CIRCADIAN GROWTH IN PORPHYRA UMBILICALIS (RHODOPHYTA): SPECTRAL SENSITIVITY OF THE CIRCADIAN SYSTEM

The circadian rhythm in growth of the red macroalga Porphyra umbilicalis (Linnaeus) J. Agardh was investigated under different spectral light conditions in laboratory-grown thalli. A free-running rhythm was observed in constant green or red light at irradiances of 2.5 to 20 μmol photons·m⁻²·s⁻¹, whereas arhythmicity occurred in constant blue light at 6–20 μmol photons·m⁻²·s⁻¹. The circadian oscillator controlling growth rhythmicity in Porphyra uses most of the visible sunlight spectrum and possibly multiple photoreceptors with a high sensitivity for blue light and a lower sensitivity for red light. This was inferred from three experimental results: (1) The free-running period, τ, of the growth rhythm decreased with increasing irradiance, from approximately 25 h at 2.5 μmol photons·m⁻²·s⁻¹ to 22 h at 20 μmol photons·m⁻²·s⁻¹ in red or green light, (2) Dark pulses of 3 h duration, interrupting otherwise continuous green or red light, caused advances during the subjective day and delays during the subjective night; the circadian oscillator in Porphyra can discriminate darkness from green or red light, and (3) Low-irradiance blue light pulses (2.5 μmol photons·m⁻²·s⁻¹) shifted the growth rhythm in red light of higher irradiance (e.g. 10 μmol photons·m⁻²·s⁻¹), and a strong, high amplitude, type 0 phase response curve was obtained that is usually observed with light pulses shifting a circadian rhythm in otherwise continuous darkness.     

Photophobic stop-response in a dinoflagellate: Modulation by preirradiation

Gyrodinium dorsum Kofoid responds photophobically to flashes of blue light. The photophobic response consists of a cessation of movement (stop-response). Without background light and after a flash fluence above 10 J m⁻², 75–85% of the cells show a stop-response, while only 50% of the cells show this response at 5 J m⁻². With a flash fluence of 5 J m⁻², background light of different wavelengths either increases (614 nm. 5.5–18.2 μmol m⁻² s⁻¹) or decreases (700 nm, 18.4–36.0 μmol m⁻² s⁻¹) the stop-response. Two hypotheses for the mechanism of the modulation by background light of the photophobic response are discussed: an effect of light on the balance of the photosynthetic system (PS I/PS II) or an effect on a phytochrome-like pigment (P_r/P_fr). This study supports the idea that a phytochrome-like pigment works in combination with a blue light-absorbing pigment. It was also found that cells of Gyrodinium dorsum cultured in red light (39.8 μmol m⁻²) had a higher absorption in the red region of the absorption spectra than those cultured in white light (92.7 μmol m⁻²).     

Asparagine and regulation of photoinduced rhythm in Penicillium claviforme

A photosensitive reaction involved in the expression and regulation of the endogenous sporulation rhythm in Penicillium claviforme Bainier CBS 126-23 has been described earlier by our team. The present work shows that asparagine plays a central role in this periodic system. The 24–26 h periodicity, which becomes desynchronized over a few days, was affected by supplying asparagine (1 to 25 m M ). a) The rhythm remained synchronized for at least 3 weeks, for all the asparagine concentrations used, b) The period increased successively from one cycle to the next (from 35±3 h to 73±8 h over 6 cycles) for 1 m M asparagine. This period lengthening became less and less accentuated as the asparagine concentration was increased. At ≥10 m M , the period was stable; it was 33±5 h for 10 m M and 22±1.5 h for 25 m M asparagine. Otherwise asparagine could not elicit rhythmicity in darkness or in dim continuous light (≤5 μW m⁻²).     

