The differential effects of C-16,17-dihydro gibberellins and related compounds on stem elongation and flowering in Lolium temulentum

Plants of Lolium temulentum L. cv. Ceres grown under short days (SDs) can be induced to initiate inflorescences either by exposure to one long day (LD) or by single applications of some gibberellins (GAs), which also enhance the flowering response to one LD. Single doses of up to 25 μg per plant of C-16, 17-dihydro-GA₅ were about as effective as GA₅ for promoting flowering after one LD but inhibited stem elongation by up to 40% over three weeks. The promotion of flowering but not the inhibition of elongation by 16, 17-dihydro-GA₅ was reduced in SDs or in LDs low in far-red (FR) radiation. With shoot apices cultured in vitro, 16, 17-dihydro-GA₅ was more florigenic than GA₃ for apices excised after one LD of 14 h or more, but less florigenic for apices excised from plants in shorter days. 16, 17-Dihydro-GA₅ was ineffective compared with GA₁, GA₃ and GA₅ for α-amylase production by half-seeds of Lolium, a response concordant with its effect on stem elongation. As with GA₅, 16, 17-dihydro derivatives of GA₁, GA₃, GA₂₀ and several other GAs were more effective for flowering and less effective for stem elongation than the GAs from which they were derived. Hydroxylation at C-17 and/or C-16 generally reduced the effectiveness of 16, 17-dihydro-GA₅ for flowering. These results extend the known features of GA structure which favour flowering relative to stem elongation in L. temulentum. Moreover, C-16, 17-dihydro-GA₅ mimics, in its daylength- and wavelength-dependence and lack of stem elongation, characteristics of the LD stimulus in L. temulentum.     

Gibberellins and Stem Growth as Related to Photoperiod in Silene armeria L

Stem growth and flowering in the long-day plant Silene armeria L. are induced by exposure to a minimum of 3 to 6 long days (LD). Stem growth continues in subsequent short days (SD), albeit at a reduced rate. The growth retardant tetcyclacis inhibited stem elongation induced by LD, but had no effect on flowering. This indicates that photoperiodic control of stem growth in Silene is mediated by gibberellins (GA). The objective of this study was to analyze the effects of photoperiod on the levels and distribution of endogenous GAs in Silene and to determine the nature of the photoperiodic after-effect on stem growth in this plant. The GAs identified in extracts from Silene by full-scan combined gas chromatography-mass spectrometry (GC-MS), GA₁₂, GA₅₃, GA₄₄, GA₁₇, GA₁₉, GA₂₀, GA₁, GA₂₉, and GA₈, are members of the early 13-hydroxylation pathway. All of these GAs were present in plants under SD as well as under LD conditions. The GA₅₃ level was highest in plants in SD, and decreased in plants transferred to LD conditions. By contrast, GA₁₉, GA₂₀, and GA₁ initially increased in plants transferred to LD, and then declined. Likewise, when Silene plants were returned from LD to SD, there was an increase in GA₅₃, and a decrease in GA₁₉, GA₂₀, and GA₁ which ultimately reached levels similar to those found in plants kept in SD. Thus, measurements of GA levels in whole shoots of Silene as well as in individual parts of the plant suggest that the photoperiod modulates GA metabolism mainly through the rate of conversion of GA₅₃. As a result of LD induction, GA₁ accumulates at its highest level in shoot tips which, in turn, results in stem elongation. In addition, LD also appear to increase the sensitivity of the tissue to GA, and this effect is presumably responsible for the photoperiodic after-effect on stem elongation in Silene.     

