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1.
Genotypic and exogenous factors affecting shoot regeneration from anther callus of linseed (Linum usitatissimum L.) 总被引:1,自引:0,他引:1
Summary The objective of this study was to investigate factors affecting the regeneration capacity of linseed anther culture. Four different environmental conditions in a phytotron were tested with regard to their effects on anther donor plants of cv. Hella. Anther response and shoot regeneration from anther callus was maximal when donor plants were grown in a 16 hrs-day at 14°C day/8°C night temperature. Anthers of four linseed genotypes were cultured on different media. Maximum shoot regeneration was achieved when the induced calli were transferred onto a modified N6 medium containing zeatin (1 mg l-1). Most of the calli regenerated shoots in the second subculture on regeneration media. Shoots were rooted on modified B5 or MS media containing NAA (0.1 mg l-1). Cytological examinations of incubated anthers and root tips of regenerated plants indicated that the anther calli were derived from microspores.Abbreviations B5
Gamborg's (1975) medium
- BAP
6-benzylaminopurine
- 2,4D
dichlorophenoxyacetic acid
- N6
Chu's (1978) medium
- NAA
-naphthaleneacetic acid
- MS
Murashige & Skoog's (1962) medium
- ZEA
zeatin 相似文献
2.
B. S. Ahloowalia 《Euphytica》1982,31(3):755-759
Summary A procedure for plant regeneration from callus culture of potato, Solanum tuberosum L. is described. Calli were induced from 1–2 mm long shoot apices of potato cultivars Cara and A25/19 on half-strength Murashige and Skoog's medium (half-MS) supplemented with 3.2 mg IAA (indole-3-acetic acid), 1.0 mg kinetin (6-furfurylamino)purine], and 0.5 mg 2,4-D [2,4-dichlorophenoxy)acetic acid]/1. Sixty percent explants produced nodular calli on this medium within 30 days. Calli differentiated into shoot-primordia when subcultured on half-MS medium supplemented with 0.5 mg 2,4-D and 1.0 mg zeatin [6-(4-hydroxy-3-methybut-2 enylamino)amino purine]/1. Differentiated calli on half-MS medium without growth hormones produced complete plantlets which were cloned on the same medium and transferred into soil. 相似文献
3.
T. Yamada 《Euphytica》1989,44(3):181-186
Summary Callus cultures were induced from hypocotyl sections of 24 varieties of white clover (Trifolium repens L.). The calli did not show any significant difference of growth among the varieties. After the calli has been transferred to three regeneration media, green-spot formation was observed on calli derived from some seedlings. Remarkable intra- and intervarietal variations in the emergence of green spots and some trends between the origin of varieties and the frequency of green spots were observed. In most cases, the green spots turned brown without showing further differentiation, and only two genotypes formed shoots. A callus from a seedling of the Swedish variety Undrom has sustained high levels of plant regeneration throughout 24 months of culture. Protoplasts derived from this selected genotype were divided into cell colonies. 8P (Kao, 1977) medium containing 0.5 mg/1 2,4-D and 0.5 mg/1 kinetin was the most suitable medium for inducing divisions in protoplasts. When subcultured into solid B5 medium, the colonies produced calli, which when transferred to a regeneration medium, formed shoots. This genotype is expected to a useful subject for genetic engineering of white clover.Abbreviations 2,4-D
2,4-dichlorophenoxyacetic acid
- IAA
indole-3-acetic acid
- 2ip
6-, -dimethylallylamino purine
- NAA
-naphthaleneacetic acid 相似文献
4.
