Ultrastructural Changes in Leaves of Cichorium during Somatic Embryogenesis

A detailed electron microscopy study of early cellular eventsduring somatic embryogenesis in leaves of Cichorium is described.Leaves on in-vitro grown plantlets were sectioned and put at35°C, in darkness, in an agitated liquid induction medium.No sign of embryogenic predetermination, such as thick cellwall, dense cytoplasm and enlarged nucleus, could be seen inany cell before treatment. Perivascular cells were the firstto react. Addition of glycerol (330 mM) allowed the arrest ofembryogenic cells at an activated stage. The main events werea thickening of the wall, with extracellular secretion and anaccumulation of Ca²⁺ in the vacuole, demonstrated by an antimonateprocedure. After 5 d, leaves were transferred to glycerol-freemedium where multicellular proembryos could be observed. Theyshowed reduced vacuoles, cortical microtubules, numerous multivesicularbodies and lipid globules. The embryoid cells were lined alongthe mesophyll lacunae by an extracellular secretion with a tubularstructure; histochemical tests proved its complex lipo-glyco-proteicnature.Copyright 1993, 1999 Academic Press Cichorium, extracellular tubular protein, somatic embryogenesis, vacuolar calcium     

Somatic embryogenesis and plant regeneration from protoplasts of Cichorium intybus L. x Cichorium endivia L.

Somatic embryos and adult plants were regenerated from mesophyll protoplasts of a clone of chicory 474 (Cichorium intybus L. x Cichorium endivia L.). Embryos were obtained in three different ways:

胡桃楸胚性愈伤组织诱导与体细胞胚胎发生

胡桃楸是东北东部山地阔叶红松林的重要组成树种。因其被大量采伐,资源日趋枯竭。体细胞胚胎发生是快速繁殖和人工种子研制的基础,对遗传改良有重要意义。为探讨不同外植体、植物生长调节物质种类及配比对胡桃楸培养物的影响,建立了胡桃楸体胚发生及再生植株体系。结果表明:合子胚为外植体时最易形成胚性愈伤组织,外植体最佳取材时期为5～6月。胡桃楸胚性愈伤组织最适诱导为MS+1.0mg·mL-12,4-D+0.5mg·mL-16-BA;体细胞胚的诱导、发育和分化的适宜的培养基为附加蔗糖60g.L-1、水解酪蛋白700mg·mL-1时不添加任何生长调节物质的MS培养基。     

SEM Characterization of an Extracellular Matrix Around Somatic Proembryos in Roots of Cichorium

Roots of in vitro plantlets of a hybrid Cichorium intybus L.x C. endivia L. placed for 10 d in an agitated liquid inductionmedium in darkness at 35 °C give somatic embryos of varioussizes which disrupt the epidermis. Proembryos can be observedinside the root; they show a fibrillar network linking the surfacecells. The network is observed in agitated and static liquidmedium; it is not well developed on solid medium. It is notremoved by lipid solvents and pectinase but disappears partlywith protease. Ether-methanol (1:1 v/v) for 45 min and Tris-HC1buffer for 3 h at 30 °C destroy it. As in animal cells suchexternal proteic networks are constituents of an extracellularmatrix linked to the cytoskeleton, we tested microtubule destabilizationby colchicine and cold treatments which removed the network;this effect was reversed by DMSO and high temperature. Cichorium, extracellular matrix, extracellular proteins, somatic embryogenesis     

非洲紫罗兰叶片体细胞胚培养及快繁技术研究

以非洲紫罗兰叶片为材料进行胚状体诱导及快繁技术研究.结果表明:.在MS NAA0.1mg/L BA0.1 mg/L 2,4-D1.0 mg/L的培养基上培养15d利于诱导胚性细胞分化,起始黑暗培养5～10d可提高胚性细胞分化率;在MS BA0.05～1mg/L的培养基上可诱导胚状体大量发生;在MS NAA0.1mg/L十BA0.1 mg/L的培养基上能够获得茎芽快速增殖;在1/2MS NAA0.01mg/L的培养基上可以生根.     

