Direct Somatic Embryoid Formation on Immature Embryos of Trifolium repens, T. pratense and Medicago sativa, and Rapid Clonal Propagation of T. repens

By direct somatic embryogenesis in vitro a clone of asepticplantlets can be raised from a single immature embryo of Trifoliumrepens (white clover) within about 6 weeks of pollination. Embryoidsare induced directly from intact zygotic embryonic tissue ona culture medium containing 0·025 or 0·05 mg 1^–1BAP and 1·0 g 1^–1 yeast extract. Similar directsomatic embryogenesis has also been achieved for Trifolium pratense(red clover) and Medicago sativa (lucerne). Applications ofembryo propagation by direct somatic embryogenesis are discussed,particularly in relation to multiple screening of host genotypesfor analysis of host/pathogen and legume/Rhizobium interactions. Trifolium repens L., Trifolium pratense L., Medicago sativa L., clover, lucerne, tissue culture, embryoid, somatic embryogenesis, legumes     

Auxin and heat shock activation of a novel member of the calmodulin like domain protein kinase gene family in cultured alfalfa cells

A calmodulin like domain protein kinase (CPK) homologue wasidentified in alfalfa and termed MsCPK3. The full-length sequenceof cDNA encoded a 535 amino acid polypeptide with a molecularweight of 60.2 kDa. The deduced amino acid sequence showed allthe conserved motifs that define other members of this kinasefamily, such as serine-threonine kinase domain, a junction regionand four potential Ca²⁺-binding EF sites. The recombinant MsCPK3protein purified from E. coli was activated by Ca²⁺and inhibitedby calmodulin antagonist (W-7) in in vitro phosphorylation assays.The expression of MsCPK3 gene increased in the early phase ofthe 2,4-D induced alfalfa somatic embryogenesis. Heat shockalso activated this gene while kinetin, ABA and NaCl treatmentdid not result in MsCPK3 mRNA accumulation. The data presentedsuggest that the new alfalfa CPK differs in stress responsesfrom the previously described homologues and in its potentialinvolvement in hormone and stress-activated reprogramming ofdevelopmental pathways during somatic embryogenesis. Key words: Medicago sativa, CPK, stress, 2,4-D, phosphorylation, somatic embryogenesis.     

Development of a Superficial Meristem During Somatic Embryogenesis from Immature Cotyledons of Soybean (Glycine max L.)

Initial events were studied in the development of an embryogenicmeristem during somatic embryogenesis from in vitro culturedimmature cotyledons of soybean. The presence of 2,4-D in theculture medium led to the formation of a superficial embryogenictissue associated with the abaxial epidermis of 3 mm cotyledons.Additionally, 2,4-D initiated rapid non-morphogenic periclinaldivision in the parenchyma tissues of the cotyledon. Consequentinternal expansion disrupted and eventually ruptured the apparentlyquiescent adaxial epidermis. The profound difference in thein vitro response between abaxial and adaxial epidermes is discussedin relation to their relative roles in nutrient transport duringseed development in vivo. Somatic embryogenesis, transfer cells, Glycine max     

Storage Lipid Accumulation by Zygotic and Somatic Embryos in Culture

In vitro accumulation of storage lipids occurs in zygotic andsomatic embryos of Brassicu napus L. The concentration of sucrosein the medium modified the pattern of storage lipid accumulationin zygotic and somatic embryos. The sucrose concentration atwhich the maximum amount of lipid is accumulated by the twotypes of embryos is different Analysis of fatty acid compositionshowed that the same fatty acids are present in embryos in vivoand those cultured in vitro although there are quantitativedifferences. The possibility of using this type of system forin vitro production of valuable plant metabolites is discussed Embryo cloning, somatic embryogenesis, in cilro culture, storage lipids, Brussica napus, oilseed rape     

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     

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     

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     

Ultrastructural Studies of Somatic Embryos of Eucalyptus nitens and Comparisons with Zygotic Embryos Found in Mature Seeds

Although somatic embryogenesis has been observed in tissuesfrom a limited number of Eucalyptus species cultured in vitro,no comparisons have been made of the morphology and structureof eucalypt somatic embryos and zygotic embryos found in matureseeds. We used scanning and transmission electron microscopy,in conjunction with histological analysis, to compare maturezygotic embryos with somatic embryos of the commercially-importanttemperate eucalypt Eucalyptus nitens. Apart from differencesin the nature of the outer coating enclosing both embryo types,somatic embryos of E. nitens were observed to have strong similaritieswith zygotic embryos in seeds in terms of their overall size,morphology and internal cellular organization. Many cells inboth sexually-produced and somatic embryos contained numerouslipid-rich globular bodies. The wider significance of theseobservations is discussed with regard to their potential applicationsin eucalypt plantation biotechnology programmes. Copyright 2000Annals of Botany Company Eucalyptus nitens, shining gum, somatic embryo, tissue culture, ultrastructure, zygotic embryo     

