CN100484398C - In vitro conservation method of churysanthemum by reducing macroelements in the medium - Google Patents
In vitro conservation method of churysanthemum by reducing macroelements in the medium Download PDFInfo
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- CN100484398C CN100484398C CNB2007100193466A CN200710019346A CN100484398C CN 100484398 C CN100484398 C CN 100484398C CN B2007100193466 A CNB2007100193466 A CN B2007100193466A CN 200710019346 A CN200710019346 A CN 200710019346A CN 100484398 C CN100484398 C CN 100484398C
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Abstract
The invention relates to a method for conserving chrysanthemum in vitro through reducing major element in the medium, which is special for the in vitro conservation of the chrysanthemum germplasm resource. The invention comprises the steps of: taking the suckers of the chrysanthemum as the explants, and axillary buds for subculture, and conserving on the 1/2MS, 1/2MS (1/2NH4+) or 1/4MS medium containing 6-BA0.3mg/L and NAA0.1mg/L. The survival rate for a 12-month conservation is 100%, 8 months longer than that of conservation on the normal MS medium. After the conservation material recovers to normal growth, the descendant is proved to have no genetic variance through the detection of POD, EST and ISSR. The invention uses the method of conserving chrysanthemum test-tube plantlet through reducing major element in the medium and identifies the genetic stability of the descendant, which proves that the plants grow normally after one-year conservation and the descendant has no genetic variation.
Description
One, technical field
The present invention relates to be undertaken the method for chrysanthemum {in vitro} conservation, be exclusively used in chrysanthemum germ plasm resource {in vitro} conservation by macroelement in the minimizing medium.
Two, technical background
Chrysanthemum (Dendranthema * grandiflorum Ramat.) is one of China's ten great tradition famous flowers and the world's four big cut-flowers, have view and admire, eat, various value such as medicinal.China is the centre of origin of cultivating chrysanthemum and the distribution center of Chrysanthemum germ plasm resource, surplus the Chrysanthemum 40 kind China distribute have 20 surplus kind, surplus the cultivating chrysanthemum kind reaches 3000.There is height heterozygosity in cultivating chrysanthemum in heredity, offspring's proterties is separated, be difficult to preserve germ plasm resource by seed, and mainly carry out vegetative propagation by cuttage, need expend a large amount of soils, man power and material and carry out the maternal preservation and the cottage propagation of seedling, and in long-term vegetative propagation process, be prone to the people for mixing and planting the sexual involution phenomenon.
On producing, present seedling owing to tissue culture industrialization production not only will be complied with the demand in fast changing supply and demand market but also be subjected to the restriction of the season of growth again, making that the expansion of some materials is numerous does not have a practical significance in certain phase, it temporarily need be preserved, when the development of producing makes these materials become once more to need, it can be quickly recovered to normal fast numerous application state.Simultaneously, the summer high temperature high humidity, subculture pollutes easily, it if can be carried out the short-term preservation and then can get over the summer safely.
For overcoming the shortcoming that chrysanthemum tradition field planting preserves and solving the realistic problem of tissue culture industrialization in producing, the research of carrying out the {in vitro} conservation of chrysanthemum germ plasm resource seems urgent day by day.{in vitro} conservation, have not time-consuming, do not take a lot of work, be difficult for causing that germ plasm resource mixes, keep advantages such as germplasm merit, and be convenient to the exchange of virus-free germplasm.Along with nearly decades of being in full swing of cultured in vitro technology, reaching the slow growth method {in vitro} conservation technology that prolongs subculture time purpose by the external environmental condition that changes the culture growth and also obtained fast development.Since the nineties in 20th century, the researcher successfully carried out lily, Mengzi garden balsam, yellowish colored lily, dendrobium candidum etc. the test tube {in vitro} conservation of flowers germ plasm resource, but macroelement is preserved the chrysanthemum test-tube plantlet, the Shang Weiyou report in the present domestic utilization minimizing medium.
Three, summary of the invention
Technical problem the objective of the invention is at present chrysanthemum germ plasm resource field planting preservation workload big, be subject to the influence of extreme natural calamity and damage by disease and insect, and defectives such as the normal subculture preservation of tissue culture switching is frequent, cost height, a kind of method of carrying out the chrysanthemum {in vitro} conservation by macroelement in the minimizing medium is provided, be used for chrysanthemum germ plasm resource {in vitro} conservation, it is normal not only to preserve after 1 year plant strain growth, and hereditary variation does not take place the offspring who preserves material.
