Soil Moisture Rather than Soil Nutrient Regulates the Belowground Bud Bank of Rhizomatous Species <i>Psammochloa villosa</i> in Arid Sand Dunes

In arid and semi-arid sand dune ecosystems, belowground bud bank plays an important role in population regeneration and vegetation restoration. However, the responses of belowground bud bank size and composition to sand burial and its induced changes in soil environmental factors have been rarely studied. In arid sand dunes of Northwestern China, we investigated belowground bud bank size and composition of the typical rhizomatous psammophyte Psammochloa villosa as well as three key soil environmental factors (soil moisture, total carbon and total nitrogen) under different depths of sand burial. Total buds and rhizome buds increased significantly with increasing burial depth, whereas tiller buds first increased and then decreased, with a peak value at the depth of 20–30 cm. Soil moisture increased significantly with sand burial depth, and was positively correlated with the number of all buds and rhizome buds. Soil total carbon concentration first increased and then decreased with sand burial depth, and total nitrogen concentration was significantly lower under deep sand burial than those at shallow depths, and only the number of tiller buds was positively correlated with soil total nitrogen concentration. These results indicate that soil moisture rather than soil nutrient might regulate the belowground bud bank of P. villosa, and that clonal psammophytes could regulate their belowground bud bank in response to sand burial and the most important environmental stress (i.e., soil moisture). These responses, as the key adaptive strategy, may ensure clonal plant population regeneration and vegetation restoration in arid sand dunes.     

Flower Morphogenesis in Rosa hybrida 'Mercedes' as Studied by Cryo-scanning Electron and Light Microscopy. Effects on Light and Shoot Position on a Branch

Flower bud development in Rosa hybrida cv. 'Mercedes' was studied in shoots grown at different irradiances and sprouting from axillary buds at different branch positions. Cryo-scanning electron microscopy and light microscopy were used to visualize, characterize and determine flower morphogenesis during early shoot development. Up to the moment of visible flower bud appearance on the plant, flower morphogenesis was divided into nine stages. This classification was based on external and internal characteristics of the primordium. All shoots of the rose 'Mercedes' whether positioned uppermost or second on a branch and whether grown at 300 or 150 μmol m^-2 s^-1 PAR (12 h d^-1) developed equally up to flower stage 7, i.e. the stage just before visible initiation of stamen and pistils. Signs of flower bud abortion were the compactness of the flower bud at developmental stage 7 (height/width < 1·5) and the sprouting of axillary buds positioned just below the flower bud primordium. It was concluded that once a flower bud has reached a height to width ratio larger than 1·5, and once stamen and pistil developmental has started, it has passed the critical developmental stage in which abortion may occur. Flower developmental stage was closely related to shoot length. This relationship was not affected by irradiance level nor by shoot position on a branch. Therefore, cultivation treatments aimed to improve flower production by reducing flower abortion, such as supplementary lighting, will be most effective when applied during the first 2 weeks of shoot growth in which the flower develops up to stage 7.     

Regeneration capacity from buds on roots and rhizomes in five herbaceous perennials as affected by time of fragmentation

Variation in seasonal sprouting pattern from roots and rhizomes of perennial herbaceous plants influence the success of plant proliferation ability, invasiveness and escape from weed control measures. The latter often rely on methods, which repeatedly fragment the underground system, thereby trigger adventitious and axillary buds to sprout, and consequently reduce the amount of stored energy. If carried out at times when no re-growth occurs, treatments will have little effect on weed populations, but cost much in terms of labour and energy. The purpose of this experiment was to determine the seasonal variation in bud sprouting capacity after fragmentation. Five troublesome perennial weed species, collected in northern and southern Sweden, were grown outdoors in Uppsala, Sweden (N 59°49′, E 17°39′), from May 2009 to January 2010. Cut root and rhizome fragments, taken at two weeks intervals from July to January, were used to evaluate bud sprouting capacity, which was statistically analyzed using generalized additive models. In Elytrigia repens from southern Sweden and Sonchus arvensis sprouting capacity was significantly impaired during a period from September to November. In Equisetum arvense and Tussilago farfara sprouting was low between July and November where after it increased. In contrast, Cirsium arvense and E. repens from northern Sweden sprouted readily throughout the period. Except for E. repens, a model by populations was significantly better than one based on latitudinal origin. The result suggests a species-specific timing of treatments in weed management, avoiding the non-effective autumn period for E. arvense, S. arvensis and T. farfara, and in some cases in E. repens.     