Histology of Callogenesis and Somatic Embryogenesis Induced in Stem Fragments of Cork Oak (Quercus suber) Cultured In Vitro

Calluses able to produce somatic embryos were formed duringin vitro culture of shoot fragments of cork oak (Quercus suberL.).Histological monitoring of these fragments during cultureshowed that it was the cortical parenchyma cells which underwentdedifferentiation before calluses were formed by repeated divisions.The calluses consisted of parenchyma cells surrounded by a fewlayers of meristematic cells. Proembryos formed in groups aroundthe edge of some calluses. Histological examination showed thatthey were produced by the evolution of two different categoriesof cell: one category had the appearance of ‘embryogenic’cells with very thick walls, a small vacuole rich in starchand a well-developed nucleus with a prominent nucleolus. Theother cells were very bulky with large vacuoles; their morphologywas similar to that of suspensor cells encountered in embryogenesisin gymnosperms. The ontogenic stages were similar to those describedin zygotic embryos of the genus Quercus. Nevertheless, mostof the embryonic structures deviated from normal developmentand at all stages produced secondary proembryos. Cork-oak, Quercus suber L, histology, callogenesis, somatic embryogenesis, embryogenic cells, starch, secondary embryogenesis     

There is No Somatic Meiosis in Embryogenic Leaves of Cichorium

Several papers dealing with carrot cell cultures describe meiosis-likedivisions and haploid cells prior to somatic embryogenesis.We have studied the first division in embryogenic mesophyllcells of a diploidCichorium intybus L. and of a tetraploid hybridC.intybus L.xC. endivia L. which undergo direct somatic embryogenesisfrom single cells when leaf fragments are placed in a liquidagitated inductive medium (modified MS with 1x10^-7M NAA and2.5x10^-6M 2-iP), in darkness, at 35°C. MicrosporogenesisinC. intybus provided aspects of meiosis for comparison. Inleaves incubated in inductive conditions, DAPI staining of nucleishowed normal mitosis on days 3–6; about 0.6% cells inprophase had undergone spontaneous endoreduplication leadingto a tetraploid somatic embryo. Immunocytochemistry of tubulinrevealed the constant presence of a preprophase band, as ina normal mitosis. The first pluricellular somatic embryos becamevisible on day 5 of culture. Flow cytometric determination ofnuclear DNA on days 4, 5 and 6 did not show any peak correspondingto the 1C DNA level for the diploid plant or to the 2C DNA levelfor the tetraploid. Instead there was a weak but constant peakat the 4C and 8C levels. We conclude that inCichorium leaves,the first division of somatic embryogenesis is a normal mitosis,with a small shift to endoreduplication. In our opinion, somaticmeiosis is not a prerequisite during direct somatic embryogenesis. Cichorium ; chicory; somatic embryogenesis; cell division; flow cytometry; tubulin     

The Use of Single Somatic Embryo Culture in Propagating and Regenerating Lucerne (Medicago sativa L.)

Embryogenic cultures of lucerne (Medicago sativa L.) cv. Robothave been established and propagated on medium containing yeastextract. These cultures consisted of unorganized callus tissuebearing embryogenic centres which increased in size during subculture,yielding new regenerated somatic embryos at the end of each20-d subculture. A development in the propagation of the embryogenic cultureswas the establishment of single embryo culture in hormone-freemedium where, in selected cases, the process of recurrent somaticembryogenesis (RSE) took place on the hypocotyl of explantedembryos. The process was independent of supporting callus tissueand occurred on simple defined medium. Single embryos underwenteither plantlet development or continued RSE on the hypocotyl.One third of the regenerated plantlets showed RSE after thetwo to three trifoliate leaf stage. In these cases shoot developmentstopped and only somatic embryo production took place. In vitrocloning of regenerated plantlets allowed us to reproduce eachparticular genotype before transplantation into soil. Lucerne (alfalfa), Medicago sativa L., somatic embryogenesis, single embryo culture     

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     

Genotype, explant and position effects on organogenesis and somatic embryogenesis in eggplant (Solanum melongena L.)

