Evidence that Daminozide, but not Two Other Growth Retardants, Modifies the Fate of Applied Gibberellin A9 in Chrysanthemum morifolium Ramat

Interactions between three growth retardants and gibberellinA₉ (GA₉) in Chrysanthemum morifolium Ramat. cv. Bright GoldenAnne grown in short days have revealed that the particular retardantemployed modifies the response to this gibberellin. When plants were given a foliar spray of daminozide (a substitutedsuccinamic acid), the effects of a subsequent application ofGA₉ to each lateral shoot, on both stem length and the rateof inflorescence development, were relatively small. However,GA₉ was highly active on plants previously sprayed with piproctanylbromide (a quaternary ammonium, piperidinium compound) or onthose given a compost drench of chlorphonium chloride (a quaternaryphosphonium retardant). In the absence of GA₉ all three retardantsreduced stem length and delayed flowering. Irrespective of the extent of the responses to various dosesof GA₉ (1–50 µg per shoot), a close relationshipwas maintained between internode extension and earliness offlowering, as in previous studies with retardants and othergibberellins. On plants which had received chlorphonium chlorideGA₃ and GA₁₃ were highly active and poorly active, respectively. The data suggest that daminozide could act as a retardant notonly by blocking the biosynthesis of gibberellins but also,wholly or partly, by restricting the metabolism or action ofendogenous gibberellins.     

Effects of Growth Retardants, Gibberellic Acid and Indol-3-ylacetic Acid on Stem Extension and Flower Development in the Pot Chrysanthemum (Chrysanthemum morifolium Ramat)

The growth retardants chlorphonium chloride, daminozide anda new, quaternary ammonium compound, piproctanyl bromide, allreduced shoot length and delayed the time of flowering of thepot chrysanthemum (Chrysanthemum morifolium Ramat) cv. BrightGolden Anne grown throughout in short days. The retardants delayedflowering by reducing the rate of flower bud development andnot by influencing bud initiation. In the case of chlorphoniumchloride and daminozide, a single dose of 20 or 40 µggibberellic acid (GA) completely overcame the effects on bothstem length and flowering, whereas when piproctanyl bromidehad been applied GA did not always bring about a total reversal.Responses to GA were recorded a few days after its application.Neither the retardants nor Ga altered leaf number. Only whenpiproctanyl bromide was the retardant did indol-3-ylacetic acidproduce a small but significant increase in stem length at flowering. The results are consistent with a theory of retardant actionin which gibberellins play the dominant role and strongly suggestthat these hormones are a major factor influencing both stemextension and the rate of flower-bud development in the chrysanthemum.They may promote flower development and thus hasten floweringby attracting assimilates to these organs. Chrysanthemum morifolium Ramat, stem extension, flower development, growth retardants, gibberellic acid, indol-3-ylacetic acid     

Size of the Chrysanthemum Shoot Apex in Relation to Inflorescence Initiation and Development

The size of the apical dome of Chrysanthemum morifolium Ramat.at the transition to inflorescence initiation in continuouslight (long days) was not systematically influenced by eitherthe temperature or the irradiance under which the plants weregrown. It was generally 0.26 mm in diameter and c. 3.6 x 10^–3mm³ in volume when the first bract was initiated. The dimensionsof the apical dome of plants in short days were only slightlysmaller at this stage. Similarly, each step in the further developmentof the chrysanthemum inflorescence was associated with a narrowrange of apex sizes, indicating that inflorescence initiationand development are closely related to apex size. Chrysanthemum morifolium Ramat, shoot apex, inflorescence initiation     