Contrasting bud bank dynamics of two co-occurring grasses in tallgrass prairie: implications for grassland dynamics

Because most shoot recruitment in perennial grasses occurs from belowground axillary buds, bud dynamics determine plant population dynamics and meristem limitation to population growth. Therefore, grassland vegetation responses to environmental change or disturbance may be influenced by interspecific differences in bud banks and the patterns and environmental controls of bud development and demography. We examined bud bank dynamics in Andropogon gerardii and Dichanthelium oligosanthes in tallgrass prairie by enumerating and classifying buds throughout 15?months to determine whether grass buds live for multiple years and accumulate; whether bud natality, dormancy and outgrowth are synchronous or variable; and whether bud bank dynamics differ between these co-occurring species. Andropogon gerardii (a C₄ species) maintained a larger dormant bud bank, showed synchrony in bud development and transition to tiller, and its buds lived for multiple years. Thus, multiple previous years?? bud cohorts contributed to recruitment. By contrast, D. oligosanthes (a C₃ species) maintained a smaller dormant bud bank, had asynchronous bud development with active buds present year-round, and its buds lived for 1?year. Buds played different roles in the dynamics of each species, allowing A. gerardii to over-winter and recruit new spring tillers and D. oligosanthes to survive and recruit new tillers following summer dormancy. These differences in bud bank age structure, phenology, and dynamics between these species suggest greater demographic buffering and time-lag effects in A. gerardii populations. Interspecific differences in bud bank structure and dynamics may explain and help predict grassland responses to environmental change.     

Effects of thidiazuron and N6-benzylaminopurine on shoot regeneration of Phalaenopsis

Adventitious bud formation from the vegetative buds of the flower stalks of Phalaenopsis occurred on Vacin and Went medium with 15% coconut water and 5 to 40 μM thidiazuron (TDZ) or 40 μM N⁶-benzylaminopurine. The highest efficiency of induction was achieved with 5 or 10 μM TDZ. Adventitious buds developed into shoots on VWC medium. TDZ was more effective than BAP in stimulating the axillary buds of intact shoots to develop. Regenerated shoots rooted after about two months of culture on VWC medium with 1% sucrose. Shoot tips excised from the regenerated shoots initiated protocorm-like bodies after two months of culture on VWC medium.     

Light and nitrogen nutrition regulate apical control in Rosa hybrida L.

Apical control is defined as the inhibition of basal axillary bud outgrowth by an upper actively growing axillary axis, whose regulation is poorly understood yet differs markedly from the better-known apical dominance. We studied the regulation of apical control by environmental factors in decapitated Rosa hybrida in order to remove the apical hormonal influence and nutrient sink. In this plant model, all the buds along the main axis have a similar morphology and are able to burst in vitro. We concentrated on the involvement of light intensity and nitrate nutrition on bud break and axillary bud elongation in the primary axis pruned above the fifth leaf of each rose bush. We observed that apical control took place in low light (92 μmol m⁻² s⁻¹), where only the 2-apical buds grew out, both in low (0.25 mM) and high (12.25 mM) nitrate. In contrast, in high light (453 μmol m⁻² s⁻¹), the apical control only operates in low nitrate while all the buds along the stem grew out when the plant was supplied with a high level of nitrate. We found a decreasing photosynthetic activity from the top to the base of the plant concomitant with a light gradient along the stem. The quantity of sucrose, fructose, glucose and starch are higher in high light conditions in leaves and stem. The expression of the sucrose transporter RhSUC2 was higher in internodes and buds in this lighting condition, suggesting an increased capacity for sucrose transport. We propose that light intensity and nitrogen availability both contribute to the establishment of apical control.     