Effect on the Progeny of Applying Different Day Length and Hormone Treatments to Parent Plants of Lactuca scariola

Seedlings of the self-fertilizing species Lactuca scariola L. grown continuously in 8 h days did not flower even one year from sowing. Seedlings grown in 16 h days uatil flower buds appeared 96 days after germination were either transferred to 8 h days or treated weekly with gibberellic acid (GA₃), abscisic acid (ABA) or chlormequat (CCC) and retained, together with untreated control plants, in 16 h days. Each growth regulator caused characteristic morphological changes in the treated plants. All these plants flowered and produced seeds but the seeds showed distinct differences in weight, in their time to germination and in the seedlings which they produced. Germination and seedling characters depended on the light regime during germination as well as on the chemical applied to the parent plant and the rate of application. The parental treatment also affected the shape and size of the seedlings on a given day after germination, and certain treatments of the parent plant (transfer from long to short days and treatment with CCC in long days) advanced the flowering date of the seedlings. The gibberellin level in the seeds was raised, in increasing order, by treatment of the parent plant with 100 mg/1 GA₃, transfer from long to short days, 10 mg/1 GA₃, and 5000 mg/l CCC. It is suggested that the effect of day length on plant performance is mediated by the level of growth regelating substances within the plant and that the behaviour of seeds can be modified by the parental environment via the accumulation of different levels of certain growth factors in the seeds. A rise of one growth substance in the parent plant can result in the accumulation of a different one in the seeds.     

Environmental control of growth and development of Scrophularia marilandica

Summary Seedlings of Scrophularia marilandica were grown at different combinations of day/night temperature and photoperiod under controlled conditions. The species flowered in long days. The stems of plants grown at low temperature and short photoperiod failed to elongate. Treatment with gibberellic acid (GA₃) simulated the effect of increasing temperature and photoperiod and caused stem elongation in plants which would otherwise not have elongated. Application of GA₃ to plants grown at high temperature and long photoperiod resulted in increased stem elongation and flowering. The growth retardant (2-chloroethyl)trimethylammonium chloride (CCC) had little effect on rosette plants grown at low temperature and short photoperiod. Application of CCC to +GA₃ plants grown at a higher temperature and long photoperiod gave a significant increase in stem height. The interaction between temperature and applied GA is described in an experiment using plants grown at high and low temperatures for varying periods of time.This work was supported by National Science Foundation Grant GB 17483.     

Allogibberic acid: An inhibitor of flowering in Lemna perpusilla

Allogibberic acid (I) has been identified as the compound responsible for the inhibition of flowering, increase in frond multiplication rate and decrease in frond size produced in Lemna perpusilla 6746 by autoclaved, unbuffered aqueous solutions of gibberellic acid (VII). 13-Deoxyallogibberic acid (IV), a product of autoclaving aq. GA₇ (VIII) solutions, also inhibits flowering in L. perpusilla and is about 10 times more active than allogibberic acid.     

The effect of gibberellic acid on the buoyancy of Spirodela intermedia W. Koch

Under laboratory conditions concentrations of gibberellic acid (GA₃) up to 0.1 mg 1^?1 had little effect on the growth of Spirodela intermedia W. Koch. However, at higher concentrations up to 3 mg 1^?1, growth was affected; frond air spaces changed shape and size, roots were shed, fissures developed in the adaxial epidermis, and the plants lost buoyancy. These changes were accompanied by an increase in water content. It is suggested that the anatomical modification induced by GA, suppress the buoyancy effect of the aerenchyma by allowing the entrance of water into the lacunae. The potential relationship to the action of herbicides is discussed.     

The effects of hormones and saccharides on growth and flowering of green and herbicides-treatedChenopodium rubrum L. plants

The medium forin vitro culture of green and SANDOZ herbicides-treatedChenopodium rubrum L. plants contained saccharides and hormones in different concentrations. Five days after sowing, the plants were exposed to non-inductive (15 long days—LD) or inductive (6 short days—SD + 9 LD) photoperiodic conditions. The length of hypocotyl and cotyledon blade were measured and percentage of flowering was scored. Gibberellic acid (GA₃) stimulated hypocotyl growth of green and photobleached plants under SD and inhibited under LD conditions. Indole-3-acetic acid (IAA) slightly stimulated hypocotyl growth of green plants only under LD conditions. Benzylaminopurine (BAP) inhibited hypocotyl growth regardless of photoperiodic regime. The optimal concentration of glucose or saccharose for flowering in green and SANDOZ-treated plants was 5%. In green SAN 9785-treated plants exogenous saccharides compensated lack of photosynthates to bring about full flowering, but SAN 9789-treated plants needed in addition GA₃.     

