INHIBITION OF CELL PROLIFERATION AND EXPANSION IN VITRO BY THREE STEM GROWTH RETARDANTS

Three inhibitors of stem elongation, Amo, CCC, and Phosfon, inhibit cell division and expansion in tissues cultured in vitro. However, contrary to the case in intact plants, gibberellic acid does not prevent the retardant-induced inhibition in vitro. Supplementary auxin is also without effect in preventing the inhibition. Thus, the effect of the retardants cannot be simply that of inhibiting gibberellin or auxin synthesis. With respect to growth, carrot, chrysanthemum, and geranium tissues are equally sensitive to all 3 retardants, whereas tobacco tissues are considerably more resistant to Amo and apparently unaffected by CCC.     

EVIDENCE ON THE SITE OF ACTION OF GROWTH RETARDANTS

1. The ability of five growth retardants to inhibit the GA-inducedand endogenous growth of Avena leaf sections has been investigated.The retardants vary in effectiveness. The order, from most effectiveto least, is Phosfon D, Amo-1618, C011, CCC and B995. 2. The inhibition of growth caused by Phosfon D and Amo-1618is not reversed by GA. It is apparent that the retardants donot compete with GA at the site of GA-action. 3. Addition of IAA will partially reverse the inhibition inducedby Phosfon D or Amo-1618. It is concluded that the retardantsact in part in Avena leaf sections by interfering with the auxinmetabolism of the tisssue. ¹ Supported in part by grants G-14578 and GB-1950 from the NationalScience Foundation ² Present address: Department of Botany, University of Washington,Seattle, Washington     

Morphogenetic responses of tomato plants to combined and individual applications of gibberellic acid,Phosfon and B-nine

Summary Two growth retardants, B-nine (N-dimethylamino succinamic acid) and Phosfon (2,4-dichlorobenzyl-tributyl phosphonium chloride) were applied to tomato plants, either singly or in combination with gibberellic acid (GA), in order to determine various morphogenetic responses. GA (5 ml of 10^– M ⁴ per plant) and B-nine (5 ml of 1.56×10^–2 M per plant) were applied as foliar spray whereas Phosfon (1.5×10^–3 M in 10 ml of water per plant) was applied as soil amendment. Growth retardation by Phosfon persisted through the time of harvest and was somewhat neutralized by GA. Fruit set and extent of seediness of fruits were the maximum in Phosfon-treated plants compared to others. Plants receiving B-nine, however, recovered from the initial growth retardation and indicated no residual action at harvest. GA in combination with B-nine produced significantly greater vegetative growth and dry weight accumulation than did GA alone. This indicated that applied and endogenous GA responded differently to different growth retardants. None of the treatments had any noticeable effect on the time of flowering.     

SHOOT HISTOGENESIS: THE EARLY EFFECTS OF GIBBERELLIN UPON STEM ELONGATION IN TWO ROSETTE PLANTS

Sachs , Roy M., Charles F. Bretz , and Anton Lang . (U. California, Los Angeles.) Shoot histogenesis: The early effects of gibberellin upon stem elongation in two rosette plants. Amer. Jour. Bot. 46(5): 376–384. Illus. 1959.—Within 24 hr. after the application of gibberellic acid (GA) to vegetative plants of biennial Hyoscyamus and of the long-day plant Samolus, a considerable increase in mitotic activity was observed in the pith, cortical, and vascular tissues of the rosette axis immediately below the apical meristem. As the treatment continued, the zone of cell division increased commensurate with the increase in length of the stem; the new cell divisions formed transverse walls predominantly and thus contributed to stem elongation. The cell contribution from the apical meristem was but a small fraction of the total produced by the subapical tissues, suggesting that the induced subapical mitotic activity is the main site of tissue development in the shoot. There was no evidence for cell elongation for at least 72 hr. after application of GA, and, hence, the initial increase in stem length was due solely to an increase in cell number. With regard to the general problem of shoot histogenesis, our data for the rosette plants and those for Xanthium and Chrysanthemum showing extensive cell division far below the apical meristem, are in full agreement with the studies by Bindloss (1942) with tomato, and support her conclusion that “. . . it is no longer possible to think that the chief center of cell division is in a relatively short zone 60 to 100 microns from the stem tip . . . and that cell division activity in the promeristem is not solely responsible for stem length.” On the contrary, the mitotic activity in the subapical regions is undoubtedly responsible for the major part of the cells found in the stem.     