In vitro micropropagation of the macarronesian evergreen treePersea indica (L.) K. Spreng

Summary Shoot propagation ofPersea indica (L.) K. Spreng was achieved using seedling axillary buds cultured on MS (Murashige and Skoog, 1962) medium with 1 mg/l (2.8 μM) N⁶-benzyladenine (BA). Forty percent of the obtained shoots did not elongate, but showed bud proliferation, which was maximal (three axillary buds per shoot) at the end of the seventh subculture. Sixty percent of the shoots elongated, did not show bud proliferation, and formed calluses at their base. Successful rooting (84.6%) was achieved dipping the base of each elongated shoot in 3 g/l (16.11 mM) indolebutyric acid (IBA) for 1–2 s, and transferring to half strength MS medium without growth regulators. These shoots presented an acclimatization success of 100%. Results suggest that micropropagated elongated shoots ofP. indica can be adequately used in reforestation programs.     

Changes after Decapitation in Concentrations of Indole-3-Acetic Acid and Abscisic Acid in the Larger Axillary Bud of Phaseolus vulgaris L. cv Tender Green

Early changes in the concentrations of indole-3-acetic acid (IAA) and abscisic acid (ABA) were investigated in the larger axillary bud of 2-week-old Phaseolus vulgaris L. cv Tender Green seedlings after removal of the dominant apical bud. Concentrations of these two hormones were measured at 4, 6, 8, 12 and 24 hours following decapitation of the apical bud and its subtending shoot. Quantitations were accomplished using either gas chromatography-mass spectrometry-selected ion monitoring (GS-MS-SIM) with [¹³C₆]-IAA or [²H₆]-ABA as quantitative internal standards, or by an indirect enzyme-linked immunosorbent assay, validated by GC-MS-SIM. Within 4 hours after decapitation the IAA concentration in the axillary bud had increased fivefold, remaining relatively constant thereafter. The concentration of ABA in axillary buds of decapitated plants was 30 to 70% lower than for buds of intact plants from 4 to 24 hours following decapitation. Fresh weight of buds on decapitated plants had increased by 8 hours after decapitation and this increase was even more prominent by 24 hours. Anatomical assessment of the larger axillary buds at 0, 8, and 24 hours following decapitation showed that most of the growth was due to cell expansion, especially in the intermodal region. Thus, IAA concentration in the axillary bud increases appreciably within a very few hours of decapitation. Coincidental with the rise in IAA concentration is a modest, but significant reduction in ABA concentration in these axillary buds after decapitation.     

Carbohydrates Modulate the In Vitro Growth of Olive Microshoots. I. The Analysis of Shoot Growth and Branching Patterns

The rate of microshoot proliferation during the micropropagation of olive (Olea europaea L.) plants is limited by the low rates of both bud sprouting and growth of secondary shoots following subculturing. The aim of this study was to determine (1) the effects of sucrose and mannitol on shoot growth, (2) whether either of these sugars modifies the pattern of shoot development of the explants, and (3) the influence of apical dominance on explant development. Working with single-node microcuttings of Olea europaea L. cv. Maurino with two opposite axillary buds, we added 17, 34, or 68 g L^?1 of sucrose or mannitol to the medium as the primary carbon source. Shoot development was classified as either (a) an outgrowth of the first bud on an explant (shoot-type A), (b) an outgrowth of the second bud (shoot-type B), or (c) an outgrowth of an axillary bud on either an A- or B-type shoot (shoot-type C). Explant survival, fresh-mass production, and patterns of shoot development were influenced by the type and concentration of sugar used. Mannitol promoted the sprouting and growth of A-, B-, and C-type shoots more than sucrose. The developmental responses observed indicate that the growth of axillary meristems of in vitro olive explants is not regulated by apical dominance. The results demonstrate that the sugar alcohol plays an important role in the developmental regulation of olive explants. Mannitol may also protect against detrimental effects associated with in vitro growth conditions.     

