Equivalence between Pfr and Cyclic AMP in the Induction of d-Usnic Acid Dehydrogenase in the Lichen Evernia prunastri

d-Usnic acid dehydrogenase is induced in Evernia prunastri thalli by a supply of exogenous d-usnic acid in light. This effect is enhanced by red light pulses through a two step way: a very rapid increase of activity after the first 10 minutes of red light, which is not reversed by far-red light, and a slow enhancement following successive red light pulses at the beginning of each hour of incubation. The last response is completely reversed by far-red following red light. Although induction of the enzyme is not achieved in the dark, 0.1 and 0.5 millimolar cyclic AMP, or 0.1 millimolar dibutyryl cyclic AMP substitutes light action and, then, the enzyme is produced. In addition, phytochrome—far red-absorbing form—increases the amount of endogenously produced cyclic AMP and this effect is shown to be photoreversible when ethylenediaminetetraacetic acid is inhibiting adenylate cyclase.     

Phytochrome-mediated development of glycine oxidation by mitochondria in cucumber cotyledons

The development of glycine oxidation activity in mitochondria in etiolated cucumber ( Cucumis sativus L., cv. Shinfushinari) cotyledons is regulated by phytochrome. This conclusion is based on two lines of evidence. 1. The oxidation activity was increased by continuous illumination of far-red light. 2. It was also increased by brief red light pulses, the effect of which was reversed by brief far-red light pulses. The light-induced increase in glycine oxidation and in glycine decarboxylase (EC 2.1.2.10) activity in the cotyledons was inhibited by cycloheximide, but not by chloramphenicol. While glycine oxidation activity continued to increase during light-illumination for 20 h, malate oxidation activity increased for 6 to 8 h after illumination and decreased thereafter. This transient increase in the activity of malate oxidation was also induced by red light pulses and the effect of the red light was reversed by far-red light pulses.     

Factors Affecting Urease Activity in the Lichen Evernia prunastri (L.) Ach

In the lichen Evernia prunastri increased urease activity inthe presence of urea is enhanced by phosphate buffer and respirablereserves and decreased by desiccation. Although stimulatory,exogenous urea is not essential and may act as both an enzymeactivator and inducer. The previously observed decline in ureaseactivity on prolonged urea treatment, attributed to in vivoenzyme inactivation by phenolic lichen substances, is prevented,but not reversed, by in vitro additions of dithiothreitol. Evernia prunastri urease activity, enzyme inactivation, enzyme induction desiccation lichen     

The Photoresponse of S-Adenosylmethionine Decarboxylase Activity in Leaves of Pharbitis nil

S-Adenosylmethionine decarboxylase activity in leaves of Pharbitisnil increased dramatically at lights-on and then gradually decreasedin the light. The enzymatic activity fell dramatically at lights-offthen increased slightly in darkness. Photoinduction was preventedby cycloheximide and the enzymatic activity fell dramaticallyupon treatment with cycloheximide in the light. ¹Present address: Sakuya Konohana Kan, Osaka City Parks Association,Tsurumi-ku, Osaka, 538 Japan     

The participation of phytochrome in the signal transduction pathway of salt stress responses in Mesembryanthemum crystallinum L.

Continuous irradiation of Mesembryanthemum crystallinum plantswith light of equal amounts of photosynthetically active radiation,but widely different red:far red ratios was used to intervenein phytochrome-mediated signal transduction pathways in thepresence and absence of salt stress. Light with a low ratioof red:far red (in contrast to light with a high ratio of red:farred), caused induction of PEP carboxylase activity, accumulationof the CAM isoform of PEP carboxylase, and the accumulationof malate anion. Taking these as indicators of CAM inductionit is concluded that phytochrome can participate in the signaltransduction pathway leading to CAM in M. crystallinum. A lowratio of red: far red light acted synergystically with saltstress in the induction of these CAM indicators. The simplestinterpretation of this interaction is that the phytochrome-mediatedeffects and salt stress effects acted on the same signal transductionpathway. The accumulation of pinitol was also increased by light witha low ratio of red:far red, consistent with the existence ofa stress syndrome in M. crystallinum which utilizes a commontransduction pathway. A low ratio of red:far red light induced a strong shade avoidanceresponse and, compared to light with a high red:far red ratio,modified chlorophyll content and betacyanin pigment complement. Plants grown in light with a low ratio of red:far red floweredearlier than plants grown in light with a high red:far red ratio. It is concluded that phytochrome can participate in the signaltransduction pathway leading to the induction of both CAM andthe processes which result in pinitol accumulation and pigmentationin M. crystallinum, as well as in the mediation of shade avoidanceand flowering responses. Key words: Mesembryanthemum crystallinum, CAM, phytochrome, signal transduction, drought stress     