CONTROL OF FLOWER FORMATION BY GROWTH RETARDANTS AND GIBBERELLIN IN SAMOLUS PARVIFLORUS,A LONG-DAY PLANT

The growth retardants AMO–1618 and CCC inhibited flower formation and stem elongation in Samolus parviflorus, a long-day rosette plant, under inductive conditions. The vegetative growth of the plants, as measured by leaf formation, was affected only slightly, or not affected at all. Application of gibberellic acid (GA₃) reversed completely the inhibition both of flower formation and of stem elongation caused by AMO, but relatively larger amounts of GA were required to reverse the CCC inhibition of stem elongation than that of flower formation. When applied under short-day conditions, AMO had no effect on the level of applied GA required for flower induction. When applied following long-day treatment the retardant caused some reduction of flower formation after marginal numbers of long days, but had no effect when enough long days to cause 100% flower formation were given. Other evidence indicates that the growth retardants act by inhibiting the synthesis of endogenous gibberellin. In LD plants, at least part of the action of inductive environmental conditions consists in causing an increase of gibberellin synthesis, supporting the hypothesis that relatively high GA levels are necessary for the production of the floral stimulus in this group of plants, as in long-short-day plants. The experiments with CCC indicate that stem elongation and flower formation in Samolus can be separated, and that the effect of GA on flower formation is not necessarily dependent on its effect on stem elongation.     

UV-B-induced Inhibition of Stem Elongation and Leaf Expansion in Pea Depends on Modulation of Gibberellin Metabolism and Intact Gibberellin Signalling

Information on the involvement of elongation-controlling hormones, particularly gibberellin (GA), in UV-B modulation of stem elongation and leaf growth, is limited. We aimed to study the effect of UV-B on levels of GA and indole-3-acetic acid (IAA) as well as involvement of GA in UV-B inhibition of stem elongation and leaf expansion in pea. Reduced shoot elongation (13%) and leaf area (37%) in pea in response to a 6-h daily UV-B (0.45 W m^?2) exposure in the middle of the light period for 10 days were associated with decreased levels of the bioactive GA₁ in apical stem tissue (59%) and young leaves (69%). UV-B also reduced the content of IAA in young leaves (35%). The importance of modulation of GA metabolism for inhibition of stem elongation in pea by UV-B was confirmed by the lack of effect of UV-B in the le GA biosynthesis mutant. No UV-B effect on stem elongation in the la cry-s (della) pea mutant demonstrates that intact GA signalling is required. In conclusion, UV-B inhibition of shoot elongation and leaf expansion in pea depends on UV-B modulation of GA metabolism in shoot apices and young leaves and GA signalling through DELLA proteins. UV-B also affects the IAA content in pea leaves.     

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     

SHOOT HISTOGENESIS: SUBAPICAL MERISTEMATIC ACTIVITY IN A CAULESCENT PLANT AND THE ACTION OF GIBBERELLIC ACID AND AMO-1618

Sachs , R. M., A. Lang , C. F. Bretz and Joan Roach . (U. California, Los Angeles.) Shoot histogenesis: subapical meristematic activity in a caulescent plant and the action of gibberellic acid and Amo—1618. Amer. Jour. Bot. 47(4): 260—266. Illus. 1960.–Studies on gibbereilininduced stem formation in rosette plants (Sachs et al., 1959) have shown that a zone of intensive meristematic activity, arising below the existing apical meristem, is almost solely responsible for stem histogenesis, i.e., the formation of the cells constituting the elongate stem. An extensive subapical zone of meristematic activity is also present in caulescent plants, such as Chrysanthemum morifolium, Amo-1618 ([4-hydroxy-5 isopropyl-2 methylphenyl] trimethylammonium chloride, 1-piperidine carboxylate) completely inhibits subapical meristematic activity in chrysanthemum, causing the plants to assume a dwarfed, rosette-like habit of growth. Gibberellic acid, applied either simultaneously, or following the Amo—1618 treatment, completely prevents or reverses the effect of Amo—1618, making the plants retain or resume their normal growth habit. Amo—1618 and gibberellic acid have relatively little effect upon the activity of the apical meristem of Chrysanthemum. Thus, while the apical meristem proper (eu- or promeristem) is the site of shoot organization and the ultimate source of the cells of the entire shoot, the subapical zone of division, termed the subapical meristem, is largely responsible for stem histogenesis in caulescent as well as in rosette plants. Gibberellins, or native, gibberellin-like substances appear to regulate the activity of the subapical meristem and thus to play an important role in shoot development. Amo—1618 and related compounds seem to exert their dwarfing effect in plants by acting as antagonists of gibberellins, at least with respect to the latters' function in regulating the subapical meristematic activity in the shoot.     