Effect of light quality (blue, red) and fluence rate on the synthesis of pigments and pigment-proteins in maize and black pine mesophyll chloroplasts

Maize ( Zea mays L. hybrid ZP-704) and black pine ( Pinus nigra Arn.) were grown for five days at low fluence rate (0.4–4.0, μmol m^–2 s⁻¹) in blue or red light. Compared to red light of the same fluence rate, blue light effects in maize were repressive for the accumulation of Chita, b , carotenoids and light-harvesting complex-2 (LHC-2) proteins. The maximal reduction of proteins bound to the light-harvesting complex of photosystem 2 and pigments was attained at different fluence rate levels. In black pine, blue light compared to the red of the same fluence rate level either activated or reduced accumulation of pigments and LHC proteins, the effect being dependent on its fluence rate level. At fluence less than 3.0 μmol m⁻² s⁻¹ blue light was more efficient for the synthesis of Chi a, b and carotenoids, hut for LHC-2 complexes, fluence rates between 0.4 and 1.5 [μmol m⁻² s⁻¹ were more effective. In pine the effects of the two lights on the accumulation of pigments and LHC proteins were demonstrated separately and were dependent on fluence rate level. This suggests irradianoe-controlled activation/deactivation of the photoreceptor at the level of the cell.     

Effect of riboflavie and cyanide on blue light induction of betacyanin formation in Amamnthus caudatus seedlings

The role of phyto chrome and flavins in blue light induction of betacyanin formation was studied in etiolated, three-day-old Amaranthus caudatus L. seedlings, using the criterion of far-red reversibility and exogenously applied riboflavin and KCN. The effect of riboflavin was studied using high fluence rate blue light (42.7 :nmol m⁻²s⁻¹nm⁻¹ at 450 nm). When present in the incubation medium during illumination, riboflavin promoted the far-red reversibility with short light treatments and suppressed the inductive action of continuous illumiaation. If added after light treatments, it promoted betacyanin formation. The filtration of blue light through the riboflavin solution caused profound changes in light quality without affecting the far-red reversibility after 30 mm illumination. The effect of 1 mM KCN was tested with 70'% lower fluence of blue light. Cyanide caused the suppression of the inductive effect with 5 min blue light, which was accompanied by an enhancement of betacyanin induction by the terminal far-red light pulse. With 30 min blue light, however, it caused the appearance of far-red reversibility. The inductive effect of continuous blue illumination was slightly promoted by this Inhibitor. These results demonstrate that the effect of blue light on the pbyto chrome system is complex, whereas the physiological (inductive) action of the flavin triplet state is limited to low fluence, short blue light treatments.     

Relative effectiveness and interaction of ultraviolet-B, red and blue light in anthocyanin synthesis of apple fruit

The effect of light on anthocyanin production in apple ( Malus pumila Mill. cv. Jonathan) skin disks was investigated, with prolonged irradiation from different light sources. High fluence rates of white light provided from a xenon lamp were unable to produce large amounts of anthocyanin, and anthocyanin production became saturated at about 30 W m⁻². When UV-B light, provided by a fluorescent lamp which had an emission peak at 312 nm, was combined with the white light, anthocyanin production was synergistically stimulated and increased up to the highest fluence rates of white light tested (44 W m⁻²). This UV-B light was more effective than red and blue light provided from fluorescent lamps, but anthocyanin production became saturated at about 1.7 W m⁻². However, simultaneous irradiation with red and UV-B light had a synergistic effect. UV-B light was also effective in increasing anthocyanin production in whole fruit. Therefore this synergism seemed to have an important role in the development of the desirable red skin color under field light conditions. The results of aminoethoxyvinylglycine treatment suggested that ethylene was not involved in the stimulative effect of UV-B light.     