Role of Light in 5-Aminolevulinic Acid Formation in Wild Strain and Mutant C-2A' Cells of Scenedesmus obliquus

In dark-grown wild strain cells of Scenedesmus obliquus, 5-aminolevulinicacid (ALA) formation was induced by irradiation with a weakblue light, as in its mutant C-2A' cells. The induction wasinhibited by distamycin A, 6-methylpurine, cycloheximide andchloramphenicol. After the light induction, the ALA formationcould proceed in the dark as well as in the light, in such heterotrophicallygrown wild type cells, but not in the greening mutant C-2A'cells. In the latter, ALA formation was dependent on red light,as well as on blue light, in the presence of CMU. The amountsof protochlorophyll in the mutant cells increased upon cessationof illumination and decreased with subsequent irradiation withblue and red light. The possible role of protochlorophyll asa photoreceptor in regulation of ALA formation in the mutantcells is discussed. ¹Present address: Laboratory of Chemistry, Faculty of Medicine,Teikyo University, Otuka, Hachioji, Tokyo 192-03, Japan. (Received January 17, 1981; Accepted April 30, 1981)     

The Effect of Phosphate Buffer on the Physiology of the Lichen Evernia prunastri

The physiological consequences of incubating either fresh ordesiccated thalli of Evernia prunastri in phosphate buffer orwater, in the presence or absence of added urea, was investigated.Phosphate buffer, with or without added urea, induced an immediateand sustained inhibition of photosynthesis. This was enhancedby prior desiccation. Urea in water also caused a reductionin photosynthesis but had little effect on respiration, whichwas initially enhanced by phosphate buffer but subsequentlydeclined. Release of intracellular K indicated a slower butsubstantial loss of membrane integrity in the presence of phosphatebuffer or, to a lesser extent, urea. Intracellular Na concentrationsrose initially on incubation in sodium phosphate buffer andthen declined, implying the occurrence of membrane damage. Urea-inducedurease activity was sustained in the presence of dithiothreitolwhen expressed on a unit protein basis. However, a decline wasobserved when results were calculated on a thallus dry weightbasis. The previously reported loss of urease activity on prolongedincubation in phosphate buffer is now suggested to be a consequenceof general buffer-induced damage rather than a specific urea-inducedsynthesis of inhibitory phenolic compounds. Evernia prunastri, cation location, lichen phenols, phosphate buffer, photosynthesis, respiration, urease activity     

Photostimulation of Hydroxypyruvate Reductase Activity in Peroxisomes of Pharbitis nil Seedlings: I. Action Spectrum

Hydroxypyruvate reductase activity in etiolated cotyledons ofPharbitis nil is highly stimulated by white light. The actionspectrum shows three effective regions: blue, red and far red.The main characteristics of this high irradiance reaction responseis a high blue efficiency and a low red efficiency. Experimentswith herbicide-treated plants demonstrated that chlorophyllis not involved in the regulation but suggest that a specificblue-absorbing pigment is involved, in addition to phytochrome. (Received November 22, 1983; Accepted June 20, 1984)     

Regulation of Calmodulin- and Dopamine-Stimulated Adenylate Cyclase Activities by Light in Bovine Retina