How plants grow up

A plant's lateral structures, such as leaves,branches and flowers, literally hinge on the shoot axis,making its integrity and growth fundamental to plant form.In all plants, subapical proliferation within the shoot tip displaces cells downward to extrude the cylindrical stem.Following the transition to flowering, many plants show extensive axial elongation associated with increased subapical proliferation and expansion. However, the cereal grasses also elongate their stems, called culms, due to activity within detached intercalary meristems which displaces cells upward, elevating the grain-bearing inflorescence. Variation in culm length within species is especially relevant to cereal crops, as demonstrated by the high-yielding semi-dwarfed cereals of the Green Revolution. Although previously understudied, recent renewed interest the regulation of subapical and intercalary growth suggests that control of cell division planes,boundary formation and temporal dynamics of differentiation, are likely critical mechanisms coordinating axial growth and development in plants.     

GIBBERELLIN RELATIONSHIPS IN THE ‘ALASKA’ PEA (PISUM SATIVUM)

'Alaska’ peas (Pisum sativum L.) grown under a 16-hr photoperiod at 20 ± 1 C and an 8-hr dark period at 16 ± 1 C in their ontogeny exhibit two periods of sensitivity to applied gibberellin (GA), namely, prior to and subsequent to but not during the linear phase of stem elongation. This paper describes experiments conducted primarily with seedlings. Growth-saturating doses of GA, applied to dry seeds before planting (10⁻³ m) and to the shoot tips of 3-day-old seedlings (10 μg), evoked growth rates equal to the growth rate of etiolated seedlings. Sensitivity of seedlings to applied GA decreased with age through the first 2 to 3 weeks of development; by the time seedlings were about 14 days of age and had four elongating internodes they no longer responded to applied GA. As endogenous growth rate diminished late in ontogeny, the plants again became sensitive to applied GA. Growth response was used as a criterion for determining apparent translocation of applied GA. ‘Alaska’ pea seedlings appeared to transport GA, both acropetally from the cotyledons and basipetally from the shoot tip, to all internodes with remaining extension potential. Excision of both cotyledons at any time during the first 9 days of development caused a significant reduction of growth rate, and applied GA did not restore normal growth rate. No evidence was found that the cotyledons supply endogenous GA to the shoot axis in normal seedling development. It is suggested that the normal growth rate of light-grown ‘Alaska’ peas is correlated with the rate of synthesis of GA and that GA is rate-limiting for stem elongation during early seedling development and during the period of decreasing growth rate and onset of apex senescence.     

Developmental changes in the gibberellin-induced growth response in stem segments of light-grown pea genotypes

The effects of GA on stem elongation were studied using segments from one tall and three dwarf light-grown pea genotypes varying in endogenous hormone content. Stem segments were cut at two distinct ages: when the fourth internode was at about 6–13% of full expansion (early-expansion) or at 18–25% of full expansion (mid-expansion). Light microscopy and flow cytometry were used to demonstrate that GA does not induce cell division in excised pea stem segments. The growth studied here was strictly elongation. Measurement of final segment length after 48 hours and high resolution measurement of growth kinetics over 20 hours using an angular position transducer were done on segments treated with hormone solutions. Our data indicate that the action of GA on stem elongation can be classified into two distinct modes. The first, apparent in early-expansion stem segments, shows distinct growth kinetics and is independent of the endogenous IAA concentration of the segments. Quantitation of IAA by GC/MS in early-expansion segments of wild type pea incubated with gibberellin shows that an increase in IAA concentration is part of the GA response in such segments. The second mode of GA action is evinced in mid-expansion segments. Whereas there is no short term (<20 h) response to GA alone (as determined by growth kinetics), there is a long term (48 h) response whose magnitude decreases across the genotypes with decreasing endogenous hormone content. Growth responses indicate that in mid-expansion segments exogenous GA acts by enhancing IAA action but appears to be unable to augment endogenous IAA content. Contradictory reports of the response of excised stem segments to GA can be reconciled when tissue genotype and developmental stage are considered.     