Benzyladenine-induced stimulation of 5-aminolevulinic acid accumulation under various light intensities in levulinic acid-treated cotyledons of etiolated cucumber

Benzyladenine (BA) stimulated 5-aminolevulinic acid (ALA) accumulation in the presence of levulinic acid during illumination with 43 μmol m⁻² s⁻¹ light in excised etiolated cotyledons of cucumber ( Cucumis sativus L. cv. Aonagajibai). A short dark-pretreatment (6 h) with BA eliminated the lag phase of ALA accumulation. The rate of ALA accumulation during the steady-state phase in cotyledons pretreated with BA for a long period (14 h) was considerably accelerated compared to that in cotyledons pretreated with BA for 6 h. The rate of ALA accumulation during the lag phase was saturated at a very low light fluence (<1.4 μmol m⁻² s⁻¹) in both BA-pretreated and water-control cotyledons. The steady-state rate of ALA accumulation increased with increasing light fluence up to 43 μmol m⁻² s⁻¹ (parallel to that of Chl formation) in water-control cotyledons. In contrast, in cotyledons pretreated with BA for either 6 or 14 h, the steady-state rate reached a plateau at a very low light fluence. Based on the above results together with our finding that there are two components of Chl formation (M. Dei, 1984. Physiol. Plant. 62: 521–526) possible intermediate steps of Chl biosynthesis pathway affected by BA and light intensity are discussed.     

Influence of red light on the activity of phosphofructokinase in Chlorella kessleri

In crude extracts of the unicellular green alga Chlorella kessleri Fott et Novákóva grown in red light the activity of the glycolytic enzyme phosphofructokinase (PFK, EC 2.7.1.11) is about 40% higher compared to white light conditions giving the same dry matter production. Application of cycloheximide and density labelling with D₂O indicate that this increase depends on the de novo synthesis of the enzyme: Twelve h of illumination at a fluence rate of 7 × 10¹⁸ quanta m⁻² s⁻¹ (11.6 μmol m⁻² s⁻¹) suffice to saturate the effect. In autotrophically grown algae maximal increase in enzyme saturate the effect. In autotrophically grown algae maximal increase in enzyme activity is reached in light of 680 nm, while in 3-(3,4-dichlorophenyl)-1,1-dimethyl urea (DCMU)-poisoned, glucose-fed cells, light of wavelengths around 727 nm is most effective. Involvement of a phytochrome-like photoreceptor is discussed.     

Phytochrome control of hypocotyl extension in light-grown Chenopodium rubrum

The regulation of hypocotyl extension in light-grown Chenopodium rubrum L. seedlings by light analogous to dense vegetation canopy shade has been monitored. Hypocotyl extension was controlled by both the quantity and quality of the actinic light. At the higher of the two background photon fluence rates which were used (10.0 μmol m⁻²s⁻¹ in the 400–700 nm waveband), increasing the proportion of phytochrome calculated to exist as Pfr resulted in greater inhibition of growth. At the lower photon fluence rate (1.0 μmol m⁻²s⁻¹ in the 400–700 nm waveband), a biphasic response was observed in which minimum inhibition was observed at intermediate photoequilibria. Although photosynthesis was not directly involved in the photomorphogenetic responses, it did play an indirect quantitative role in determining the response.     

Effect of temporary changes in light intensity on carbon transport, partitioning and respiratory loss in young tomato seedlings raised under different light intensities

Tomato plants were grown under light intensities of 36 or 90 W m⁻² [photosynthetically active radiation (PAR)], and then the light intensity was changed to 36, 90 or 180 W m⁻² for 8 h to investigate the effect of temporary changes in light intensity on the carbon budget of photoassimilates from the third leaf using a ¹⁴CO₂ steady-state feeding method. In the plants that were raised under 90 W m⁻², the photosynthetic rate increased when the light intensity was increased to 180 W m⁻², whereas no increase occurred in the plants that were raised under 36 W m⁻². Although the total amount of carbon fixed during the 8-h light period showed a large difference between plants grown at the two initial light intensities, the proportion of carbon exported during the light period did not differ apparently, irrespective of the change in light intensity. However, the amount of carbon exported during the time course was higher in plants that were raised under 90 W m⁻² than those raised under 36 W m⁻², irrespective of the change in light intensity. The partitioning pattern of ¹⁴C-photoassimilates was not changed by the change in light intensity, irrespective of whether the light intensity was increased or not. However, the amount of ¹⁴C-photoassimilates accumulated in each part differed according to the two initial light intensities. The carbon transport from a source leaf was also investigated through a quantitative analysis of carbon balance.     