The relative importance of genotype and explant, and their interactionsfor in vitro plant regeneration via both organogenesis and somaticembryogenesis in Solanum melongena (eggplant) has been studied.Hypocotyl, cotyledon and leaf explants of four commerciallygrown Indian cultivars, Pusa Purple Long, Long White Cluster,Pusa Kranti, and Pusa Purple Cluster were used in the study.A combination of benzyladen-ine (11.1 µM) and indoleaceticacid (2.9 µM) was found to be optimum for shoot regeneration.Naphthalene acetic acid induced embryogenesis in all the threeexplants; 32.2µM was optimum for hypocotyl explants while10.7µM yielded maximum number of somatic embryos fromcotyledon and leaf explants. Genotype, explant and genotype-explantinteraction had highly significant effects on both organogenesisand somatic embryogenesis with genotype exerting maximum effecton both these processes. Pusa Purple Long was found to be themost responsive genotype for regeneration of both adventitiousshoots and somatic embryos among the cultivars. Among the explants,hypocotyls yielded the maximum number of adventitious shootsfollowed by cotyledons and leaves. The embryogenic responseof leaves and cotyledons was, however, significantly higherthan that of hypocotyl explants. Significant differences formorphogenetic potential were also observed within a single explant(hypocotyl). There was a basipetal gradient for organogenesis(i.e. decrease in number of shoots from base to apex) whilethe terminal hypocotyl segments showed better embryogenic potentialthan the median segments. Key words: Solarium melongena, organogenesis, somatic embryogenesis, genotype, explant, position effect     

Somatic Embryogenesis in Brassica nigra (Koch)

Four genotypes of Brassica nigra were tested for their abilityto produce somatic embryos in vitro. Seedling-derived hypocotylexplants cultured in MS medium with p-chlorophenoxyacetic acid,-naphthaleneacetic acid and adenine gave rise to embryos thatcould germinate into seedlings with a high frequency on transferto medium containing benzylaminopurine riboside and p-chlorophenoxyaceticacid. Ebryogenesis was highest in leaf explants followed bystem and hypocotyls. Comparison of the embryogenic responseof hypocotyl segments differing in age indicated an increasein the frequency of response with increasing age of the explants.However, germination of embryos into seedlings declined withincreasing age of the explant. Embryogenesis was higher in MSmedium compared to five other media with similar growth regulatorcomposition. Genotypic differences exist for frequency of embryogenesisand subsequent maturation into seedlings. Key words: Brassica nigra, somatic embryogenesis, growth regulators, plant regeneration     

Callus Culture of Sainfoin (Onobrychis viciifolia) and Plant Regeneration through Somatic Embryogenesis

Callus of sainfoin (Onobrychis viciifolia Scop.) was initiatedfrom stem and root explants which were obtained from seedlingsgrowing in vitro, on Linsmaier Skoog (LS) medium supplementedwith 1 mg l^–1 2, 4-D and 1 mg l^–1 BA or only 1 mgl^–1 BA, and the Vacin and Went medium without hormones.Somatic embryos were formed on LS medium containing 1 m l^–1BA. Embryos developed into complete plants on filter paper saturatedwith hormone-free LS medium. Onobrychis viciifolia, somatic embryogenesis, callus culture, plant regeneration     

Somatic Embryogenesis and Its Hormonal Regulation in Tissue Cultures of Freesia refracta

Somatic embryogenesis can be induced in tissue cultures of Freesiarefracta either directly from the epidermal cells of explants,or indirectly via intervening callus. These two pathways ofsomatic embryogenesis can be controlled and regulated by varyingthe combinations and levels of exogenous hormones. When younginflorescence segments were cultured in vitro on modified N₄(MN₄) medium supplemented with 2 mg l^–1 indoleacetic acid(IAA) and 3 mg l^–1 6-benzylaminopurine (BAP), some ofthe epidermal cells began to exhibit the features of embryogeniccells. These cells produced embryoids and developed into newplants through direct somatic embryogenesis. If the same explantswere placed on Murashige and Skoog's (MS) medium containing2 mg l^–1 IAA, 05 mg l^–1 BAP and 05 mg l^–1naphthaleneacetic acid (NAA), pale-yellow translucent nodularcalluses appeared on the surface of the explants. When thiskind of callus was transferred to MN6 medium with 2 mg l^–1IAA and 3 mg l^–1 BAP, embryoids formed which further developedinto plantlets. The regenerated plants were morphologicallynormal and possessed the normal diploid chromosome number of2n = 22. A similar result has also been obtained with youngleaf explants of this plant. The early segmentations of embryogeniccells and the development of embryoids were studied using histologicaland scanning electron microscopic techniques, and the resultshave been discussed in association with the ontogeny and originof the embryoids. Freesia refracta Klatt, somatic embryogenesis, plant regeneration, exogenous hormones     