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。     

Label-Free Quantitative Proteomics of Embryogenic and Non-Embryogenic Callus during Sugarcane Somatic Embryogenesis

The development of somatic cells in to embryogenic cells occurs in several stages and ends in somatic embryo formation, though most of these biochemical and molecular changes have yet to be elucidated. Somatic embryogenesis coupled with genetic transformation could be a biotechnological tool to improve potential crop yields potential in sugarcane cultivars. The objective of this study was to observe somatic embryo development and to identify differentially expressed proteins in embryogenic (E) and non-embryogenic (NE) callus during maturation treatment. E and NE callus were cultured on maturation culture medium supplemented with different concentrations (0.0, 0.75, 1.5 and 2.0 g L^-1) of activated charcoal (AC). Somatic embryo formation and differential protein expression were evaluated at days 0 and 21 using shotgun proteomic analyses. Treatment with 1.5 g L^-1 AC resulted in higher somatic embryo maturation rates (158 somatic embryos in 14 days) in E callus but has no effect in NE callus. A total of 752 co-expressed proteins were identified through the SUCEST (The Sugarcane EST Project), including many housekeeping proteins. E callus showed 65 exclusive proteins on day 0, including dehydrogenase, desiccation-related protein, callose synthase 1 and nitric oxide synthase. After 21 days on maturation treatment, 14 exclusive proteins were identified in E callus, including catalase and secreted protein. NE callus showed 23 exclusive proteins on day 0 and 10 exclusive proteins after 21 days on maturation treatment, including many proteins related to protein degradation. The induction of maturation leads to somatic embryo development, which likely depends on the expression of specific proteins throughout the process, as seen in E callus under maturation treatment. On the other hand, some exclusive proteins can also specifically prevent of somatic embryos development, as seen in the NE callus.     

Effect of Gamma Irradiation on Embryogenic Avocado Cultures and Somatic Embryo Development

Embryogenic avocado cultures were exposed to ionizing irradiation in order to determine its effect on proliferation and subsequent somatic embryo development. The approximate PD₅₀ as determined by linear regression is 35 Gy 2 weeks after irradiation for Fuerte 2.11.1 and 4 weeks after irradiation for T362 2.11.1. Irradiation of embryogenic cultures did not significantly affect the number of early stage Fuerte 2.11.1 somatic embryos that developed directly from irradiated cultures; however, 10–50 Gy inhibited somatic embryo development. Irradiation of T362 2.11.1 embryogenic cultures at 25–50 Gy inhibited the number of intermediate and mature stages of somatic embryos that developed directly from irradiated cultures, and 50 Gy inhibited somatic embryo maturation. Inhibition of somatic embryo development could be partially offset by proliferation of irradiated embryogenic cultures as suspensions. Irradiation up to 10 Gy significantly increased the number of mature Fuerte 2.11.1 somatic embryos that developed from suspension cultures. Irradiation with doses up to 25 Gy stimulated development of heart stage T362 2.11.1 somatic embryos; however, mature somatic embryo development was suppressed at dosages of 10 Gy and greater.     

Direct Somatic Embryogenesis in Roots of Cichorium: Is Callose an Early Marker?

Direct somatic embryogenesis can be obtained from epidermaland cortical cells in roots from in vitro Cichorium plantlets.The first embryogenic cells are seen after six days of culturein darkness, at 35 °C, in a liquid medium supplemented withNAA (1 x 10^–7 M), 6-dimethylallyl-amino-purine (2·5x 10^–6 M), sucrose (0.03 M) and glutamine (1·7x 10^–3 M). Embryogenic cells undergo first a linear andthen a globular segmentation, with increasing cytoplasmic density.These cells and young embryoids show aniline blue fluorescence.SEM allows the same microglobular pattern to be seen on thesurface of young embryoids and on young microspores of Cichoriumused as controls. In this root system, callose deposition seemsto be an early marker in somatic embryogenesis. Somatic embryogenesis, callose, Cichorium     

Histology of Organogenic and Embryogenic Responses in Cotyledons of Somatic Embryos of Quercus Suber L

