Changes in the Polypeptide Composition during the Ontogenetic Development of the Shoot Apex of Crocus sativus

The shoot apex development during the life cycle of Crocus sativus L. was characterized by light microscopy and two-dimensional gel electrophoresis. Using silver staining of polyacrylamide gels, numerous quantitative and qualitative changes in the populations of polypeptides were observed during transition from vegetative to prefloral and from prefloral to floral stages. Using 80 g protein, we were able to detect 352 polypeptidic spots. In comparison with the vegetative apex, 89 new polypeptides were identified in the prefloral meristem and 29 polypeptides were missing. In the reproductive meristem, 94 new spots were identified and 44 spots were missing. Thus, substantial quantitative and qualitative changes in the populations of polypeptides occurred during the prefloral stage, a point of no return in plant development, i.e., and before floral primordia initiation.     

Rates of cell division in the young prefloral shoot apex ofChrysanthemum segetum L.

Summary The rate of cell division was determined by the colchicine induced metaphase-accumulation technique in the young prefloral shoot apex of the quantitative long-day plantChrysanthemum segetum L. growing under conditions favourable to flowering (16-hour photoperiod; 124Em^–2s^–1; 22 °C). Cell cycle duration was evaluated in relation to the location of the cells in the intact apex. The cell cycle durations were 53.5 hours, 47.4 hours, and 97.7 hours in the axial, lateral and subapical central cells respectively. Compared with previous results, these data give evidence of the major role played by the early increase in cell division rate of axial cells in the new pattern of the prefloral shoot apex at its initial stage of development. By comparison with the vegetative shoot apex, the cell cycle duration was preferentially shortened in the axial zone; it was only slightly altered in the lateral zone while it was lengthened in the vacuolating subapical central cells. In the three zones within the prefloral shoot apex, the duration of mitosis was constant (3.2 to 3.3 hours) and the same as in the vegetative shoot apex.     

Changes in the Pattern of Cell Division in the Shoot and Root Meristems of Lolium perenne during the Transition from Vegetative to Floral Growth

For Lolium perenne cv. Cropper, a system which resulted in 100%flowering comprised 90 short days (SD) at 4 ?C (vernalization)and 30 SD at 18 ?C followed by 8 long days (LD). The mitoticindex and G1 and G2 percentages were measured in the shoot androot apices of plants following 2, 5 or 8 LD and in SD controlssampled at the beginning and end of induction. Identical measurementswere made in plants given 48 SD at 18 ?C followed by 2, 5 or8 LD; plants remained vegetative in response to this treatmentlacking vernalization. Significant increases in both mitoticindex and meristem size occurred in the shoot apex in LD followingthe vernalizing, but not the non-vernalizing, treatment. A clusterof mitoses in the apical dome of the shoot apex was unique tothe vernalized plants given 5 or 8 LD. However, an increasein root meristem size occurred regardless of vernalization,but a significant increase in the mitotic index was limitedto vernalized plants given 5 or 8 LD. Whilst the vernalization-LDtreatment resulted in an increase in the G2 percentage in theshoot apex following 2, 5 or 8 LD, no such alteration was observedin the root meristem. Thus, the changes to the cell cycle whichcorrelated with flowering were increased mitotic indices andG2 percentages in the shoot apex at each sampling time and increasedmitotic indices in the root apex following 5 and 8 LD. Key words: Cell division, flowering, Lolium perenne L.     

INFLORESCENCE DEVELOPMENT IN BRASSICA CAMPESTRIS L.

Vegetative seedlings of the Ceres strain Brassica campestris L., a quantitative, long-day plant, were induced to flower by exposure to a 16-hr, long-day cycle. Cytohistological and cytohistochemical changes associated with inflorescence development were examined. Developing shoot apices were classified in vegetative, transitional, and reproductive stages. The vegetative apex possessed a biseriate tunica, central zone, peripheral zone and pith-rib meristem. The transitional stage at 48 hr was marked by an increase in size and by a stratification of the upper cell layers of the shoot apex with a concurrent decrease of apical cytohistochemical zonation. The reproductive stage was initiated at 58 hr by periclinal cell divisions in the 3rd and 4th cell layers of the flank region. Cytohistochemical zonation in the vegetative apical meristem was restored in the floral apex. An “intermediate developmental” phase was not observed between the vegetative and reproductive stage.     