Regeneration of Plants from Protoplasts of Arabidopsis thaliana L. cv. Columbia (C24), Via Direct Embryogenesis

This report describes a protocol for the regeneration of fertileplants from mesophyll protoplasts of Arabidopsis thaliana raceColumbia (C24). Regeneration was rapid and reproducible. Theprotocol is especially novel in that a large proportion of regeneratingprotoplasts regenerated via direct somatic embryogenesis. Protoplastsisolated from in vitro-grown plants entered sustained divisionafter 3–5 d in culture medium and over a period of severaldays 6–22% of protoplasts underwent at least one celldivision. Approximately 2–16% of these protoplasts continuedto divide and after 3 weeks in culture had formed macroscopiccolonies, of which 70–80% were regular embryo-like structures.Four weeksafter release from the alginate culture matrix andtransfer to solid medium in the light, 68–88% of thesestructures had produced well-developed shoots. Shoots couldbe maintained in culture or established in peat blocks. Theregenerated plants were fertile. Key words: Arabidopsis thaliana, protoplast, regeneration, embryogenesis, dicamba     

Polyamine Levels in Relation to Growth and Somatic Embryogenesis in Tissue 6Medicago Sativa L.

Polyamine levels in petiole-derived tissue cultures of two highlyregenerable Medicago sativa L. genotypes were determined duringthe embryo induction and embryo differentiation phases of somaticembryogenesis. Putrescine levels increased 27–32-foldduring the 10 d on 2, 4-D- and kinetin-containing embryo inductionmedium and fell sharply following transfer to growth substance-freeembryo differentiation medium. The rapid increase in putrescinecontent occurred during a period of relatively little growthwhile the decline coincided with the initiation of rapid tissuegrowth on embryo differentiation medium. The addition of putativeinhibitors of putrescine or spermidine biosynthesis to the embryoinduction medium led to reduced levels of polyamines, particularlyof putrescine, in cultures of both genotypes but subsequentsomatic embryo formation was inhibited in cultures of one genotypeonly. It was concluded that the pronounced change in putrescinemetabolism was not specifically associated with embryogenesis,but appeared to be related generally to re-programming of cellsinto a new pattern of in vitro development. Key words: Medicago sativa, polyamines, somatic embryogenesis     

Age and growth of planktonic squids Cranchia scabra and Liocranchia reinhardti (Cephalopoda, Cranchiidae) in epipelagic waters of the central-east Atlantic

Statolith microstructure was studied in two abundant planktoniccranchiids, Cranchia scabra (56 specimens, 38–127 mm mantlelength, ML) and Liocranchia reinhardti (34 specimens, 99–205mm ML) sampled in epipelagic waters of the western part of theGulf of Guinea (tropical Atlantic). Growth increments were revealedin ground statoliths of both species. It was possible to distinguishtwo growth zones in statolith microstructure by their colourin reflected light of the microscope: the translucent postnuclearzone and pale white opaque zone. Assuming that growth incrementsin statoliths were produced daily, ages of the largest immatureC.scabra and L.reinhardti were 166 and 146 days, respectively.Both cranchiids are fast-growing squids with growth rates inlength resembling those of juveniles of tropical ommastrephidsand Thysanoteuthis rhombus. Liocranchia reinhardti grows faster:its growth rate in ML is approximately twice that of same-agedC.scabra. The life cycle of both cranchiids consists of twophases. During their epipelagic phase, C.scabra and L.reinhardtifeed and grow rapidly from paralarvae to immature young in theepipelagic waters, attaining 120–130 and 170–200mm ML by ages of 4–5 months, respectively. Then they changetheir life style to a deepwater phase.     

Uniformity of Plants Regenerated by Direct Somatic Embryogenesis from Zygotic Embryos of Trifolium repens

A total of 55 regenerants from direct somatic embryogenesison three zygotic embryos of Trifolium repens have been examinedfor uniformity with respect to morphological markers, chromosomenumber, breeding behaviour and banding patterns produced bySDS-polyacrylamide gel electrophoresis of total leaf proteinsand isoelectric focussing of leaf peroxidase, esterase and leucineaminopeptidase isozymes. Differences were observed between clones,but no differences were detected among primary and secondaryregenerants from the same zygotic embryo. The data support theconcept that direct somatic embryogenesis on immature zygoticembryos is a conservative, clonal regeneration process. Trifolium repens, clover, somatic embryogenesis, somaclonal variation, embryo culture, isozymes