BLUE LIGHT IN THE DEVELOPMENT OF FERN GAMETOPHYTES AND ITS INTERACTION WITH FAR-RED AND RED LIGHT

Two effects of blue light on the development of Onoclea sensibilis spores are demonstrated. Brief irradiation promotes the protonemal or filamentous type of growth, and the rate of filament elongation is greater than in darkness. Longer periods of irradiation induce the formation of 2-dimensional prothallia. Blue-light treatments which promote filament elongation interact with elongation-promoting far-red light. Far-red irradiation alone promotes filament elongation to a greater extent than blue light, but a blue-light irradiation, either following or preceding far-red treatment, strongly inhibits the far-red promotion. In darkness, a slow recovery from the blue-light-induced loss of sensitivity to far-red takes place. The recovery may be greatly accelerated by interposing a red-light treatment between blue and far-red irradiation.     

Phytochrome-mediated branch formation in protonemata of the mossCeratodon purpureus

We have analyzed light induction of side-branch formation and chloroplast re-arrangement in protonemata of the mossCeratodon purpureus. After 12 hr of dark adaptation, the rate of branch formation was as low as 5%. A red light treatment induced formation of side branches up to 75% of the dark-adapted protonema. The frequency of light induced branch formation differed between cells of different ages, the highest frequency being found in the 5th cell, the most distal cell studied from the apex. We examined the effect of polarized light given parallel to the direction of filament growth. The position of branching within the cell depended on the vibration plane of polarized red light. Branch formation was highest when the electric vector of polarized light vibrates parallel to the cell surface and is fluence rate dependent. The positional effect of polarized red light could be nullified to some extent by simultaneous irradiation with polarized far-red light. An aphototropic mutant,ptr116, shows characteristics of deficiency in biosynthesis of the phytochrome chromophore and exhibits no red-light induced branch formation. Biliverdin, a precursor of the phytochrome chromophore, rescued the red-light induced branching when added to the medium, supporting the conclusion that phytochrome acts as photoreceptor for red light induced branch formation. The light effect on chloroplast re-arrangement was also analyzed in this study. We found that polarized blue light induced chloroplast re-arrangement in wild-type cells, whereas polarized red light was inactive. This result suggests that chloroplast re-arrangement is only controlled by a blue light photoreceptor, not by phytochrome inCeratodon.     

Comparative development of heavily asymmetric-cordate gametophytes of <Emphasis Type="Italic">Anemia phyllitidis</Emphasis> (Anemiaceae) focusing on meristem behavior

Development of heavily asymmetric cordate gametophytes of Anemia phyllitidis (Anemiaceae), one of the schizaeoid ferns, was examined using a sequential observation technique; epi-illuminated light micrographs of the same growing gametophytes were taken approximately every 24 h. The apical cell-like wedge-shaped cell was produced once from the terminal cell of a germ filament, but it stopped dividing soon after production of one or two derivative cells. Without a functional apical cell, the gametophyte developed by intercalary growth until the early stage of wing formation, and then the multicellular (pluricellular) meristem arose from the lower lateral side of the gametophyte. This was in sharp contrast to the observation that the multicellular meristem forms in place of the apical cell in typical cordate gametophytes. Loss of the functional apical cell probably caused a site-shift in the multicellular meristem of the Anemia phyllitidis gametophyte during evolution from apical to lateral. The results suggest that apical cell-based and multicellular meristems are primarily independent of each other. The multicellular meristem produced cells equally in the distal and proximal directions to form wings in both directions but proximally produced cells divided much less frequently. As a result, a heavily asymmetric gametophyte was formed.     

AN INTERPRETATION OF DOSE-RESPONSE CURVES FOR LIGHT-INDUCED CELL ELONGATION IN FERN PROTONEMATA

Protonemata of Onoclea sensibilis and Diyopteris filix-mas elongate in response to both red and far-red light. The promotion caused by far-red is larger than that caused by red light. This phenomenon differs from a typical response to phytochrome, the photoreceptor pigment immediately suggested by the activity of red and far-red light. The phenomenon has been explained by two different hypotheses, one of which holds that phytochrome is solely responsible for the response, whereas the other postulates an interaction between phytochrome and P₅₈₀, a yellow-green light absorbing pigment, to account for the response. The hypothesis that phytochrome is the sole photoreceptor leads to some specific predictions concerning the shapes of the dose-response curves for light-induced protonema elongation. These predictions were tested with both continuous and short-term irradiation. In all instances saturating far-red light caused greater elongation than did saturating red light, and no dose of red light duplicated the activity of saturating far-red light. Other experiments tested the interactions of red and far-red light and the effects of different doses of yellow-green light on protonema elongation. The results of many of the experiments were not in agreement with the hypothesis that phytochrome is the sole photoreceptor, whereas they were in agreement with the assumption that filament elongation is controlled by both phytochrome and P₅₈₀.     

