CN104686324A - Phalaenopsis amabilis anti-browning tissue culture method taking lemon extract as anti-browning culture medium - Google Patents

Phalaenopsis amabilis anti-browning tissue culture method taking lemon extract as anti-browning culture medium Download PDF

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CN104686324A
CN104686324A CN201510064734.0A CN201510064734A CN104686324A CN 104686324 A CN104686324 A CN 104686324A CN 201510064734 A CN201510064734 A CN 201510064734A CN 104686324 A CN104686324 A CN 104686324A
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browning
medium
culture
lemon extract
differentiation
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CN104686324B (en
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项艳
赵康
任洁
沈周高
冯琳
赵华琳
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Anhui Agricultural University AHAU
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Anhui Agricultural University AHAU
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Abstract

The invention discloses a phalaenopsis amabilis anti-browning tissue culture method taking a lemon extract as an anti-browning culture medium. The culture medium comprises a primary culture medium and a proliferation and differentiation culture medium, wherein each of the primary culture medium and the proliferation and differentiation culture medium respectively contains a certain volume of natural lemon extract. The tissue culture method disclosed by the invention comprises the steps of carrying out explant disinfection, carrying out primary culture, carrying out proliferation and differentiation culture, carrying out rooting culture, exercising seedlings, transplanting and the like. According to the tissue culture method, the culture medium containing natural additives is used for playing a role in preventing and treating the common browning problem of phalaenopsis amabilis, and meanwhile, the browning problem of a differentiation stage is prevented and treated in an assisted manner by adopting different cutting manners, so that a combined anti-browning method is formed. The method disclosed by the invention is high in stability and high in success rate, is environment-friendly and can be applied to repeated production annually; the problems of low success rate and no environment-friendliness in the existing methods are solved, so that the method has great practical application significance.

Description

A kind of Moth orchid anti-browning tissue culture method that is anti-browning medium with lemon extract
The application is application number: 201410003340X, and the applying date is: 2013-4-27, and denomination of invention is: the divisional application of a kind of Moth orchid anti-browning tissue culture method and anti-browning medium
Technical field
The present invention relates generally to field of plant tissue culture, specifically a kind of Moth orchid anti-browning tissue culture method and anti-browning medium.
Background technology
Explant browning is the major issue run in Plant Tissue Breeding.There are some researches show, cause the main cause of brownization to act on natural substrate aldehydes matter by polyphenol oxidase and form quinone and cause, browning can be controlled preferably occur by adding antioxidant and adsorbent.
The reason of brownization is produced for these, there are some researches show that active carbon is the effect that can play anti-browning in the early time, because the principle of active carbon anti-browning is the suction-operated of active carbon, and the suction-operated of active carbon own is limited, that is we can not add a large amount of active carbons in every bottle, so the suction-operated of active carbon is in a small amount smaller, once the harmful components of absorption reach capacity, substantially just effect is not had, therefore need to change fresh culture in incubation, and growing of plant is continuous print process, strict demand is had to the inherent subenvironment of cultivating, frequent replaced medium is unfavorable for the nutrient component generation effect in medium, and in switching process, there is the risk of pollution, high-frequency switching can strengthen pollutes dead probability, also just say that the effect of active carbon anti-browning has serious defect.There are some researches show again that illumination is influential to brownization of Initial culture subsequently, result shows, 1000lx and 3000lx light intensity is cultivated can reduce melting brown rate, and the Brown that 2000lx light intensity is cultivated is serious, significant difference.Be not difficult to find that these methods also exist certain defect and incomprehensive and not environmentally, the research for the anti-browning of whole cultivation stage and the anti-browning method of a comparison system is still very few.
Moth orchid has another name called phalaenopsis (Phalaenopsis amabilis), the orchid family (Orchidaceae) phalaenopsis belongs to (Phalaenopsis) perennial herbaceous plant that grows nonparasitically upon another plant, there is the Moth orchid of the title of " cattleya queen ", because its flower shape such as butterfly with different colors dances in the air, beautiful in colour, with a slim and graceful figure, elegant, extremely welcome on flowers market at home and abroad, always be the favorite of consumer.And Moth orchid is except potted plant, being also suitable for especially being used as cut-flower, is the top grade flower material of artistic flower arrangement.
