improvement as the method for in-vitro breeding indirect regenerated plant of watermelon cotyledon of the present invention, the seed sprouting step is: seed is peelled off shell soak 3.5~4.5 hours in 30 ℃ of running water after, the seed that will shell then binds up with gauze and immerses among 10% liquor natrii hypochloritis, places the sterilization 10 minutes of vibrating on the shaking table; Then the seed that shells is washed with sterile water.Again the seed that shells after the above-mentioned flushing is inoculated into according to the ratios that add 20 gram sucrose and 7 gram agar in every liter of MS minimal medium and makes and the pH value is on 5.8 the medium; Cultivated 30 hours down prior to the dark condition of 28 ℃ of incubators, treat that 90% above seed base-root exposes after, transfer to again and continue cultivation the illumination condition of culturing room 3000 luxs (LX) under, cotyledon expansion after 4~5 days.
As a kind of improvement of the method for in-vitro breeding indirect regenerated plant of watermelon cotyledon of the present invention, in the callus induction step: explant is the cuboid that long 0.5cm, wide 0.2cm and surface have 3~4 road scalpel cuts.
The present invention has specifically considered following several factors role in the present invention in production process:
One, the difference of illumination condition is to the influence of watermelon evoked callus: found that the callus of inducing is faint yellow graininess under dark condition, and glossy; As shown in Figure 3 and Figure 4.Obviously effective than the callus of inducing under the 3000LX illumination condition (as depicted in figs. 1 and 2).
Two, different hormone combinations are to the influence of callus induction and plant regeneration:
1), different hormone combinations are to the influence of callus induction:
In every liter of MS minimal medium, add on the basis of 20 gram sucrose, 7 gram agar, add NAA, BA, the KT hormone of different proportionings, and to regulate its pH value be 5.8, make corresponding inducing culture, specifically as shown in table 1:
18 kinds of made inducing cultures of different proportioning hormones of table 1
| Medium numbering number of medium | Hormone concentration (mg/L) concentration of hormone | ||
| NAA | BA | KT | |
| Y1 Y2 Y3 Y4 Y5 Y6 Y7 Y8 (inducing culture A) Y9 Y10 Y11 (inducing culture B) Y12 Y13 Y14 Y15 Y16 Y17 Y18 | 0.5 0.5 0.5 0.5 0.5 0.5 1.0 1.0 1.0 1.0 1.0 1.0 2.0 2.0 2.0 2.0 2.0 2.0 | 0.5 0.5 1.0 1.0 2.0 2.0 0.5 0.5 1.0 1.0 2.0 2.0 0.5 0.5 1.0 1.0 2.0 2.0 | 1.0 2.0 1.0 2.0 1.0 2.0 1.0 2.0 1.0 2.0 1.0 2.0 1.0 2.0 1.0 2.0 1.0 2.0 |
With capital glad class watermelon explant and Yi Xuan class watermelon explant, be inoculated in respectively on the above-mentioned inducing culture, cultivated 20 days down in 25 ℃ dark conditions, induce to obtain corresponding callus.
The result shows: adopt the Y8 medium (promptly to add in every liter of MS minimal medium on the basis of 20 gram sucrose, 7 gram agar, add 1.0mg NAA, 0.5mg BA and 2.0mg KT again) induce capital glad class watermelon callus effect best: inductivity height not only, and the callus quality of inducing is good, there is not brownization of explant situation to take place, as shown in Figure 3.The Y8 medium is defined as inducing culture A.Adopt the Y11 medium (promptly in every liter of MS minimal medium, to add on the basis of 20 gram sucrose, 7 gram agar, add 1.0mg NAA, 2.0mg BA and 1.0mg KT again) induce Yi Xuan class watermelon callus effect best: inductivity height not only, and the callus quality of inducing is good, there is not brownization of explant situation to take place, as shown in Figure 4.The Y11 medium is defined as inducing culture B.
2), different hormone combinations are to the influence of callus regeneration indefinite bud frequency:
In every liter of MS minimal medium, add IAA, BA, the KT hormone of different proportionings, and to regulate its pH value be 5.8, make corresponding differential medium.The Yi Xuan class watermelon callus that capital glad class watermelon callus that above-mentioned inducing culture A (being the Y8 medium) is induced and above-mentioned inducing culture B (being the Y11 medium) induce, forward to respectively on the above-mentioned different differential medium, and move on under the light and to continue to cultivate 30 days, obtain indirect regenerated adventitious bud.Hormone-content and corresponding callus differentiation frequency in the differential medium are as shown in table 2.
