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1.
Plant regeneration from leaf tissues of four North Dakota genotypes of potato (Solanum tuberosum L.)
Y. D. Park D. H. Ronis A. A. Boe Z. M. Cheng 《American Journal of Potato Research》1995,72(6):329-338
An efficient plant regeneration system was developed fromin vitro leaf tissues of four North Dakota potato genotypes. The best medium for genotype ND860-2 was Murashige and Skoog medium with 20.0 μM IAA and 11.4 μM zeatin riboside. Two to three weeks of initial dark treatments had a significant effect in reducing the time for shoot regeneration and increasing the number of regenerated shoots. Four antibiotics commonly used inAgrobacterium- mediated transformation were tested for their effects on shoot regeneration. Shoot induction was completely inhibited by kanamycin at 15 mg/L and hygromycin at 4 mg/L or higher, but not by carbenicillin (except at 1000 mg/L) and cefotaxime. Hygromycin significantly stimulated shoot induction at 1 mg/L. 相似文献
2.
Nowadays, many researches were conducted in minimizing tissue culture technology due to the overhead of cost needed. The purpose of this study was to investigate the effects of using five kinds of organic additives at four level concentrations responsive to the number of shoots produced for eight weeks in culture. Stem segment explants of Celosia sp. were cultured on MS medium that have been supplemented with different kinds of extract juice that serve as organic additives which are mature coconut, young coconut, papaya, banana and tomato at 20, 30, 50 and 70 ml L-1. The numbers of shoot on each explant were recorded and the mean of ten replicates explants were calculated. Among the media used, young coconut water at 70 ml L1- induced the highest shoot regeneration (14.21+/-8.26), followed by mature coconut water at 50 ml L-1 (13.14+/-10.33). Banana and tomato juice promote highest shoot regeneration of stem segments at 50 ml L-1 that produced 9.57+/-4.68 and 9.28+/-5.82 shoots per explants, respectively. While the lowest concentration which at 20 ml L-1 of papaya juice showed highest shoot regeneration (10.50+/-3.45) produced among the three other concentration tested. Statistical results showed that there were significant differences interactions effects (p<0.05) in terms of number of shoot regenerated between the types of extracts juices determined by ANOVA test. Comparing number of shoots regenerated that were cultured in control media, it showed higher than all of experimental medium composition. There were no big different in cost required in preparation of control media and the experimental media. Applications of five kinds of local fruit in tissue culture media should be considered since it responsive in shoot regeneration. 相似文献
3.
以蝴蝶兰幼嫩花梗诱导的无菌苗叶片为外植体,以MS为基本培养基,研究不同暗培养时间和TDZ浓度对蝴蝶兰叶片诱导不定芽的影响。结果表明:暗培养和TDZ对接种的蝴蝶兰叶片的成活率均具有显著影响,暗培养60 d时,叶片的存活率在90%以上,而在同一暗培养时间条件下,叶片的存活率随着TDZ浓度的增加而上升;在TDZ浓度为3.0 mg/L,暗培养60 d时,蝴蝶兰存活叶片不定芽的诱导率最高,达到93.45%;诱导的不定芽数最多,平均每个外植体诱导的不定芽数为13.22个。综合考虑外植体的成活率、不定芽诱导率和诱导的不定芽数,蝴蝶兰叶片诱导不定芽的最佳条件为:MS+TDZ 3.0 mg/L,暗培养60 d。 相似文献
4.
苎麻茎尖的组织培养及其诱导植株的再生 总被引:8,自引:0,他引:8
对苎麻50号品系的茎尖进行组织培养并诱导植株再生。结果表明:最适茎尖转绿和分化的培养基是1/2MS 6-BA1.0mg/L CH300mg/L的液体培养基,茎尖分化率为100%。最适成苗培养基为MS 6-BA0.5mg/L IAA0.1mg/L CH300mg/L,成苗率是53.3%。扩繁培养基为MS 6-BA0.3 ̄1.0mg/L,繁殖系数达6.7。适宜生根培养基为1/2MS NAA0.01mg/L。最佳茎尖剥取材料是无菌试管苗,茎尖长以0.3mm带1 ̄2个叶原基为宜。从茎尖接种培养成苗到移栽需4个月左右。 相似文献
5.