" V31 " is a kind of Moth orchid safflower series, with the Peduncle Length of overlength, and good inflorescence arrangement, the colored shape of the golden mean of the Confucian school and pattern, special flower motif, wins the welcome of the numerous producers and consumer, for many years pursued, be the outstanding person in Moth orchid always.But the brownization problem of orchid in tissue culture procedures is multiple common, almost inevitable, brownization can cause the death of plant, and the plant in namely cultivating can not proceed to cultivate, so prevent brownization from being the problem will doing one's utmost to solve in orchid tissue cultures.
Summary of the invention
The object of the present invention is to provide a kind of Moth orchid anti-browning tissue culture method, the brownization problem that can be occurred Moth orchid tissue culture procedures by the method is improved, and improves survival rate, increases healthy plantlet in vitro quantity thus increases final output.
The present invention also aims to provide a Plants anti-browning tissue culture medium (TCM); This medium can significantly improve to the brownization problem occurred in plant tissue culture process.
Technical solution problem of the present invention adopts following scheme:
One Plants anti-browning group training medium, its feature is, each stage medium is made up of following component:
(1) Initial culture base
6-BA 8.0mg, NAA 0.5mg, marigold extract 175mg, agar 8g, sucrose 30g is added, medium pH=5.6 in often liter of MS minimal medium; Or
6-BA 8.0mg, NAA 0.5mg, lemon extract 150mg, agar 8g, sucrose 30g is added, medium pH=5.6 in often liter of N6 minimal medium; Or
6-BA 8.0mg, NAA 0.5mg, tomato extract solution 300mg, agar 8g, sucrose 30g is added, medium pH=5.6 in often liter of MS minimal medium; Or
BA 8.0mg, NAA 0.5mg, rosemary, Xue MingRosma rinus officinalis extract 110mg, agar 8g, sucrose 30g is added, medium pH=5.6 in often liter of MS minimal medium;
(2) Proliferation, Differentiation medium
6-BA 8.0mg, NAA 0.5, marigold extract 175mg Coconut Juice 150g, agar 8g, sucrose 30g, medium pH=5.6 are added in often liter of B5 minimal medium; Or
+ 6-BA 8.0mg, NAA 0.5mg, lemon extract 150mg, Coconut Juice 150g, agar 8g, sucrose 30g is added, medium pH=5.6 in often liter of N6 minimal medium; Or
6-BA 8.0mg, NAA 0.5mg, tomato extract solution 300mg, Coconut Juice 150g, agar 8g, sucrose 30g is added, medium pH=5.6 in MS minimal medium; Or
6-BA 8.0mg, NAA 0.5mg, rosemary, Xue MingRosma rinus officinalis extract 110mg, Coconut Juice 150g, agar 8g, sucrose 30g, medium pH=5.6 are added in MS minimal medium.
The present invention provides a kind of Moth orchid anti-browning tissue culture method simultaneously, and comprise explant sterilization, Initial culture and Proliferation, Differentiation and cultivate, culture of rootage, hardening and transplanting, its feature is,
Described Initial culture refers to:
The explant of disinfecting is accessed on the Initial culture base described in claim 1,25 ± 1 DEG C, illumination 1500-2000Lx; Light application time is 10-12 hour/day, cultivates 5-6 week;
Described Proliferation, Differentiation is cultivated and is referred to:
By the Proliferation, Differentiation medium described in the tissue access claim 1 that brownization does not occur after Initial culture, 25 ± 1 DEG C, illumination 1500-2000Lx; Light application time is 10-12 hour/day, is cultured to and differentiates seedling.
Described culture of rootage refers to:
The unrooted seedling of the height of seedling 2cm after being cultivated by Proliferation, Differentiation, by every bottle of 1 strain, is inoculated in MS+6-BA 1.0mg/L+NAA 0.2mg/L+ agar 8g/L+ sucrose 30g/L medium, cultivates 2 weeks.
Described hardening refers to:
Seedling after culture of rootage was proceeded to root media again every 25-30 days, 2-3 time so repeatedly; Opened by seedling bottleneck after strong sprout, place 2-3 day in culturing room half shading, period keeps the skin wet in good time, makes plantlet in vitro progressively adapt to external environment, reaches the object of hardening.
Described transplanting refers to:
The sphagna of disinfecting is soaked with clear water, then sloughs moisture unnecessary in sphagna with dewaterer and produce without water droplet to hand-tight the holding of sphagna, stand-by; Be separately dispersion shape by the root system of seedling during transplanting, central filler sphagna, then wrap up whole root system with sphagna, then shoot root portion is immersed in nutrient solution, absorb after nutrient solution until sphagna and carry out Bao Miao again, transplant.
