几种药用芳香植物组织培养快速繁殖的研究
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摘要
以洋甘菊、留兰香、薰衣草、药用鼠尾草、牛至、百里香这些有较高药用价值的芳香植物为试材,探讨了这6种芳香植物离体培养过程中基本培养基、植物激素对外植体生长发育、增殖和生根的影响,筛选出适合每种植物增殖和生根的培养基。进行快速繁殖,建立了无菌试管苗体系。
基本培养基MS适合于洋甘菊、留兰香、薰衣草、牛至。MS培养基比改良MS培养基更有利于百里香的生长,药用鼠尾草苗较小(仅两片叶,几乎无茎杆)时Nitsch培养基比MS培养基更有利于外植体的生长,药用鼠尾草苗较大(四片叶)时MS培养基比Nitsch培养基更有利于外植体的后期生长。
洋甘菊最适增殖培养基为MS+BA0.2mg/L+IBA0.06mg/L。洋甘菊易生根,加有NAA(0.1-1.5mg/L)或IBA(0.1-1.5mg/L)的MS培养基中都可以诱导出大量的根。组培苗移栽易成活。在BA和IBA的组合,对幼茎加粗有影响。
留兰香的最佳增殖培养基MS+BA0~0.1mg/L+IBA0~0.04mg/L。接种在加有NAA(0~2mg/L)的MS培养基上,茎上可长出大量的气生根,而培养基内部的生根数量则相对较少。从生根率、生根数及苗的生长综合考虑,留兰香生根培养基中NAA的浓度为0.1~0.5mg/L较理想。留兰香的幼茎用NAA浸泡处理2小时后,可在瓶外扦插生根繁殖,扦插在珍珠岩+园土(1∶1)中生根良好。
薰衣草的最佳增殖培养基为MS+BA1.0mg/L。BA对薰衣草嫩茎增殖有极显著影响,而 BA×IBA交互作用对薰衣草嫩茎增殖影响不显著。薰衣草的最佳生根培养基为MS+IBA0.5mg/L。
牛至的最佳增殖培养基为MS+2.0mg/LBA+IBA0.02mg/L。牛至易生根,试验结果表明NAA、IBA、IAA三种激素处理后生根率多在90%以上。牛至的根形成后易老化、褐化,在炼苗移栽时应注意选择适宜的时间,不宜太晚。
药用鼠尾草的最佳增殖培养基MS+BA0.8mg/L,BA对药用鼠尾草平均嫩芽增殖有极显著的影响。最佳生根培养基1/2MS+IBA0.8mg/L+蔗糖20g。
百里香的最佳增殖培养基MS+BA1.5mg/L+IBA0.08mg/L,平均增殖倍数4.24;最佳生根培养基以1/2MS培养基为基本培养基,附加0.5mg/L IBA,2%蔗糖浓度,生根率可达100%。
The materials of medicinal aromatic plants Chamomilla recutita L, Mentha spicata L, Lavandula angustifolia Mill, Origanum vulgare L, Salavia officinalis L and
Thymus serpyllum L.var.mongolicus Ronn were used to establish the in vitro plant and develop a feasible and practicable system of, to study the effect of some phytohormones on growth, development and proliferation in vitro, to choose the suitable media of the six plants. Multiple shoots were produced from the base of buds after the establishment of the culture.
Regard to Chamomilla recutita L, Mentha spicata L, Lavandula angustifolia Mill, Origanum vulgare L MS basal media is suit, but infancy Origanum vulgare L grew better on Nitsch medium than MS medium. To Thymus serpyllum L.var.mongolicus Ronn of growth, MS medium is better than amend MS medium.
Regard to Chamomilla recutita L, multiplication and growth of shoots were optimum with MS+ BA0.2mg/L+IBA0.06mg/L. MS medium with NAA(0.1~1.5mg/L) or IBA(0.1-1.5mg/L) can induced lots of roots, the survival rate after transplantation was higher. cuttings were stronger on MS medium with BA×IBA than MS media with BA or MS media with IBA.
Regard to Mentha spicata L, multiplication and growth of shoots were optimum with MS+BA0~0.1mg/L+IBA0~0.04mg/L. plant of regene ration are easy to root. The ratio of rooting can reach 100% in MS+ NAA(0.1~0.5mg/L).And plants produce many aerial roots. And cuttage of Mentha spicata L out of bottles were studied .
Regard to Lavandula angustifolia Mill, the optimum propagation medium is MS+BA1.0mg/L; the optium-rooting medium is MS+IBA0.5mg/L. The survival rate after transplantation was not high. Growth of stem-tip is better than stem.
Regard to Origanum vulgare L, shoot-tips as explants, the optimum propagation medium is MS+2.0mg/LBA+IBA0.02mg/L. The ratio of rooting can reach 100% in MS and 1/2MS
media, but a number of roots are thinner and fewer, and do not survive after transplant. So it is necessary that hormone should be added in medium.