Gibberellins, Endogenous and Applied, in Relation to Flower Induction in the Long-Day Plant Lolium temulentum

Changes in endogenous gibberellin-like substances (GAs) and related compounds in the shoot apices of Lolium temulentum during and after flower induction by one long day was examined for plants grown in three consecutive years. The total GA level in the shoot apical tissue was high (up to 42 micrograms per gram dry weight, or 3 × 10⁻⁵ molar GA₃ equivalents), increasing several-fold on the day after the long day and then declining. Of the many GA-like substances present, the putative polyhydroxylated components—with HPLC retention times between those of GA₈ (three hydroxyls) and GA₃₂ (four hydroxyls), and accounting for about a quarter of the total GA activity—were most consistent and striking in their changes. Their level in the apices increased 3- to 5-fold on the day after the long day and then subsided. When various GAs were applied to plants in noninductive short days, flower initiation was induced by several, most notably by GA₃₂, GA₅, 2,2-dimethyl GA₄, GA₃, and GA₇. GA₃₂ was most like one long day in eliciting a strong flowering response while having little effect on stem growth, whereas GA₁ had the opposite effect. It is suggested that highly hydroxylated C-19 GAs may play a central role in the induction of flowering in this long-day plant.     

Gibberellins in Relation to Flowering and Stem Elongation in the Long Day Plant Silene armeria

Two long days induced some flowering and 4 or more long days caused 100% flowering in Silene armeria. On long days microscopically detectable flower primordia were first seen after 6 days, which is at least 1 day before the start of stem elongation. Both gibberellin A₃ and A₇ caused flowering on short days, but the results were variable and flowering was never 100%. Three different gibberellins were detected in Silene extracts. The pattern of gibberellins extracted from plants on short and long days was qualitatively the same, but on long days gibberellin content was up to 100% higher than on short days. Only small amounts of diffusible gibberellins were obtained from Silene shoot tips (including very young leaves) on short days. However, on long days the diffusible gibberellins increased by as much as 10-fold after 4 to 6 long days but then declined somewhat after 10 long days. The gibberellins extracted from the shoot tips at the completion of the diffusion period also increased under long days, although the increase was not as large as for the diffusible gibberellins. An A₅-like gibberellin present in extracts was not detected in diffusates.     

Genetic Regulation of Development in Sorghum bicolor: V. The ma(3) Allele Results in Gibberellin Enrichment

Sorghum bicolor genotypes, near isogenic with different alleles at the third maturity locus, were compared for development, for responsiveness to GA₃ and a GA synthesis inhibitor, and occurrence and concentrations of endogenous GAs, IAA, and ABA. At 14 days the genotype 58M (ma₃^Rma₃^R) exhibited 2.5-fold greater culm height, 1.75-fold greater total height, and 1.38-fold greater dry weight than 90M (ma₃ma₃) or 100M (Ma₃Ma₃). All three genotypes exhibited similar shoot elongation in response to GA₃, and 58M showed GA₃-mediated hastening of floral initiation when harvested at day 18 or 21. Both 90M and 100M had exhibited hastening of floral initiation by GA₃ previously, at later application dates. Tetcyclacis reduced height, promoted tillering, and delayed flowering of 58M resulting in plants which were near phenocopies of 90M and 100M. Based on bioassay activity, HPLC retention times, cochromatography with ²H₂-labeled standards on capillary column GC and matching mass spectrometer fragmentation patterns (ions [m/z] and relative abundances), GA₁, GA₁₉, GA₂₀, GA₅₃, and GA₃ were identified in extracts of all three genotypes. In addition, based on published Kovats retention index values and correspondence in ion masses and relative abundances, GA₄₄ and GA₁₇ were detected. Quantitation was based on recovery of coinjected, ²H₂-labeled standards. In 14 day-old-plants, total GA-like bioactivity and GA₁ concentrations (nanograms GA/gram dry weight) were two- to six-fold higher in 58M than 90M and 100M in leaf blades, apex samples, and whole plants while concentrations in culms were similar. Similar trends occurred if data were expressed on a per plant basis. GA₁ concentrations for whole plants were about two-fold higher in 58M than 90M and 100M from day 7 to day 14. Concentrations of ABA and IAA did not vary between the genotypes. The results indicate the mutant allele ma₃^R causes a two- to six-fold increase in GA₁ concentrations, does not result in a GA-receptor or transduction mutation and is associated with phenotypic characteristics that can be enhanced by GA₃ and reduced by GA synthesis inhibitor. These observations support the hypothesis that the allele ma₃^R causes an overproduction of GAs which results in altered leaf morphology, reduced tillering, earlier flowering, and other phenotypic differences between 58M and 90M or 100M.     