Blue, red and blue plus red light control of chlorophyll content and CO2 gas exchange in barley leaves: Quantitative description of the effects of light quality and fluence rate

The dependence of the Chl content and the rate of CO₂ gas exchange (RGE) on both blue and red quanta fluence rates have been studied in primary leaves of barley ( Hordeum vulgare L. cv. Viner). Empirical equations connecting the two photosynthetic indices with fluence rates of blue or red light were developed. These equations consist of 3 (Chl content) or 2 (RGE) terms, each reflecting the involvement of a specific reaction in the long-term light control of the development of the photosynthetic apparatus. On the basis of the equations the effects of mixed blue plus red light on both the Chl content and RGE were calculated. An additive mode of the co-action of blue and red light in the range of high PFDs (10–170 μmol m⁻² s⁻¹) becomes evident from the comparison of the experimental results and calculated data. The results indicate the involvement of phytochrome, cryptochrome and chlorophyll in the long-term regulation of the Chl content and RGE.     

Benzyladenine-induced stimulation of two components of chlorophyII formation in etiolated cucumber cotyledons

Excised etiolated cotyledons of cucumber ( Cucumis sativus L. cv. Aonagajibai) were continuously irradiated under various intensities of white light. The rate of chlorophyII (Chi) formation during the lag phase reaches a plateau at fluence rates above 1.4 urmol m⁻² s⁻¹. This is true in both water-control and benzyladenine (BA)-pretreated cotyledons. In cotyledons pretreated for 14 h with BA in darkness (in which case, Chl formation is stimulated by BA during both the lag and the steady-state phases), the increase in the steady-state rate of Chl formation with increasing light in tensity is stimulated compared to that of the water control over the range of fluence rates, 0. 25-43 urmol m⁻² s⁻¹. In cotyledons pretreated for 6 h with BA in darkness (only Chl formation during the lag phase is stimulated), only an increase in fluence rate from 0.25 to 1.4 umol m⁻² s⁻¹ causes a higher increase in the Chl formation in the BA-treated cotyledons than in the water control. The time course of Chl formation shows that the BA-induced late-appearing effect (stimulation of the steady-state rate) is almost absent at low intensity illumination, but the BA-induced fast-appearing effect (elimination of the lag phase) is effective at all intensities. From this evidence, the Chl-forming process apparently consists of two components, whose periods of operation or light-intensity requirements are different. BA stimulates the rates of the respective components in both the fast and the late-appearing effects.     

Light effects on in vitro adventitious root formation in axillary shoots of mature Prunus serotina

Light effects on in vitro adventitious root formation in axillary shoots of a 95-year-old black cherry ( Prunus serotina Ehrh.) were examined using microcuttings derived from cultured vegetative buds. Three studies were performed: 1) complete darkness and 4 levels of continuous white light irradiance were tested at 70, 278, 555 and 833 μmol m⁻² s⁻¹; 2) white, red, yellow and blue light were tested to assess the importance of spectral quality; and 3) the effect of blue light at intensities of 7,15, 22 and 30 μmol m⁻² s⁻¹ was also studied, Measurements included rooting percentage, total number of roots per shoot, and shoot and root dry weight. There was a strong negative effect of white light intensity upon root formation. Blue light between 15 and 22 μmol m⁻²: s⁻¹ significantly retarded root formation and completely inhibited it at 36 μmol m⁻² s⁻¹. Shoots treated with yellow light exhibited the highest rooting percentage, mean number of roots per shoot, and root dry weight.     