Regard to Salavia officinalis L, the optimum propagation medium is MS+BA0.8mg/L.The effect of BA,IBA on bud multiplication is significant. The best rooting medium is optimum with 1/2MS+IBA0.8mg/L+ sucrose 20g/L.
Regard to Thymus serpyllum L, the optimum propagation medium is MS+BA1.5mg/L+IBA0.08mg/L, the optimum-rooting medium is 1/2MS+IBA0.5mg/L+ sucrose 20g/L.The ratio of rooting can reach 100%.
基本培养基MS适合于洋甘菊、留兰香、薰衣草、牛至。MS培养基比改良MS培养基更有利于百里香的生长,药用鼠尾草苗较小(仅两片叶,几乎无茎杆)时Nitsch培养基比MS培养基更有利于外植体的生长,药用鼠尾草苗较大(四片叶)时MS培养基比Nitsch培养基更有利于外植体的后期生长。
洋甘菊最适增殖培养基为MS+BA0.2mg/L+IBA0.06mg/L。洋甘菊易生根,加有NAA(0.1-1.5mg/L)或IBA(0.1-1.5mg/L)的MS培养基中都可以诱导出大量的根。组培苗移栽易成活。在BA和IBA的组合,对幼茎加粗有影响。
留兰香的最佳增殖培养基MS+BA0~0.1mg/L+IBA0~0.04mg/L。接种在加有NAA(0~2mg/L)的MS培养基上,茎上可长出大量的气生根,而培养基内部的生根数量则相对较少。从生根率、生根数及苗的生长综合考虑,留兰香生根培养基中NAA的浓度为0.1~0.5mg/L较理想。留兰香的幼茎用NAA浸泡处理2小时后,可在瓶外扦插生根繁殖,扦插在珍珠岩+园土(1∶1)中生根良好。
薰衣草的最佳增殖培养基为MS+BA1.0mg/L。BA对薰衣草嫩茎增殖有极显著影响,而 BA×IBA交互作用对薰衣草嫩茎增殖影响不显著。薰衣草的最佳生根培养基为MS+IBA0.5mg/L。
牛至的最佳增殖培养基为MS+2.0mg/LBA+IBA0.02mg/L。牛至易生根,试验结果表明NAA、IBA、IAA三种激素处理后生根率多在90%以上。牛至的根形成后易老化、褐化,在炼苗移栽时应注意选择适宜的时间,不宜太晚。
药用鼠尾草的最佳增殖培养基MS+BA0.8mg/L,BA对药用鼠尾草平均嫩芽增殖有极显著的影响。最佳生根培养基1/2MS+IBA0.8mg/L+蔗糖20g。
百里香的最佳增殖培养基MS+BA1.5mg/L+IBA0.08mg/L,平均增殖倍数4.24;最佳生根培养基以1/2MS培养基为基本培养基,附加0.5mg/L IBA,2%蔗糖浓度,生根率可达100%。
The materials of medicinal aromatic plants Chamomilla recutita L, Mentha spicata L, Lavandula angustifolia Mill, Origanum vulgare L, Salavia officinalis L and
Thymus serpyllum L.var.mongolicus Ronn were used to establish the in vitro plant and develop a feasible and practicable system of, to study the effect of some phytohormones on growth, development and proliferation in vitro, to choose the suitable media of the six plants. Multiple shoots were produced from the base of buds after the establishment of the culture.
Regard to Chamomilla recutita L, Mentha spicata L, Lavandula angustifolia Mill, Origanum vulgare L MS basal media is suit, but infancy Origanum vulgare L grew better on Nitsch medium than MS medium. To Thymus serpyllum L.var.mongolicus Ronn of growth, MS medium is better than amend MS medium.
Regard to Chamomilla recutita L, multiplication and growth of shoots were optimum with MS+ BA0.2mg/L+IBA0.06mg/L. MS medium with NAA(0.1~1.5mg/L) or IBA(0.1-1.5mg/L) can induced lots of roots, the survival rate after transplantation was higher. cuttings were stronger on MS medium with BA×IBA than MS media with BA or MS media with IBA.
Regard to Mentha spicata L, multiplication and growth of shoots were optimum with MS+BA0~0.1mg/L+IBA0~0.04mg/L. plant of regene ration are easy to root. The ratio of rooting can reach 100% in MS+ NAA(0.1~0.5mg/L).And plants produce many aerial roots. And cuttage of Mentha spicata L out of bottles were studied .
Regard to Lavandula angustifolia Mill, the optimum propagation medium is MS+BA1.0mg/L; the optium-rooting medium is MS+IBA0.5mg/L. The survival rate after transplantation was not high. Growth of stem-tip is better than stem.
