Somatic Embryogenesis and Plant Regeneration from Leaf Callus of Hordeum vulgare

Explants obtained from the basal portion of leaves of Hordeumvulgare (cv. Karan 92) gave rise to callus when cultured onMurashige and Skoog (MS) basal medium supplemented with 2, 4-dichlorophenoxyaceticacid (2, 4-D). Initially, the callus was friable, shiny-whiteand watery but subsequently some compact, nodular callus appeared.The latter were cultured on MS medium containing 0.05 mg l^–12, 4-D and 0.1 mg l^–1 N6-furfurylaminopurine (kinetin),when plantlets were generated. Histological studies showed thatplantlet regeneration occurred by the formation of somatic embryos.The regenerated plants had the normal diploid chromosome number(2n = 14). Hordeum vulgare, barley, somatic embryogenesis, tissue culture, plant regeneration     

Somatic Embryogenesis and Plant Regeneration from Cultured Leaf Explants of Zea mays

Young leaf segments of Zea mays L. seedlings were cultured onMurashige and Skoog's basal nutrient medium supplemented with2 mg l^–1 2, 4-D and sub-cultured on medium containing8 mg l^–1 2,4-D. Two types of callus tissues appeared—embryogenicand non-embryogenic. The embryogenic callus tissue producednumerous somatic embryos which on transfer to media containinglow amounts of 2,4-D or ABA produced plantlets. Callus tissuesexhibited embryogenic potential for more than 1 year. Zea mays L. cv. Ageti-76, Zea mays L. cv. N-L-D-Comp., maize, leaf, callus, somatic embryogenesis, regeneration     

Histology of Somatic Embryogenesis from Leaf Explants of the Oil Palm Elaeis guineensis

Histological analysis was carried out during the sequence ofevents which lead to the obtaining of somatic embryos of oilpalm. Calluses from the division of perivascular cells formedat the veins of young leaf explants. Subsequent proliferationof histologically similar nodules was by means of a cambium-likezone. Under certain conditions these calluses consisted almostentirely of meristematic cells. They then differentiated rapidly:the cambium-like zone fragmented, leading to protuberance inwhich the cells divide rapidly; epidermal structures were formed,with a network of procambial strands, and synthesis of storagelipids accompanied the formation of these embryo-like structureswhich developed into clumps of true somatic embryos, each witha shoot apex and a root apex. Other structures frequently observedduring in vitro culture are also described and show that alternatepathways do exist. The structure and evolution of somatic embryosare compared to those of zygotic embryos. Storage lipids emergeas an early tracer of the satisfactory development of tissuetowards somatic embryogenesis. Oil palm, Elaeis guineensis, histology, somatic embryogenesis, callogenesis, storage lipids     

Genotype Dependent Somatic Embryogenesis and Regeneration from Leaf Base Cultures of Sorghum bicolor

A simple and reproducible protocol for callus induction and regeneration of plantlets from leaf base cultures of agronomically important Indian cultivars of Sorghum bicolor(L.) Moench (296 Band RS 585) has been developed. A strong genotype dependent response was observed and the genotype 296 B was found to be the most responsive as compared to the other genotypes tested. Cultures were raised from the III, IV and V leaf bases, excised from 12-day-old in vitro raised plantlets and cultured on Callus Induction Medium (CM). Callus initiation took place after 10-14 days of culture. The explants were maintained on this medium for 30- 35 days, after which they were transferred to Regeneration Medium (RM). Histological examination indicated that somatic embryogenesis was prevalent in the leaf base cultures and the embryos started to germinate after 15-20 days of transfer to RM. Plantlets with complete shoot and root system have been raised with as many as 30 plantlets regenerating from a single explant. These plantlets could be easily separated from one another and transferred to culture tubes for faster growth and development. Later, individual plants numbering more than 50 were transferred to pots containing soil: soilrite (1:1) for hardening. A high regeneration frequency of up to 40 % could be obtained in the genotype 296 B followed by 10.8 % in the genotype RS 585 and 7.8 % in C 43.     