Anatomical analysis of growth and developmental patterns in the internode of deepwater rice

Submergence of the stem induces rapid internodal elongation in deepwater rice (Oryza sativa L. cv. Habiganj Aman II). A comparative anatomical study of internodes isolated from airgrown and partially submerged rice plants was undertaken to localize and characterize regions of growth and differentiation in rice stems. Longitudinal sections were examined by light and scanning-electron microscopy. Based on cell-size analysis, three zones of internodal development were recognized: a zone of cell division and elongation at the base of the internode, designated the intercalary meristem (IM); a zone of cell elongation without concomitant cell division; and a zone of cell differentiation where neither cell division nor elongation occur. The primary effects of submergence on internodal development were a threefold increase in the number of cells per cell file resulting from a decrease in the cell-cycle time from 24 to 7 h within the IM; an expansion of the cell-elongation zone from 5 to 15 mm leading to a threefold greater final cell length; and a suppression of tissue differentiation as indicated by reduced chlorophyll content and a lack of secondary wall formation in xylem and cortical sclerenchyma. These data indicate that growth of deepwater-rice internoes involves a balance between elongation and differentiation of the stem. Submergence shifts this balance in favor of growth.Abbreviations GA gibberellin - IM intercalary meristem     

Light-induced inhibition of elongation growth in sunflower hypocotyls

Summary The long-term effects of white light (WL) on epidermal cell elongation and the mechanical properties and ultrastructure of cell walls were investigated in the subapical regions of hypocotyls of sunflower seedlings (Helianthus annuus L.) that were grown in darkness. Upon transition to WL a drastic inhibition of epidermal cell elongation was observed. However, the mechanical properties of the inner tissues (cortex, vascular bundles, and pith) were unaffected by WL. Thus, the light-induced decrease in cell wall plasticity measured on entire stems occurs exclusively in the peripheral tissues (epidermis and 2 to 3 subepidermal cell layers).An electronmicroscopic investigation of the epidermal cell walls showed that they are of the helicoidal type with the direction of microfibrils monotonously changing during deposition. This cell wall type was identified by the appearance of arced patterns of microfibrils in cell walls sectioned oblique to the plane of their synthesis. WL irradiation did not change the periodicity of this pattern nor the thickness of the lamellae. Thus, the inhibition of cell elongation was not caused or accompanied by a shift in the direction of microfibril deposition in the growth-limiting outer tissues. However, cell wall thickness, the number of lamellae and hence the amount of cellulose oriented parallel and transverse to the longitudinal cell axis increased in WL. This may account for the effect of WL on the reduction of cell wall plasticity and growth.Abbreviations D darkness - PATAg periodic acid-thiocarbohydracide-silver protein - WL white light     

Promotive and inhibitory effects of uniconazole and prohexadione on the sprouting of bulbils of Chinese yam,Dioscorea opposita

Gibberellin A₁ (GA₁), GA₃ and GA₄ inhibited the sprouting of nondormant bulbils of Chinese yam, Dioscorea opposita, where the effectiveness of the GAs was as follows: GA₄>GA₁+GA₃. Uniconazole and prohexadione, plant growth retardants, promoted the sprouting of half-dormant bulbils. By contrast, these retardants inhibited the sprouting of nondormant bulbils. Gibberellin A₃ (GA₃) and A₄ (GA₄) which were applied to the stems of the sprouted bulbils, promoted stem elongation, but GAs applied to the bulbous parts inhibited this process. The effectiveness of the GAs on stem elongation was as follows: GA₃+GA₄ for the promotion and GA₄ > GA₃ for the inhibition. Uniconazole applied to the stem inhibited the stem elongation of the sprouted bulbils. These results suggest the possible involvement of endogenous GAs in the induction and maintenance of bulbil dormancy of D. opposita, as well as in the bulbil sprouting and subsequent stem elongation.     