Summary Foreign DNA was introduced into cell suspension cultures and leaf tissue of Eustoma grandiflorum Griseb. (lisianthus) by microprojectile bombardment. For this purpose a low-cost bombardment device that uses a helium flux to accelerate microprojectiles was built. When cell suspensions were used, an average of 4.1 Kan resistant calli were recovered per shot after 4 months' cultivation on selective medium. Most of the Kan resistant plants regenerated from calli were positive to GUS assay. Both the nptII and gus genes were successfully amplified from alkali-treated leaves of putative transgenic plants by PCR analysis. Transgenic plants were not recovered from bombarded leaves. Considering the host range specificity of Agrobacterium, and the response of the species to plant regeneration from suspension culture, microprojectile bombardment is, at present, the most efficient procedure for genetic transformation of lisianthus.Abbreviations BA
6-benzyladenine
- Cx
cefotaxime
- 2,4 D
(2,4-dichlorophenoxy) acetic acid
- FDA
fluorescein diacetate
-
gus
-glucuronidase
- IAA
indole-3-acetic acid
- IBA
indole-3-butyric acid
- 2iP
(2-isopentenyl) adenine
- Kan
kanamycin
-
nptII
neomycin phosphotransferase II
- PCR
polymerase chain reaction 相似文献
5.
花生与其近缘野生种间细胞融合及杂种愈伤组织的形成 总被引:1,自引:1,他引:0
本研究旨在为体细胞杂交法在花生育种中的应用奠定基础。将花生栽培种Krapts和野生种A. stenosperma幼叶解离的原生质体,用PEG方法融合后,置于添加2 mg/L毒莠定(Pic)、0.1 mg/L苯基噻二唑基脲(TDZ)、2%的椰乳、5 g/L聚乙烯吡咯烷酮(PVP)和0.1% 2-吗啉乙磺酸(MES)的改良MSB5(MS无机盐+B5有机成分)液体培养基中进行浅层培养。5周后将形成的小愈伤组织转移到添加3 mg/L玉米素(ZT)、0.2 mg/L 6-苄氨基嘌呤(BAP)、0.1 mg/L 萘乙酸(NAA)的固体培养基上进行培养,促使愈伤组织增殖。观察发现,融合处理的原生质体在液体培养基上培养4天后开始分裂,2周后形成直径约300 μm的细胞团,5周后小愈伤组织直径可达2~3 mm。当将小愈伤组织转移到固体培养基上后,愈伤组织迅速增殖,并获得大量愈伤组织。提取愈伤组织DNA进行PCR检测,部分愈伤组织扩增出了双亲特异的DNA条带或双亲都不具有的新条带,说明愈伤组织来自于融合细胞。 相似文献
6.
Microspore response of three- way cross maize hybrid genotype 3AL/95 (Zea mays L.) was studied under simplified isolation and culture conditions. Fertile plant production was achieved through abundant plant
regeneration. As a total, microspores of 160 tassels were inoculated and five sustainable microspore derived callus cultures
(SMC) were obtained. Hybrid seeds (ML SC), which were produced by crossing of regenerates from two SMCs, gave rise to subsequent
vigorous and fertile progeny. The response of the 3AL/95 and ML SC microspores was studied in three liquid culture media in
order to improve the early viability of microspores. Them N6M medium provided better survival of cultured microspores (p = 5%) than the ppN6M/89 and the YPM-G media. The pH 5.8 in mN6M medium revealed significant increase (p = 1%) in microspore viability as compared to pH 3.0. The ML SC microspores showed higher viability(30%) on the first day
of culture in the mN6M than those of the3AL/95 (19%) but without improved rate of callus formation and plant regeneration.
This revised version was published online in August 2006 with corrections to the Cover Date. 相似文献
7.
B. S. Ahloowalia 《Euphytica》1987,36(2):659-665
Summary Plants were regenerated from callus cultures initiated from immature embryos of barley, Hordeum vulgare L. Immature embryos from seven diverse genotypes were cultured on modified Murashige and Skoog (MS) medium supplemented with 1.5 mg 2,4-D and 6.5 mg IAA/l. Of the 249 embryos cultured, 30% initiated callus within 8 days. Subculture of callus for 80 to 100 days on half-MS medium supplemented with 0.5 mg/l 2,4-D and 1.0 mg/l zeatin resulted in organogenesis. Culture of organogenic calli for 30 days on half-MS medium without growth regulators produced plants which originated mostly via multiple shoot formation. Callusing response of the tested genotypes ranged from zero to 44%; however, only 23% of the calli were regenerative. Regenerated plants included variants for chlorophyll deficiency, plant height, stem thickness, spike shape, pollen fertility, seed set and ploidy. 相似文献
8.
