CN102823503A - Tissue culture medium for propagating anthurium buds by using buds - Google Patents
Tissue culture medium for propagating anthurium buds by using buds Download PDFInfo
- Publication number
- CN102823503A CN102823503A CN2012103633492A CN201210363349A CN102823503A CN 102823503 A CN102823503 A CN 102823503A CN 2012103633492 A CN2012103633492 A CN 2012103633492A CN 201210363349 A CN201210363349 A CN 201210363349A CN 102823503 A CN102823503 A CN 102823503A
- Authority
- CN
- China
- Prior art keywords
- bud
- medium
- buds
- culture medium
- tissue culture
- Prior art date
- Legal status (The legal status is an assumption and is not a legal conclusion. Google has not performed a legal analysis and makes no representation as to the accuracy of the status listed.)
- Granted
Links
Landscapes
- Hydroponics (AREA)
- Micro-Organisms Or Cultivation Processes Thereof (AREA)
- Breeding Of Plants And Reproduction By Means Of Culturing (AREA)
Abstract
The invention discloses a tissue culture medium for propagating anthurium buds by using buds. The culture medium comprises a subculture medium and a rooting medium. The tissue culture medium adopts direct induction of germ-free buds and proliferation and propagation instead of callus dedifferentiation for the first time. Compared with the callus dedifferentiation, the technique can be used for fast and easily obtaining germ-free buds, can avoid variation occurred during subculture proliferation, guarantees the grade and quality of seedlings, and is beneficial to storage and production utilization of germplasm resources.
Description
Technical field
The present invention relates to tissue culture medium (TCM), relate in particular to a kind of red palm with the numerous bud culture medium for tissue culture of bud.
Background technology
The red palm (anthurium) has another name called that the peace ancestral spends, fiery crane flower etc., belongs to the Araeceae Anthurium, originates in the tropical rain forest area of South America, and all there is extensive cultivation in existing Europe, Asia, Africa.Characteristic is the warm chilly of happiness, the wet fearness drought of happiness, and happiness the moon is avoided solarization.Its flower is unique, and spadix is arranged, and is bright in colour magnificent, rich color, and leaf bract, common bract color has redness, pink, white etc., and great ornamental value is arranged.The breeding of methods such as available sowing, plant division.The flower language of the red palm be ride on the crest of success, enthusiasm, warm blood.
The red palm is important tropical cut-flower, spadix, and its Buddhist flame petal is very large, plump tool wax, that color and luster has is red, powder, white, green, double-colored etc.Its lovely luster, appearance is peculiar, applied range, economic worth is high, is present global evolution is fast, demand is bigger high-grade tropical cut-flower and pot flowers.The tropical rain forest in red palm original producton location, the available seminal propagation of the red palm, but it is long to get into flowering time.Division propagation is the red palm main mode of breeding in the past.Red palm plant base portion grows the suction bud, but plant division behind the generation root system, can divide the 3-4 strain every year, and reproduction coefficient is lower, is difficult to satisfy the required seedling of large-scale production.The quick breeding of seedling, the just clone technology of the red palm are mainly carried out in the production of present red palm seedling through tissue culture.Like this can be in the relatively short time high quality seedling of production neat and consistent, the needs that supply is produced.Through tissue culture technique sport technique segment such as produce foundation, enrichment culture, strengthening seedling and rooting that red palm seedling mainly contains regenerating system, transplant and nurse young plants in hothouses.
The domestic and international at present research report to red palm tissue culture all is to carry out callus induction with organs such as blade, petiole, stem sections; And then evoked callus differentiation indefinite bud; Variation appears in indefinite bud easily that obtain through this approach in breeding, influenced seedling original excellent genetic character.And be directly to induce stem section differentiation lateral bud with the mode of the numerous bud of bud, induce lateral bud differentiation indefinite bud to breed again, the indefinite bud that obtains through this approach can effectively be avoided the variation that occurs in the shoot proliferation process, keeps maternal plant original excellent proterties better.
Summary of the invention
The objective of the invention is to overcome the deficiency of prior art, provide a kind of red palm with the numerous bud culture medium for tissue culture of bud, this medium comprises subculture medium and root media, wherein:
Component and each components contents of every liter of (L) subculture medium are following:
(1) macroelement: potassium nitrate 1800mg/L, ammonium nitrate 1350mg/L, calcium chloride dihydrate 350mg/L, epsom salt 320mg/L, potassium dihydrogen phosphate 150mg/L, ferrous sulfate heptahydrate 27.5mg/L, disodium ethylene diamine tetraacetate 37.3mg/L;
(2) trace element: four water manganese sulphate 21.5mg/L, white vitriol 8.3mg/L, boric acid 6.0mg/L, Sodium Molybdate Dihydrate 0.2mg/L, KI 0.83mg/L, cupric sulfate pentahydrate 0.02mg/L, CoCL2 0.02mg/L;
(3) organic matter: inositol 80.0mg/L, glycine 2.5mg/L, vitamin b3 (VB
2) 6.0mg/L, puridoxine hydrochloride (VB
6) 0.45mg/L, nicotinic acid 0.45mg/L, thiamine hydrochloride (VB
1) 0.1mg/L;
(4) plant growth regulator: 6-benzyladenine 0.5-2.0mg/L, methyl 0.2-0.8mg/L;
Surplus is a distilled water.