Kinetics of growth retardant and hormone interactions in affecting cucumber hypocotyl elongation

The capacities of indole-3-acetic acid (IAA) and gibberellin A₃ (GA₃) to counteract the inhibitory effects of (2-chloroethyl) trimethylammonium chloride (CCC), 2-isopropyl-4-dimethylamino-5-methylphenyl-1-piperidinecarboxylate methyl chloride (Amo-1618), and N,N-dimethylaminosuccinamic acid (B-995) on hypocotyl elongation in light-grown cucumber (Cucumis sativus L.) seedlings were investigated. One μg of GA₃ applied to the shoot tip was sufficient to completely nullify the effect of 10 μg of Amo-1618 or 25 μg of B-995 applied simultaneously to the shoot tip, and 10 μg of GA₃ completely counteracted the effect of 10⁻³ m CCC added to the root medium. One μg of IAA counteracted the effect of 10⁻³ m CCC in the root medium, but IAA did not nullify the action of either Amo-1618 or B-995. Experiments were conducted using 2 growth retardants simultaneously, which indicated that Amo-1618 and CCC inhibit a common process, namely GA biosynthesis, essential to hypocotyl elongation. However, since the effect of CCC was overcome by applications of both GA and IAA, growth retardation resulting from treatment with CCC apparently is not due solely to inhibition of GA biosynthesis. B-995 did not interact additively with either Amo-1618 or CCC, which suggests that B-995 affects a process different from those affected by the other 2 retardants. Thus, while inhibition evoked by B-995 is reversible by applied GA, the action of B-995 does not appear to be inhibition of GA biosynthesis.     

Internodal elongation and orientation of cellulose microfibrils and microtubules in deepwater rice

Excised stem sections of deepwater rice (Oryza sativa L.) containing the highest internode were used to study the induction of rapid internodal elongation by gibberellin (GA). It has been shown before that this growth response is based on enhanced cell division in the intercalary meristem and on increased cell elongation. In both GA-treated and control stem sections, the basal 5-mm region of the highest internode grows at the fastest rate. During 24 h of GA treatment, the internodal elongation zone expands from 15 to 35 mm. Gibberellin does not promote elongation of internodes from which the intercalary meristem has been excised. The orientation of cellulose microfibrils (CMFs) is a determining factor in cell growth. Elongation is favored when CMFs are oriented transversely to the direction of growth while elongation is limited when CMFs are oriented in the oblique or longitudinal direction. The orientation of CMFs in parenchymal cells of GA-treated and control internodes is transverse throughout the internode, indicating that CMFs do not restrict elongation of these cells. Changes in CMF orientation were observed in epidermal cells, however. In the basal 5-mm zone of the internode, which includes the intercalary meristem, CMFs of the epidermal cell walls are transversely oriented in both GA-treated and control stem sections. In slowly growing control internodes, CMF orientation changes to the oblique as cells are displaced from this basal 5-mm zone to the region above it. In GA-treated rapidly growing internodes, the reorientation of CMFs from the transverse to the oblique is more gradual and extends over the 35-mm length of the elongation zone. The CMFs of older epidermal cells are obliquely oriented in control and GA-treated internodes. The orientation of the CMFs parallels that of the cortical microtubules. This is consistent with the hypothesis that cortical microtubules determine the direction of CMF deposition. We conclude that GA acts on cells that have transversely oriented CMFs but does not promote growth of cells whose CMFs are already obliquely oriented at the start of GA treatment.     

Effects of ethylene and gibberellic Acid on cellular growth and development in apical and subapical regions of etiolated pea seedling

Subhook swelling of 4-day-old etiolated pea seedlings (var. Alaska), caused by 0.5 microliter per liter ethylene, was prevented by preincubation and continued growth in 0.1 mm gibberellic acid (GA). The subhook region exhibited normal elongation and cell size and volume. However, inhibition of elongation and cessation of cell division caused by 0.5 microliter per liter ethylene in the apical hook region of the etiolated pea stem were not overcome by GA. Most of the arrested cells were in G(2). These data suggest a possible interaction of GA and ethylene in cell enlargement in the subhook region of the etiolated pea seedlings. They also suggest a different mode of action by ethylene in the apical hook region where the ethylene effect was not counteracted by GA.