Plant regeneration from protoplasts of Iris germanica L. 总被引:1,自引:0,他引:1
Summary Protoplasts were isolated enzymatically from suspension cultures derived from embryogenic calli induced by leaf base culture of Iris germanica. In protoplast culture, the effects of glucose concentration, different sugars and combinations of 2,4-D and KIN on protoplast division and colony formation were examined. N6 medium supplemented with 0.1–1 mg/l 2,4-D, 1 mg/l KIN, 200mg/l casein hydrolysate, 250 mg/l proline, 0.2 M glucose and 20 g/l agarose was suitable for protoplast division and colony formation. When colonies formed were transferred onto hormone-free MS medium, many plantlets were regenerated through somatic embryogenesis. Thus, we could establish a plant regeneration system from protoplasts of I. germanica.Contribution from the Laboratory of Plant Breeding, Faculty of Agriculture, Miyazaki University, Japan, No. 95. 相似文献
9.
Summary Chromosome number of morphogenic and non-morphogenic calli and regenerated plants of barley were determined. Cultures were obtained from two kinds of explants, immature embryos and seedling leaves from three cultivars, Ingrid, Dissa and Golden Promise. Callus chromosome analyses were carried out during a 12 month period in a medium containing 2 mg/l of 2,4-D. Diploid cells were predominant in all cases; although in leaf-derived cultures, retraploid cells (2n=4x=28) showed a tendency to increase as time in culture increased and after more than six months in culture, diploid cells decreased to percentages of almost 70%. Aneuploid cells were generally infrequent in all cases. The source of explant has been more important than the genotype (cultivar) and the type of callus (morphogenic vs. non-morphogenic) in the chromosomal stability of cultures as time increases. From short term cultures, only 1.85% of the regenerated plants were tetraploid, the remaining were diploids. The ability of morphogenic calli to regenerate plants decreased before any significant reduction of diploid cells were observed. 相似文献
10.
The effect of colchicine on induction of embryogenesis andchromosome doubling during microspore culture was evaluated in twoF1 hybrids of spring oilseed rape (Brassica napus L.). Immediatecolchicine treatment of isolated microspores with the concentrations 50 and500 mg/L for 15 h stimulated embryogenesis and produced largeamounts of healthy-looking embryos. These normal embryos germinatedwell at 24 °C after being transferred to solid regeneration mediumand an initial period of low temperature (2 °C) for 10 days, andcould directly and rapidly regenerate vigorous plants. A high doublingefficiency of 83–91% was obtained from 500 mg/L colchicinetreatment for 15 h with low frequency of polyploid and chimeric plants.The present experiment showed that a treatment duration of 30 h revealedless positive effects on embryogenesis and doubling efficiency, especially athigher colchicine concentration (1000 mg/L). Poor embryogenesis andembryo germination were observed from ordinary microspore culturewithout change of induction medium and colchicine treatment, and severalsubcultures were required for induction of secondary embryogenesis andplant regeneration. 相似文献
11.