Comparative Potency of Nine Gibberellins

Gibberellins A₁ to A₉ have been compared, each at several doselevels, in bioassays based on extension of stems of dwarf gardenpea (Pisum sativum), dwarf bean (Phaseolus vulgaris) and Lunariaannua, of hypocotyls of cucumber (Cucumis sativus) and lettuce(Lactuca sativa), and of leaf sheaths of three dwarf mutants(d–1, d–3, d–5) of maize (Zea mays). GibberellinsA₃ (gibberellic acid) and A₇ are of high potency in most bioassays.A₈ is of negligible potency in all and is probably not a functionalhormone. The other gibberellins show a more or less marked tendencyto specificity. The plants used as bioassay material also differin the specificity of their response. Some, for example, maizedwarfs d–3 and d–5 and lettuce, respond well tomost gibberellins; others, for example, cucumber, respond onlyto a few; extreme specificity is shown by Lunaria annua which,in the unvernalized condition, responds by stem elongation onlyto gibberellin A₇. Dose/response curves of the various gibberellinsare usually parallel, but certain exceptions to this have beenfound. Possible explanations of specificity are discussed inrelation to the results obtained, and it is concluded that insufficientevidence is available to make it possible to draw any validconclusions. Current definitions of gibberellins, whether basedon chemical structure or biological activity, are unsatisfactory.     

Effects of Interactions between Low-temperature Treatments, Gibberellin (GA3) and Photoperiod on Flowering and Stem Height of Spring Rape (Brassica napus var. annua)

Exogenous gibberellin A₃(GA₃) reduced the number of leaf nodesat flowering and time to flowering and increased the stem heightat flowering in three genotypes of spring rape (Brassica napusvar.annua L.). The responses to GA₃were similar to those forlong days (LD) and low-temperature treatments, suggesting thatthe effect of photoperiod and the vernalization response areprobably mediated through gibberellins. The response to exogenousGA₃was greatest in non-cold-treated plants in short days (SD)suggesting that endogenous GAs are limiting in these conditions.CCC, an inhibitor of gibberellin biosynthesis, caused a smallincrease in the number of leaf nodes at flowering and time toflowering and a small decrease in the stem height at flowering,but unexpectedly, its effect was hardly influenced by the applicationof exogenous GA₃. Genotypes that showed the clearest responsesto the treatments with regard to the number of leaf nodes atflowering and time to flowering did not show the clearest responseswith regard to the stem height at flowering; the pattern ofresponses of the number of leaf nodes at flowering and timeto flowering was distinct from that of stem height at flowering.This indicates that flower formation and stem elongation areseparable developmental processes which may be controlled bydifferent endogenous gibberellins, different levels of a specificendogenous gibberellin, or different responses to gibberellin.Copyright 1999 Annals of Botany Company Brassica napus var. annua, gibberellin, photoperiod, spring rape, vernalization.     

A Model of Flowering in Chrysanthemum

A mathematical model of flowering in Chrysanthemum morifoliumRamat. is described which may be used to predict quantitiessuch as the number of primordia initiated by the apex, plastochronduration and apical dome mass before, during and after the transformationof the apical meristem from vegetative to reproductive development.The model assumes that primordial initiation is regulated byan inhibitor present in the apical dome. Within each plastochronthe apical dome grows exponentially, and the inhibitor concentrationdeclines through chemical decay and dilution. When the inhibitorconcentration falls to a critical level a new primordium isinitiated. There is instantaneous production of inhibitor, anda decrease in dome mass corresponding to the mass of the newprimordium. The process continues until the apical dome attainsa particular mass when the first bract primordium is produced.Subsequent primordia compete with the apical dome for substrates,and the specific growth rate of the dome declines with successiveplastochrons. Eventually, the net mass of the dome starts todecline until it is entirely consumed in the production of floralprimordia. Chrysanthemum morifoliumRamat, flowering, primordial initiation     

Activity of Gibberellins A1 to A0 in the Avena First-leaf Bioassay, and Location after Chromatography

Activity curves are determined for gibberellins A₁ to A₀ bythe Avena first-leaf bioassay method. Gibberellins A¹, A₄ andA₅ can be detected at 10^-11 or 10^-10 g/ml and give optimum activityof approximately 230 per cent elongation (water controls = 100per cent). Gibberellins A²A³, and A⁹ can be detected at 10^-3g/mland give optimum activity of approximately 200 per cent. GibberellinsA₆ and A₇ can be detected at 10^-5g/ml; GA₇ gives optimum activityof around 190 per cent. All the gibberellins except GA₈ canbe detected by this bioassay method after chromatography inn-butanol: 1.5 N ammonia (3: 1) and benzene: acetic acid: water(4: 2: 1) when applied to the paper at concentrations from O.Ito µg. The sensitivity of the method is compared withthat of other gibberellin bioassay methods.     