In cork oak (Quercus suber L.), recurrent embryogenesis is produced in vitro through autoembryony without exogenous plant growth regulators (PGRs); secondary embryos appear on the embryo axis but seldom on cotyledons. Focusing mainly on the histological origin of neoformations, we investigated the influence of the embryo axis and exogenous PGRs on the embryogenic potential of somatic embryo cotyledons. Isolated cotyledons of somatic embryos became necrotic when cultured on PGR-free medium but gave secondary embryos when cultured on media containing benzyladenine and naphthaleneacetic acid. Cotyledons of cork oak somatic embryos are competent to give embryogenic responses. Isolated cotyledons without a petiole showed a lower percentage of embryogenic response than did those with a petiole. In petioles, somatic embryos arose from inner parenchyma tissues following a multicellular budding pattern. Joined to the embryo axis, cotyledons did not show morphogenic responses when cultured on PGR-free medium but revealed budlike and phylloid formations when cultured on medium with PGRs. The different morphogenic behavior displayed by somatic cotyledons indicates an influence of the embryo axis and indicates a relationship between organogenic and embryogenic regeneration pathways.     

Somatic Embryogenesis: Factors Influencing Coordinated Behaviour of Cells as an Embryogenic Group

A number of common features are associated with a great diversityof observations of somatic embryogenesis in vitro. There arefundamental homologies between direct and indirect somatic embryogenesis,and between single-cell and multiple-cell initiation. Many ofthe observed differences can be attributed to whether or notcells require redetermination to the embryogenic state, andto differences in the nearest neighbour relationships of initiatingcells. The observed pattern of morphogenesis depends on whethera group of cells can establish and maintain coordinated behaviouras an embryogenic unit and will be influenced by factors whichaffect intercellular communication. Somatic embryogenesis, tissue culture, cell-cell interactions     

Correlation Between Appearance of Embryogenic Cells and the IAA Levels in Rice Somatic Cell Culture

Changes of endogenous IAA level and IAA action in cultured rice ( Oryza sativa L. ) somatic cells during the period from 7th to 15th day which was the transition from somatic to embryogenic cells were observed. The study was carded out in three experimental systems viz. mature caryopsis and young panicles (2 ~ 5 mm long) of rice cv. "Guangluai 4" under normal osmosis (3% sucrose), mature caryopses from rice cv. "Yanjing 2" or "Guangluai 4" under normal and higher osmosis (5% sucrose or 2.5 % sorbitol). During this period, endogenous IAA contents were greatly increased in young-panicle calli under normal osmosis and mature-caryoptic calli under higher osmosis but decreased in mature-caryoptic calli under normal osmosis. Exogenous IAA could induce the appearance of embryogenic cell from nonembryogenic callus at a lower frequency. And 2,3,5-tri-iodobenzoic acid could increase the frequency of embryogenic cell induction. From these results it could be concluded that accumulation of higher IAA level in the cultured rice cells was essential for induction of embryogenic cell appearance. Since 2,4-D was involved in all induction medium with the same concentration but exerted different effects on embryogenic cell induction, it was suggested that it might act through mediating the endogenous IAA metabolism.     

Somatic embryogenesis and plant regeneration in Cichorium intybus L. (Witloof,Compositae)

Somatic embryogenesis of Cichorium intybus L. var. Carolus is induced using cubical pieces of mature tap roots with an intervening callus phase. A Murashige and Skoog's (MS) semi solid basal medium supplemented with 2,4-dichlorophenoxyacetic acid (0.02 or 0.2 mg/l) and benzylaminopurine (0.25 mg/l) and a liquid MS medium devoid of growth regulators are used respectively for induction of callus and somatic embryoids and for further development and germination. Regeneration from the nodular proembryonal stage to the full grown embryoids occurs following different morphological pathways depending on the physical and chemical environment of the culture. Further development of these embryos into plantlets and the possibilities of application of this technique in plantbreeding have been discussed.Abbreviations MS Murashige and Skoog medium - BAP benzylaminopurine - 2,4-D 2,4-dichlorophenoxyacetic acid     

A Novel Method for Separation of Somatic Embryos from Embryogenic Suspension Cultures by Cold Treatment

This study reports a novel method for embryo separation by cold treatment of heterogeneous suspension cultures which contain embryogenic single cells, cell clusters and embryos at various stages of development. The method was applied to embryo suspension cultures of pepper (Capsicum annuum) and sugarcane (Saccharum officinarum). In both plants, single cells lost their viability dramatically over a few days while the viability of embryos remained above 95% for 25-30 days when kept at 5 °C. The effect of duration of cold treatment on embryo germination was also tested. The optimal duration of cold treatment was found to be 10 days for sugarcane and 21 days for pepper. After the cold treatment, the germination percentages were 90% and 96% for sugarcane and pepper, respectively.     