Abstract: Neural retina from most species contains 3,4-dihydroxyphenylethylamine (dopamine) receptors coupled to stimulation of adenylate cyclase activity. It has been demonstrated that release of dopamine from its neurons and subsequent occupation of dopamine receptors is increased by light. In this study, we have shown that adenylate cyclase activity in bovine retina is highly responsive to the endogenous Ca²⁺-binding protein, cal-modulin, and that calmodulin can increase dopamine-sen-sitive adenylate cyclase activity in bovine retina. We further demonstrate that both dopamine- and calmodulin-stimulated adenylate cyclase activities can be regulated by alterations in light. Bovine retinas were dissected from the eye under a low-intensity red safety light, defined as dark conditions, and incubated for 20 min in an oxygenated Krebs Henseleit buffer under either dark or light conditions. The retinas were then homogenized and adenylate cyclase activity measured in a paniculate fraction washed to deplete it of endogenous Ca²⁺ and calmodulin. Activation of adenylate cyclase activity by calmodulin, dopamine, and the nonhydrolyzable GTP analog, gua-nosine-5′-(β,γ-imido)triphosphate (GppNHp), was significantly (60%) greater in paniculate fractions from retinas that had been incubated under dark conditions as compared to those incubated under light conditions. Basal, Mn²⁺-, and GTP-stimulated adenylate cyclase activities were not altered by changes in lighting conditions. Calmodulin could increase the maximum stimulation of adenylate cyclase by dopamine in retinas incubated under either dark or light conditions, but the degree of its effect was greater in retinas incubated under light conditions. Activation of adenylate cyclase by calmodulin, dopamine, and GppNHp in paniculate fractions from retinas incubated under light conditions was indistinguishable from the activation obtained when retinas were incubated in the dark in the presence of exogenous dopamine. These results suggest that an increased release of dopamine occurs in light. The decreased response of adenylate cyclase to exogenous dopamine can then be explained by a subsequent down-regulation of dopamine receptor activity. The down-regulation of dopamine receptor activity can also regulate activation of adenylate cyclase by GppNHp and calmodulin. The results suggest that dopamine, calmodulin, and GppNHp are modulators of a common component of adenylate cyclase activity, and this component is regulated by light.     

Flowering in Pisum: the Effect of Light Quality on the Genotype If e Sn Hr

Far-red light, when given as a 16 h photoperiod extension, iamore effective than red light in reducing the flowering nodeof genotype Pisum. In contrast, when a 16 h dark period is interruptedby a 2 h light break red light is more effective than far-redlight. In addition, the stimulatory effect of a red interruptionis partially reversed by a subsequent period of far-red. However,a light interruption is not effective until over 12 h have elapsedsince the start of the previous photoperiod, regardless of whetherthe photoperiod was of 4 or 8 h duration. The results suggest that there are two light-dependent reactionscontrolling flowering in peas, one operating through the phytochromesystem with high levels of Pfr suppressing production of flowerinhibitor by the sn gene and a second requiring continuous illuminationwith wavelengths above 700 nm. The role of time measurementin the photoperiod response in peas is suggested to be filledby the proportion of time the Sn gene is effectively producinginhibitor. The photoperiod response in peas is not independentof temperature or plant age since the activity of gene Sn isalso varied by these factors.     

Effect of Cycloheximide on the Inverse Control by Phytochrome of the Expression of Two Nuclear Genes in Barley (Hordeum vulgare L.)

The accumulation of mRNAs encoded by two phytochrome-regulatedgenes in barley (Hordeum vulgare L.) was examined after a singlered light pulse in presence of cycloheximide. The initial increasein mRNA encoding the major light harvesting chlorophyll a/bbinding protein (LHCP) could still be observed indicating thatno protein synthesis-requiring step is essential for the transductionchain. The phytochrome-induced decrease in mRNA encoding NADPH:protochlorophyllideoxidoreductase was considerably slowed. (Received February 22, 1988; Accepted June 8, 1988)     

Effects on Phytochrome Controlled Germination Produced by Far-Red Irradiation of Seeds Before and During Rehydration