Described explant sterilization refers to:
Cut raw tender leaf then from plant, running water washes away silt, and cleaning solution soaks 10min and removes surface smut, tap water 3h, be placed on superclean bench: the alcoholic solution of volumetric concentration 75% soaks 35s, afterwards aseptic water washing 3 times, then uses the HgCl of volumetric concentration 0.2% 2solution soaks 5-7min, aseptic water washing 8 times, soaks 4-8min afterwards and proceeds in culture dish, blot the Initial culture bases to be accessed such as adhesive water with 500mg/L PVP.
The inventive method tool has the following advantages or effect:
1. the present invention adopts natural additive marigold and lemon to add in medium as additive, first time natural materials is added in medium the effect playing anti-browning, compare with active carbon with traditional chemical reagent, these natural materials are natural pure, environmental protection, utilizes benefit materials contained by additive self to play the effect of anti-browning.
2. the present invention adopts several different minimal medium and natural additive to combine, and have found the assembled scheme of optimized anti-browning, and scheme is unique, can have multiple choices, for the anti-browning in Moth orchid group training process from now on provides thinking and solution.
4. in the present invention's in the end stage, access in the medium not adding anti-browning reagent and normally take root after plantlet in vitro growing way is stablized, few generation brownization, plays cost-saving object.
5. the present invention can play in first generation and breeding the effect preventing brownization, compared with conventional method more comprehensively, the problem of anti-browning is solved from each stage, thus survival rate and the quality of plantlet in vitro is improved, certain facilitation is played to the growth of plantlet in vitro self simultaneously, a large amount of high-quality seedlings can be obtained.
6. the plantlet in vitro melting brown rate in the present invention is low, nutrient health, and warm photosynthetic reason, growing way is vigorous.
Embodiment
Below by way of specific embodiment, technical solution of the present invention is described further.
Following examples MS culture medium prescription: containing KNO in often liter of medium 3(1900mg/L), NH 4nO 3(1650mg/L), MgSO 47H 2o (370mg/L), KH 2pO 4(170mg/L), CaCl 2(330mg/L), KI (0.83mg/L), H 3bO 3(6.2mg/L), MnSO 4h 2o (16.9mg/L), ZnSO 47H 2o (8.6mg/L), CuSO 45H 2o (0.025mg/L), CoCl 26H 2o (0.025mg/L), Na 2moO 42H 2o (0.25mg/L), FeSO 47H 2o (27.85mg/L), Na 2eDTA (37.25mg/L), glycine (2.0mg/L), nicotinic acid B3 (0.5mg/L), thiamine hydrochloride B1 (0.1mg/L), puridoxine hydrochloride B6 (0.5mg/L), inositol (100mg/L).
B5 medium is filled a prescription: KNO 3(2500mg/L), (NH 4) 2sO 4(134mg/L), NaH 2pO 4h 2o (150mg/L), MgSO 47H 2o (250mg/L), CaCl 2(124mg/L), KI (0.75mg/L), H 3bO 3(3mg/L), MnSO 4h 2o (10mg/L), ZnSO 47H 2o (2mg/L), CuSO 45H 2o (0.025mg/L), CoCl 26H 2o (0.025mg/L), Na 2moO 42H 2o (0.25mg/L), FeSO 47H 2o (27.85mg/L), Na 2eDTA (37.25mg/L), nicotinic acid B3 (1mg/L), thiamine hydrochloride B1 (100mg/L), puridoxine hydrochloride B6 (1mg/L), inositol (100mg/L).
N6 culture medium prescription: KNO 3(2830mg/L), (NH 4) 2sO 4(463mg/L), MgSO 47H 2o (185mg/L), KH 2pO 4(400mg/L), CaCl 2(125mg/L), KI (0.8mg/L), H 3bO 3(1.6mg/L), MnSO 4h 2o (3.3mg/L), ZnSO 47H 2o (1.5mg/L), FeSO 47H 2o (27.85mg/L), Na 2eDTA (37.25mg/L), glycine (2.0mg/L), nicotinic acid B3 (0.5mg/L), thiamine hydrochloride B1 (1mg/L), puridoxine hydrochloride B6 (0.5mg/L).