Component and each components contents of every liter of (L) root media are following:
(1) macroelement: potassium nitrate 900mg/L, ammonium nitrate 675mg/L, calcium chloride dihydrate 175mg/L, epsom salt 160mg/L, potassium dihydrogen phosphate 75mg/L, disodium ethylene diamine tetraacetate 37.3mg/L, ferrous sulfate heptahydrate 27.5mg/L;
(2) trace element: four water manganese sulphate 21.5mg/L, white vitriol 8.3mg/L, boric acid 6mg/L, KI 0.83mg/L, Sodium Molybdate Dihydrate 0.2mg/L, cupric sulfate pentahydrate 0.02mg/L, CoCL2 0.02mg/L;
(3) organic matter: inositol 80.0mg/L, glycine 2.5mg/L, thiamine hydrochloride (VB
1) 0.1mg/L, puridoxine hydrochloride (VB
6) 0.45mg/L, nicotinic acid 0.45mg/L;
(4) plant growth regulator: methyl 0.3-0.6mg/L;
Surplus is a distilled water.
The red palm of the present invention with the subculture in the numerous bud culture medium for tissue culture of bud, the compound method of root media is:
The preparation of 1 mother liquor and preservation
1.1 for ease of sampling, the various mother liquors of suitable preparation earlier are divided into macroelement mother liquor, micro-mother liquor, organic matter mother liquor and each plant growth regulators mother liquor.Sucrose, agar should not be made into mother liquor, directly claim appearance when needing;
1.2 the macroelement mother liquid concentration becomes 100 times of solution, organic matter, micro-mother liquor are made into 200 times of solution, and the concentration of plant growth regulating reagent mother liquor is made into 1mg/ml;
1.3 mother liquor is selected aseptic distilled water, deionized water or ultra-pure water preparation for use, uses the water that boiled when producing in a large number;
1.4 during preparation macroelement mother liquor, each component should be dissolved separately, mix by the order of nitrogen, calcium, magnesium, phosphorus one by one the back, otherwise cause deposition easily;
1.5 trace element, organic matter, plant growth regulator mother liquor are used brown bottle and are installed and place refrigerator to preserve;
1.6 should in time use after the mother liquor preparation, period of storage should not be above 1 month;
1.7 find that mother liquor has deposition, or growth of microorganism arranged, or algal grown is arranged, should pass into disuse.
2 culture medium preparation
2.1, measure various mother liquors in proportion according to culture medium prescription;
2.2 in dosing container, put into about pure water more than 1/2 of preparing the preparing culture medium total amount, and add an amount of sugar, add the mother liquor of aequum then while stirring one by one;
But 2.3 add after the agar heat fused, also can directly add agar powder during if any mixing plant, supply the total amount of required preparing culture medium then with pure water, stirring gets final product;
2.4 the sugar in the medium, in a large amount of tissue cultivating seedling are produced, general available commercially available white sugar, but preferably garden beet is not sugared with sucrose;
2.5 regulate the pH value to 5.8 of medium with the sodium hydroxide of the hydrochloric acid of 1.0 mol or 1.0 mol;
2.6 will dividing as early as possible, prepared culture medium installs in the culture vessel, in order to avoid culture medium solidifying or retrogradation and be difficult to packing;
2.7 should note during the packing medium avoiding medium to be bonded on the bottleneck,, before lid bottle cap or bottle stopper, must clean bottleneck with clean gauze if be stained with medium.
3 medium sterilizations
3.1 being loaded in the high-pressure sterilizing pot, the medium that branch is installed sterilizes;
3.2 the heating initial stage when the air pressure of sterilizing pan disinfection room reaches 0.05Mpa, is opened condensation trap, drains cold air in the disinfection room;
3.3, keep temperature and pressure sterilization 15-20 minute when the disinfection room internal gas pressure reaches 0.11Mpa, when temperature reaches 121 ℃, picks up counting;
3.4 close the heating power supply switch, by slow exhaust mode discharging hot gas, when reducing to atmospheric pressure, opens indoor air pressure to be sterilized sterilization pot cover or door, take out medium;
3.5 medium should place little air to flow and the clean environment cooling of few dust, cultivates vessel otherwise in the cooling intake process, cause mycotic spore to get into, and produces mould contamination.
4 medium storage
4.1 medium should be joined existing usefulness as far as possible at present;
4.2 can be at air clean and immobilising environment short time storage medium, should pass into disuse but storage surpasses 1 month medium.