Technical scheme the present invention comprises by reducing the method that macroelement in the medium carries out the chrysanthemum {in vitro} conservation:
With chrysanthemum pin bud is explant, with 75% ethanol surface sterilization 30s, and aseptic water washing 2 times, again with 0.1% mercuric chloride sterilization 8min, behind the aseptic water washing 5 times, the stem section that is cut to 1 joint of defoliation band inserts in the MS medium; Behind the 20d axillalry bud of sprouting is transferred to MS+0.3mg.L
-16-BA+0.1mg.L
-1Carry out enrichment culture on the NAA medium; The stem section that behind the 30d indefinite bud of breeding is cut into 2 joints of defoliation band changes 1/2MS (macroelement all reduces by 1/2 amount) or 1/2MS (1/2NH over to
4 +) (NH
4NO
3Reduce by 3/4 amount, all the other macroelement reduce by 1/2 amount) or 1/4MS (macroelement all reduces by 3/4 amount), preserve on the medium of all additional 6-BA0.3mg/L and NAA0.1mg/L.
Contain sucrose 3%, agar 0.7% in the above medium, pH is 6.0 (before the autoclave sterilizations), 23 ± 2 ℃ of condition of culture, intensity of illumination 2000~3000lux, light application time 12h/d.
The method of beneficial effect {in vitro} conservation chrysanthemum provided by the invention germ plasm resource compared with prior art has following advantage and good effect:
1. method of carrying out the chrysanthemum {in vitro} conservation by macroelement in the minimizing medium provided by the present invention, be used for chrysanthemum germ plasm resource {in vitro} conservation, test-tube plantlet preserves that survival rate still is 100% after 12 months, and plant strain growth is normal, and the test-tube plantlet on the normal MS medium was only survived 4 months.
2. the inventive method is preserved 12 months chrysanthemum test-tube plantlet, and the ISSR amplification bands of a spectrum and the contrast of its offspring POD, EST isodynamic enzyme zymogram and primer I 35 do not have difference, preserve material settling out, and genetic variation does not take place.
3. the present invention utilizes first and reduces in the medium macroelement and preserve the chrysanthemum test-tube plantlet and its offspring is carried out genetic stability identify, preserves with traditional chrysanthemum field planting and compares, and can save shelf space, and workload is little.
4. can prevent many generation breeding back kind sexual involutions and virus infections, guarantee the good property and the purity of germplasm.
5. broken the restriction of vegetation season, material can be provided at any time, had the saving storage space simultaneously, be convenient to transportation and advantage such as exchange.
6. can prevent the loss of germ plasm resource.
7. heavy subculture work in reduce producing, and reduce the waste of human and material resources resource unnecessary in the production operation process provides necessary approach for actual production reduces production costs and increases economic efficiency.
Four, description of drawings
Preserve 6 months test-tube plantlet on the different medium nutrient levels of Fig. 1
The test-tube plantlet of preserving 12 months on the different medium nutrient levels of Fig. 2 is followed successively by from the right side on a left side: 1/2MS (1/2NH
4 +), 1/2MS, 1/4MS
Fig. 3 preserves plant recovers to cultivate 25d on enrichment culture the left figure of upgrowth situation: the right figure of CK: preserve plant
The upgrowth situation of Fig. 4 regeneration plant domestication 25d
Fig. 5 regeneration plant is transplanted 3 months upgrowth situation of booth
Fig. 6 transplants 3 months regeneration plants of booth and is followed successively by with the right side of the contrast that contrasts plant and leaf shape from a left side: CK, 1/2MS (1/2NH
4 +), 1/2MS, 1/4MS
The left figure of Fig. 7 isodynamic enzyme zymogram: the right figure of POD isodynamic enzyme zymogram: EST isodynamic enzyme zymogram
The ISSR amplification of Fig. 8 primer I 35
Annotate: (M) 100 bp dna molecular amount mark CK: contrast: (1) 1/2MS (1/2NH
4 +); (2) 1/2MS; (3) 1/4MS;
Five, embodiment
The method of {in vitro} conservation chrysanthemum germ plasm resource provided by the present invention, its embodiment is as follows:
1. the {in vitro} conservation of chrysanthemum germ plasm resource: with ' the Olympic torch ' (Dendranthema * grandiflorum Ramat. ' Aoyunhuoju ') (public kind of this seminar seed selection, old kerria of the document that sees reference, Fang Weimin etc. the potted plant little chrysanthemum series of chrysanthemum new varieties one summer flower type. the gardening journal, 2005,32 (3): 567) kind is for supplying the examination material.Getting ' the Olympic torch ' pin bud is explant, with 75% ethanol surface sterilization 30s, and aseptic water washing 2 times, again with 0.1% mercuric chloride sterilization 8min, behind the aseptic water washing 5 times, the stem section that is cut to 1 joint of defoliation band inserts in the MS medium.Behind the explant inoculation 5d, the axillary bud sprouting rate is 83.3%; Behind the 20d axillalry bud is transferred to MS+0.3mg.L
-16-BA+0.1mg.L
-1Carry out enrichment culture on the NAA medium; The stem section that behind the 30d indefinite bud of breeding is cut into 2 joints of defoliation band changes 1/2MS (macroelement all reduces by 1/2 amount) or 1/2MS (1/2NH over to
4 +) (NH
4NO
3Reduce by 3/4 amount, all the other macroelement reduce by 1/2 amount) or 1/4MS (macroelement all reduces by 3/4 amount), preserve on the medium of additional 6-BA0.3mg/L and NAA0.1mg/L.