Hormone-content and corresponding callus differentiation frequency in table 2 differential medium
| Differential medium numbering number of medium | Hormone concentration (mg/L) concentration of hormone differentiation | Callus differentiation frequency frequency of calli | |||
| IAA | BA | KT | Yi Xuan | The capital is glad | |
| F1 F2 F3 F4 F5 | 0.00 0.00 0.00 0.00 0.05 | 2.0 2.0 4.0 4.0 2.0 | 0.0 2.0 0.0 2.0 0.0 | 0±0 0±0 2.1±4.2 0±0 4.2±4.8 | 0±0 2.1±4.2 0±0 0±0 6.3±8.0 |
| F6 F7 F8 F9 *F10 F11 F12 | 0.05 0.05 0.05 0.10 0.10 0.10 0.10 | 2.0 4.0 4.0 2.0 2.0 4.0 4.0 | 2.0 0.0 2.0 0.0 2.0 0.0 2.0 | 8.3±0 6.2±4.2 4.2±4.8 6.3±8.0 12.5±4.8 4.2±4.8 8.3±6.8 | 10.4±4.2 6.3±8.0 6.2±4.2 4.2±8.4 18.8±4.2 6.3±8.0 8.3±0 |
The result shows: Yi Xuan and the complete dedifferentiation callus of Jing Xin two class watermelons all reach the highest regeneration frequency on F10 differential medium (being to add 0.1 milligram of IAA, 2.0 milligrams of BA and 2.0 milligrams of KT in every liter of MS minimal medium), be respectively 12.5 ± 4.8% and 18.8 ± 4.2%, and regenerated adventitious bud is light green, glossy, as Fig. 5, shown in Figure 6.
The present invention has successfully obtained by Yi Xuan and the indirect regenerated adventitious bud of Jing Xin two class watermelons, and has obtained whole plant by elongation, culture of rootage---the watermelon indirect regenerated plant.The present invention has set up the indirect regenerating system of good watermelon, and for somaclonal variation is induced, improvement of genes, anther culture, protoplast cultivation and research such as fusion and multiploid induction and application provide foundation.
All medium that use among the present invention are all regulated pH value to 5.8 with NAOH or the HCL of 1mol/L, constant temperature sterilization 20min between 121~126 ℃.The MS minimal medium is the plant tissue minimal medium of Murashige and Skoog1962 invention.
Description of drawings
Fig. 1 is the callus figure that " Yi Xuan " induces under the 3000LX illumination condition;
Fig. 2 is the callus figure that " capital is glad " induced under the 3000LX illumination condition;
Fig. 3 is the shooting figure under " Yi Xuan " the callus Stereo microscope of inducing under dark condition;
Fig. 4 is the shooting figure under " capital is glad " the callus Stereo microscope of inducing under dark condition;
Fig. 5 is the shooting figure under " Yi Xuan " callus regenerated adventitious bud Stereo microscope;
Fig. 6 is the shooting figure under " capital is glad " callus regenerated adventitious bud Stereo microscope.
Embodiment
With reference to above-mentioned accompanying drawing, the specific embodiment of the present invention is elaborated.A kind of method of in-vitro breeding indirect regenerated plant of watermelon cotyledon is characterized in that may further comprise the steps:
1, seed sprouting:
Selecting Jing Xin and Yi Xuan class cultivating watermelon kind for use is material, and the sprouting step of two kinds of seeds is:
Seed soaks after about 4 hours in 30 ℃ of running water peels off shell, and the seed that will shell then binds up with gauze that to immerse concentration be among 10% the liquor natrii hypochloritis, placing on the shaking table vibration sterilization 10 minutes; Then the seed that shells is repeatedly washed with sterile water;
The seed that shells after the above-mentioned flushing is inoculated into according to the ratios that add 20 gram sucrose and 7 gram agar in every liter of MS minimal medium makes and the pH value is on 5.8 the medium; Cultivated 30 hours down prior to the dark condition of 28 ℃ of incubators, treat that 90% above seed base-root exposes after, transfer to again and continue cultivation the 3000LX of culturing room illumination condition under, cotyledon expansion after 4~5 days.
2, callus induction:
1), choose the strong position of regeneration capacity between the plumular axis of above-mentioned 4 age in days seedling aseptic seedling and the cotyledon, be cut into the cuboid that is about the wide about 0.2cm of 0.5cm, draw under the 3-4 as explant on the cuboid surface with scalpel.