Effect of ultraviolet radiation on accumulation and leakage of 86Rb+ in guard cells of Vicia faba

The effects of UV-C (254 nm), UV-A (365 nm) and broad-band UV (280–380 nm) on guard cells of Vicia faba L. cv. Long Pod were investigated in the presence of white light (450 μmol m⁻² s⁻¹). UV-C (7 μmol m⁻² s⁻¹) was found to cause leakage of ⁸⁶Rb⁺ from guard cells, while UV-A (0.3 μmol m⁻² s⁻¹) stimulated increased uptake in these cells. A relatively small stimulatory effect was observed by broad-band UV (3 μmol m⁻² s⁻¹) during the first 30 min of irradiation with an apparent equilibration of influx and efflux thereafter. Leakage of ⁸⁶Rb⁺ from guard cells continued despite the removal of UV-C and an increase in the amount of white light from 450 to 1500 μmol m⁻² s⁻¹, suggesting that membranes were irreversibly damaged. Irradiation of guard cells with UV-C for 30, 45 and 90 min indicated that these cells began to be affected already by 30 min UV-C irradiation.     

Blue, red and blue plus red light control of chloroplast pigment and pigment-proteins in corn mesophyll cells: Irradiance level-quality interaction

Corn ( Zea mays L. cv. OP Golden Bantum) was grown under low irradiance blue, red or blue plus red light. Red was more effective than blue light for synthesis of Chl a, b and light-harvesting proteins (LHC-2) associated with photosystem 2(PS2). Blue light was slightly more effective for synthesis of light-harvesting proteins (LHC-1) associated with photosystem 1 (PS1), but below a fluence rate of 1 μmol m⁻² s⁻¹ the response to blue vs that to red depended on irradiance level. Blue light containing a small amount of red light was as effective as red light for Chl a and b synthesis, but no more effective than blue light for LHC-2 synthesis. Adding small amounts of blue light to red repressed the effect of red light on LHC-2 synthesis and produced irradiance response curves similar to those produced by blue alone for LHC-2 synthesis. This repression by blue light depended on the ratio of red to blue and the level of the blue light.     

Stem extension rate in light-grown plants. Evidence for an endogenous circadian rhythm in Chenopodium rubrum

Stem extension in light-grown plants of Chenopodium rubrum L. ecotype selection 184 (50°10'N; 150°35'W) was recorded continuously for periods up to one week at constant temperature. Stem extension rate measurements were made with linear voltage-displacement transducer devices. At the beginning of experiments, the 3rd intenode above the cotyledons was about 5 mm long. Stem extension rate exhibited a rhythmic behaviour in continuous white light (20 W m⁻²), and in continuous darkness with a period of approximately 23 h. In continuous darkness, the amplitude of the rhythm damped out very quickly after 24 h and a second peak was just measurable. The mean value of the stem extension rate was dependent on the light fluence before the experiments. This overt rhythm, which could be observed at the individual plant or even internode level, exhibited the characteristics of an endogenous circadian rhythm. There was no correlation of the peak time to local time. The peak time was determined by the time of transfer from dark to light for dark periods equal to or longer than 8 h, and the phase was shifted by the time of transfer from light to dark at the proper phase of a pre-existing rhythm.     

Inhibition of hypocotyl elongation by ultraviolet-B radiation in de-etiolating tomato seedlings. I. The photoreceptor

Broad-band UV-B radiation inhibited hypocotyl elongation in etiolated tomato ( Lycopersicon esculentum Mill. cv. Alisa Craig) seedlings. This inhibition could be elicited by < 3 μmol m⁻² s⁻¹ of UV-B radiation provided against a background of white light (> 620 μmol m⁻² s⁻¹ between 320 and 800 nm), and was similar in wild-type and phytochrome-1-deficient aurea mutant seedlings. These observations suggest that the effect of UV-B radiation is not mediated by phytochrome. An activity spectrum obtained by delivering 1 μmol m⁻² s⁻¹ of monochromatic UV radiation against a while light background (63 μmol m⁻² s⁻¹ showed maximum effectiveness around 300 nm, which suggests that DNA or aromatic residues in proteins are not the chromophores mediating UV-B induced inhibition of elongation. Chemicals that affect the normal (photo)chemistry of flavins and possibly pterins (KI, NaN, and phenylacetic acid) largely abolished the inhibitor) effect of broad-hand UV-B radiation when applied to the root zone before irradiation. KI was effective at concentrations < 10⁻⁴ M , which have been shown in vitro to be effective in quenching the triplet excited stales of flavins but not fluorescence from pterine or singlet states of flavins. Elimination of blue light or reduction of UV-A, two sources of flavin excitation, promoted hypocotyl elongation, but did not affect the inhibition of elongation evened by UV-B. Kl applied after UV-B irradiation had no effect on the inhibition response. Taken together these findings suggest that the chromophore of the photoreceptor system invoked in UV-B perception by tomato seedlings during de-etiolation may be a flavin.     