The red palm of the present invention with the method for the numerous bud tissue culture of bud is:
1. bud induces
As explant, cut off blade in the tender stem of the red palm of fine clip robust growth, no damage by disease and insect, clean 1-2 time with the water that is added with a little liquid detergent; And scrub internode gently with banister brush; Rinse well with flowing water again, then on superclean bench with the stem section with 75% alcohol disinfecting 30 seconds, aseptic water washing 3 times; Again with 0.1% mercuric chloride sterilization 10min, aseptic water washing 5~6 times.The material that has disinfected is cut into the sections that has 1-2 lateral bud, and base portion is inoculated in downwards in the medium of induced bud then.When explant is cultivated for the first time, need secretly cultivate about 10 days entirely, be put under the low light level again and cultivate, about cultivation stem section through about 20 days can induce sprouting, and then moves to the place cultivation of seeing light.
2. the enrichment culture of bud
The sprouting of inducing acquisition is seeded to induces the differentiation bud of growing thickly to carry out the shoot proliferation of bud on the subculture medium, general 40 days subcultures once, the subculture material all is placed on the cultivation indoor cultivation, culturing room's temperature is (25 ± 2) ℃, illumination 12h.d
-1, illuminance 1500lx.
3. what take root induces
When budling grows to moon 2.0cm, will go to root induction on the root media by single cutting-out on the bud of growing thickly than healthy and strong bud seedling, all the other bud seedlings go to and proceed enrichment culture on the subculture medium.Culture of rootage need be cultivated under the low light level about 10 days, and this moment, the base portion of seedling formed white projection, and elongation gradually, can form obvious young root after 15 days, grew up to complete plantlet gradually, should progressively increase illumination this period and make seedling become sturdy.
4. the take root transplanting of seedling
The abundant lignification of seedling of waiting to take root, blade is unfolded, and the leaf look dark green, and the caulom elongation can be carried out the booth transplanting during the about 3.0cm of height of seedling.Take out earlier seedling during transplanting, clean the medium of base portion after, transplant on the usefulness of sterilizing through 0.1% potassium permanganate is grown seedlings the good seedling medium of support; About 100-120 strain seedling is transplanted in every holder, irrigates normal root water, keeps certain temperature and humidity; Temperature is controlled at 25 ℃ ± 5 ℃, humidity about 70%, matrix see dried see wet for well; Too wet meeting causes mashed root, and it is withered that blade appears in too dried meeting, and will regularly spray medicine and carry out diseases prevention and handle.
Advantage of the present invention is:
1, adopts first without the callus dedifferentiation; Directly induce aseptic bud and expand numerous propagation with the numerous bud of bud; This technology than obtain through callus aseptic bud material sooner, easier; And can effectively avoid the variation that occurs in the shoot proliferation process, and guaranteed the quality and the quality of seedling, help germ plasm resource and preserve and produce and utilize;
2, carry out the red palm with the numerous bud enrichment culture of bud with subculture medium, summer, cultivation temperature remained on 25-28 ℃, and winter, cultivation temperature kept about 20 ℃, and the subculture seedling moon is bred 3.8 times, and a year reproduction coefficient is 3.8
12, it is many that the subculture seedling directly breaks up bud, and bud is healthy and strong, and growth is neat, and the leaf look dark green;
3, cultivate rooting rate and reach 99% with the root media seedling of taking root, when temperature is 25-28 ℃, can go out root about 15 days, well developed root system, on average going out the root amount has the 6-8 bar, can transplant in 30 days, and transplanting survival rate reaches 95.5%.
Embodiment
With embodiment the present invention is described further below, but the present invention is not limited to these embodiment.
Embodiment 1:
The red palm is with the numerous bud culture medium for tissue culture of bud, and this medium comprises subculture medium and root media, wherein:
Component and each components contents of every liter of (L) subculture medium are following:
(1) macroelement: potassium nitrate 1800mg/L, ammonium nitrate 1350mg/L, calcium chloride dihydrate 350mg/L, epsom salt 320mg/L, potassium dihydrogen phosphate 150mg/L, ferrous sulfate heptahydrate 27.5mg/L, disodium ethylene diamine tetraacetate 37.3mg/L;
(2) trace element: four water manganese sulphate 21.5mg/L, white vitriol 8.3mg/L, boric acid 6.0mg/L, Sodium Molybdate Dihydrate 0.2mg/L, KI 0.83mg/L, cupric sulfate pentahydrate 0.02mg/L, CoCL2 0.02mg/L;
(3) organic matter: inositol 80.0mg/L, glycine 2.5mg/L, vitamin b3 (VB
2) 6.0mg/L, puridoxine hydrochloride (VB
6) 0.45mg/L, nicotinic acid 0.45mg/L, thiamine hydrochloride (VB
1) 0.1mg/L;
(4) plant growth regulator: 6-benzyladenine 0.5mg/L, methyl 0.2mg/L;
Surplus is a distilled water.