Effects of sediment burial disturbance on the vegetative propagation of Phalaris arundinacea with different shoot statuses

Shoot status, such as orientation and connection to the root system, and sediment burial depth after flooding disturbances have important ecological consequences on the post-flooding growth and vegetative reproduction of emergent macrophytes in wetlands. In the present study, we investigated the effect of shoot status (vertical, prostrate, or detached) and sediment burial depth (0.5 or 10 cm) on biomass accumulation and propagule production in Phalaris arundinacea (Poaceae) using an outdoor mesocosm system. In contrast to our prediction that shallow sediment burial would activate the axillary buds on prostrate shoots and regenerate more ramets, significantly fewer new ramets, rhizomes, buds, and biomass accumulation formed in P. arundinacea as the shoots changed from vertical to prostrate. Deeper sediment burial resulted in lower biomass and propagule production in plants with prostrate shoots, whereas vertical shoots increased the number of ramets. P arundinacea with detached shoots also produced a number of propagules after shallow or deep sediment burial, which might be important for the long-distance dispersal of P. arundinacea. These results suggest that P. arundinacea is a potentially invasive species in many lacustrine wetlands, particularly those with a high sedimentation rate, due to its high capacity for vegetative propagation.     

Micropropagation of Camptotheca acuminata decaisne from axillary buds, shoot tips, and seed embryos in a tissue culture system

Summary Micropropagation of the anti-cancer plant Camptotheca acuminata Decaisne from axillary buds and seed embryos was investigated. Axillary buds from greenhouse seedlings required a period of culture in media free of N⁶-benzyladenine (BA) before multiple shoot induction began. Direct induction of multiple shoots on BA-containing medium resulted in high mortality of the axillary buds. Multiple shoot induction from the greenhouse axillary buds was best achieved on B5 with 4.4 μM BA+0.5μM α-naphthaleneacetic acid, forming an average of three 2-mm tall shoots per bud in 8 wk. Elongation of these multiple shoots was successful at a lower BA level (0.22 μM) on B5 medium. Both in vitro and ex vitro rooting of the microcuttings was feasible with indole-3-butyric acid in the culture media, but ex vitro rooting led to high plantlet survival. Seed embryos were not ideal explants for multiple shoot induction. Shoot tips and axillary buds of in vitro-germinated seedlings showed an optimal multiple shoot formation on B5 with 8.9 μM BA, double the optimal BA level for greenhouse axillary buds. Using axillary buds to propagate C. acuminata plants in vitro is feasible for mass propagation of desired clonal lines high in camptothecin concentrations.     

Florigen is involved in axillary bud development at multiple stages in Arabidopsis

The wide variety of plant architectures is largely based on diverse and flexible modes of axillary shoot development. In Arabidopsis, floral transition (flowering) stimulates axillary bud development. The mechanism that links flowering and axillary bud development is, however, largely unknown. We recently showed that FLOWERING LOCUS T (FT) protein, which acts as florigen, promotes the phase transition of axillary meristems, whereas BRANCHED1 (BRC1) antagonizes the florigen action in axillary buds. Here, we present evidences for another possible role of florigen in axillary bud development. Ectopic overexpression of FT or another florigen gene TWIN SISTER OF FT (TSF) with LEAFY (LFY) induces ectopic buds at cotyledonary axils, confirming the previous proposal that these genes are involved in formation of axillary buds. Taken together with our previous report that florigen promotes axillary shoot elongation, we propose that florigen regulates axillary bud development at multiple stages to coordinate it with flowering in Arabidopsis.     