Callus induction and plant regeneration from anther and inflorescence culture of Sorghum 总被引:1,自引:0,他引:1
Summary Twenty-five inbred lines, including grain and forage types from the USA and China, two hybrids, one Sorghum almum, and one Parasorghum (S. versicolor) were tested for their response to anther culture. Three nutrient media were effective in inducing anther calli from six cultivars (Xin White, TX 403-TSB, DDY Sommer Milo, TX 2779, Brawley, and Spur Federal) and one was effective for plant regeneration for one cultivar, Xin White. Averaged over media, callus induction frequency (number of calli per 100 anthers) was highest in cultivars Xin White and TX 403-TSB (6.7 and 3.9%, respectively). The means of cultivars for media C17-2 and Ms-t-z-2, 4.3 and 3.2%, respectively, were superior to that for medium 85D3-2 (0.1%). Expressed as an average of the six cultivars and three media the mean calli induction frequency was 2.6%; however, differential responses of genotype and medium were noted. Among the 10 regeneration media tested, medium MS-d-4 containing Murashige and Skoog basal components plus 2.0 mg/l indole-3-acetic acid (IAA) and 2.5 mg/l kinetin was the most effective for plant regeneration. Numbers of albino plants and calli developing only roots increased directly with callus-induction time, whereas the frequency of plant regeneration decreased. Regenerated plants had varied numbers of chromosomes in root tip cells: 10, 15, 20, 40, and 60. The 29 regenerated plants that reached maturity, however, were highly fertile and contained only 10 bivalents in pollen mother cells. Normal chromosome number and behavior for the regenerated plants suggest that induced calli originated from cells other than microspores. However, spontaneous chromosome doubling in microspore-derived haploids may occur. The appearance of albinos also implies that haploids may have been produced from anther culture.Joint contribution of the Dept. of Agronomy and USDA-ARS, Kansas Agricultural Experiment Station, Manhattan, KS 66506-5501, USA. Contribution no. 88-566-J. 相似文献
12.
Summary Shoot development through morphological transformation in spikelets occurred after segments of young unemerged orchardgrass (Dactylis glomerata L.) inflorescences were cultured on Linsmaier and Skoog's RM medium supplemented with 0, 4.52×10-4, 4.52×10-3 and 2.26×10-2 mM 2,4-dichlorophenoxyacetic acid (2,4-D) or naphthaleneacetic acid (NAA). Effects on shoot formation were better with 2,4-D than NAA in all concentrations tested. The callus initiated from the primary culture on high 2,4-D medium was reproducible, but no evidence of shoot proliferation was noted. The shoots developed into healthy plantlets after being reared on RM medium not supplemented with hormones.Contribution from South Dakota Agricultural Experiment Station Journal Article No. 1741. 相似文献
13.
Optimization of culture conditions for improved plant regeneration efficiency from wheat microspore culture 总被引:1,自引:0,他引:1
The production of haploid plants through microspore culture is a very important tool for plant breeding. However, progress in microspore culture for many species has been hampered by a number of factors that have resulted in low recovery of regenerated green plants. In this study, a series of experiments were conducted to increase the regeneration of haploid green plants from isolated wheat microspores. The use of different basal media and variations in media components resulted in the increased recovery (approximately double) of regenerated haploid wheat plants. Our findings demonstrate that CHB medium, in combination with 2,4-d, was a better medium for embryoids induction and plant regeneration than medium MC17 with either 2,4-d or PAA growth hormones. Wheat microspores cultured without ovary co-cultivation did not respond. Furthermore, high efficiency of microspore derived embryoids (up to 296 MDEs per 100 anthers) and green plant regeneration (up to 71 green plants per 100 anthers) were achieved by the use of gelrite instead of agarose as a gelling agent, and by the addition of media additives such as spent medium or MET. 相似文献
14.
Summary Use of 2,4-D was superior to NAA or IAA for embryogenic callus initiation or maintenance in barley cultivar Bruce. A concentration of at least 2.0 mg/l 2,4-D was desirable for culture initiation. The developmental size of the embryo was more important than embryo age for obtaining embryogenic calli. Even brief exposures (20–40 days) of calli to concentrations of higher than 5.0 mg/l 2,4-D or 10.0 mg/l NAA resulted in inhibition of subsequent plant regeneration and therefore, concentrations above these could not be used for maintenance cultures. In the long-term maintenance cultures, the best production of embryogenic calli was with 0.1 mg/l and 1.0 mg/l 2,4-D. 相似文献
15.