Seeds irradiated with red light and then re-dried will respondto this light treatment on subsequent rehydration in the dark.If such high-Pfr seeds are irradiated in the dry state withfar-red light immediately before rehydration the percentagegermination is significantly reduced in the case of Plantagomajor and Sinapis arvensis but increased in Bromus steriliswhere Pfr inhibits germination. This effect of far-red lightcan be reversed by red light despite the fact that red lightalone has no effect on dry seed. This is due to the interconversionof Pfr and the red light absorbing phytochrome intermediatecomplex meta-Fa. If there is a delay between far-red irradiationand rehydration of Sinapis seeds, the inhibitory effect of thefar-red irradiation becomes progressively less the longer thedelay. This reduction in effectiveness of far-red is interpretedin terms of a dark reversal of meta-Fa to Pfr with a half-lifeof about 4–6 h. The reappearance of Pfr is either veryslow or docs not occur in dehydrated Plantago seeds, as far-redtight given 96 h prior to hydration is just as inhibitory asfar-red light given immediately before hydration. Meta-Fa doesappear to revert to Pfr in darkness in Bromus seeds, but onlyvery slowly. The rapid increase in effectiveness of red irradiationduring rehydration of high-Pfr Plantago seeds suggests that,in this species, the pre-treatment used in preparation of high-Pfrseeds may increase the receptivity or amount of the Pfr reactionpartner. Key words: Phytochrome intermediates, Seeds, Germination     

Photoinduction of Spore Germination in Marchantia polymorpha L. is Mediated by Photosynthesis

The effects of light on spore germination (protrusion of protonemata)in the liverwort Marchantia polymorpha L. were examined. Sporegermination was found to be light dependent and light irradiationfor 10 h or longer was necessary. Test using specific wavelengthsshowed that the entire spectrum from near UV to red light waseffective, red light being the most effective. Spore germinationcould be induced by intermittent irradiation with 15-min redlight pulses given every 1 or 2 h for 24 h. The effect of intermittentred light was not reversed by subsequent or simultaneous far-redlight irradiation. However, spore germination was inhibitedby the photosynthesis inhibitor DCMU (100 µM). Completeinhibition of spore germination was found when DCMU was givenduring the light period. When DCMU was applied during the darkperiods, only a slight reduction of germination rate was observed.Further, it was found that Chl formed in the spores during imbibitionin darkness. Light sensitivity increased at nearly the samerate as the appearance of Chl. Moreover, spore germination wasinduced in total darkness by the addition of glucose to themedium. These results clearly indicate that photosynthesis mediatesthe photoinduction of spore germination in Marchantia polymorpha. (Received May 13, 1999; Accepted July 14, 1999)     

Effect of far-red light pulse on induction and production of flowers in Lemna paucicostata 6746 in darkness

A short-day duckweed, Lemna paucicostata 6746, was exposed tocontinuous darkness at 26^?C, and the changes in the floral parameters(3) due to far-red and/or red light pulse given at various timesof the dark period were studied. Parameters a (vegetative growth rate) and (flowering ratio)were respectively decreased and increased with a far-red lightpulse given at the outset of the dark period. The decreaseda and the increased remained almost unchanged until the 7thhour, but returned to their initial levels thereafter. The far-redlight actions on a and were reversed by subsequent exposureto red light. Parameter P₁ (pre-flower induction period) wasextended by 1 day when far-red and/or red pulse was given atabout the 7th hour of the dark period. A far-jed pulse givenat the outset of the dark period only affected parameter P₂(flower induction period). Although the sensitivity of P₂ tored light increased with time, its sensitivity to far-red lightremained constant and at about the 7th hour was equally sensitiveto far-red and red lights. Both red and far-red pulses givenlater than the 7th hour were increasingly ineffective on P₂.The red/far-red reversibility occurred only for the action onP₂ of the far-red pulse applied during the early dark period.Parameter P₄ (flower production period) varied rhythmicallyin length with a far-red puke, the maximum shortening and extensionbeing induced by the pulse given at about the 7th and 19th hours,respectively. The sensitivity of P₄ to red light also changedrhythmically with an inverse phase angle to the rhythmic responseto farred light, and the far-red and red light actions werereversed respectively by subsequent red and far-red lights. These findings suggested that multiple timing devices includingan hourglass-type clock and a circadian clock are involved induckweed flowering. (Received October 25, 1978; )     