Ubiquitination and filamentous structure of cytidine triphosphate synthase

Living organisms respond to nutrient availability by regulating the activity of metabolic enzymes. Therefore, the reversible post-translational modification of an enzyme is a common regulatory mechanism for energy conservation. Recently, cytidine-5′-triphosphate (CTP) synthase was discovered to form a filamentous structure that is evolutionarily conserved from flies to humans. Interestingly, induction of the formation of CTP synthase filament is responsive to starvation or glutamine depletion. However, the biological roles of this structure remain elusive. We have recently shown that ubiquitination regulates CTP synthase activity by promoting filament formation in Drosophila ovaries during endocycles. Intriguingly, although the ubiquitination process was required for filament formation induced by glutamine depletion, CTP synthase ubiquitination was found to be inversely correlated with filament formation in Drosophila and human cell lines. In this article, we discuss the putative dual roles of ubiquitination, as well as its physiological implications, in the regulation of CTP synthase structure.     

AN ANALYSIS OF STAMEN FILAMENT GROWTH OF NIGELLA HISPANICA

The post-meiotic stamen filament of Nigella hispanica L. under greenhouse conditions grows in length from 1 mm to approximately 10 mm at maturity in 16 days. Analysis of the filament epidermis suggests that the intercalary meristem is diffuse along the filament with a mid-point of activity near the center of the filament. The point of maximal activity, while initially central, is variable as cell division nears completion. Measurement of cell lengths along filaments suggests that an elongation gradient from base to tip is operative in filaments 1 mm and longer. Average cell lengths of epidermal cells increase faster than do those of terminal cells. Once average cell length begins to increase in any region of the epidermis it continues to do so until flower maturity. At maturity the longest epidermal cells are near the filament base and the shortest cells are at the tip. The differences between cell division and cell elongation patterns suggest that these two processes are controlled by different sites or substances. A comparison is made between the development of the Nigella filament and other determinate organs having intercalary meristems.     

Light Dependence of Chloroplast Replication and Starch Metabolism in the Moss Polytrichum commune

Spores of Polytrichum conwtuine were grown on a mineral salt solution with or without sucrose and exposed to continuous white light, continuous darkness, red light and/or far-red light. With sucrose, germination and filament growth occurred in all conditions, Without sucrose, germination and filament growth occurred only in light. Two phytochrome mediated responses of the chloroplasts were demonstrated. Chloroplast replication occurred in continuous white light and red light of 15 min/6 hours. In continuous darkness and in far red light of 15 min/6 hours, the size of the chloroplasts increased; but no replication occurred. Both the chloroplast replication and chloroplast size were red, far-red light reversible. When changed from one continuous light environment to another, a lag period occurred before the chloroplasts responded to the new environment. Electron micrographs of sections and in vivo staining of the chloroplasts with iodine solution demonstrated that the change in size of the chloroplasts was at least partially due to the synthesis and degradation of starch.     

Calcium and pH patterning at the apical meristem are specifically altered by photoperiodic flower induction in Chenopodium spp.

The apical meristem of the short‐day plant Chenopodium rubrum responds to photoperiodic flower induction with specific changes of pH and Ca²⁺ patterning immediately after the inductive dark span. The red–far‐red reversibility of the pH and Ca²⁺ patterning in response to night break treatments was measured in order to distinguish between the effect of the prolonged dark span per se and the specific effect of photoperiodic flower induction. In addition, the pH and Ca²⁺ patterning in C. rubrum was compared with the long‐day plant Chenopodium murale. The pH was visualized using the fluorescent probe carboxy SNARF‐1. Calcium ion concentrations were studied using a combination of Ca²⁺‐probes Fluo‐3 and Fura Red. It was observed that the specific changes in pH and Ca²⁺ patterning at the apical meristem of C. rubrum were abolished by the red‐light break. This effect was fully reversed with a subsequent single far‐red treatment. These observations infer the influence of phytochrome on both pH and Ca²⁺ patterning. Changes in pH and Ca²⁺ patterning upon flower induction were observed in both long‐day and short‐day plants. These results support the hypothesis that changes of pH and [Ca²⁺] in cells of the apical meristem are part of the pathway in signal transduction triggering flower initiation.     