Stimulation of the Flowering of Pharbitis nil Chois. by Gibberellin A3 : Time Dependent Action at the Apex

Gibberellin A₃ (GA₃) stimulated flowering when it was appliedto the shoot apex of seedlings of Pharbitis nil, dwarf strainKidachi; but, not when it was applied to the cotyledons. GA₃applied to the plumule before or shortly after the start ofan inductive dark period promoted both flowering and shoot elongation;but, the later the time of application during the dark periodless the promotion of flowering, although marked promotion ofshoot elongation always took place. The variation with time in the response of flowering to GA₃indicates that early floral processes at the apex are stimulatedby GA₃, but that subsequent processes are insensitive to it.The early processes of floral stimulus produced by a 16 hr inductivedark period probably are completed within 20 hr at 28°Cafter the end of the dark period. At low temperatures, suchas 15 and 20°C, early floral processes continued for morethan 40 hr. When cotyledons were removed at various times, the export ofthe floral stimulus to the shoot apex was apparent within hoursof the generation of the floral stimulus in the cotyledons,which started with the passage of the critical 9-hr dark period. (Received February 18, 1981; Accepted March 24, 1981)     

Abnormalities in Chrysanthemum Regenerated from Long Term Cultures

Plants regenerated from leafy callus of Chrysanthemum morifoliumRamat. maintained for 9 years (LC plants) were compared to thoseregenerated from leafy callus maintained for 1 month (SC plants)in order to assess the effects of long-term culture. LC plantsdiffered morphologically from those derived from the 1-monthculture. Aberrant forms, proliferation of apical buds, variableleaf shapes and stunted growth were observed in 15 per centof the LC plants. The remaining 85 per cent were characterizedby excessive growth of lateral shoots. Flowers were smallerand irregularly formed in most LC plants. Although the growthrates of plants in both LC and SC groups were similar, floweringwas delayed considerably in the LC plants. Application of GA₃or IAA had no effect in restoring normal form. Genetic instability,chimeral rearrangement and residual hormone effects are offeredas possible explanations for the abnormalities observed. Tissue culture, Chrysanthemum morifolium, phenotypic variability     

Uptake and distribution of the growth retardant, aminozide, in relation to control of latera shoot elongation in Chrysanthemum morifolium

The uptake, stability and redistribution of the plant growth retardant, aminozide, in ‘pinched’ plants of Chrysanthemum morifolium Ramat. cv. Lemon Princess Anne were examined in relation to control of lateral shoot elongation. Foliar uptake was most rapid over the first few hours, and was almost complete within 72 h. More of the available aminozide was taken up by the young lateral shoots than by older foliage on the main stem. The aminozide content of entire plants generally remained constant over several weeks, indicating that the compound was relatively stable within the plant. The time scale and pattern of redistribution of foliar- and root-applied aminozide suggests that the compound may be translocated in both phloem and xylem. Spray application to young lateral shoots was as effective in controlling their elongation as application to all aerial organs. Basipetal transport of aminozide from lateral shoots was slight. The results are discussed in relation to the site of action of the compound and to its application in commercial practice.     