新疆棉花4个主栽品种的体细胞胚胎发生及植株再生 总被引:15,自引:0,他引:15
以新疆4个主栽棉花品种新陆中20、新陆早24、新陆早33和03298为材料, 通过不同浓度的激素组合成功地诱导获得了体细胞胚并进一步发育成苗。研究发现, 所用的4种激素组合均能有效诱导愈伤组织, 其中又以0.02 mg L-1或0.10 mg L-1 KT和0.1 mg L-1 2,4-D组合的诱导效果最佳; 两个诱导措施有利于胚性愈伤组织的产生, 即沿中柱纵切棉花下胚轴切段, 并以纵切面接触培养基; 愈伤组织诱导培养基中KNO3用量加倍。挑选黄绿色、灰绿色或浅绿色的质地疏松的愈伤组织继代于无激素且KNO3含量加倍的培养基中可产生胚性愈伤组织, 并在高比例KT/2, 4-D(0.05 mg L-1或0.10 mg L-1 KT和0.01 mg L-1 2,4-D)促进下发育成胚。借助在培养基上垫滤纸产生干燥作用, 并间隔使用强透气效果的棉塞对培养三角瓶进行透气处理, 体细胞胚可成熟发育并产生根系发达的正常再生植株。应用此法, 4个实验材料在6~8个月内即可获得大量再生苗。 相似文献
16.
Summary Protocols for plant regeneration from cotyledon explant and anther cultures of Sinapis alba have been developed for creating doubled-haploids and somaclonal variation. Among the several cultivars tested in this study, only Arda responded well to in vitro plant regeneration both from anther-as well as cotyledoncultures. Multiple shoot formation in cotyledon explants, which always followed a brief callusing phase, was found to be the best on MS medium with ZEA (1.0mg/l) and NAA (0.1mg/l). Regeneration frequency declined sharply in the absence of auxin or presence of other cytokinins and/or auxin. The frequency of shoot regeneration also declined with reduction in the photoperiod to 16h. On MS + BAP (1.0mg/l) + NAA (1.0mg/l) medium, cotyledonary explants showed profuse callusing, which could regenerate shoots on high ZEA + low NAA/IAA medium. However, it declined with progressing time in culture. Anthers, excised from fresh as well as cold pretreated buds, cultured on 10% sucrose containing MS media with different hormonal constitution, developed calli and/or embryos. Initial culture temperature was important with embryogenesis occurring only in anthers cultured at 30°C for 3 weeks. A high temperature (35°C) treatment was lethal for both callus as well as embryo formation. While BAP + NAA and ZEA + NAA/IAA supported embryogenesis, further plant regeneration from anther-or embryo-callus could be achieved in ZEA + NAA/IAA media. Some of the regenerants flowered already in vitro and had small and sterile flowers. Cytological examination of some of the root differentiating calli indicated the presence of haploid as well as diploid cells. Shoots were rooted during prolonged incubation on the same medium or on transfer to MS (reduced)/ B5 + ZEA + NAA media. 相似文献
17.
The effect of in planta TIBA and L-proline onin vitro seedlings and cell culture of sugar beet was investigated. Sterilized seeds were grownin vitro on 1/2 MS medium supplemented with 0 or3 mg/l TIBA. Calli obtained on young leaves cultured on MS medium containing 1 mg/l
BAP, were used for the initiation of cell suspension cultures using MS basal composition supplemented with 0 or 50 mM proline.
Aliquots of 1 ml from cell suspension culture were inoculated onto the first somatic embryo induction MS medium containing
TIBA 0.5 mg/l, BAP 1.0 mg/l, and proline at 0 or 50 mM. After three weeks of culture, embryogenic calli were transferred to
the second embryo induction medium supplemented with NAA and BAP at 0.2 and 0.5 mg/l, respectively. The frequency of somatic
embryos of calli obtained from in plantaTIBA together with proline treatments on average was20 which was higher than that of the other treatments.