Histoautoradiographic analysis of the thermoinductive processes in the shoot apex of Arabidopsis thaliana L. Heynh, vernalized at different stages of development

The cytochemical reactions of various zones of the shoot apexof an annual winter plant (Arabidopsis thaliana), vernalizedat two different ages (26 and 85 days), were analyzed usinghistoautoradiography after incorporation of tritiated thymidine.The following sequence of events was observed during a coldtreatment of 40 days: subapical activation (in DNA synthesis)of the rib meristem (this took place regardless of the age ofthe plants; dedifferentiation of axial cells (the beginningof which was earlier in the older plants). After cold treatment, the plants were resubmitted to warm temperaturesunder long day conditions. A re-establishment of the zonationin the meristem was seen during the first week for plants inthe "intermediate stage". The activation of axial cells increasedduring the next two weeks and a few days later both groups ofplants entered the prefloral stage followed by the formationof their first floral buds. These apical reactions were comparedto those of a French variety of A. thaliana, a quantitativelong-day plant, submitted to different photoperiods and to gibberellicacid (GA₃). (Received January 17, 1977; )     

The Structure and Development of the Vegetative Shoot Apex in Glechoma hederacea L

The development of the vegetative shoot apex of Glechoma hederaceahas been followed through a double plastochron. During this period the apex grows from c. 20 to c. 260 µin height and c. 100 to c. 300 µ in width, whilst thepair of leaves inserted at the apex base increase from o toc. 600µ in height. The width of the apex and height ofthese leaves are directly related to apex height. Some variationoccurs in the average maximal dimensions of the apex with plastochronnumber but no regular increase or decrease in these dimensionsis apparent. Both a tunica-corpus organization and cytohistological zonationis visible within the apex throughout a double plastochron.The central initiation zone shows little change in size or appearanceduring this period but the rib and flank meristems grow considerablyand undergo some differentiation. The boundaries of these zonesare not sharply defined, but normally the rib meristem givesrise to the pith, and the flank meristem forms the epidermis,cortex, and provascular tissue. The provascular tissue differentiatesacropetally and in continuity with that in the axis below.     

Structural Organization of the Shoot Apex and Axillary Bud in Slipper Spurge (Pedilanthus tithymaloides Poit.) I

The slipper spurge (Pedilanthus tithymaloides) is a small cactus-likeherbaceous plant. The shoot apex has a single tunica layer andsometimes the second layer also simulates it. There is a centralmeristem zone whose significance could not be determined. Thefirst bud meristem differentiates at the second node. The earliestbud meristem has a procambium but no shell zone was observed.The node is trilacunar. There are three bud traces and threeprophyll traces. The single prophyll is situated at right anglesto the subtending leaf.     

Surgical Experiments on the Differentiation of Vascular Tissue in the Shoot Apex of Carrot (Daucus carota L.)

Surgical techniques were applied to the shoot apex of carrot(Daucus carota L.) to test the interpretation that provasculartissue is the initial stage of vascular differentiation andto localize the sources of the influences that control its differentiation.If the apex is isolated laterally by vertical incisions leavingit at the summit of a plug of pith tissue, vascular differentiationproceeds normally and an independent vascular system is formedin the pith plug. If all leaf primordia are systematically suppressed,provascular tissue continues to differentiate as an acropetalextension of the pre-existing vascular system but no furtherdifferentiation occurs. When the apex is isolated laterallyand all leaf primordia are suppressed, provascular tissue continuesto be formed acropetally and is extended basipetally into thepith plug by redifferentiation of pith cells, but no furtherdifferentiation occurs. This tissue reacts positively to histochemicaltests for esterase indicating its vascular nature. If only oneleaf primordium is allowed to develop on an isolated shoot apex,its vascular system develops normally and extends basipetallyinto the pith plug, but there is no extension of provasculartissue into the pith plug. These results support the interpretationthat the initial stage of vascular differentiation is controlledby the apical meristem but that further maturation of vasculartissue depends upon influences from developing leaf primordia.Copyright 2000 Annals of Botany Company Provascular tissue, differentiation, carrot (Daucus carota L.), shoot apex, surgical techniques, leaf primordia     

The anatomy of the shoot apex ofHyoscyamus niger L. reversed from the generative to the vegetative state