2), when the cultivating watermelon kind be that the capital is when glad, explant is inoculated on the inducing culture A, and inducing culture A is according to the ratio that adds 20 gram sucrose, 7 gram agar, 1.0 milligrams of NAA, 0.5 milligram of BA and 2.0 milligrams of KT in every liter of MS minimal medium and to regulate the pH value be 5.8 made.
When the cultivating watermelon kind is Yi Xuanshi, explant is inoculated on the inducing culture B, and inducing culture B is according to the ratio that adds 20 gram sucrose, 7 gram agar, 1.0 milligrams of NAA, 2.0 milligrams of BA and 1.0 milligrams of KT in every liter of MS minimal medium and to regulate the pH value be 5.8 made.
3), above-mentioned 2 classes are inoculated in explant on the inducing culture, cultivated 20 days down respectively at 25 ℃ dark conditions, it is all fine to induce the back to obtain the effect of capital glad class watermelon callus and Yi Xuan class watermelon callus: i.e. inductivity height not only, and the callus quality of inducing is good, does not have brownization of explant situation to take place.
3, callus differentiation indefinite bud:
According to adding the ratio of 0.1 milligram of IAA, 2.0 milligrams of BA and 2.0 milligrams of KT in every liter of MS minimal medium and regulating the pH value is 5.8, makes differential medium.
With above-mentioned capital glad class watermelon callus and Yi Xuan class watermelon callus, forward on the differential medium respectively, and move on to group training chamber, light continues to cultivate 30 days down, obtains capital indirect regenerated adventitious bud of glad class watermelon and the indirect regenerated adventitious bud of Yi Xuan class watermelon respectively.
Capital glad class watermelon callus and Yi Xuan class watermelon callus all reach the highest regeneration frequency on above-mentioned differential medium, be respectively 12.5 ± 4.8% and 18.8 ± 4.2%; And two kinds of regenerated adventitious buds are light green, glossy.
4, above-mentioned indirect regenerated adventitious bud is extended, culture of rootage, obtain indirect regenerated plant:
With above-mentioned capital indirect regenerated adventitious bud of glad class watermelon and the indirect regenerated adventitious bud of Yi Xuan class watermelon, forward to respectively on the MS+0.1mg/L KT medium (promptly according to the ratio that adds 0.1 milligram of KT in every liter of MS minimal medium and to regulate the pH value be 5.8 made) and cultivate.
Treat that above-mentioned two kinds of indefinite buds are after growing to 1.5-2.0cm respectively on the elongation medium, again it was forwarded on the root media (promptly according to the ratio that adds 0.1 milligram of NAA in every liter of MS minimal medium and to regulate pH value be 5.8 made) of MS+0.1mg/LNAA to culture of rootage respectively 15 days, just can the opening acclimatization and transplants.
Used MS minimal medium in the above-mentioned experimentation all can be given birth to worker's biotechnology Co., Ltd available from Sigma and Shanghai.
At last, it is also to be noted that what more than enumerate only is a specific embodiment of the present invention.Obviously, the invention is not restricted to above embodiment, many distortion can also be arranged.All distortion that those of ordinary skill in the art can directly derive or associate from content disclosed by the invention all should be thought protection scope of the present invention.
Claims (3)
1, a kind of method of in-vitro breeding indirect regenerated plant of watermelon cotyledon is characterized in that may further comprise the steps:
1), seed sprouting: selecting Jing Xin or Yi Xuan class cultivating watermelon kind for use is that material carries out seed sprouting;
2), callus induction:
Choose between the plumular axis of above-mentioned 4 age in days seedling aseptic seedling and the cotyledon position as explant;
When the cultivating watermelon kind is that the capital is when glad, above-mentioned explant is inoculated on the inducing culture A, and described inducing culture A is according to the ratio that adds 20 gram sucrose, 7 gram agar, 1.0 milligrams of methyls, 0.5 milligram of six benzyladenine and 2.0 milligrams of 6-chaff aminopurines in every liter of MS minimal medium and to regulate the pH value be 5.8 made;
When the cultivating watermelon kind is Yi Xuanshi, above-mentioned explant is inoculated on the inducing culture B, and described inducing culture B is according to the ratio that adds 20 gram sucrose, 7 gram agar, 1.0 milligrams of methyls, 2.0 milligram of six benzyladenine and 1.0 milligrams of 6-chaff aminopurines in every liter of MS minimal medium and to regulate the pH value be 5.8 made;
With the above-mentioned explant that is inoculated on the inducing culture, cultivated 20 days down in 25 ℃ dark conditions, induce the acquisition callus;
3), callus differentiation indefinite bud:
According to adding the ratio of 0.1 milligram of heteroauxin, 2.0 milligram of six benzyladenine and 2.0 milligrams of 6-chaff aminopurines in every liter of MS minimal medium and regulating the pH value is 5.8, has made differential medium;
Above-mentioned callus is forwarded on the differential medium, and move on under the light and to continue to cultivate 30 days, obtain indirect regenerated adventitious bud;
4), with above-mentioned indirect regenerated adventitious bud extend, culture of rootage, obtain indirect regenerated plant.