This revised version was published online in July 2006 with corrections to the Cover Date. 相似文献
18.
Summary A maize plant resistant to 5-methyltrytophan (5MT) was selected from M2 seeds (Zea mays L. Danggin, inbred line) originating from ears treated with ethylmethane sulfonate (0.2%) at 6 hr after self-pollination. Genetic analysis of the progeny of plants selected from a medium containing 50 ppm 5MT showed that 5MT resistance was inherited as a single dominant nuclear gene. This resistance was also expressed in callus and seedling. Analysis of the free amino acids in kernels and calli showed that homozygous resistant plants (MR1) contained higher levels of total free amino acids than sensitive plants and calli. In particular, the their kernels the levels of tryptophan, threonine and serine were, respectively, 4.5, 5.9 and 6.3 times higher than those of the sensitive plants. From the results, it may be expected that mutants resistant to amino acid anologs will be useful not only for studying amino acid biosynthesis but also for improving the nutritional quality of maize.Abbreviations EMS
Ethylmethane sulfonate
- 5MT
5-methyltryptophan
- 2,4-D
2-4-dichlorophenoxyacetic acid 相似文献
19.
Summary The possibility of producing agronomically-useful somaclones via organogenesis and somatic embryogenesis from callus cultures of pea (Pisum sativum L.) was studied. Organogenic calli were induced from immature leaflets on MSB medium with NAA and BAP. Embryogenic calli were derived either from immature zygotic embryos (using 2,4-D) or from shoot apices (using picloram) of aseptically-germinated seedlings.The seed progenies (T1 to T3-generation) of primary regenerants were grown in field conditions and their phenotypic variation was evaluated and compared with control, non-tissue culture-derived plant material. In addition, electrophoretic analyses of selected isoenzyme systems and total proteins have been done. The results do not show dramatic changes in qualitative and quantitative traits. The evaluation of at least two future generations (T4, T5) is planned.Abbreviations BAP
6-benzylaminopurine
- IBA
indole-3-butyric acid
- MSB
medium (mineral salts after Murashige & Skoog, 1962, vitamins after Gamborg et al., 1968)
- NAA
-naphthalene-acetic acid, picloram-4-amino-3,5,6-trichloro picolinic acid
- 2,4-D
2,4-dichlorophenoxyacetic acid
- ORG
organogenesis
- SE
somatic embryogenesis 相似文献
20.
Powdery mildew resistance in Kentucky bluegrass genotypes regenerated from excised seed pieces 总被引:2,自引:0,他引:2
Summary Severity of powdery mildew was assessed on seven cultivars and lines of Kentucky bluegrass propagated by seed and tissue culture. Tissue culture plants were started from embryo axes cultured on Murashige and Skoog medium containing different concentrations of 2,4-dichlorophenoxyacetic acid (2,4-D) and 6-benzylaminopurine (BAP), and incubated (1 to 4 weeks) or not incubated in the dark prior to transfer to a lighted culture room. There were significant differences in disease severity (DS) among seed propagated and tissue culture regenerated plants. DS ranged from highly susceptible (100% of leaf covered by mildew) (DS=9) to resistant (DS=3.0). In some tissue culture regenerants the disease severity was significantly affected by the tissue culture process. Ten clones expressing resistance were selected, and plants propagated vegetatively. In six clones, disease resistance was sustainable in subsequent vegetatively propagated plants, while resistance was lost in four of the selected clones. Results are discussed with a view to using tissue culture to produce Kentucky bluegrass genotypes with resistance to powedery mildew.Abbreviations BAP
benylaminopurine
- 2,4-D
2,4-dichlorophenoxyacetic acid
- DS
disease severity
- MS
Murashige & Skoog
- SDW
sterile distilled water 相似文献