Component and each components contents of every liter of (L) root media are following:
(1) macroelement: potassium nitrate 900mg/L, ammonium nitrate 675mg/L, calcium chloride dihydrate 175mg/L, epsom salt 160mg/L, potassium dihydrogen phosphate 75mg/L, disodium ethylene diamine tetraacetate 37.3mg/L, ferrous sulfate heptahydrate 27.5mg/L;
(2) trace element: four water manganese sulphate 21.5mg/L, white vitriol 8.3mg/L, boric acid 6mg/L, KI 0.83mg/L, Sodium Molybdate Dihydrate 0.2mg/L, cupric sulfate pentahydrate 0.02mg/L, CoCL2 0.02mg/L;
(3) organic matter: inositol 80.0mg/L, glycine 2.5mg/L, thiamine hydrochloride (VB
1) 0.1mg/L, puridoxine hydrochloride (VB
6) 0.45mg/L, nicotinic acid 0.45mg/L;
(4) plant growth regulator: methyl 0.3mg/L;
Surplus is a distilled water.
Embodiment 2:
The red palm is with the numerous bud culture medium for tissue culture of bud, and this medium comprises subculture medium and root media, wherein:
Component and each components contents of every liter of (L) subculture medium are following:
(1) macroelement: potassium nitrate 1800mg/L, ammonium nitrate 1350mg/L, calcium chloride dihydrate 350mg/L, epsom salt 320mg/L, potassium dihydrogen phosphate 150mg/L, ferrous sulfate heptahydrate 27.5mg/L, disodium ethylene diamine tetraacetate 37.3mg/L;
(2) trace element: four water manganese sulphate 21.5mg/L, white vitriol 8.3mg/L, boric acid 6.0mg/L, Sodium Molybdate Dihydrate 0.2mg/L, KI 0.83mg/L, cupric sulfate pentahydrate 0.02mg/L, CoCL2 0.02mg/L;
(3) organic matter: inositol 80.0mg/L, glycine 2.5mg/L, vitamin b3 (VB
2) 6.0mg/L, puridoxine hydrochloride (VB
6) 0.45mg/L, nicotinic acid 0.45mg/L, thiamine hydrochloride (VB
1) 0.1mg/L;
(4) plant growth regulator: 6-benzyladenine 2.0mg/L, methyl 0.8mg/L;
Surplus is a distilled water.
Component and each components contents of every liter of (L) root media are following:
(1) macroelement: potassium nitrate 900mg/L, ammonium nitrate 675mg/L, calcium chloride dihydrate 175mg/L, epsom salt 160mg/L, potassium dihydrogen phosphate 75mg/L, disodium ethylene diamine tetraacetate 37.3mg/L, ferrous sulfate heptahydrate 27.5mg/L;
(2) trace element: four water manganese sulphate 21.5mg/L, white vitriol 8.3mg/L, boric acid 6mg/L, KI 0.83mg/L, Sodium Molybdate Dihydrate 0.2mg/L, cupric sulfate pentahydrate 0.02mg/L, CoCL2 0.02mg/L;
(3) organic matter: inositol 80.0mg/L, glycine 2.5mg/L, thiamine hydrochloride (VB
1) 0.1mg/L, puridoxine hydrochloride (VB
6) 0.45mg/L, nicotinic acid 0.45mg/L;
(4) plant growth regulator: methyl 0.6mg/L;
Surplus is a distilled water.
Embodiment 3:
The red palm is with the numerous bud culture medium for tissue culture of bud, and this medium comprises subculture medium and root media, wherein:
Component and each components contents of every liter of (L) subculture medium are following:
(1) macroelement: potassium nitrate 1800mg/L, ammonium nitrate 1350mg/L, calcium chloride dihydrate 350mg/L, epsom salt 320mg/L, potassium dihydrogen phosphate 150mg/L, ferrous sulfate heptahydrate 27.5mg/L, disodium ethylene diamine tetraacetate 37.3mg/L;
(2) trace element: four water manganese sulphate 21.5mg/L, white vitriol 8.3mg/L, boric acid 6.0mg/L, Sodium Molybdate Dihydrate 0.2mg/L, KI 0.83mg/L, cupric sulfate pentahydrate 0.02mg/L, CoCL2 0.02mg/L;
(3) organic matter: inositol 80.0mg/L, glycine 2.5mg/L, vitamin b3 (VB
2) 6.0mg/L, puridoxine hydrochloride (VB
6) 0.45mg/L, nicotinic acid 0.45mg/L, thiamine hydrochloride (VB
1) 0.1mg/L;
(4) plant growth regulator: 6-benzyladenine 0.5mg/L, methyl 0.2mg/L;
Surplus is a distilled water.