木薯体细胞胚胎发生及植株再生研究

对木薯体细胞胚胎发生的影响因素进行了优化研究。结果表明,基因型对木薯体细胞胚胎发生影响很大,在供试的六个品种中,“华南 8 号”的体细胞胚胎发生率和产胚量最高,分别为 65% 和19个;侧芽茎尖为最佳外植体,体细胞胚胎发生的最佳培养基为MS +0.5mg/L CuSO4 + 4 mg/L 2,4-D。同时,对木薯体细胞胚再生成完整植株的主要影响因素作了分析,建立了一个高效的植株再生体系。     

从长寿花嫩叶直接诱导体细胞胚和出芽

1　植物名称　长寿花 (Kalanchoeblossfeldiana) ,又名寿星花、矮生伽蓝菜。2　材料类别　盆栽植物的嫩叶片。3　培养条件　基本培养基为MS。诱导培养基 :( 1 )MS +NAA 1 .0mg·L- 1 (单位下同 ) + 6 BA1 .0 ;( 2 )MS +NAA 1 .0 ;( 3)MS + 6 BA 1 .0。生根培养基为 :( 4 ) 1 /2MS不加任何生长调节剂。以上培养基含 2 %蔗糖、0 .6%琼脂 ,pH 5 .8。培养温度( 2 5± 2 )℃。4　生长与分化情况　嫩叶外植体经 70 %酒精消毒 1 5s和 0 .1 %升汞消毒 8min后 ,以无菌水清洗。切成 1cm× 1cm大小的切段 ,接种于诱导培养基上培养。嫩叶外植…     

1-Aminocyclopropane-1-Carboxylic Acid Enhanced Direct Somatic Embryogenesis from Oncidium Leaf Cultures

Influence of the ethylene precursor 1-aminocyclopropane-1-carboxylic acid (ACC) and two ethylene inhibitors, silver nitrate (AgNO₃) and cobalt chloride (CoCl₂), on direct somatic embryogenesis were tested in vitro using leaf cultures of Oncidium cv. Gower Ramsey. Leaf cells of tips, adaxial sides and cut ends could directly form somatic embryos on a hormone-free 1/2-strength MS medium. The frequency of embryo-producing explants was 55, 52.5 and 30 %, respectively. The embryo numbers per embryo-producing explant was 20.3. ACC at lower concentrations (5 and 10 μM) significantly retarded direct embryo formation from cut ends. However, higher concentrations of ACC (20 and 50 μM) significantly promoted embryogenic response of leaf tips and adaxial sides. All concentrations of AgNO₃ and CoCl₂ significantly retarded direct embryo formation. The best response was found on 20 μM of ACC, and the frequency of embryo-producing explants were 90, 85 and 35 % on leaf tips, adaxial sides and cut ends, respectively. The embryo numbers per embryo-producing explant was 32.2. This revised version was published online in July 2006 with corrections to the Cover Date.     

Somatic Embryogenesis in Cassava: The Anatomy and Morphology of the Regeneration Process

Anatomical and morphological studies demonstrated that somaticembryos developed similarly on mature seed and clonal leaf explantsof cassava (Manihot esculenta Crantz) cultured for 20–24d on Murashige and Skoog (MS2) basal medium supplemented with4.0 mg l^–1 2,4-D (Stage 1) before transfer to MS2 basalmedium supplemented with 0–01 mg l^–1 2,4-D and 0–1mg l^–1 6-benzylaminopurine (Stage II medium). Within 7d of inoculation onto Stage I medium, cell divisions occurredin the adaxial tissues of cotyledon-piece and leaf-lobe explants,and associated with this was the development of embryogeneticprotusions and ridges on the adaxial surface. Foliose structuresand somatic embryo initials developed from these tissues oncotyledon, embryonic axis and leaf-lobe explants and, when cultureswere transferred to Stage II medium, further somatic embryodevelopment occurred. Somatic embryos apparently originatedfrom groups of cells and were identified by the presence ofa closed root axis, a shoot axis and cotyledons of similar shapeand venation to those of zygotic embryos. Somatic embryos hadno vascular connection with parental cultures. Manihot esculenta, cassava, somatic embryogenesis, tissue culture, anatomy, morphology, morphogenesis     

Plant Regeneration Through Somatic Embryogenesis in Leaf Derived Callus of Plumbago Rosea

Regeneration of Plumbago rosea L., a rare medicinal plant, via somatic embryogenesis in callus cultures derived from leaf explants was described. Optimum callus formation was achieved on semi-solid Murashige and Skoog (MS) medium supplemented with 0.25 mg dm^–3 kinetin and 2.0 mg dm^–3 1-naphthaleneacetic acid (NAA). Somatic embryogenesis was achieved upon transferring the 4-week-old callus to a medium containing 1.0 mg dm^–3 kinetic (Kn), 0.5 mg dm^–3 gibberellic acid (GA₃) and 0.1 mg dm^–3 NAA. Embryo maturation and germination was achieved on the half-strength MS basal salts supplemented with 0.01 – 0.25 mg dm^–3 Kn and 2 % (m/v) saccharose. An average of 50 – 60 plantlets were obtained from 150 mg of embryogenic callus within 4 week of subculture. Out of the 50 plantlets about 28 survived in the greenhouse.     