Contain sucrose 3%, agar 0.7% in the above medium, pH is 6.0 (before the autoclave sterilizations), 23 ± 2 ℃ of condition of culture, intensity of illumination 2000~3000lux, light application time 12h/d.
2. preserving material offspring's genetic stability identifies: ' the Olympic torch ' test-tube plantlet is gone up growth after 3 months at proliferated culture medium (contrast), its top tip and cultivation lid turn back downwards, whole strain twisted growth, and cover with aerial root on the stem section, have only top tip peak green to use, after 4 months, plant senesecence is withered.And test-tube plantlet poor growth on the medium that macroelement reduces in various degree, plant strain growth normal (Fig. 1) after 5 months, the top tip and cultivation lid (Fig. 2) after 12 months, plant middle and lower part chlorosis is withered, but the middle and upper part can be used.Macroelement has prolonged the test-tube plantlet successive transfer culture time greatly in the minimizing medium, make subculture at interval transfer 12 months subcultures for 1 time to 1 time by at ordinary times 1 month subculture, and after 12 months on 3 kinds of medium the survival rate of test-tube plantlet be 100%, comparison is according to prolonging survival 8 months; Test-tube plantlet was preserved after 12 months, the contrast test-tube plantlet of preserving with subculture 1 subnormal cultivation in 1 month is forwarded on the proliferated culture medium, the preservation material differentiates the normal indefinite bud of form after cultivating 10d, and differentiation capability is normal compared with the control, shows that preserving material recovers growth normal (Fig. 3); Behind the 30d indefinite bud of regeneration is transferred on the root media, root media is 1/2MS+0.1mg.L
-1NAA; Open behind the culture of rootage 15d and cultivate lid white silk seedling, be transplanted to behind the 7d in the perlite that high-temperature sterilization is crossed and tame, water every day once, 3~4d waters the MS nutrient solution once, is transplanted to booth (Fig. 4) behind the 25d; The transplanting booth is got plant lobus cardiacus extraction crude enzyme liquid after 2 months (method sees reference, and document how imitate by loyalty, the Zhang Shuzheng chief editor. electrophoresis [M]. Science Press, Beijing, 1999) and total DNA (method document Xiao Jun that sees reference, Yang Liguo etc. two kinds of comparisons of extracting the total DNA method of chrysanthemum. Liaoning agricultural science, 2005 (1): 40~41), find no specific band generation (Fig. 7, Fig. 8) through peroxide enzyme (POD) and esterase (EST) isodynamic enzyme, ISSR Markers for Detection.Above presentation of results reduces the chrysanthemum germplasm that macroelement was preserved 12 months in the medium and has kept good genetic stability.
The method that above-mentioned isodynamic enzyme detects is, gets plant lobus cardiacus 0.15g, adds on the 450ml buffer solution ice bath to grind to form homogenate rapidly, is transferred to 4 ℃ of centrifugal 20min of 8000rmp/min in the centrifuge tube, and supernatant is the crude extract of enzyme; The separation gel of preparation 9%, 3% concentrated glue adopt the vertical panel polyacrylamide gel electrophoresis to analyze POD and EST isodynamic enzyme, every hole point sample 20ul.Concentrate glue and adopt 100V voltage stabilizing electrophoresis, use 200V voltage stabilizing electrophoresis behind the separation gel instead.When running extremely near bottom 1cm, the bromophenol blue colour band stops electrophoresis; POD adopts the dyeing of improvement benzidine method, EST dyes with a-naphthalene ester, strong orchid, gel imaging analysis instrument (Shanghai Peiqing Science Co., Ltd, the JS-380 type) going up observation finds, the zymogram of {in vitro} conservation material offspring strain and contrast consistent (Fig. 7) illustrates that genetic variation does not take place to reduce the chrysanthemum germplasm that macroelement was preserved 12 months in the medium on protein level.