Structure of Flower in Arabidopsis thaliana: Spatial Pattern Formation

Morphological analysis of flowers was carried out in Arabidopsis thaliana wild type plants and agamous and apetala2 mutants. No direct substitution of organs takes place in the mutants, since the number and position of organs in them do not correspond to the structure of wild type flower. In order to explain these data, a notion of spatial pattern formation in the meristem was introduced, which preceded the processes of appearance of organ primordia and formation of organs. Zones of acropetal and basipetal spatial pattern formation in the flower of wild type plants were postulated. It was shown that the acropetal spatial pattern formation alone took place in agamous mutants and basipetal spatial pattern formation alone, in apetala2 mutants. Different variants of flower structure are interpreted as a result of changes in the volume of meristem (space) and order of spatial pattern formation (time).     

Improving of oilseed rape lateral root formation by physiological analogues of auxin

The aim of the present work was to study the effect of auxin physiological analogue TA-12 [1-(2-chloroethoksicarbonylmethyl)-4-naphthalenesulfonic acid calcium salt] on the formation of oilseed rape lateral root and on the mitotic activity of apical meristem cells. Spring oilseed rape (Brassica napus L. ssp. oleifera annua Metzg.) cultivar ‘Mascot’ was chosen as a test object. Anatomical, cytological and histological studies on root development suggest that compound TA-12 induces the activity of parent root pericycle cells, stimulates the formation of lateral roots and enhances the division of apical meristem cells. The auxin transport inhibitor 2,3,5-triiodobenzoic acid suppresses the division of apical meristem cells, while this process is restored by the auxin physiological analogue TA-12 and naphthaleneacetic acid. The compound TA-12, by stimulating primary root growth and lateral root induction, optimised the formation of the oilseed rape root system.     

Adventitious shoot regeneration from Begonia × erythrophylla petiole sections is developmentally sensitive to light quality

The influence of light quality on organogenesis in vitro was investigated using Begonia  ×  erythrophylla petiole explants. Pre-treatment of in vitro donor plants by growth in the dark or under far-red or blue light reduced their competence for shoot formation when compared with those grown under red or white light. Culture of competent petiole explants under far-red, blue light or in the dark reduced the number of shoots produced per explant compared to those cultured under red or white light. Explants were found to be developmentally sensitive to both far-red and blue light, because meristem, but not primordia development was inhibited. In addition, blue light inhibition of shoot formation is not mediated directly through phytochrome, as few shoots formed on explants cultured under a mixture of red and blue light which resulted in a high P _fr/ P _tot (0.82) and would allow shoot formation in the absence of blue light. Unlike the inhibitory influence of far-red light, which is reversible, exposure to blue light permanently reduces an explant's competence for shoot formation. Our results suggest that phytochrome and an independent blue light photoreceptor, possibly a cryptochrome, can regulate shoot production from B. erythrophylla petiole explants.     

Cyclin‐dependent kinase activity maintains the shoot apical meristem cells in an undifferentiated state

As the shoot apex produces most of the cells that comprise the aerial part of the plant, perfect orchestration between cell division rates and fate specification is essential for normal organ formation and plant development. However, the inter‐dependence of cell‐cycle machinery and meristem‐organizing genes is still poorly understood. To investigate this mechanism, we specifically inhibited the cell‐cycle machinery in the shoot apex by expression of a dominant negative allele of the A‐type cyclin‐dependent kinase (CDK) CDKA;1 in meristematic cells. A decrease in the cell division rate within the SHOOT MERISTEMLESS domain of the shoot apex dramatically affected plant growth and development. Within the meristem, a subset of cells was driven into the differentiation pathway, as indicated by premature cell expansion and onset of endo‐reduplication. Although the meristem structure and expression patterns of the meristem identity genes were maintained in most plants, the reduced CDK activity caused splitting of the meristem in some plants. This phenotype correlated with the level of expression of the dominant negative CDKA;1 allele. Therefore, we propose a threshold model in which the effect of the cell‐cycle machinery on meristem organization is determined by the level of CDK activity.     

The F-box protein SHORT PRIMARY ROOT modulates primary root meristem activity by targeting SEUSS-LIKE protein for degradation in rice

Root meristem activity is essential for root morphogenesis and adaptation, but the molecular mechanism regulating root meristem activity is not fully understood. Here, we identify an F-box family E3 ubiquitin ligase named SHORT PRIMARY ROOT (SHPR) that regulates primary root (PR) meristem activity and cell proliferation in rice. SHPR loss-of-function mutations impair PR elongation in rice. SHPR is involved in the formation of an SCF complex with the Oryza sativa SKP1-like protein OSK1/20. We show that SHPR interacts with Oryza sativa SEUSS-LIKE (OsSLK) in the nucleus and is required for OsSLK polyubiquitination and degradation by the ubiquitin 26S-proteasome system (UPS). Transgenic plants overexpressing OsSLK display a shorter PR phenotype, which is similar to the SHPR loss-of-function mutants. Genetic analysis suggests that SHPR promotes PR elongation in an OsSLK-dependent manner. Collectively, our study establishes SHPR as an E3 ubiquitin ligase that targets OsSLK for degradation, and uncovers a protein ubiquitination pathway as a mechanism for modulating root meristem activity in rice.     