Component and each components contents of every liter of (L) root media are following:
(1) macroelement: potassium nitrate 900mg/L, ammonium nitrate 675mg/L, calcium chloride dihydrate 175mg/L, epsom salt 160mg/L, potassium dihydrogen phosphate 75mg/L, disodium ethylene diamine tetraacetate 37.3mg/L, ferrous sulfate heptahydrate 27.5mg/L;
(2) trace element: four water manganese sulphate 21.5mg/L, white vitriol 8.3mg/L, boric acid 6mg/L, KI 0.83mg/L, Sodium Molybdate Dihydrate 0.2mg/L, cupric sulfate pentahydrate 0.02mg/L, CoCL2 0.02mg/L;
(3) organic matter: inositol 80.0mg/L, glycine 2.5mg/L, thiamine hydrochloride (VB
1) 0.1mg/L, puridoxine hydrochloride (VB
6) 0.45mg/L, nicotinic acid 0.45mg/L;
(4) plant growth regulator: methyl 0.3mg/L;
Surplus is a distilled water.
Embodiment 4:
The red palm is with the numerous bud culture medium for tissue culture of bud, and this medium comprises subculture medium and root media, wherein:
Component and each components contents of every liter of (L) subculture medium are following:
(1) macroelement: potassium nitrate 1800mg/L, ammonium nitrate 1350mg/L, calcium chloride dihydrate 350mg/L, epsom salt 320mg/L, potassium dihydrogen phosphate 150mg/L, ferrous sulfate heptahydrate 27.5mg/L, disodium ethylene diamine tetraacetate 37.3mg/L;
(2) trace element: four water manganese sulphate 21.5mg/L, white vitriol 8.3mg/L, boric acid 6.0mg/L, Sodium Molybdate Dihydrate 0.2mg/L, KI 0.83mg/L, cupric sulfate pentahydrate 0.02mg/L, CoCL2 0.02mg/L;
(3) organic matter: inositol 80.0mg/L, glycine 2.5mg/L, vitamin b3 (VB
2) VB
26.0mg/L, puridoxine hydrochloride (VB
6) 0.45mg/L, nicotinic acid 0.45mg/L, thiamine hydrochloride (VB
1) 0.1mg/L;
(4) plant growth regulator: 6-benzyladenine 2.0mg/L, methyl 0.8mg/L;
Surplus is a distilled water.
Component and each components contents of every liter of (L) root media are following:
(1) macroelement: potassium nitrate 900mg/L, ammonium nitrate 675mg/L, calcium chloride dihydrate 175mg/L, epsom salt 160mg/L, potassium dihydrogen phosphate 75mg/L, disodium ethylene diamine tetraacetate 37.3mg/L, ferrous sulfate heptahydrate 27.5mg/L;
(2) trace element: four water manganese sulphate 21.5mg/L, white vitriol 8.3mg/L, boric acid 6mg/L, KI 0.83mg/L, Sodium Molybdate Dihydrate 0.2mg/L, cupric sulfate pentahydrate 0.02mg/L, CoCL2 0.02mg/L;
(3) organic matter: inositol 80.0mg/L, glycine 2.5mg/L, thiamine hydrochloride (VB
1) 0.1mg/L, puridoxine hydrochloride (VB
6) 0.45mg/L, nicotinic acid 0.45mg/L;
(4) plant growth regulator: methyl 0.6mg/L;
Surplus is a distilled water.
Comparative Examples:
Obtain the medium of aseptic bud through callus, this medium comprises inducing culture, subculture medium and root media, wherein:
Component and each components contents of every liter of (L) inducing culture are following:
(1) macroelement: potassium nitrate 1900mg/L, ammonium nitrate 1650mg/L, calcium chloride dihydrate 400mg/L, epsom salt 370mg/L, potassium dihydrogen phosphate 170mg/L, ferrous sulfate heptahydrate 27.5mg/L, disodium ethylene diamine tetraacetate 37.3mg/L;
(2) trace element: four water manganese sulphate 22.3mg/L, white vitriol 8.6mg/L, boric acid 6.2mg/L, Sodium Molybdate Dihydrate 0.25mg/L, KI 0.83mg/L, cupric sulfate pentahydrate 0.025mg/L, CoCL2 0.025mg/L;
(3) organic matter: inositol 100.0mg/L, glycine 2.0mg/L, puridoxine hydrochloride (VB
6) 0.5mg/L, nicotinic acid 0.5mg/L, thiamine hydrochloride (VB
1) 0.1mg/L;
(4) plant growth regulator: 6-benzyladenine 0.8-1.2mg/L, 2,4 dichlorophenoxyacetic acid (2,4-D) 0.1-0.2mg/L;
Component and each components contents of every liter of (L) subculture medium are following:
(1) macroelement: potassium nitrate 1900mg/L, ammonium nitrate 1650mg/L, calcium chloride dihydrate 400mg/L, epsom salt 370mg/L, potassium dihydrogen phosphate 170mg/L, ferrous sulfate heptahydrate 27.5mg/L, disodium ethylene diamine tetraacetate 37.3mg/L;
(2) trace element: four water manganese sulphate 22.3mg/L, white vitriol 8.6mg/L, boric acid 6.2mg/L, Sodium Molybdate Dihydrate 0.25mg/L, KI 0.83mg/L, cupric sulfate pentahydrate 0.025mg/L, CoCL2 0.025mg/L;
(3) organic matter: inositol 100.0mg/L, glycine 2.0mg/L, puridoxine hydrochloride (VB
6) 0.5mg/L, nicotinic acid 0.5mg/L, thiamine hydrochloride (VB
1) 0.1mg/L;
(4) plant growth regulator: 6-benzyladenine 1.5-2.0mg/L, kinetin (KT) 0.5-1.0mg/L;
Surplus is a distilled water.