Regulation of Separase in Meiosis: Separase is Activated at the Metaphase I-II Transition in Xenopus Oocytes during Meiosis

Separase is a cysteine protease conserved in all eukaryotes and functions to remove the sisterchromatid cohesion in anaphase by cleaving the SCC1 subunit of the cohesin complex. Theregulation of separase activity as the degradation of its inhibitor, securin, and the downregulationof the inhibitory phosphorylation has never been directly investigated in themeiotic cell cycle of vertebrates. In this study, we cloned the full-length gene encodingXenopus separase from an oocyte cDNA library. Purified xSeparase can cleave the human ?-kleisin subunit of cohesin in vitro but cannot bind with hSecurin when these two proteins areco-expressed in 293T cells. Similar to its human counterpart, xSeparase cleaves itself uponactivation but at a single site. The cleavage site is conserved with one of the three selfcleavagesites in hSeparase. Using self-cleavage as a reporter for its activation, wedemonstrated that xSeparase was transiently activated between the two meioses and may beinvolved in the homologous chromosome separation, as observed in other organisms. Takingthe advantage of the inability of xSecurin to interact with hSeparase, we demonstrated that theCSF extract re-inhibit both full-length and auto-cleaved hSeparase, indicating thatphosphorylation inhibition of separase does occur under the physiological condition. Inaddition, we found that the endogenous xSecurin was accumulated in response toprogesterone-induced oocyte maturation, and was degraded at both the anaphase I and II in anAPC/C-dependent manner.     

DNA Methylation and Embryogenic Competence in Leaves and Callus of Napiergrass (Pennisetum purpureum Schum.)

Quantitative and qualitative levels of DNA methylation were evaluated in leaves and callus of Pennisetum purpureum Schum. The level of methylation did not change during leaf differentiation or aging and similar levels of methylation were found in embryogenic and nonembryogenic callus.     

Factors Affecting Formation of Somatic Embryos and Embryogenic Callus from Unemerged Inflorescences of a Graminaceous Crop Pennisetum

Differentiation of somatic embryos was dependent on the concentrationof auxin and the mineral medium. Low levels of auxin 2,4-D inN₆ medium, a low ammonium nutrient, favoured the formation ofsomatic embryos, while on MS medium containing high ammoniumcompact tissues appeared. At higher levels of auxin, irrespectiveof nutrient medium, compact tissues were formed. The originof compact tissue on N₄ medium could be traced to somatic embryo-likestructures. This tissue regenerated into somatic embryos onhormone-free N₆ medium whereas on MS medium thalloid structuresappeared. Pennisetum, unemerged inflorescence, somatic embryo, embryogenic callus     

Enhanced Agrobacterium-mediated Transformation of Embryogenic Calli of Upland Cotton via Efficient Selection and Timely Subculture of Somatic Embryos

Agrobacterium-tumefaciens-mediated transformation of cotton embryogenic calli (EC) was enhanced by choosing appropriate EC and improving efficiency of coculture, selection cultivation, and plant regeneration. After 48-h cocultivation, the number of β-glucuronidase (GUS)-positive calli characterized by yellow, loose, and fine-grained EC was twofold greater than that of gray, brown, and coarse-granule EC. It indicated that efficiency of transient transformation was affected by EC morphology. And transient transformation efficiency was also improved by cocultivation on the medium adding 50 mg l⁻¹ acetosyringone at 19°C for 48 h. Subculturing EC on the selection medium with low cell density was beneficial to production of more kanamycin-resistant (Km-R) calli lines. From an original 0.3-g EC, an average of 20 Km-R calli lines were obtained from a selection dish and the GUS-positive rate of Km-R clones was 81.97%. A large number of normal plants were rapidly regenerated on the differentiation medium with dehydration treatments and the GUS-positive rate of regeneration plants was about 72.60%. Polymerase chain reaction analysis of GUS-positive plantlets revealed a 100% positive detection rate for neomycin phosphotransferase II gene and uidA. Southern blot of transgenic plants regenerated from different Km-R calli lines demonstrated that the target gene, mostly with the low copy number, has been integrated into the cotton genome. Shen-Jie Wu and Hai-Hai Wang should be considered as joint first authors