落叶松体细胞的胚胎发生

简要回顾了重要用材树种落叶松体细胞胚胎发生的研究历史,并对落叶松体细胞胚胎发生的基本步骤、影响体细胞胚胎发生的因素及其主要应用,进行了综述,同时就落叶松体胚发生的研究趋势作了展望.     

Histological Analysis of Organogenesis and Somatic Embryogenesis Induced in Immature Tissues of Stylosanthes scabra

A well established protocol for in vitro germination of Stylosanthesscabra zygotic embryos was achieved. The response of S. scabraembryonic tissues cultured in vitro was highly dependent onthe kind of growth regulator used. Organogenesis was obtainedby using BAP, otherwise somatic embryogenesis was induced by2, 4-D. Histological aspects of both methods of regenerationwere evaluated. Endogenous neoformed buds seem to develop fromdeepseated vascular nodule structures into callus tissue. Besides,a direct somatic embryogenesis of a multicellular origin issuggested. Stylosanthes scabra, histology, organogenesis, somatic embryogenesis     

乔纳金叶片培养胚状体发生体系的建立

利用乔纳金无菌苗叶片培养,成功地诱导出胚状体并获得再生植株。具体步骤如下:Ⅰ.在MS BA2.0mg.L-1 IAA6.0mg.L-1 2,4-D0.3mg.L-1培养基上预诱导6d;Ⅱ.在MS BA2.0mg.L-1培养基上胚性细胞发生胚状体;Ⅲ.在MS BA0.5mg.L-1 IAA0.1mg.L-1上壮苗培养20d;Ⅳ.在MS IBA0.8mg.L-1 IAA0.7mg.L-1培养基上小植株生根。     

Identification of a Phosphoprotein Expressed During Somatic Embryogenesis in Wheat Leaf Base Cultures

2,4-D mediated induction of somatic embryogenesis in wheat is enhanced in the presence of Ca⁺⁺ and its removal by EGTA reduces the response significantly. Changes that occur at the polypeptide level following 2,4-D treatment were analysed. Intense cell division activity was discernable in the leaf base explants within an hour of treatment. Changes in protein profiles were prominent in the membrane fraction as compared to the soluble fraction. The protein profile of the leaf base culture with somatic embryos was distinct from the calli induced from mature embryos on a 2,4-D containing medium. The role of Ca²⁺ in the induction of somatic embryogenesis was demonstrated by the use of EGTA (a calcium chelator), verapamil, nifedipine (calcium channel blockers), W7 (calmodulin antagonist) and Li (PI inhibitor). ^{In vitro} protein phosphorylation studies showed that 2,4-D, calcium and related treatments inhibit phosphorylation of proteins. In the membrane fraction proteins, accumulation of polypeptides at the low molecular weight range was seen in samples treated with verapamil and W7, and a 30 kO polypeptide in the samples treated with calmodulin antagonist, W7. Autoradiography of membrane fraction proteins displayed the presence of a 16 kO protein phosphorylated in samples treated with verapamil, nifedipine and W7. It thus appears that 2,4-D and Ca⁺⁺ prevent the phosphorylation of this phosphoprotein. These results thus indicate the action of 2,4-D via the Ca²⁺-CaM signaling pathway in triggering the induction of somatic embryogenesis.     

云杉属树种的体细胞胚胎发生

综述了云杉属树种体细胞胚胎发生的研究现状,其中包括：（1）影响云杉属树种体细胞胚胎发生及其植株再生的因素;（2）云杉属树种体细胞胚胎发生的形态学和细胞组织学研究。并展望了云杉属树种体细胞胚胎发生的应用前景及研究方向。     

Factors Affecting Somatic Embryogenesis from Cotyledonary Explants of Safflower

Frequency of safflower (Carthamus tinctorius L.) somatic embryogenesis, number of somatic embryos per responding explant and somatic embryo maturation and germination were affected by genotype, explant age, carbon source, and ethylene. Among 8 cultivars tested, 7 were embryogenic with varying frequencies. The best response was obtained with cv. Girna. Whole cotyledonary explant from 10-d-old plants was best responding compared to 5- or 15-d-old ones. Among different carbon sources, sucrose at 87.6 mM concentration was most suitable for embryo induction, maturation and germination. Of the different ethylene inhibitors, silver nitrate at 50 [micro ]M concentration significantly increased the embryogenic frequency and also the number of embryos per responding explant. Silver nitrate has pronounced effect on embryo maturation but had no effect on germination.