Moth orchid anti-browning tissue culture method comprises the following steps:
(1) selection of explant and the preparation of natural additive and sterilizing
Choose the tender leaf of giving birth to then in tender leaf or plantlet in vitro, raw tender leaf needs through following sterilization process then: cut from plant, running water washes away silt, washing agent immersion bubble 10min also brushes away surface smut gently with soft brush, tap water 3h, be placed on superclean bench: the alcoholic solution of volumetric concentration 75% soaks 35s, afterwards aseptic water washing 3 times, then uses the HgCl of volumetric concentration 0.2% 2solution soaks 7min, aseptic water washing 8 times, to proceed in culture dish the medium to be accessed such as suck dry moisture afterwards with 500mg/L PVP immersion 6min; Employ the Disinfection Effect after PVP (polyvinylpyrrolidone) and improve 4 times than the solution sterile rate originally do not used.
To choose plantlet in vitro be explant is that not need the process through sterilization to be directly placed in superclean bench stand-by.
The natural additive that the present invention chooses is marigold, lemon, tomato, rosemary, Xue MingRosma rinus officinalis, needs to be prepared into sterile solution in advance.The marigold chosen shortly past viewing period is taken flower and cleans, squeeze juice, by juice solids removed by filtration residue, then filters to make in medium that the sterilizing to be added of aseptic extract completes in superclean bench with sterilizing filter and uses.Band epidermis lemon squeeze juice, by juice solids removed by filtration residue, then filters to make in medium that the sterilizing to be added of aseptic extract completes with sterilizing filter and uses in superclean bench.Band epidermis tomato squeeze juice, filters juice, then filters to make in medium that the sterilizing to be added of aseptic extract completes in superclean bench with sterilizing filter and use.Rosemary, Xue MingRosma rinus officinalis plant puts into the first boiling water boiling 0.5h of water, then keeps water temperature 90 ° to boil 2.5h, by juice solids removed by filtration residue, then filters to make in medium that the sterilizing to be added of aseptic extract completes in superclean bench with sterilizing filter and uses.
(2) Initial culture
The blade handled well is cut to the fritter of normal 0.5cm*0.5cm, or again the fritter of 0.5cm*0.5cm is laterally cut into small pieces from centre again; By in each medium in above-mentioned fritter access table 1, at 25 ± 1 DEG C, illumination 1500-2000Lx; Cultivate under the condition of light application time 10-12 hour/day, often organize medium treatment and divide 3 repetitions, each process 9 bottles.Average melting brown rate result (cultivating 6 weeks) in 6 weeks is as shown in table 1, brownization does not wherein occur in 2 weeks in the 3rd, 9,12,30 4 group, in 6 weeks, average melting brown rate is less than 5.
Table 1 Initial culture base
Often kind of medium all adds 6-BA 8.0mg/L+NAA 0.5mg/L+ agar 8g/L+ sucrose 30g/L, pH=5.6.
(3) Proliferation, Differentiation is cultivated
Cultivate in each increment differential medium do not occurred in the tissue access table 2 of brownization, condition of culture: 25 ± 1 DEG C, illumination 1500-2000Lx; Light application time is 10-12 hour/day, and wherein the 3rd, 4,5,10 group brownization did not occur in 3 weeks, and the average melting brown rate in 6 weeks is lower than 3%, and the rate of increase improves more than 5 times, differentiation cycle time 8d.
Table 2 Proliferation, Differentiation medium
Often kind of medium all adds 6-BA 8.0mg/L+NAA 0.5mg/L+ agar 8g/L+ sucrose 30g/L, pH=5.6.Often group process is all repeat for 3 times, each process 9 bottles.
(4) culture of rootage
Get the unrooted seedling of height of seedling 2cm, by every bottle of 1 strain, be inoculated in MS+6-BA 1.0mg/L+NAA 0.2mg/L+ agar 8g/L+ sucrose 30g/L medium, in 2 weeks, grow 4-6 bar root, in 6 weeks, under the condition not using anti-browning reagent, brownization does not occur.
(5) hardening and transplanting
Seedling after taking root proceeded to root media again every 25-30 days, 2-3 time so repeatedly, and such seedling is superior in quality, can stand the impact that external environment is brought.Opened by seedling bottleneck after strong sprout, place 2-3 day in culturing room half shading, period keeps the skin wet in good time, makes plantlet in vitro progressively adapt to external environment, reaches the object of hardening.
The sphagna of disinfecting is soaked with clear water, then with dewaterer slough moisture unnecessary in sphagna (sphagna degree of dehydration with hand-tight hold without water droplet be produced as should), stand-by.Be separately dispersion shape by the root system of seedling during transplanting, the a little sphagna of central filler, wrap up whole root system with sphagna again, then seedling is sent in nutritive cube (nutritive cube nutrient solution is the solution that the mother liquor of MS medium dilutes after 10 times), sphagna is gently pressed onto the underwater of nutritive cube.Bag Miao Shiyao accomplishes that degree of tightness is suitable for.First by populated with sphagna for cave dish, then can dig 1 duck eye with tweezers in the middle of the dish of each cave, seedling root system put into wherein, gently presses.3000-4000 times of bactericide to be sprayed after transplanting in time and carry out prevention process.After general cultivation 3 ~ 5 days without the need to watering, but suitably should increase air humidity.