Vegetative axillary bud dormancy induced by shade and defoliation signals in the grasses

Vegetative axillary bud dormancy and outgrowth is regulated by several hormonal and environmental signals. In perennials, the dormancy induced by hormonal and environmental signals has been categorized as eco-, endo- or para-dormancy. Over the past several decades para-dormancy has primarily been investigated in eudicot annuals. Recently, we initiated a study using the monoculm phyB mutant (phyB-1) and the freely branching near isogenic wild type (WT) sorghum (Sorghum bicolor) to identify molecular mechanisms and signaling pathways regulating dormancy and outgrowth of axillary buds in the grasses. In a paper published in the January 2010 issue of Plant Cell and Environment, we reported the role of branching genes in the inhibition of bud outgrowth by phyB, shade and defoliation signals. Here we present a model that depicts the molecular mechanisms and pathways regulating axillary bud dormancy induced by shade and defoliation signals in the grasses.Key words: axillary bud, dormancy, shade, phytochrome, defoliation, shoot branching, teosinte branched1, MAX2, cell cycle, sorghumThe dormancy and outgrowth of axillary buds is regulated by several plant hormones such as auxin, cytokinins, abscisic acid and strigolactones, and by environmental factors such as light quality, quantity and duration as well as water, temperature and nutrient status.^1–3 Since the fate of an axillary bud is regulated by such diverse hormonal and environmental signals and their interactions, the type of dormancy induced varies. In perennials, three types of bud dormancy have been identified.^4,5 Dormancy mediated by factors within the bud is known as endo-dormancy; while dormancy induced by factors within the plant but outside the bud is called paradormancy or correlative inhibition; the best known example being apical dominance. Dormancy induced due to unfavorable environmental conditions is known as eco-dormancy. Although there is an indepth knowledge about para-dormancy in annuals,⁶ few studies have been conducted on eco-dormancy. Similarly, studies of endo-dormancy have largely been restricted to low-temperature mediated growth-cessation of axillary buds of perennial plants.^7,8 To understand the regulation of dormancy and outgrowth of axillary buds in monocots, we initiated a study on the molecular mechanisms inhibiting bud outgrowth by shade and defoliation signals in sorghum. Our results published in the January 2010 issue of Plant, Cell & Environment indicate that different types of dormancy may be induced in axillary buds of annual grasses by various signals and there may be overlapping and independent molecular mechanisms mediating induction of axillary bud dormancy.     

秋水仙素浓度和处理时间对茉莉腋芽生长发育的影响

为了解秋水仙素处理对茉莉﹝Jasminum sambac (Linn.) Aiton〕腋芽生长发育的影响,以长度为0(未萌发)、3~5和8~10 mm腋芽为实验材料,对500、1000和2000 mg·L-1秋水仙素溶液分别处理24和48 h后腋芽的生长状况以及萌发枝条和叶片的生长和发育状况进行分析,同时,对各处理组花粉母细胞的减数分裂行为进行观察;在此基础上,对秋水仙素处理后茉莉腋芽及萌发枝条的各生物学效应指标进行相关性分析。结果显示：经秋水仙素处理后,各处理组腋芽的生长率和处理指数,以及萌发枝条的长度、最大节间长、最大叶长、最大叶宽、现蕾数、现蕾率、最大蕾长、最大蕾宽和开花率总体上显著(P<0.05)低于对照组(用清水处理未萌发腋芽48 h),而腋芽的抑制率和死亡率显著高于对照组。总体上看,随秋水仙素质量浓度提高,腋芽的生长率和处理指数降低,而抑制率和死亡率升高,萌发枝条的长度和最大节间长缩短,开花率升高,其他指标呈波动变化;随处理时间延长,腋芽的生长率、死亡率和处理指数降低,但抑制率升高,萌发枝条仅现蕾数和开花率降低,其他指标均逐渐提高;随腋芽长度增加,腋芽的抑制率和处理指数降低,但死亡率升高,萌发枝条的现蕾率、现蕾数、最大蕾长和开花率均呈波动变化,其他指标均降低。经秋水仙素处理后,茉莉花粉母细胞在减数分裂过程中存在落后染色体、染色体桥和微核等异常现象,且随秋水仙素质量浓度和腋芽长度增加及处理时间延长,减数分裂后期的细胞异常率逐渐升高。相关性分析结果显示：细胞异常率与腋芽生长率呈显著负相关,与腋芽死亡率呈极显著正相关;腋芽生长率与腋芽抑制率和开花率分别呈显著和极显著(P<0.01)负相关;腋芽抑制率与现蕾率呈显著正相关;处理指数与细胞异常率呈极显著负相关。研究结果表明：秋水仙素浓度和处理时间对茉莉腋芽的生长发育有一定影响;综合考虑各生物学效应指标,茉莉腋芽适宜的诱导条件为用500 mg·L-1秋水仙素溶液处理3~5 mm腋芽24 h。此外,建议将处理指数作为秋水仙素对茉莉腋芽细胞减数分裂影响效应的评价指标之一。     