Interaction of growth retardants,daylength, and gibberellins A19, A20, and A1 on shoot elongation in birch and alder

Gibberellins A₁₉, A₂₀, and A₁ were applied to seedlings of birch (Betula pubescens Ehrh.) and alder (Alnus glutinosa (L.) Gaertn.) in order to test their ability to counteract growth inhibition induced by growth retardants (ancymidol and BX-112) or short day (SD, 12 h) photoperiod. Ancymidol inhibits early and BX-112 inhibits late steps in gibberellin biosynthesis. BX-112 inhibited stem elongation in both species while ancymidol, applied as a soil drench, was effective in alder only. Growth retardants affected stem elongation mainly by inhibiting elongation of internodes. All three gibberellins were equally active when applied to seedlings treated with ancymidol; however, only GA₁ was able to counteract the growth inhibition induced by BX-112. SD-induced cessation of elongation growth in birch was counteracted by GA₁, and to some degree, by GA₂₀, while GA₁₉ was inactive. SD treatment did not induce cessation of apical growth in alder. These results are consistent with the hypothesis that of gibberellins belonging to the early C-13 hydroxylation pathway, GA₁ is the only active gibberellin for stem elongation.     

Antagonistic and Synergistic Interactions between Ancymidol and Gibberellins in Shoot Growth of Cucumber (Cucumis sativus L. )

Effects of the plant growth retardant, ancymidol, on the growthand morphology of the shoot system of cucumber (Cucumis sativusL. ) were investigated. Ancymidol inhibited stem elongation,reducing both number and length of internodes. Reduction inleaf area, attributable to a reduction in both cell size andnumber, was accompanied by an increase in chlorophyll per unitarea. The retardant decreased apical dominance and delayed anthesis.Gibberellic acid fully reversed ancymidol-induced inhibitionof stem elongation, internode length and production, and leafexpansion. GA_4/7 and ancymidol gave a synergistic promotionof stem elongation by increasing elongation of younger internodesand increasing internode production. Synergistic promotion ofpetiole elongation by this combination was also observed. Ancymidol,applied 7 d previously either to the shoot or root, severelyreduced the level of gibberellin-like activity in bleeding sapcollected from decapitated plants.     

The Relationship of Endogenous Gibberellins to Light-regulated Stem Elongation Rates in Dwarf and Normal Cultivars of Pisum sativum L.

Dwarf cultivar Progress No. 9 and normal cultivar Alaska ofPisum sativum L. were grown under conditions of darkness orred light. Red light decreased the stem elongation rate of bothcultivars. Gibberellins present during the linear phase of stemelongation were isolated and the two main components were tentativelyidentified by gas chromato-chromatography and mass spectrometryas Gibberellin A₁ and A₅. Both gibberellins varied quantitativelywithin and between cultivar and treatment groups, and the amountspresent were inversely related to stem elongation rate. Althoughthe stem elongation rate of plants grown under red light wasrepressed, endogenous gibberellin was not limiting and was asmuch as two-fold higher in red light-grown plants than in dark-grownplants. The levels of endogenous gibberellin in dawrf plantsindicated that the genetic growth limitation was not due toa gibberellin deficiency. (Received May 26, 1981; Accepted January 28, 1982)     

A Modified Micro-Drop Bioassay Using Dwarf Rice for Detection of Femtomol Quantities of Gibberellins

The sensitivity of the micro-drop assay with dwarf rice (Oryzasativa L., cv. Tan-ginbozu and cv. Waito-Q to gibberellins (GAs)was increased conspicuously by the use of assay plants thathas been treated with uniconazole (S-3307), an inhibitor ofthe biosynthesis of GAs. The Tan-ginbozu plants treated withS-3307 responded to 10 fmol/plant of GA₃ (ca. 3.5 pg/plant)and to 30 fmol/plant of gibberellins A₁, A₄, A₇, A₁₉ and A₂₀.Waito-C plants treated with S-3307 responded to 10 fmol of GA₃and to 30 fmol/plant of gibberellins A₁, A₄ and A₇. GibberellinsA₉, A₁₉ and A₂₀ had much less of an effect on the treated Waito-Cplants than did gibberellins A₁, A₃, A₄ and A₇. Furthermore,treatment with S-3307 counteracted the inhibition of growthof both cultivars by abscisic acid. Thus, the modified micro-dropassay should prove very useful for the detection of minute amountsof GAs in plant extracts. (Received October 3, 1988; Accepted March 29, 1989)     