In the inventive method, employ several minimal medium, several basic cultivation and natural interpolation are combined and has carried out full friendship experimental design, the experiment effect that many-sided consideration is final, the effect of self of natural additive is played greatly at utmost, also solve each stage be all applicable to use problem, the growth of plantlet in vitro can also be promoted while anti-browning.

Claims (6)

1. with lemon extract for an anti-browning medium, it is characterized in that, each stage medium is made up of following component:
(1) Initial culture base
6-BA 8.0mg, NAA 0.5mg, lemon extract 150mg, agar 8g, sucrose 30g is added, medium pH=5.6 in often liter of N6 minimal medium; Or
(2) Proliferation, Differentiation medium
+ 6-BA 8.0mg, NAA 0.5mg, lemon extract 150mg, Coconut Juice 150g, agar 8g, sucrose 30g is added, medium pH=5.6 in often liter of N6 minimal medium.
2., with the Moth orchid anti-browning tissue culture method that lemon extract is anti-browning medium, comprise explant sterilization, Initial culture and Proliferation, Differentiation and cultivate, culture of rootage, hardening and transplanting, is characterized in that,
Described Initial culture refers to:
The explant of disinfecting is accessed on the Initial culture base described in claim 1,25 ± 1 DEG C, illumination 1500-2000Lx; Light application time is 10-12 hour/day, cultivates 5-6 week;
Described Proliferation, Differentiation is cultivated and is referred to:
By the Proliferation, Differentiation medium described in the tissue access claim 1 that brownization does not occur after Initial culture, 25 ± 1 DEG C, illumination 1500-2000Lx; Light application time is 10-12 hour/day, is cultured to and differentiates seedling.
3. a kind of Moth orchid anti-browning tissue culture method that is anti-browning medium with lemon extract according to claim 2, is characterized in that: described culture of rootage refers to:
The unrooted seedling of the height of seedling 2cm after being cultivated by Proliferation, Differentiation, by every bottle of 1 strain, is inoculated in MS+6-BA 1.0mg/L+NAA 0.2mg/L+ agar 8g/L+ sucrose 30g/L medium, cultivates 2 weeks.
4. the Moth orchid anti-browning tissue culture method that a kind of described in Claims 2 or 3 is anti-browning medium with lemon extract, is characterized in that: described hardening refers to:
Seedling after culture of rootage was proceeded to root media again every 25-30 days, 2-3 time so repeatedly; Opened by seedling bottleneck after strong sprout, place 2-3 day in culturing room half shading, period keeps the skin wet in good time, makes plantlet in vitro progressively adapt to external environment, reaches the object of hardening.
5. a kind of Moth orchid anti-browning tissue culture method that is anti-browning medium with lemon extract according to claim 4, is characterized in that: described transplanting refers to:
The sphagna of disinfecting is soaked with clear water, then sloughs moisture unnecessary in sphagna with dewaterer and produce without water droplet to hand-tight the holding of sphagna, stand-by; Be separately dispersion shape by the root system of seedling during transplanting, central filler sphagna, then wrap up whole root system with sphagna, then shoot root portion is immersed in nutrient solution, absorb after nutrient solution until sphagna and carry out Bao Miao again, transplant.
6. a kind of Moth orchid anti-browning tissue culture method that is anti-browning medium with lemon extract according to claim 2, is characterized in that: described explant sterilization refers to:
Cut raw tender leaf then from plant, running water washes away silt, and cleaning solution soaks 10min and removes surface smut, tap water 3h, is placed on superclean bench, and the alcoholic solution of volumetric concentration 75% soaks 35s, aseptic water washing 3 times afterwards, then use the HgCl of volumetric concentration 0.2% 2solution soaks 5-7min, aseptic water washing 8 times, soaks 4-8min afterwards and proceeds in culture dish, blot the Initial culture bases to be accessed such as adhesive water with 500mg/L PVP.
CN201510064734.0A 2013-04-28 2013-04-28 A kind of be anti-browning culture medium with Fructus Citri Limoniae extract iris anti-browning tissue culture method Expired - Fee Related CN104686324B (en)

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