《Journal of Crop Improvement》2013,27(4):432-446
Broccoli (Brassica oleracea var. italica) is an important nutritionally rich vegetable cole crop grown in the world. Environmental stress, pests, and diseases cause enormous yield losses because of a limited gene pool. Genetic manipulation is becoming an important method for broccoli improvement. The objective of present study was to evaluate the potency of thidiazuron (TDZ) as a plant growth regulator in evoking morphogenic responses in leaf and petiole explants of broccoli. An efficient, reproducible, and high frequency plant regeneration protocol has been standardized in broccoli cv. Solan green head. Leaf and petiole explants were cultured on Murashige-Skoog (MS) medium, supplemented with a wide range of TDZ concentrations. The following treatments were designed for efficient in vitro shoot regeneration: TDZ alone, TDZ with adenine, TDZ with naphthalene acetic acid (NAA), and TDZ with indole acetic acid (IAA). Among the 36 combinations of growth regulators used, the highest percentage of leaf explants producing shoot (89.25%) was recorded on MS medium containing 1.0 μM TDZ and 0.107 μM NAA. The multiple shoot regeneration response of petiole explant producing shoots (91.55%) was obtained on MS medium containing 2.0 μM TDZ and 0.107 μM NAA. Shoot multiplication and elongation were obtained on the same medium. For root regeneration in in vitro regenerated shoots, different concentrations of NAA were applied. High frequency (100%) root regeneration response with healthy and vigorous roots was observed on MS medium supplemented with 0.54 μM NAA. The regenerated plantlets with well-developed shoots and root system were transferred to pots containing cocopeat and successfully acclimatized. We recommend 1.0 μM TDZ with 0.107 μM NAA and 2.0 μM TDZ and 0.107 μM NAA combinations for adventitious shoot regeneration from leaf and petiole explants in broccoli cv. Solan green head respectively. This is the first report on high frequency organogenesis from leaf and petiole explants of broccoli cv. Solan green head using thidiazuron. 相似文献
6.
Intact immature flower buds of African violet (Saintpaulia ionantha H. Wendl.) were used as explant sources for in vitro studies. The effect of exogenous hormones, NAA and BAP on the indirect organogenesis of this species was observed. Callus was formed on the cut end (base) of pedicels of floral buds where they were in contact with the medium. When maintained on the same medium, callus was differentiated into adventitious shoots after 10 weeks in culture. MS media supplemented with 2.0 mg L(-1) NAA and 1.0 mg L(-1) BAP gave the highest number of sterile or vegetative floral buds from the surface of callus of the explants, but these buds failed to develop further. The floral buds were expanded as abnormal flowers. The floral structures were smaller in size compared to intact flowers. Petals (corolla) were white to purple in colour but did not form any reproductive organs, i.e., stamens or pistils. All sterile or vegetative floral buds and abnormal flowers survived for 3 months in culture but failed to reach anthesis. 相似文献
7.
以王氏唇柱苣苔(Chirita wangiana)叶片为外植体进行组培离体快繁研究,并利用流式细胞术对组培苗进行遗传稳定性分析。结果表明:最佳初代诱导培养基为MS添加0.5 mg/L 6-BA+0.1 mg/L NAA;最适继代培养基为MS添加0.5 mg/L 6-BA+0.05 mg/L NAA;最适生根培养基为1/2 MS培养基添加0.5 mg/L IBA和15 g/L蔗糖,所有生根培养基获得的组培苗移栽驯化成活率达到92%以上。组织学切片检测表明,王氏唇柱苣苔叶片为外植体所形成芽体均为器官发生方式形成。流式细胞术检测表明,组培苗倍性没有变化,基因组大小与母本相比仅发生了1.86%的减少;染色体数目为2n=36,跟母本一致,植株形态特征上也无变异。研究结果可为王氏唇柱苣苔的园艺应用快速提供大量遗传稳定的种苗。 相似文献
8.
花生幼叶芽诱导和植株再生研究 总被引:12,自引:2,他引:12
从萌发9-10d的花生幼嫩叶片上切取中段作外植体,接种MS+BA 3mg/L NAA 0.8mg/L AgNO3 2mg/L诱芽培养基,12-14d后产生丛生芽点,芽诱导率达78.9%,平均每外植体产生9个丛生芽。4周后转至MS BA 3mg/L AgNO3 2mg/L诱导芽伸长,诱导生根后获得再生植株。 相似文献
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10.