A study was made of the anatomical structure of the shoot apices ofHyoscyamus niger L. in plants which were transferred from a long-day to a short-day regime after the initiation of the inflorescence. After a certain time these plants are reverted to the vegetative stage with the inhibition of the development of further flower buds and the renewed production of rosette leaves. The inflorescence apex consisted of a few superficial layers of cells and a corpus composed of slightly elongated cells. The anatomical structure of the apices which were reverted into the vegetative state resembled that of shoot apices in the intermediate stage. The apex had several layers of small cells, under which there was a group of small but irregularly arranged cells which passed into the rib meristem. The shoot apices of plants transferred from a long to a short-day regime at different time intervals after fulfilling the requirements of minimal photoperiodic induction thus, on the short day, display morphological and anatomical characteristics of various degrees of transition from generative to vegetative stage.     

Characterization of Stelar Initiation in Shoot Apices of Ferns

Procambium is commonly recognized as a vascular meristem inshoot apices of vascular plants. Prestelar tissue comprisingprovascular tissue (PVT) and pith mother cells (PMCs) immediatelysubjacent to the single cell layer of promeristem has been consideredto represent the initial stage of stelar differentiation precedingprocambium and rib meristem in ferns. In addition to characterizationof PVT and PMCs on the basis of cell morphology, cytologicalfeatures and developmental continuity with procambium and ribmeristem, four lines of evidence from studies of shoot apicesof Matteuccia struthiopteris and Osmunda cinnamomea supportthis interpretation of initial differentiation. (1) Differentialstaining by safranin-fast green and crystal violet-erythrosinshows that PVT and PMCs differ in colour reactions from promeristemand resemble procambium and pith meristem, respectively. (2)Comparative ultrastructural study reveals qualitative differencesin the cell membrane system, nuclei, cytoplasm, vacuoles andplastids between promeristem and PVT but similarity of PVT toprocambium. (3) Large droplets of tannins occur in promeristembut not in PVT, PMCs and procambium. (4) Cytochemical studyof the shoot apex of Osmunda shows that carboxylesterase activityis strongly demonstrated in PVT and procambial cells but notin promeristem cells and PMCs. These observations further substantiatethe interpretation that PVT represents initial vascular differentiationand PMCs reflect a commitment to pith development.Copyright1995, 1999 Academic Press Initial vascular differentiation, provascular tissue, differential staining, ultrastructure, tannins, carboxylesterase, shoot apex, Matteuccia struthiopteris, Osmunda cinnamomea     

Electron microscopic study of the mitochondria in the apical meristem of a wheet shoot in ontogeny]

The mitochondria of apical meristem cells in the wheat (Triticum aestivum L.) shoot were studied during ontogenesis using electron microscope and morphometrical methods. Changes in their structure were followed from the juvenile mitochondria of the seed embryonic ear cells. The parameters of the "average" mitochondrion, such as profile area, outer membrane length, were shown to differ relatively weakly during the periods with different meristem activity. Changes in the internal structure of the mitochondria having the developed system of crystae in the actively growing apices and those with weakly developed crystae in the resting seed or low active "waiting meristem" are much more pronounced. The relative volume of mitochondria, their number per unit of cytoplasm volume and total length of membranes suffer relatively insignificant changes during the vegetative phase and increase markedly during the prefloral phase when the apex is preparing itself for generative differentiation.     

Morpho-histogenic studies on tendrils of Passiflora

The ontogenetic development of the tendril and its associatedorgans is investigated in 17 species of Passiflora. The shootapex shows a single tunica layer though the second layer simulatestunica. The cytohistological zonation is not a constant feature.In P. caerulea Linn., it is distinct at leaf initiation butin P. pruinosa Mast., P. vespertilio Linn., and P. watsonianaMast., it is indistinct. The main axillary bud differentiatesfrom the peripheral meristem of the shoot apex. The differentiationof this bud into floral and tendril menstems occurs at a nodeimmediately below the shoot apex in P. minima Blanco. and Pracemosa Brot. In other species this differentiation generallyoccurs at the lower nodes. The floral meristem is initiatedas an accessory bud from this bud, thus forming a bud complex.The residuum of the bud complex develops as a tendril. The thirdaccessory bud which does not originate from this bud complex,develops into a vegetative branch. The fundamental nature ofthe vascular relationship between the flower, tendril, accessorybud, subtending leaf, and the axis is similar in most of theinvestigated species.     