Weak red light plays an important role in awakening the photosynthetic machinery following desiccation in the subaerial cyanobacterium Nostoc flagelliforme

The subaerial cyanobacterium Nostoc flagelliforme can survive for years in the desiccated state and light exposure may stimulate photosynthetic recovery during rehydration. However, the influence of light quality on photosynthetic recovery and the underlying mechanism remain unresolved. Exposure of field collected N. flagelliforme to light intensity ≥2 μmol photons m⁻² s⁻¹ showed that the speed of photosystem II (PSII) recovery was in the following order: red > green > blue ≈ violet light. Decreasing the light intensity showed that weak red light stimulated PSII recovery during rehydration. The chlorophyll fluorescence transient and oxygen evolution activity indicated that the oxygen evolution complex (OEC) was the activated site triggered by weak red light. The damaged D1 protein accumulated in the thylakoid membrane during dehydration and is degraded and resynthesized during dark rehydration. PsbO interaction with the thylakoid membrane was induced by weak red light. Thus, weak red light plays an important role in triggering OEC photoactivation and the formation of functional PSII during rehydration. In its arid habitats, weak red light could stimulate the awakening of dormant N. flagelliforme after absorbing water from nighttime dew or rain to maximize growth during the early daylight hours of the dry season.     

CONJUGATION IN SPIROGYRA1

Conjugating filaments of Spirogyra were examined with both light and electron microscopes. Initially 2 or more filaments of Spirogyra were attached by mucilagenous material. Papillae appeared first in one filament and then in adjacent positions on the other filament. Subsequent growth of papillae separated the conjugating filaments; wall microtubules disappeared in papillae as they elongated. Golgi activity then increased markedly only in the male filament; mucilage production by these Golgi coincided with contraction of the male gamete from its cell wall and may be responsible for its subsequent migration. The end walls separating papillae dissolved to form the conjugation tube, allowing gamete union. The male protoplast then migrated through the tube and further cytoplasmic condensation formed an elliptical-shaped zygote. During the migration phase, zygote wall formation was initiated and numerous active Golgi apparently contributed material to it. Early zygote maturation was characterized by rapid wall formation and an increase in lipid droplets.     

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.     

Der Einfluss des Lichtes auf die Bildung von Blattprimordien am Vegetationskegel der Keimlinge vonSinapis alba L

Summary Seedlings of white seeded mustard (Sinapis alba L.) have been investigated with respect to the influence of light (red, far-red, white) on the rate of formation of primordia at the apex. The results show that the formation of primordia is strongly increased by light and that this control is exerted mainlyvia the phytochrome system and the high energy reaction )=blue, far-red reaction) of photomorphogenesis (cf.Mohr 1962). Apparently photosynthesis can also be important in the case that the supply of organic material limits the rate of those growth processes which have been induced by the photomorphogenetically effective radiation.The morphological appearance of the stem apex and of the youngest primordia is the same in light and dark. It is concluded that light increases the rate of primordia formation by promoting the mitotic activity in the apical meristem. Growth of the primary leaves of the mustard seedling is also greatly promoted by light. Both the phytochrome system and the high energy reaction system are involved. Experiments indicate that this control by light is exerted in a way similar to the light control of the growth of the cotyledons (Mohr 1959b).

---

---

Mit 7 Textabbildungen     

THE RELATIONSHIP BETWEEN THE PROMOTION OF ELONGATION OF FERN PROTONEMATA BY LIGHT AND GROWTH SUBSTANCES

Germinating spores of the fern Onoclea sensibilis L. were grown in darkness, so that they developed as filaments (protonemata). Brief daily exposure of the filaments to red, far-red or blue light increased the rate of filament elongation. Filament elongation was also promoted by indoleacetic acid. When filament elongation was promoted with both indoleacetic acid and exposure to light, the growth promotions caused by red and far-red light were additive to auxin-induced growth. Blue light promoted elongation only at sub-optimal concentrations of auxin. Elongation induced by guanine was additive to red- and far-red-induced elongation. Gibberellic acid had no effect on elongation under any condition. Blue-light-induced elongation resembled auxin-induced elongation in its requirement for exogenous sucrose and sensitivity to inhibition by parachlorophenoxyisobutyric acid. Red and far-red light were active regardless of the presence or absence of sucrose and promoted elongation at a concentration of parachlorophenoxyisobutyric acid which completely inhibited blue-light-induced elongation.