花生胚小叶的离体再生及筛选压力选择 总被引:1,自引:0,他引:1
以花生胚小叶为外植体,优化离体再生条件,通过对再生苗进行筛选,为外源基因的遗传转化提供实验依据。研究表明,不同基因型胚小叶的再生能力差异显著,在供试基因型中中花8号不定芽诱导率和成苗率最高,且外植体状态最好。中花8号胚小叶再生的最佳诱导培养基为MSB + 6-BA(4.5mg/L)+NAA(1mg/L)+AgNO3(2mg/L),最佳诱导培养时间为21d。对中花8号再生苗进行筛选浓度实验,草丁膦(PPT)为20mg/L时,可筛选出抗性苗;300mg/L的卡那霉素(Km)可用于较小幼苗筛选,而对较大幼苗则需将Km的浓度提高至400mg/L以上。 相似文献
11.
利用改良的草丁膦筛选系统快速而有效筛选转基因大豆 总被引:1,自引:1,他引:0
为提高大豆(Glycine max(L.)Merrill)遗传转化效率建立了一种快速而有效的草丁膦筛选系统.将刺伤的子叶节外植体接种于含有pCAMBIA3201载体的LBA4404农杆菌溶液.目前利用草丁膦筛选转基因大豆的常规方法是在含有5 mg/L草丁膦的芽诱导培养基和含有3~5 mg/L草丁膦的芽伸长培养基上进行筛选.利用此常规筛选方法所获得的大多数植株是非转化体,从而导致转化效率变低,为1.6%;而且这种方法极大地延迟了芽的伸长过程,使多数不定芽的伸长发生在农杆菌处理后的21~41周.为此,对常规草丁膦筛选方法进行了改良.首先将外植体放置在不含有除草剂的芽诱导培养基上培养3周,然后转到含有4 mg/L草丁膦的芽伸长培养基上进行筛选.此时,多数不定芽仅在7~12周内便可伸长.当芽长到3~5 cm时,从外植体上切下来转到含有1~5 mg/L草丁膦的根诱导培养上进行进一步的筛选.结果表明,在添加有3 mg/L草丁膦根培养基上,转化效率达到最大值为6.7%.不定芽对根培养基中的除草剂反应迅速,仅在10d天内所有非转化体都变枯死亡.利用这种改良的筛选系统,大多数转基因植株仅在8~16周内便可获得.Southern杂交结果证实了外源基因稳定地整合在大豆基因组中.GUS检测和除草剂抗性分析结果表明,被整合的外源基因在大豆细胞中得到了稳定的表达. 相似文献
12.
2个葡萄品系外植体愈伤组织诱导和植株再生 总被引:12,自引:0,他引:12
进行了无核白、红地球2个葡萄品系外植体愈伤组织诱导和植株再生的研究。通过葡萄品系无核白、红地球叶片和叶柄外植体的愈伤组织的诱导、再分化,以器官发生途径实现植株再生。结果表明:(1)愈伤组织诱导以MS+BA5mg/L+NAA0.5mg/L+蔗糖40g/L培养基最佳,诱导率为35%;同一葡萄品种的叶片与叶柄诱导愈伤组织的频率基本相同,而红地球外植体诱导愈伤组织的频率高于无核白;(2)不定芽的诱导再生以1/2MS+BA0.5mg/L+NAA0.05mg/L+CH500mg/L+蔗糖30g/L培养基最佳,平均诱导率达35.4%;叶柄来源的愈伤组织诱导不定芽的频率高于叶片愈伤组织;(3)根系的诱导以1/2MS+KT0.5mg/L+IBA1.0mg/L+AC2g/L+蔗糖15g/L培养基最佳,无核白和红地球来源的不定芽诱导生根频率基本相同,都在80%以上。 相似文献
13.