2, the method for in-vitro breeding indirect regenerated plant of watermelon cotyledon according to claim 1 is characterized in that described seed sprouting step is:
Seed is peelled off shell soak 3.5~4.5 hours in 30 ℃ of running water after, and the seed that will shell then binds up with gauze and immerses among 10% liquor natrii hypochloritis, places the sterilization 10 minutes of vibrating on the shaking table; Then the seed that shells is washed with sterile water;
The seed that shells after the above-mentioned flushing is inoculated into according to the ratios that add 20 gram sucrose and 7 gram agar in every liter of MS minimal medium makes and the pH value is on 5.8 the medium; Cultivated 30 hours down prior to the dark condition of 28 ℃ of incubators, treat that 90% above seed base-root exposes after, transfer to again and continue cultivation culturing room's 3000 lux illumination conditions under, cotyledon expansion after 4~5 days.
3, the method for in-vitro breeding indirect regenerated plant of watermelon cotyledon according to claim 2 is characterized in that described callus induction step is: described explant has the cuboid of 3~4 road scalpel cuts for long 0.5cm, wide 0.2cm and surface.
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Cited By (6)
| Publication number | Priority date | Publication date | Assignee | Title |
|---|---|---|---|---|
| CN102047842B (en) * | 2009-11-10 | 2012-07-25 | 东北农业大学 | Method for directly regenerating plants by adopting citrullus lanatus cotyledon nodes |
| CN104304032A (en) * | 2014-11-07 | 2015-01-28 | 四川农业大学 | Method suitable for efficient induction and plant regeneration of multi-genotype watermelon somatic embryos |
| CN104871972A (en) * | 2015-05-18 | 2015-09-02 | 浙江省农业科学院 | High-frequency regeneration system establishment method for effectively controlling watermelon adventitious bud waterlogging phenomenon |
| CN109136259A (en) * | 2018-10-09 | 2019-01-04 | 北京市农林科学院 | A kind of watermelon High-efficient Genetic Transformation and transgenic plant identification method |
| CN109997690A (en) * | 2018-11-15 | 2019-07-12 | 齐齐哈尔大学 | A method of improving watermelon tissue-cultured seedling transplanting survival rate |
| CN112931214A (en) * | 2021-03-30 | 2021-06-11 | 安徽省农业科学院园艺研究所 | Watermelon in-vitro culture method |
-
2006
- 2006-02-24 CN CNB200610049596XA patent/CN100366145C/en not_active Expired - Fee Related
Cited By (7)
| Publication number | Priority date | Publication date | Assignee | Title |
|---|---|---|---|---|
| CN102047842B (en) * | 2009-11-10 | 2012-07-25 | 东北农业大学 | Method for directly regenerating plants by adopting citrullus lanatus cotyledon nodes |
| CN104304032A (en) * | 2014-11-07 | 2015-01-28 | 四川农业大学 | Method suitable for efficient induction and plant regeneration of multi-genotype watermelon somatic embryos |
| CN104304032B (en) * | 2014-11-07 | 2016-07-13 | 四川农业大学 | The Citrullus vulgaris somatic embryo being applicable to polygene type is efficiently induced and plant regeneration method |
| CN104871972A (en) * | 2015-05-18 | 2015-09-02 | 浙江省农业科学院 | High-frequency regeneration system establishment method for effectively controlling watermelon adventitious bud waterlogging phenomenon |
| CN109136259A (en) * | 2018-10-09 | 2019-01-04 | 北京市农林科学院 | A kind of watermelon High-efficient Genetic Transformation and transgenic plant identification method |
| CN109997690A (en) * | 2018-11-15 | 2019-07-12 | 齐齐哈尔大学 | A method of improving watermelon tissue-cultured seedling transplanting survival rate |
| CN112931214A (en) * | 2021-03-30 | 2021-06-11 | 安徽省农业科学院园艺研究所 | Watermelon in-vitro culture method |
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