The relative significance for stem elongation and flowering in Lolium temulentum of 3β-hydroxylation of gibberellins

In previous experiments with many gibberellins (GAs) and GA derivatives applied to Lolium temulentum L., quite different structural requirements were evident for stem elongation on the one hand and for the promotion of flowering on the other. Whereas hydroxylation at carbons 12, 13 and 15 enhanced flowering relative to stem growth, the reverse was the case at carbon 3 (L.T. Evans et al. 1990, Planta 182, 97–106). The significance of hydroxylation at carbon 3 is examined in this paper. The application of inhibitors of 3β-hydroxylation, including C/D-ring-rearranged GAs, reduced stem growth but, in the case of the two acylcyclohexanediones, increased the flowering response when applied on the inductive long day. Later applications of the acylcyclohexanediones, made after floral initiation had occurred, were inhibitory to flowering, suggesting that subsequent inflorescence development requires 3β-hydroxylated GAs. Applications of the 3α-hydroxy epimers of GA₁, GA₃ and GA₄ gave slightly less promotion of flowering in comparison with the 3β-hydroxy GAs, but far less promotion of stem elongation, except in the case of 3-epi-GA₄, which was comparable to GA₄. The 3α-hydroxy epimer of 2,2-dimethyl GA₄ gave less promotion of flowering than its 3β-hydroxy epimer but almost no promotion of stem elongation. The 3α-hydroxy epimers of GA₃ and 2,2-dimethyl GA₄ did not act as competitive inhibitors of the stem elongation elicited by GA₃ and 2,2-dimethyl GA₄, respectively. These results extend the differences in GA structure which favour flowering as opposed to stem elongation, and indicate that 3-hydroxylation and its epimeric configuration are of much greater importance to stem elongation than to flower initiation in Lolium.     

GA3和Spd对杜鹃开花期光合特性和抗氧化系统的影响

为探讨GA_3和Spd对杜鹃(Rhododendron simsii)开花花期和开花品质的影响,研究了外源GA_3和Spd对杜鹃开花期光合特性和抗氧化系统的变化。结果表明,外源GA_3对花期有显著的提前作用,Spd对花期有明显的延迟作用,但两者均使花期延长、花径增大且成花率提高。GA_3和Spd处理提高了花期叶片的光合色素含量和净光合速率(Pn)、气孔导度(Gs)和胞间CO_2浓度(Ci);GA_3处理提高了叶片的蒸腾速率(Tr),而Spd使叶片的Tr下降,两者均有效缓解了末花期叶绿素含量的下降。GA_3和Spd处理显著降低了花瓣MDA含量,提高了抗氧化酶SOD、POD和CAT活性,并减缓了末花期SOD的下降,有效延缓了衰老进程,延长花期。以1 600 mg L~(–1) GA_3和0.10 mmol L~(-1) Spd处理效果较好,能有效提高杜鹃花的观赏品质。     

Studies on Flowering Responses of Urena lobata

Urena lobata L. is a qualitative short-day plant with a critical dark period of about 12 hr. A minimum of 12 short days are required for floral initiation. Gibberellic acid (GA₃) sprayed onto the leaves promoted flowering. The growth retardant, (2-chloroethyl)-trimethylammonium chloride (CCC) markedly inhibited flowering and stem elongation. This inhibition was reversed by subsequent application of GA₃.     