Component and each components contents of every liter of (L) root media are following:
(1) macroelement: potassium nitrate 950mg/L, ammonium nitrate 825mg/L, calcium chloride dihydrate 200mg/L, epsom salt 185mg/L, potassium dihydrogen phosphate 85mg/L, disodium ethylene diamine tetraacetate 37.3mg/L, ferrous sulfate heptahydrate 27.5mg/L;
(2) trace element: four water manganese sulphate 21.5mg/L, white vitriol 8.3mg/L, boric acid 6mg/L, KI 0.83mg/L, Sodium Molybdate Dihydrate 0.2mg/L, cupric sulfate pentahydrate 0.02mg/L, CoCL2 0.02mg/L;
(3) organic matter: inositol 80.0mg/L, glycine 2.5mg/L, thiamine hydrochloride (VB
1) 0.1mg/L, puridoxine hydrochloride (VB
6) 0.45mg/L, nicotinic acid 0.45mg/L;
(4) plant growth regulator: methyl 0.3-0.6mg/L;
Surplus is a distilled water.
The medium that utilizes the foregoing description 1 and Comparative Examples to process carries out tissue culture to the red palm, can find out that from the result of following table the technical indicator of embodiment far surpasses Comparative Examples.
Claims (2)
1. a red palm is with the numerous bud culture medium for tissue culture of bud, and this medium comprises subculture medium and root media, it is characterized in that:
Component and each components contents of every liter of (L) subculture medium are following:
(1) macroelement: potassium nitrate 1800mg/L, ammonium nitrate 1350mg/L, calcium chloride dihydrate 350mg/L, epsom salt 320mg/L, potassium dihydrogen phosphate 150mg/L, ferrous sulfate heptahydrate 27.5mg/L, disodium ethylene diamine tetraacetate 37.3mg/L;
(2) trace element: four water manganese sulphate 21.5mg/L, white vitriol 8.3mg/L, boric acid 6.0mg/L, Sodium Molybdate Dihydrate 0.2mg/L, KI 0.83mg/L, cupric sulfate pentahydrate 0.02mg/L, CoCL2 0.02mg/L;
(3) organic matter: inositol 80.0mg/L, glycine 2.5mg/L, vitamin b3 (VB
2) 6.0mg/L, puridoxine hydrochloride (VB
6) 0.45mg/L, nicotinic acid 0.45mg/L, thiamine hydrochloride (VB
1) 0.1mg/L;
(4) plant growth regulator: 6-benzyladenine 0.5-2.0mg/L, methyl 0.2-0.8mg/L;
Surplus is a distilled water.
2. the red palm according to claim 1 is characterized in that with the numerous bud culture medium for tissue culture of bud:
Component and each components contents of every liter of (L) root media are following:
(1) macroelement: potassium nitrate 900mg/L, ammonium nitrate 675mg/L, calcium chloride dihydrate 175mg/L, epsom salt 160mg/L, potassium dihydrogen phosphate 75mg/L, disodium ethylene diamine tetraacetate 37.3mg/L, ferrous sulfate heptahydrate 27.5mg/L;
(2) trace element: four water manganese sulphate 21.5mg/L, white vitriol 8.3mg/L, boric acid 6mg/L, KI 0.83mg/L, Sodium Molybdate Dihydrate 0.2mg/L, cupric sulfate pentahydrate 0.02mg/L, CoCL2 0.02mg/L;
(3) organic matter: inositol 80.0mg/L, glycine 2.5mg/L, thiamine hydrochloride (VB
1) 0.1mg/L, puridoxine hydrochloride (VB
6) 0.45mg/L, nicotinic acid 0.45mg/L;
(4) plant growth regulator: methyl 0.3-0.6mg/L;
Surplus is a distilled water.