Effects of UV-C and UV-B on cytomorphology and water permeability of inner epidermal cells of Allium cepa

Changes of cytomorphology and water permeability of inner epidermal cells of Allium cepa L. cvs Spartan and Keep Well were investigated with the light microscope after irradiation with UV-C (254 nm) and UV-B (280 and 310 nm). The sequence of the investigated changes of viscosity, protoplasmic streaming, organelle shape and water permeability was the same with 254 as with 280 nm. although a higher dose of 280 nm was needed to produce the same biologically equivalent effect. However, when calculated as a percentage of the lethal dose, the initial doses that produced the effects were the same for 254 and 280 nm. No changes could he observed at the cellular level after the cells were irradiated with 310 nm. The lethal dose depended upon the time between irradiation and observation. At 254 nm it was 1.1 kJ m⁻² up to 1 h after irradiation and dropped to 860 J m⁻² when measured 24 and 48 h later. At 280 nm a dose of 2.8 kJ m⁻² killed the cells within I h while the dose needed after 24 and 48S h was 1.99 kJ m⁻². The minimum doses which caused the different cytomorphological effects did not depend upon the observation time. Normal cell structure and functions that were altered immediately alter irradiation did not recover. Doses that were not immediately effective alter irradiation caused no later damage. Doses which increased water permeability were much higher than doses which influenced cytomorphological parameters of the cell.     

Influence of solar ultraviolet radiation on photosynthesis and motility of marine phytoplankton

Abstract: The effects of solar ultraviolet radiation (UV) on carbon uptake, oxygen evolution and motility of marine phytoplankton were investigated in coastal waters at Kristineberg Marine Research Station on the west coast of Sweden (58° 30'N, 11° 30'E). The mean irradiances at noon above the water surface during the investigation period were: photosynthetic active radiation (PAR, 400–700 nm) 1670 μmol m⁻² s⁻¹; ultraviolet-A radiation (UV-A, 320–400 nm) 35.9 W m⁻² and ultraviolet-B radiation (UV-B, 280–320 nm) 1.7 W m⁻². UV-B radiation was much more attenuated with depth in the water column than were PAR and UV-A radiation. UV-B radiation could not be detected at depths greater than 100–150 cm. Inhibition of carbon uptake by UV-A and UV-B in natural phytoplankton populations was greatest at 50 cm depth and the effects of UV-B were greater than those of UV-A. At depths greater than 50 cm there was almost no effect of ultraviolet radiation on carbon uptake. PAR, UV-A and UV-B decreased oxygen evolution by the dinoflagellate Prorocentrum minimum . Inhibition of oxygen evolution was greater after 4 h than 2 h but it was not possible to distinguish the negative effects of the different light regimes. The motility of P. minimum was not affected by PAR, UV-A and UV-B. The importance of exposure of phytoplankton to different light regimes before being exposed to natural solar radiation is discussed.     

Sporulatim in the fungus Verticillium agaricinum: Reversal of blue light inhibition by Ultraviolet radiation

In colonies ranging from 3- to 5-days-old, light in general stimulates conidiation in Verticillium , including V. agaricinum and several strains of V. albo-atrum . However, when growth was started by inoculating with conidial suspension spread evenly over the plate, it was found that blue light inhibited conidiation in our strain of V. egaticinum . We most light-sensitive phase was around 9 h after inoculation. A broad band blue light pulse of 10 J m⁻² saturated the response. The inhibitory effect of blue light could be reversed by a subsequent ultraviolet (UV) radiation, but a further effect of blue light was lost after the UV pulse. Blue light inhibition was also prevented by IJV radiation administered before the blue light.