尾叶桉U6遗传转化再生体系的建立 总被引:1,自引:0,他引:1
以桉树品种尾叶桉U6叶盘为外植体,选用MS培养基为基本培养基,附加激素6-BA,IAA,IBA,NAAA,通过研究不同激素浓度组合对外植体愈伤诱导及不定芽分化的影响,建立了较好的遗传转化再生体系.结果表明,尾叶桉U6叶盘最适分化培养基为MS 6-BA 2.0 mg/L 2,4-D 1 mg/L IAA 0.2 mg/L 蔗糖30 g/L 琼脂粉5 g/L;小苗的最佳生根培养基为MS NAA 0.2 mg/L mA 0.5 m/L 蔗糖30 g/L 琼脂粉5 g,L.40mg/L卡那霉素可以抑制叶盘的分化;20 mg/L卡那霉素可以抑制再生植株的生根.2种抑菌抗生素中,头孢霉素对叶片再生影响较大;而250 mg/L的羧苄青霉素能有效地抑制农杆菌菌株EHA105的生长,却对尾叶桉叶盘的芽分化影响不大,为适宜的抑菌抗生素.3种农杆菌LBA4404,EHA105,GV3101的菌液浸染桉树叶盘,统计其愈伤组织GUS染色率,以EHA105对外植体的浸染能力最强,达83.3%. 相似文献
14.
Regeneration potentials in Gerbera jamesonii Bolus ex. Hook f. from tissues culture system was studied using leaf, petiole and root explants. In vitro regeneration, callus induction and root formation were optimized by manipulation of growth regulators during organogenesis. Various kinds of plant growth regulators such as 6-Benzylaminopurine (BAP), alpha-Naphthalene acetic acid (NAA), 2, 4-Dichlorophenoxyacetic acid (2,4-D), Indole-3-acetic acid (IAA), Indole-3-Butyric acid (IBA), N6-[2-Isopentenyl]adenine (2iP), Kinetin and Zeatin were used to initiate cultures. These plant growth regulators were added to Murashige and Skoog medium in different combinations and concentrations. Adventitious shoots were obtained from petiole explants cultured on Murashige and Skoog (MS) medium supplemented with 2.0 mg L(-1) BAP and 0.5 mg L(-1) NAA. Effectiveness of shoot regeneration medium, type of growth regulator used and duration of induction period were investigated. Leaf explants cultured on MS medium supplemented with 1.0 mg L(-1) BAP and 2.0 mg L(-1) 2, 4-D showed the best results for callus induction. Root explants were found to be non-regenerative in all experiments conducted. Petiole segment was identified as the best explant for regeneration of this species. Regenerated plants were rooted on Murashige and Skoog basal medium. Plantlets were then transferred to field with 75% survival rate. 相似文献
15.
Shirley Yee Birt Stevens Shirlyn Coleman Jane E. A. Seabrook Xiu-Qing Li 《American Journal of Potato Research》2001,78(2):151-157
The shoot/plantlet regenerationin vitro of seven potato (Solanum tuberosum L.) cultivars from petioles with intact leaflets was assessed using six treatment combinations-a basal medium with or without silver thiosul-phate (STS) or thidiazuron (TDZ) at two concentrations (2 or 0.5 mg/l) of the indoleacetic acid (IAA). The basal medium consisted of Murashige and Skoog (MS) salts and vitamins supplemented with 3 mg/1 6-benzylaminopurine, and 1 mg/1 gibberellic acid, 30 g/l sucrose, and 7.0 g/l PHYTOAGAR. Two full sets repeats and one partial set repeat of independent experiments were conducted and all produced similar results. Silver thiosulphate decreased the regeneration frequency and number of shoots per callus. No significant changes were observed with thidiazuron. Regeneration rates of (100% ) with up to 20 shoots/plantlets per callus were achieved at 2 mg/1 IAA with cultivars Désirée, Kennebec, Niska, and Lenape. These cultivars still showed high regeneration rates (87%–98% ) on media with 0.5 mg/1 IAA, and good regeneration rates were also achieved by the other three cultivars (48%, 94%, and 50% for Chieftain, Russet Burbank, and Shepody, respectively). Even with the single medium protocol (0.5% IAA without thiosulphate or thidiazuron), Désirée, Lenape, and Niska exhibited a regeneration rate of 98%. The use of petiole-with-leaflet explants could be ideal for the regeneration step of potato genetic transformation protocol because of their high regeneration efficiency and their small cut surface area forAgrobacterium elimination after co-incubation. 相似文献
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17.