Revisiting the fate of buds: size and position drive bud mortality and bursting in two coexisting Mediterranean Quercus species with contrasting leaf habit

Understanding the relationships between bud size and position and bud fate through time is crucial for identifying and subsequently modeling the mechanisms underlying tree architecture. However, there is a lack of information on how bud size drives crown architectural patterns in coexisting tree species. We studied bud demography in two coexisting Mediterranean oak species with contrasting leaf habit (Quercus ilex, evergreen; Q. faginea, deciduous). The main objective was to analyse the effect of bud size on the fate of buds with different positions along the shoot (apical, leaf axillary and scale-cataphyll axillary buds). The number, length and position of all buds and stems were recorded in marked branches during 4 years. Study species presented different strategies in bud production and lifespan. The evergreen species showed greater mortality rate than the deciduous one, which produced larger buds. Bud size and position were highly related since apical buds where longer than axillary ones and bud length declined basipetally along the stem. Apical buds had also higher chances of bursting than axillary ones. Within positions, longer buds presented a higher probability of bursting than shorter ones, although no absolute size threshold was found below which bud bursting was impaired. In Q. ilex, four-year-old buds were still viable and able to burst, whereas in Q. faginea practically all buds burst in their first year or died soon after. Such different bud longevities may indicate contrasting strategies in primary growth between both species. Q. ilex is able to accumulate viable buds for several ages, whereas Q. faginea seems to rely on the production of large current-year buds with high bursting probability under favourable environmental conditions.     

In vitro propagation of cashew from young trees

Summary Regeneration of cashew (Anacardium occidentale L.) from shoot explants of young grafts of mature tree origin is described. Establishment of shoot cultures was affected by season of collection, source, and type of explant. Explants from young grafts established better than those collected from field trees, and nodal cuttings regenerated better than shoot tips. Maximum percentage bud break and minimum contamination was noticed when shoots were collected in dry months (January to May). Pre-conditioning of stock plants by hormonal spray with 6-benzyladenine (BA) and gibberellic acid (GA₃) and brief presoaking of shoots in BA had no significant effect on culture establishment. MS (Murashige and Skoog, 1962) medium with half-strength major nutrients, 2.74 mM l-glutamine, 87.6 mM sucrose, and 2.25 gl⁻¹ phytagel was ideal for culture initiation. Inclusion of 0.1% polyvinylpyrrolidone (PVP-360) in the media reduced phenolic exudation. Solidified media was superior to liquid medium. Sucrose/glucose as energy source was found essential in the medium and had significant effect on percentage bud break and shoot development. A repeatable axillary shoot-bud induction was obtained on the above basal medium containing thidiazuron (TDZ) alone and in combination with BA. TDZ at 0.45 μM was best for axillary shoot-bud proliferation (4.5 buds per shoot) with maximum response (100%). Bud elongation could be stimulated in multiple shoots on medium containing 116.8 mM sucrose. In vitro rooting on auxin media and pulsing microshoots in 10 mM naphthalenaacetic acid (NAA) was ineffective. Rooting inability was, however, overcome by a micrografting procedure.     