Effect of GA4+7 on growth and cellular change in uniconazole-treated hibiscus

Hibiscus rosa-sinensis Jane Cowl in 1.5–1 pots were given a soil drench of 0.2 mg uniconazole, pruned 2 weeks later, and treated with a foliar application of GA₄₊₇ at 0, 25 (once or four times every 2 weeks), 50 (once or twice every 4 weeks), or 100 mg L^-1. One application of GA₄₊₇ at 100 mg L^-1, two applications at 50 mg L^-1, and four applications at 25 mg L^-1 were more active in partially restoring stem elongation and caused nearly normal leaf production than other GA treatments, but promoted the abscission of the lower leaves. The size of the individual leaves, but not stem diameter, increased following GA₄₊₇ application. Multiple applications of GA₄₊₇ stimulated flowering of the retarded plants. Uniconazole resulted in short pedicels bearing short cells with increased diameter, as well as larger pith, vascular, and cortical tissues than the untreated control. Four applications of 25 mg L^-1 GA₄₊₇ to uniconazole-treated plants resulted in long pedicels, having long cells similar to the control. Results of the histological study suggest that uniconazole either slowed cell division or caused cell division to cease early.     

Effect of Gibberellic Acid and Monophenols on Flowering of lmpatiens balsamina in Relation to the Number of Inductive and Non-inductive Photoperiodic Cycles

A single treatment of plants with GA₃ (gibberellic acid) is not adequate to cause induction under LD (long day: 24-h photo-period) condition, but its effect is added to the sub-threshold induction caused by one SD (short day: 8-h photoperiod) cycle. Floral bud initiation is hastened, and the number of floral buds and flowers per flowering plant increases in plants receiving a single treatment with the combination GA₃+ SA (salicylic acid) accompanying a single SD cycle. However, the increase on 10 replicate basis is more marked in plants receiving three treatments with the combination GA₃+β-N (β-naphthol) and five treatments with the combination GA₃+ SA accompanying six and 10 SD cycles, respectively. The number of floral buds and flowers decreases with an increase hi the number of SD cycles, but it is higher in plants treated with GA₃, SA or GA₃+β-N than in the water-treated controls. — Under long days, treatment of plants with the combinations GA₃+ SA or GA₃+β-N accelerates the initiation as well as increases the number of floral buds. While a minimum of five treatments with GA₃ or of 25 with SA or β-N alone is needed for floral bud initiation under a 24-h photoperiod, three treatments are adequate to induce floral buds with the combination GA₃+ SA or GA₃+β-N under continuous illumination. Ten or more treatments with these combinations under a 24-h photoperiod produce more flowers than the same treatments under an 8-h photoperiod.     

Gibberellic Acid Reduces Flowering Intensity in Sweet Orange [Citrus sinensis (L.) Osbeck] by Repressing CiFT Gene Expression