Regard to Origanum vulgare L, shoot-tips as explants, the optimum propagation medium is MS+2.0mg/LBA+IBA0.02mg/L. The ratio of rooting can reach 100% in MS and 1/2MS
media, but a number of roots are thinner and fewer, and do not survive after transplant. So it is necessary that hormone should be added in medium.
Regard to Salavia officinalis L, the optimum propagation medium is MS+BA0.8mg/L.The effect of BA,IBA on bud multiplication is significant. The best rooting medium is optimum with 1/2MS+IBA0.8mg/L+ sucrose 20g/L.
Regard to Thymus serpyllum L, the optimum propagation medium is MS+BA1.5mg/L+IBA0.08mg/L, the optimum-rooting medium is 1/2MS+IBA0.5mg/L+ sucrose 20g/L.The ratio of rooting can reach 100%.
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Kintzion,S. 1999,Somatic embryogenesis and in vitro rosmarinic acid accumulation in Salvia officinalis and S.fruticosa leaf callus culture. Plant Cell Reports ,18(6) : 462-466
Kaltimani.K.N,Reddy.YN 1998,Effect of leaves on rooting of stem cuttings of Japanese Mint. Kamataka Journal of Agricultural Sciences,11(3):853-854
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Kothari,S.K,Sinah.VP 1996,The effect of row spacing and ritroge fertilization on the growth and oil yield composition of Japanese mint. Journal of Mendicinal and Aromatic Plant Sciences,18(1):17-21
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Menghini.A,Capuccella.M. 1994,Micropropagation of common chamomile Informatore Agrario , 50(22):76-77
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Monne-Bosch.S, Mueller. M., Schwareez. K 2001, Diterpenes and antioxidative protection in drought-stressed Saliva officinalis plants. Journal and Plant Physiology, 158(11):1431-1437
Olszowska.O.,Furmanowa M. 1990, Micropropagation of Salvia officinalis by shoot buds Plants Medica 56(6):637
Prasad,B,L,S.2000,Influence of growth regulations and methods of application on rooting of thyme (Thymus valgaris L.) cutting. In Spices and Aromatic Plants,202-206
Preety Singh,Srivastava S.K,Misra A.2001, Excretion of butyl hydrogen phthalate by iron efficient Menthaspicata L.var MSS-5 under iron stress. Joural of Plant Biology,28(1):111-114
Perry,N.B,Anderson R.E 1999, Essential oils from Dalmatian sage (Salvia offoconalis L.) :variations among individuals,plant parts, seasona and sites.Journal of Agricultural and Food Chemistry,47(5):2048-2054
Panov-Filotheov,H.,Bosabalidis A.M, Karataglis.S.2001,Effect of copper toxicity on leaves of Oregamo. Annals of Botany,88(2):207-214
Rady,M,R. 2000,Mcriopropagation of Lavandula officinalis L. through shoot tip culture of mature plants .Egyptian Journal of Horticulture ,27(3) :305-314
Rusera.R.,1999,In vitro culture of mint (M. piperta) with a high coefficient of multiplication. Rasteniev DniNauki ,36(4):201-203
Siva,C,D,E,P. 1999,Early rooting in rosemary (Rosmarinus officinalis L.)cuttings under the influence of chemical treatments and collecting time. Acta horticulture,No.502:213-217
Sanchez-gras,M,C . 1996,Micropropagation of Lavandula latifolia through nodal bud culture of mature plants. Plant cell, Tissue and organ culture , 45(3):259-261
Savithri Bhat, Priti.Maheshwari Sushil kumrr 2002, Mentha species :in vitro regenration and genetic transformation. Molecular Biology Today, 3(1):11-23
Siddique M.A.A, Paul T.M 1994, Influence of IBA on the induction of rooting in Salvia officinalis L.
Advances in Plant Sciences, 7(1):170-172
Shetty,K., Curtis. O.P, Levin R.E,1996, Specific interation of mucoid strains of Pseudomonas spp. With oregano (Origanum vulgare) clones and the Relationship to prevention of hyperhydric in tissue culture. Journal of Plant Physiologo,149(5):605-611
Tawfik,A.A. Read P.E 1992, Stimulation of growth and monterpene production of sage (Saliva officinalis) by benzyladenine in vitro. Plant Growth Regulator Society of America Quarterly, 20(4):200-206
Tsuro,M..2000,Efficient plant regeneration from multiple shoots formed in the leaf-derived callus of Lavandula vera.using the “open culture system ”. Scientia Horticulture,86 (1):81-88
Tavoletti.S, Standardi.A 1994,Raspomse to in vitro of twochamomile (Matricaria chamomillial) population with different ploidy levels. Journl of Genetics & Breeding. 48(2):125-130
Youssef,A,A 2000,Effect of salt stress on the essential oil content and composition of Rosmarinus officinalis callus cultures . Egyptian Journal of Horticulture,27(1):69-79
Zheljazkov.V.D, Topalor. V 1996, Effect of planting time and density on yieldsfrom