The bud and root sprouting capacity of Alternanthera philoxeroides after over-wintering on sediments of a drained canal

Alternanthera philoxeroides (Mart.) Griseb. is one of many aggressive invasive plants that can grow in diverse habitats. Aquatic A. philoxeroides forms dense floating mats over the water surface. However, when water levels decrease during winter, some mats become stranded on exposed sediments and are thus exposed to air. Do the stems of these mats possess the capacity to develop new shoots during the next growing season? In this study, we examined the sprouting of sediment-stranded over-wintering mats of A. philoxeroides. Stems of the over-wintering mats were divided into three types (dry, withered, and fresh stems) depending on moisture content and were immersed in water for 4 weeks to observe the sprouting of axillary buds and roots. The results showed that withered stems yielded much more biomass than dry or fresh stems. Stem moisture content significantly affected the sprouting rate and the length growth rate of buds and roots. Dry stems lacked reproductive capacity. The sprouting rate and length growth rate of the buds and roots were higher in fresh stems than in withered stems. Furthermore, the mean values of the bud sprouting rate and the bud length growth rate were highest during the first week, i.e., most of buds sprouted within 1 week or less. Our results suggest that more than 70% (on a dry weight basis) of the stems in stranded mats possessed rapid sprouting capacity even after over-wintering on the sediment for more than 2 months. This strategy may be an adaptation to the fluctuations inherent in many aquatic habitats, and it possibly explains why A. philoxeroides can flourish even after a dry winter. Handling editor: S. M. Thomaz     

Seasonal Effects in the Hormonal Control of Growth in the Submerged Aquatic Macrophyte Ceratophyllum demersum

The season dependent changes in growth response to treatment with auxin or gibberellin were studied in the aquatic macrophyte Ceratophyllum demersum. Control plants show, under experimental conditions, a maximum growth in length in February. In the same period most of the lateral buds appear. Growth of the lateral buds occurs later. IAA causes a stimulation of growth in length from late November or December until February, in concentrations of 10^?9M and 10^?6M. There is almost no stimulation of lateral bud formation by IAA, only a slight increase from late November until December occurs by the lowest concentrations used. The highest concentration used, 10^?4M, is in most cases supraoptimal for lateral bud formation; only when plants become dormant (August), this high dose may stimulate the process. GA₃, in concentrations of 10^?9, 10^?6 or 10^?4M, exhibits a dose dependent increase of the response with respect to growth in length and lateral bud formation. The response occurs earlier than that for IAA: already early in November, or December, until February. Growth of the lateral buds may show only a slight stimulation by IAA as well as GA in winter. From February until April all GA concentrations used could cause a small increase of the growth of sprouts. In the case of IAA, however, only the lowest concentration could cause a small increase.     

Axillary bud proliferation and organogenesis of <Emphasis Type="Italic">Euphorbia pulchurrima</Emphasis> winter rose

Summary Protocols for both axillary bud proliferation and shoot organogenesis of Euphorbia pulchurrima Winter Rose^TM were developed using terminal buds and leaf tissues. Greenhouse-grown terminal buds were placed on Murashige-Skoog (MS) basal medium supplemented with various concentrations of either benzlyaminopurine (BA) or thidiazuron (TDZ). Explants produced the greatest number of axillary buds on media containing between 2.2 and 8.8 μM BA. The number of explants that produced axillary buds increased with increasing BA concentration. TDZ at concentrations between 2.3 and 23.0 μM caused hyperhydricity of shoots and were not effective in promoting shoot proliferation. The most calluses and shoots were produced from leaf midvein sections from in vitro grown plants placed on the medium containing 8.8–13.3 μM BA and 17.1 μM indole-3-acetic acid (IAA) for 1 mo. before transferring to the medium containing only BA. Adventitious buds were produced only from red-pigmented callus, and explants that produced callus continued to produce adventitious shoots in the presence of IAA. Five-mo.-old shoots derived from shoot culture or organogenesis rooted readily in artificial soil with or without treatment with indolebutyric acid, and were acclimatized in the greenhouse.