Growth changes in the shoot apex of Sinapis alba during transition to flowering

The aim of the work was to report morphological changes whichoccur in the shoot apex during the morphogenetic switch to floweringin the model long day (LD) plant, Sinapis alba. During the floraltransition induced by 1 LD the growth rate of all componentsof the shoot apex is modified profoundly. The earliest changes,detected at 24 h after start of LD, include a decrease in plastochronduration and an increase of growth of leaf primordia. One daylater, the meristem dome starts to increase in volume, apicalinternodes have an increased height and there is a precociousoutgrowth of axillary meristems. All these changes precede initiationof flower primordia, which starts at about 60 h after the startof LD. Later changes include meristem doming, a decrease inthe plastochron ratio and a shift to a more complex phyllotaxis.All the changes, except the decreased plastochron ratio, arecharacteristics of an apex with an increased tempo of growth.The stimulation of longitudinal growth (height of apical intemodes)is more marked and occurs earlier than the reduction of radialgrowth (plastochron ratio). Key words: Axillary meristem, internode growth, leaf growth, plastochron ratio, plastochron duration     

A Note on the Manipulation of Flower Symmetry inAntirrhinum majus

Treatments consisting of maceration of the centre of the shootapical meristem or localized application of the plant hormone,indoleacetic acid (IAA), to apical flower buds or the estimatedcentre of the shoot apex were made to test their effect, ifany, on flower shape or symmetry. Both types of treatment affectedflower symmetry. IAA treatment was most successful, but it alsoaffected the completeness of the flower, producing a small numberof reduced flowers. Alteration of symmetry was, however, themain response to treatment.Copyright 1999 Annals of Botany Company Antirrhinum majusL., flower symmetry mutants, microsurgical and microhormonal treatments, apical meristem, flower buds.     

Location of cell cycle changes in relation to morphological changes in the shoot apex ofSilene coeli-rosa immediately before sepal initiation

Summary Changes in morphology, the mitotic index and the proportions of cells in G₁ and G₂ were measured in shoot meristems ofSilene coeli-rosa immediately before floral morphogenesis in order to determine whether the known changes to the cell cycle at this time are restricted to a particular region of the apex. Twenty-eight day-old plants were given either 7 long days (LD) plus 2 short days (SD) (day 8 of the LD treatment) or 9 SD [day 8 of the SD control (SDC) treatment]. Plants were sampled on day 8 every 2 h for 12 h and the various cell cycle measurements were performed on sections of the apical meristem. In the inductive LD treatment there was a peak in the mitotic index at 13.00 h and, possibly, the start of another at 19.00 h. At 21.00 h all meristems in this treatment initiated sepals. The mitotic activity at 13.00 and 19.00 h in the LD treatment was a result of significant increases in the mitotic index in the axial, lateral and central sub-axial areas of the apex compared with the corresponding zones in the SDC treatment. At 13.00 h of day 8, 80% of cells were in G₂ phase in the axial region in the LD treatment whilst 85% of cells were in G₁ in the axial zone in the SDC treatment. In the other zones significantly more cells were in G₂ in the LD compared with the SDC treatment as was the case at 19.00 h although not to the same extent as the axial zone at 13.00 h. Thus these data emphasize, for the first time, the mitotic activation and predominance of the G₂ population of cells particularly in the axial zone of shoot meristems in the LD treatment. These data are discussed in relation to the synchronisation of cell division which could occur in the prefloral shoot meristem at this time, affecting each shoot apical zone.Abbreviations LD long day - SD short day - SDC short day control     

Aspects of Morphogenesis in a Dorsiventral Fern, Pteridium aquilinum (L.) Kuhn: With one Plate and ten Figures in the Text

The formation of the horizontal dorsiventral rhizome of Pteridiumaquilinum from the erect radial axis of the young sporelingis described. The shoot apex and the inception of leaves andbuds at the apical meristem have been investigated, and theirinception is shown to be essentially similar in long and shortshoots, later differences being due to differing rates of growthand internodal elongation in the two types of shoot.     

Some Cytological Changes accompanying the Regeneration of Meristematic Activity at the Apex of Decapitated Roots of Vicia faba L.