The method of above-mentioned ISSR molecular markers for identification is, get the plant lobus cardiacus in little glass mortar with liquid nitrogen mixing grind away.Sample total DNA extract with reference to the CTAB method (the method document Xiao Jun that sees reference, Yang Liguo etc. two kinds of comparisons of extracting the total DNA methods of chrysanthemum. Liaoning agricultural science, 2005 (1): 40~41).Amplified reaction adopts 20.0ul reaction system (see Table 1, all reagent are all given birth to logical biotechnology Co., Ltd available from Nanjing), in the PTC-100 of U.S. MJ Research company
TMCarry out pcr amplification in the type amplification instrument, response procedures is: 95 ℃ of pre-sex change 5min; 94 ℃ of sex change 45s, 55 ℃ of renaturation 40s; 72 ℃ are extended 70s, 45 circulations; 72 ℃ are extended 7min, 10 ℃ of preservations.After amplified reaction finishes, respectively add 6 * bromophenol blue 0.4ul in ISSR amplified production reactant liquor, behind the centrifugal mixing, each is drawn mixed liquor 6.5ul and injects point sample hole electrophoresis on 2% Ago-Gel, and gel contains 0.05% ethidium bromide (EB).Electrode buffer is 1 * Tris-acetate (TAE), 180 volts of separation voltages, behind electrophoresis 50~60min in gel imaging analysis instrument (Shanghai Peiqing Science Co., Ltd, the JS-380 type) going up observation finds, the ISSR amplified band of its primer I 35 of {in vitro} conservation material offspring strain is consistent with contrast, do not have specific band to produce (Fig. 8), illustrate that genetic variation does not take place to reduce the chrysanthemum germplasm that macroelement was preserved 12 months in the medium on molecular level.
Table 1 PCR reaction system
Annotate: the sequence of primer I 35 is (AG)
8TA
Claims (1)
1, carry out the method for chrysanthemum {in vitro} conservation by macroelement in the minimizing medium, comprising:
With chrysanthemum pin bud is explant, with 75% ethanol surface sterilization 30s, and aseptic water washing 2 times, again with 0.1% mercuric chloride sterilization 8min, behind the aseptic water washing 5 times, the stem section that is cut to 1 joint of defoliation band inserts on the MS medium; Behind the 20d axillalry bud of sprouting is transferred to MS+0.3mg.L
-16-benzyladenine+0.1mg.L
-1Carry out enrichment culture on the methyl medium; The stem section that behind the 30d indefinite bud of breeding is cut into 2 joints of defoliation band changes MS or the NH that macroelement all reduces by 1/2 amount over to
4NO
3Reduce by 3/4 amount, all the other macroelement reduce the MS of 1/2 amount or the MS that macroelement all reduces by 3/4 amount, preserve on the medium of all additional 6-benzyladenine 0.3mg/L and methyl 0.1mg/L;
Contain sucrose 3%, agar 0.7% in the above medium, pH is 6.0,23 ± 2 ℃ of condition of culture, intensity of illumination 2000~3000lux, light application time 12h/d.
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CN102726298B (en) * | 2012-07-03 | 2013-07-17 | 中国农业科学院作物科学研究所 | Cryopreservation method for in vitro shoot tips of petunia hybrida |
CN103609448B (en) * | 2013-11-28 | 2016-01-20 | 安徽科技学院 | Preservation method for stevia rebaudiana germplasm |
CN104255453B (en) * | 2014-09-09 | 2016-03-30 | 安徽科技学院 | A kind of store method of stevia plantlet in vitro |
CN104170743A (en) * | 2014-09-09 | 2014-12-03 | 安徽科技学院 | Culture medium for preserving tissue culture seedlings of stevia rebaudiana |
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CN104170742A (en) * | 2014-09-09 | 2014-12-03 | 何克勤 | Method for preserving tissue culture seedlings of stevia rebaudiana idioplasm |
CN107509634B (en) * | 2017-09-30 | 2019-06-25 | 绍兴文理学院元培学院 | A kind of gold thread grass tissue cultures and rapid propagation method |
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