In Citrus, gibberellic acid (GA₃) applied at the floral bud inductive period significantly reduces flowering intensity. This effect is being used to improve the fruit set of parthenocarpic cultivars that tend to flower profusely. However, the molecular mechanisms involved in the process remain unclear. To contribute to the knowledge of this phenomenon, adult trees of ‘Salustiana’ sweet orange were sprayed at the floral bud inductive period with 40?mg?L^?1 of GA₃ and the expression pattern of flowering genes was examined up to the onset of bud sprouting. Trees sprayed with paclobutrazol (PBZ, 2,000?mg L^?1), a gibberellin biosynthesis inhibitor, were used to confirm the effects, and untreated trees served as control. Bud sprouting, flowering intensity, and developed shoots were evaluated in the spring. GA₃ significantly reduced the number of flowers per 100 nodes by 72% compared to the control, whereas PBZ increased the number by 123%. Data of the expression pattern of flowering genes in leaves of GA₃-treated trees revealed that this plant growth regulator inhibited flowering by repressing relative expression of the homolog of FLOWERING LOCUS T, CiFT, whereas PBZ increased flowering by boosting its expression. The activity of the homologs TERMINAL FLOWER 1, FLOWERING LOCUS C, SUPPRESSOR OF OVEREXPRESSION OF CONSTANS 1, and APETALA1 was not affected by the treatments. The number of flowers per inflorescence, in both leafy and leafless inflorescences, was not altered by GA₃ but increased with PBZ; the latter paralleled LEAFY relative expression. These results suggest that GA₃ inhibits flowering in Citrus by repressing CiFT expression in leaves.     

Gibberellins and Inhibitors in Relation to Flowering of White Clovers (Trifolium repens L.)

Flower primordia appeared sooner and flowering intensity increasedas day length was extended beyond 8 h (short day) in two whiteclovers: cv. Tamar and cv. Tammisto, originating from Israeland Finland, respectively. Application of GA₃ under short dayscaused Tamar to flower more intensively as much as the doseof GA₃ was increased, but it did not affect the flowering ofTammisto. The level of gibberellin-like substances in stolon apices washigher under long (16 h) than under short days in both cultivars.The level of inhibitors extracted from leaves was not affectedby day length in Tamar. However, in Tammisto this level wasalmost twice as high under short than under long days. It issuggested that the presence of a relatively high level of inhibitorsin Tammisto when grown under short days interfered with theactivity of gibberellins in its effect on flowering. ABA wasamong the inhibitors: its application under long days had noeffect on flowering, but it increased the number of stolons.Possibly inhibitors other than ABA are involved in the preventionof flowering. Leaf expansion responded to day length and GA₃ and ABA applicationin a similar way as the response of flowering, i.e. towardsflowering the size of the leaves increased.     

Effects of growth regulators,steroids and estrogen fraction from sage plants on flowering of a long day plant,Salvia splendens,grown under non-inductive light conditions

The flowering ofSalvia splendens Sellow under noninductive short days is promoted by exogenous application of estrogen fraction isolated from flowering sage plants, gibberellin GA₄₊₇ and to some extend N⁶-benzyladenine and estradiol. The most active is the combination of GA₄₊₇ with estrogen fraction. No synergistic action of GA₄₊₇ with N⁶-benzyladenine estradiol was found.     

Gibberellins in Relation to Growth and Flowering in Pharbitis nil Chois

Flowering can be modified by gibberellins (GAs) in Pharbitis nil Chois. in a complex fashion depending on GA type, dosage, and the timing of treatment relative to a single inductive dark period. Promotion of flowering occurs when GAs are applied 11 to 17 hours before a single inductive dark period. When applied 24 hours later the same GA dosage is inhibitory. Thus, depending on their activity and the timing of application there is an optimum dose for promotion of flowering by any GA, with an excessive dose resulting in inhibition. Those GAs highly promotory for flowering at low doses are also most effective for stem elongation (2,2-dimethyl GA₄ GA₃₂ > GA₃ > GA₅ > GA₇ > GA₄). However, the effect of GAs on stem elongation contrasts markedly with that on flowering. A 10- to 50-fold greater dose is required for maximum promotion of stem elongation, and the response is not influenced by time of application relative to the inductive dark period. These differing responses of flowering and stem elongation raise questions about the use of relatively stable, highly bioactive GAs such as GA₃ to probe the flowering response. It is proposed that the `ideal' GAs for promoting flowering may be highly bioactive but with only a short lifetime in the plant and, hence, will have little or no effect on stem elongation.