Priority Applications (1)
| Application Number | Priority Date | Filing Date | Title |
|---|---|---|---|
| CN 201210363349 CN102823503B (en) | 2012-09-26 | 2012-09-26 | Tissue culture medium for propagating anthurium buds by using buds |
Applications Claiming Priority (1)
| Application Number | Priority Date | Filing Date | Title |
|---|---|---|---|
| CN 201210363349 CN102823503B (en) | 2012-09-26 | 2012-09-26 | Tissue culture medium for propagating anthurium buds by using buds |
Publications (2)
| Publication Number | Publication Date |
|---|---|
| CN102823503A true CN102823503A (en) | 2012-12-19 |
| CN102823503B CN102823503B (en) | 2013-08-14 |
Family
ID=47326981
Family Applications (1)
| Application Number | Title | Priority Date | Filing Date |
|---|---|---|---|
| CN 201210363349 Expired - Fee Related CN102823503B (en) | 2012-09-26 | 2012-09-26 | Tissue culture medium for propagating anthurium buds by using buds |
Country Status (1)
| Country | Link |
|---|---|
| CN (1) | CN102823503B (en) |
Cited By (7)
| Publication number | Priority date | Publication date | Assignee | Title |
|---|---|---|---|---|
| CN103011969A (en) * | 2012-12-25 | 2013-04-03 | 浙江农林大学 | Medium specialized for plant tissue culture, and preparation method thereof |
| CN104663465A (en) * | 2015-03-31 | 2015-06-03 | 桂林市一峰食品有限公司 | Culture medium for heartleaf houttuynia herb tissue culture |
| CN104719167A (en) * | 2015-03-31 | 2015-06-24 | 桂林市一峰食品有限公司 | Tissue culture medium for herba houttuyniae |
| CN105010141A (en) * | 2015-07-09 | 2015-11-04 | 虞龙 | Anthurium rapid propagation method |
| CN106900555A (en) * | 2017-03-21 | 2017-06-30 | 钦州市林业科学研究所 | Amomum viosum test tube plant division culture medium and once-seedling forming tissue culture plant division quick-breeding method |
| CN109906938A (en) * | 2019-03-07 | 2019-06-21 | 三明市农业科学研究院 | A kind of method of red palm germ plasm resource Plantlet in vitro |
| CN114208670A (en) * | 2021-12-16 | 2022-03-22 | 四川韵然景观园林工程有限公司 | Culture medium and culture method for fast propagation of woody flower plants |
Citations (4)
| Publication number | Priority date | Publication date | Assignee | Title |
|---|---|---|---|---|
| CN1623372A (en) * | 2004-12-02 | 2005-06-08 | 广东省珠海市园艺研究所 | Tissue cultivating fast reproducing method for pot culturing red palm seedling |
| CN1813525A (en) * | 2005-01-31 | 2006-08-09 | 肖尊安 | Culture medium for anthurium andraeanum tissue culture and tissue culture seedling breeding method |
| CN101642053A (en) * | 2009-08-25 | 2010-02-10 | 浙江大学 | Cold-resistant anthurium induction culturing method |
| CN101785429A (en) * | 2009-12-01 | 2010-07-28 | 东莞市生物技术研究所 | Method for improving rapid differentiation and bud formation of anthurium andraeanum callus |
-
2012
- 2012-09-26 CN CN 201210363349 patent/CN102823503B/en not_active Expired - Fee Related
Patent Citations (4)
| Publication number | Priority date | Publication date | Assignee | Title |
|---|---|---|---|---|
| CN1623372A (en) * | 2004-12-02 | 2005-06-08 | 广东省珠海市园艺研究所 | Tissue cultivating fast reproducing method for pot culturing red palm seedling |
| CN1813525A (en) * | 2005-01-31 | 2006-08-09 | 肖尊安 | Culture medium for anthurium andraeanum tissue culture and tissue culture seedling breeding method |
| CN101642053A (en) * | 2009-08-25 | 2010-02-10 | 浙江大学 | Cold-resistant anthurium induction culturing method |
| CN101785429A (en) * | 2009-12-01 | 2010-07-28 | 东莞市生物技术研究所 | Method for improving rapid differentiation and bud formation of anthurium andraeanum callus |
Non-Patent Citations (8)
| Title |
|---|
| 《上海农业学报》 20011231 张桂和等 "安祖花茎段培养与离体繁殖" 第13-16页 1-2 第17卷, 第3期 * |
| 《中南林学院学报》 20050630 蔡能等 "安祖花离体培养快速繁殖技术的优化" 第85-88页 1-2 第25卷, 第3期 * |
| 《亚热带植物科学》 20111231 陈丽文等 "红掌茎段侧芽离体快繁技术研究" 第42-43页 1-2 第40卷, 第2期 * |
| 《辽宁农业职业技术学院学报》 20070331 关丽霞等 "红掌叶不同部位愈伤组织的诱导及植株再生" 第25-27页 1-2 第9卷, 第1期 * |
| 关丽霞等: ""红掌叶不同部位愈伤组织的诱导及植株再生"", 《辽宁农业职业技术学院学报》, vol. 9, no. 1, 31 March 2007 (2007-03-31), pages 25 - 27 * |
| 张桂和等: ""安祖花茎段培养与离体繁殖"", 《上海农业学报》, vol. 17, no. 3, 31 December 2001 (2001-12-31), pages 13 - 16 * |
| 蔡能等: ""安祖花离体培养快速繁殖技术的优化"", 《中南林学院学报》, vol. 25, no. 3, 30 June 2005 (2005-06-30), pages 85 - 88 * |
| 陈丽文等: ""红掌茎段侧芽离体快繁技术研究"", 《亚热带植物科学》, vol. 40, no. 2, 31 December 2011 (2011-12-31), pages 42 - 43 * |
Cited By (9)
| Publication number | Priority date | Publication date | Assignee | Title |