Physiological Controls on the Production of Cleistogamous and Chasmogamous Flowers in Lamium amplexicaule L

Plants of Lamium amplexicaule, grown under short-day field conditionsin Northern California produce predominantly closed flowers.Under long-day field conditions, plants may produce up to 50per cent open flowers, the same total number of flowers beingproduced under each daylength regime. A 20 ml drop of GA₃ or GA₇ (100µM) was applied to themain shoot apex of plants growing under short-day conditions,and all subsequently produced flowers opened. CCC, an inhibitorof gibberellin synthesis, was applied (0.06 per cent) to thesoil of seedlings grown under long-day conditions. The CCC-treatedplants were dwarfed and bore only closed flowers. With GA₇ appliedexogenously to the CCC-treated shoots, inhibition was released,resulting in elongated internodes and open flower production.The timing of flower production and internodal extension inLamium amplexicaule are positively correlated. When floral primordiawere removed from main shoots, the average internode lengthsdecreased. The number of nodes produced in treated plants wasincreased as a result of flower removal. Exogenous GA₇ (10 µM)applied to the nodes from which flowers were removed resultedin internodal extension but had no effect on node number. Twoprocesses that may contribute to the control of the productionof open and closed flowers in Lamium amplexicaule are: (1) anincreasing anther sac size from lower to upper node flowersthat may exert control locally, via GN production, on corollaexpansion, and (2) a photoperiodic control. Lamium amplexicaule L, henbit, cleistogamy, chasmogamy, gibberellins, gibberellic acid (GA₃), (2 chloroethyl) trimethylammonium chloride (cycocel)     

Effects of a New Plant Growth Retardant (E)-1-(4-Chlorophenyl)-4,4-dimethyl-2-(1,2,4-triazol-1-yl)-1-penten-3-ol (S-3307) on the Growth and Gibberellin Content of Rice Plants

The properties and mode of action of a new plant growth retardant,(E)-1-(4-chlorophenyl)-4,4-dimethyl-2-(1,2,4-triazol-1-yl)-1-penten-3-ol(S-3307), were investigated. When a dipping method was used,S-3307 at 2.2 ? 10^-7 M (0.064 ppm) retarded the growth of riceplants by 50% of the value found for the control. The retardationof growth was removed by a gibberellin application (8.7?10^-5M). S-3307 had nearly no effect on the shoot elongation inducedby gibberellin. The amounts of gibberellin-like substances inrice shoots were decreased by S-3307 treatment in proportionto the degree of growth retardation. This observation was confirmedwith GA₁ and GA₁₉, the main gibberellins in the rice plant.Our results indicate that S-3307 inhibits gibberellin biosynthesisin rice plants. (Received November 7, 1983; Accepted March 21, 1984)     

Flow Cytometric Determination of Relative Nuclear DNA Contents in Bicellulate and Tricellulate Pollen

Nuclear DNA content in mature pollen was measured with a flowcytometer Pollen of Lilium longiflorum, Dendranthema grandiflora(syn Chrysanthemum monfolium) and Zea mays was chopped and stainedwith the DNA fluorochrome DAPI DNA levels, expressed as arbitraryC values, were compared with those of nuclei isolated from leafor root material of the same plants In mature tricellulate pollen the generative cell is dividedafter second pollen mitosis into two sperm cells Tricellulatepollen from maize and chrysanthemum gave rise to one large 1Cpeak and, only in the case of chrysanthemum, a much smallerone at the 2C level These results suggest that the haploid nucleiof the vegetative as well as both sperm cells in tricellulatepollen are arrested in the G₁ stage of nuclear division Thesmall 2C peak in the case of chrysanthemum probably arose froma fraction of pollen with the sporophytic chromosome number(2n pollen) In contrast to this, mature bicellulate lily pollengave rise to two identical peaks at the 1C and the 2C levelFrom this result it was concluded that in bicellulate pollen,the 1C peak is caused by the signal of the haploid vegetativenucleus arrested in the G₁ stage of nuclear division, whereasthe 2C peak originates from the haploid generative nucleus whichhas already undergone DNA synthesis and is arrested in G₂ Lilium longiflorumThunb, lily, Dendranthema grandiflora Tzelev (syn Chrysanthemum morifolium Ramat ), chrysanthemum, Zea maysL, maize, male gametophytic cells, vegetative cells, generative cells, sperm cells, unreduced pollen, sporophytic cells, relative nuclear DNA contents, replication stage     