The changes that took place in mitotic index (MI), labellingindex (LI) and the relative proportions of interphase nucleiwith different amounts of DNA have been investigated duringthe regeneration of meristematic activity at the apex of rootsof Vicia faba over the 144 h period following removal of thecap and apical mm of the meristem. Measurements were also madeof the corresponding changes that took place as cells were displacedbasally along the root from the apex over the experimental period.In both parts of the root, MI and the relative proportions ofnuclei with different DNA contents changed from levels similarto those at the apex of the controls at the start and end ofthe experiment to levels resembling those found in more matureparts of the root at 24 and 48 h. In contrast to these results,LI declined over the experimental period. These cytologicalchanges were aresult of the development of lateral root primordiain both the apical 2 mm of the decapitated roots and as cellswere displaced out of the meristem into more basal parts ofthe root. It was concluded that the events leading to the regenerationof meristematic activity at the apex of roots from which thecap and apical mm of the meristem were removed, are no differentfrom those which result in lateral formation as cells are displacedbasally along the primary root from the apex, and they takeplace over the same time interval in both systems.     

Effects of Developing Leaves on Stelar Pattern Development in the Shoot Apex of Matteuccia struthiopteris

A developmental study of the normal shoot apex of Matteucciastruthiopteris suggested that patterned stelar differentiationis initiated immediately beneath the single layer of promeristemand occurs prior to the initiation of the youngest leaf primordium.A developmental study in which all leaf primordia were suppressed,with or without lateral isolation of the terminal meristem byvertical incisions, has confirmed this interpretation of stelardifferentiation. Experimentally-induced changes in the tissueimmediately below the promeristem were reflected in the resultingmature structure of the stele. Failure of leaf gap initialsto differentiate, if all leaf primordia were suppressed at theincipient stage, resulted in a mature stele without leaf gaps.Similarly the disappearance of pith mother cells after severalweeks of leaf removal was associated with the formation of astele without pith. Leaf influence was further assessed by allowingone primordium to develop while all others were suppressed.The developing leaf had a small promoting effect on caulinevascular tissue differentiation but its major impact on theexpansion of the parenchymatous tissues of the stele. Characteristicprotoxylem and protophloem failed to differentiate when allleaves were suppressed and, when leaf was allowed to develop,formed only in relation to the leaf.Copyright 1995, 1999 AcademicPress Leaf influence, vascular pattern formation, experimental surgery, shoot apex development, protoxylem, protophloem, Matteuccia struthiopteris     

Experimental and Analytical Studies of Pteridophytes: XXX. Further Investigations of the Formation of Buds and Leaves in Dryopteris aristata Druce

The influence of the shoot apex upon leaf and bud formationin the fern Dryopteris aristata has been investigated by furtherexperiments on puncturing the apical cell. When the apical cellgroup is damaged, leaf primordia, which may be orientated abnormally,continue to be formed on the meristem, but one or more budsmay also arise. The observations reported here indicate thata zone at the periphery of the apical meristem is particularlyreactive when the apical cell group is damaged, the majorityof buds being induced in this region. The extent of damage tothe apex may affect the sequence of organogenesis: when damageis extensive buds tend to be formed immediately, subsequentprimordia developing as leaves; when the damage is confinedto the apical cell, or extends to only a few of its segments,bud formation tends to be delayed. It is concluded that the effect of the apical cell on organformation is exercised through the growth and organization ofthe apex as a whole.     

Histochemical Study of Photoperiodic and Low Temperature Effects on Floral Induction of Spinacia oleracea

Shoot apices of Spinacia oleracea plants have been induced toflower either by: (a) subjecting leaves to 24 h long day, or(b) exposure to a short photoperiod but displaced by 8 h (displacedshort day) in the usual 24 h short-day cycle, or (c) exposureto low temperature (5 °C) during the dark period of thenormal short day. A quantitative cytochemical assay of pentosephosphate pathway activity during floral induction indicatesan approximate doubling of the rate of activity when comparedto that of vegetative apices (short day) (21 °C). Exposure to either low temperature, or a displaced short photoperiodstimulates pentose phosphate pathway activity in the shoot apexin a manner similar to that seen by long-day induction. Thischange in metabolic activity is accompanied by changes in theshape of the shoot apex which resembles that seen at an earlystage during floral induction. Spinacia oleracea, pentose phosphate pathway, shoot apex, glucose-6-phosphate dehydrogenase, floral induction, chilling, displaced short day