|---|---|---|---|---|
| CN103011969A (en) * | 2012-12-25 | 2013-04-03 | 浙江农林大学 | Medium specialized for plant tissue culture, and preparation method thereof |
| CN103011969B (en) * | 2012-12-25 | 2014-11-05 | 浙江农林大学 | Medium specialized for plant tissue culture, and preparation method thereof |
| CN104663465A (en) * | 2015-03-31 | 2015-06-03 | 桂林市一峰食品有限公司 | Culture medium for heartleaf houttuynia herb tissue culture |
| CN104719167A (en) * | 2015-03-31 | 2015-06-24 | 桂林市一峰食品有限公司 | Tissue culture medium for herba houttuyniae |
| CN105010141A (en) * | 2015-07-09 | 2015-11-04 | 虞龙 | Anthurium rapid propagation method |
| CN106900555A (en) * | 2017-03-21 | 2017-06-30 | 钦州市林业科学研究所 | Amomum viosum test tube plant division culture medium and once-seedling forming tissue culture plant division quick-breeding method |
| CN109906938A (en) * | 2019-03-07 | 2019-06-21 | 三明市农业科学研究院 | A kind of method of red palm germ plasm resource Plantlet in vitro |
| CN109906938B (en) * | 2019-03-07 | 2021-10-29 | 三明市农业科学研究院 | Anthurium germplasm resource in vitro preservation method |
| CN114208670A (en) * | 2021-12-16 | 2022-03-22 | 四川韵然景观园林工程有限公司 | Culture medium and culture method for fast propagation of woody flower plants |
Also Published As
| Publication number | Publication date |
|---|---|
| CN102823503B (en) | 2013-08-14 |
Similar Documents
| Publication | Publication Date | Title |
|---|---|---|
| CN102823503B (en) | Tissue culture medium for propagating anthurium buds by using buds | |
| KR101587707B1 (en) | Producing method of orchid seedlings | |
| CN103190347B (en) | Teapot dates tissue culturing method | |
| CN105284620B (en) | A kind of method that Superearly peach bybrid embryo saves seedling | |
| CN104521715B (en) | Sealing water planting cutting propagation method for gardenias with flower buds | |
| CN107047319B (en) | A kind of method for tissue culture and root media of ginkgo | |
| CN103798145A (en) | Culture medium for tissue culture of vernonia amygdalina del. | |
| CN104585037A (en) | Tissue culture rapid-propagation method of beaucarnea recurvata | |
| CN103798144A (en) | Culture medium for tissue culture of toona ciliate roem. | |
| CN103314862B (en) | A kind of method of efficient acquisition Chunlan detoxification seedling | |
| CN103782912B (en) | Culture medium for red cassia tree tissue culture | |
| CN101946704B (en) | Method for regenerating Chinese rose plant by using immature seed as explant | |
| CN109729980A (en) | A kind of Mao Hanshi based on LED light source tissue culture and rapid propagation methods of volume bis- | |
| CN102657085A (en) | In-vitro rapid propagation method for tissue culture of broad-leafed notopterygium | |
| CN102217549A (en) | Culture method of rieger begonias test tube flowers | |
| CN102613089B (en) | High-efficient in-vitro propagation method of 20-year-old schima superba big tree | |
| CN106489739A (en) | A kind of production method of Flos Carthami Rosa floribunda test tube flower | |
| CN103598093B (en) | A kind of abductive approach of blueberry embryoid | |
| CN100391333C (en) | Aseptic seedling tissue culturing and test tube seedling hardening off and transplating technology for anthurium andraeanum | |
| CN110122333A (en) | A kind of method that flame tree seed stratification is taken root | |
| CN105746358A (en) | Tissue culture formula for Euonymus phellomanus and culture method | |
| CN108849510A (en) | Rooting method in clematis kind ' Avant-Garde ' tissue-cultured seedling bottle | |
| CN103392594A (en) | Draceana arborea tissue culture seedling rooting induction technology | |
| CN107155882A (en) | A kind of medicinal bletilla striata aseptic seeding fast seedling-cultivating method | |
| CN107155894A (en) | A kind of green ridge walnut somatic embryo method for culturing seedlings |
Legal Events
| Date | Code | Title | Description |
|---|---|---|---|
| C06 | Publication | ||
| PB01 | Publication | ||
| C10 | Entry into substantive examination | ||
| SE01 | Entry into force of request for substantive examination | ||
| C14 | Grant of patent or utility model | ||
| GR01 | Patent grant | ||
| CF01 | Termination of patent right due to non-payment of annual fee | ||
| CF01 | Termination of patent right due to non-payment of annual fee |
Granted publication date: 20130814 Termination date: 20160926 |