Phase Change in Hedera helix L: II. THE POSSIBLE BOLE OF ROOTS AS A SOURCE OF SHOOT GIBBERELLIN-LIKE SUBSTANCES

When synthesis was estimated by the agar diffusion techniqueboth basal and lateral adventitious roots of Hedera helix L.in the juvenile growth phase were shown to synthesize gibberellin-likesubstances. Seedlings and cuttings from juvenile ivy could begrown in water culture for several weeks. When roots were excisedfrom these plants shoot growth was reduced in comparison withthat of intact plants. The stems, apices, and leaves of derootedseedlings and cuttings contained lower levels of extractablegibberellin-like substances than comparable organs of intactplants. The major zone of gibberellin-like activity in intactplants co-chromatographed with gibberellins A₁ and A₃. Whenthese gibberellins were applied to plants grown in culture theywere found to promote growth of intact but not derooted plants.These findings are discussed in relation to the role of rootfactors and particularly gibberellins in phase change.     

Effects of Irradiance and Temperature on Flowering of Chrysanthemum morifolium Ramat. in Continuous Light

The short-day plant Chrysanthemum morifolium cv. Polaris initiatedflower buds in all irradiances of continuous light from 7.5to 120 W m^–2. As the irradiance increased, the transitionto reproductive development began earlier and the number ofleaves initiated before the flower bud was reduced. The autumn-floweringcultivars Polaris and Bright Golden Anne, and the summer-floweringGolden Stardust were also grown in continuous light at differenttemperatures; all initiated flower buds at temperatures from10 to 28 °C but only the buds of Golden Stardust developedto anthesis and then only at 10 and 16°C. Flower initiationbegan earliest at 16–22 °C, and the number of leavesformed before the flower bud was increased at 28°C. GoldenStardust was exceptional in that the number of leaves formedwas also increased at 10 °C. Axillary meristems adjacentto the terminal meristem initiated flower buds rapidly at 10°C but not at 28 °C in all three cultivars. These resultsare discussed in relation to the autonomous induction of flowerinitiation and the effects of the natural environment on floweringof chrysanthemum. Chrysanthemum morifolium Ramat, flowering, irradiance, temperature     

Inhibition of Rooting of Cuttings by Gibberellic Acid: With one Figure in the Text

Gibberellic acid inhibited rooting but increased extension ofpea and bean stem cuttings. Indolylacetic acid usually had acontrary effect both on extension and on root initiation. Itwas found possible to separate the effects of gibberellic acidon extension and rooting. Small doses of gibberellic acid appliedto the bases of cuttings reduced rooting without increasingextension. Small apical doses increased extension without reducingrooting. Disbudding cuttings prevented extension, but gibberellicacid inhibited rooting of disbudded cuttings as strongly asthat of normal cuttings. It has thus been found necessary todiscard an earlier hypothesis that inhibition of rooting bygibberellic acid was a consequence of a diversion of essentialmetabolites to the extending apical regions of the cutting.The antagonism between gibberellic acid and indolylacetic acidwas non-competitive. Gibberellin A₁, known to occur naturallyin Phaseolus, was as active a rooting inhibitor as gibberellicacid. It is now believed that inhibition of rooting of cuttingsby gibberellins is a direct local effect, preventing those earlycell divisions involved in transformation of mature stem tissuesto a meristematic condition.