为解决油菜组织培养中组培苗生根细短、移栽不易成活的问题,以甘蓝型半冬性油菜转化pCAMBIA1301空载体的再生植株为材料,从生根时间、根长、根重、苗高、苗重、总重、生根数、生根率等方面,以MS和B5为基础培养基,分别使用琼脂糖、琼脂粉及植物凝胶为凝固剂时再生苗的生根效率,得到了两种基础培养基的最适凝固剂组合;在以上两种组合的培养基中分别加入不同浓度蔗糖,进一步比较生根情况和成本,认为含20 g/L蔗糖的B5琼脂粉培养基为最优配方。利用优化后的生根培养基配方,极大地促进油菜组培苗的生根长度和数目,提高后期移栽成活率。 相似文献
18.
R. Ayadi L. Hamrouni M. HananaM. Trifi M.L. Khouja 《Industrial Crops and Products》2011,33(2):474-480
The present study report a protocol for the efficient in vitro propagation of kenaf (Hibiscus cannabinus L., an industrial crop having high cellulosic fiber content) on hormone free MS medium using the shoot apex and nodal explants. Shoot tips and nodes were isolated from 15 days old seedlings cultivated on MS medium. Different combinations and concentrations of auxin/cytokinin were used and added to the MS medium to assess the shoot and root induction of theses explants. Several subcultures were drived in order to enhance the multiplication rate. Healthy and well developed in vitro propagated shoots were transferred for acclimatization under greenhouse conditions in pots filled with different substrates (sand + compost or perlite). Our results showed that shoots could elongate and root within 4-6 weeks on MS basal medium without any callus formation. However, addition of growth regulators to the MS medium leaded to a decrease in shoot and root induction rates. Indeed, the highest shoot regeneration frequency (90.5%) was obtained on MS control medium. Elongated shoots were transferred onto the same hormone free MS medium using five subcultures where the multiplication rate reached the highest value (3.66) at the fifth and last step. The in vitro rooted plantlets were acclimatized in greenhouse and successfully transplanted to natural conditions with 70% survival. 相似文献
19.
不同处理方法对马铃薯茎尖成苗率的影响 总被引:2,自引:0,他引:2
试验以带马铃薯病毒的N88为材料,分别在40℃/25℃(4 h/20 h)的变温环境中,培养2、3、4周处理后茎尖剥离;以N88和D575试管苗为材料,在加入0,20,30 mg·L-1病毒唑的培养基中处理40 d后茎尖剥离。茎尖培养基为MS+0.05 mg·L-1 NAA+0.1 mg·L-1 6-BA+0.1 mg·L-1 GA3+4 g·L-1琼脂粉+30 g·L-1白砂糖的改良固体培养基,30 d后开始调查成苗率,每隔10 d调查1次,直到60 d,统计茎尖成苗率。结果表明:2周变温处理的茎尖成苗率和对照接近,但脱毒率有所提高;4周变温处理剥离茎尖成苗率最低,60 d成苗率仅为15%,脱毒率为100%;病毒唑浓度对不同材料的茎尖成苗率影响不同,其中D575经过20 mg·L-1病毒唑处理,茎尖培养60 d后成苗率最高达到83.3%,PVS脱除率为40%;材料N88在加入20 mg·L-1和30 mg·L-1浓度病毒唑的培养基中培养40 d后茎尖剥离,60 d成苗率分别为40.0%和41.7%,PVY、PLRV的脱毒率为100%。 相似文献
20.
To reduce the time period for in vitro regeneration in annatto (Bixa orellana L.), a highly efficient two-stage plant regeneration protocol had been developed that can be used commercially. Different types of explants: nodal shoot tips, shoot tips and single nodes from in vitro grown seedlings were inoculated onto the Murashige and Skoog (MS) medium supplemented with different concentrations and combinations of plant growth regulators. Highest number of shoot buds was obtained when nodal shoot tip explants were inoculated onto MS medium supplemented with 31.1 μM N6-benzyladenine (BA) and 14.7 μM phenylacetic acid (PAA). PAA in combination with BA exhibited a synergistic effect on shoot multiplication and elongation. Sub-culturing of the shoots onto the MS medium supplemented with BA (13.3 μM) and PAA (7.3 μM) produced elongated shoots. Elongated shoots when inoculated onto the MS medium supplemented with 4.9 μM indole-3-butyric acid (IBA) produced optimal rooting. The rooted plantlets were hardened and their field survival rate after 6 weeks time was 73%. 相似文献