Changes in Stoichiometry among PSI, PSII and Cyt b6-f Complexes in Response to Chromatic Light for Cell Growth Observed with the Red Alga Porphyra yezoensis

Stoichiometry among 3 thylakoid components, PSI and PSII andCyt b6-f complexes, was determined with the red alga Porphyrayezoensis with special reference to the regulation of PSI/PSIIstoichiometry in response to light regime. The ratio of PSIto PSII abundance was four times greater in thalli grown underorange light which excites mainly phycobilisome, thus PSII,than that under red light which excites preferentially Chl a,thus PSI. Cyt b₆-f abundance remained almost constant. The PSIand PSII content was regulated separately under the two growthlight conditions as was also observed with the red alga Porphyridiumcruentum by Cunningham et al. [(1990) Plant Physiol. 93: 888].This differs from the cyanophyte Synechocystis PCC 6714 whereadjustment occurs only in the PSI content [(1987) Plant CellPhysiol. 28: 1547]. However, results on the marine cyanophyteSynechococcus NIBB 1071 indicate that changes in the PSI/PSIIsoichiometry is similar to red algae. In this species, as inthe red algae, more than one PSII is associated with each phycobilisome.The light regime also induced changes in the phycobiliproteincomposition in Porphyra yezoensis. Under PSII light, phycoerythrinincreased, and phycocyanin decreased, while under PSI lightthe response was reversed. The change suggests an occurrenceof complementary chromatic adaptation. (Received April 8, 1994; Accepted June 1, 1994)     

Amitriptyline reduces olfactory neuron adenylyl cyclase activity

Adenylyl cyclase plays an important role in olfactory signaltransduction. Recently, a novel type III adenylyl cyclase hasbeen localized in olfactory neurons (Pfeuffer et al., 1989;Bakalyar and Reed, 1990). Because amitriptyline (AMI), a tricyclicantidepressant, appears to have an inhibitory effect on adenylylcyclase activity in other in other neuronal tissue (Yamaokaet al., 1988; Wong et al., 1991), we measured the effect ofAMI on forskolin-stimulated adenylyl cyclase activity in membranepreparations of olfactory mucosa from adult rats. In the presenceof 5'-guanylyl-imidodiphosphate, AMI (0.5–8.0 µM)inhibited forskolin-stimulated adenylyl cyclase activity ina dose-dependent manner. To determine whether this effect wasspecific for olfactory neurons, as opposed to other cells inthe olfactory epithelium, rats were unilaterally bulbectomizedin order to reduce selectively the number of olfactory neuronson the side ipsilateral to the bulbectomy. In membrane preparationsfrom unilaterally bulbectomized animals we saw significantlylower adenylyl cyclase activity in ipsilateral olfactory mucosa,compared with adenylyl cyclase activity from non-bulbectomizedmucosa. These results indicate that AMI inhibition of adenylylcyclase activity is primariy localized in olfactory neurons.     

Red and blue light-stimulated proton efflux by epidermal leaf cells of the Argenteum mutant of Pisum sativum

Light stimulates leaf expansion in dicotyledons by increasingapoplastic acidification, cell wall loosening and solute accumulationfor turgor maintenance. Red and blue light enhance growth viadifferent photo-systems, but the cellular location and modesof action of these systems is not known. Here, the effect of red and blue light was studied on transportprocesses in epidermal cells of expanding leaves of the Argenteummutant of Pisum satlvum. Both red and blue light caused extraceiiuiaracidification by isolated epidermal tissue, which was stimulatedby extracellular K⁺ and inhibited by DCCD at 0.1 mol m^–3.Acidification induced by red compared with blue light showeddifferent saturating kinetics in fluence rate-response curves.Under near saturating light conditions the effects of red andblue light were additive. The red light-induced acidificationwas inhibited by far-red light while the blue light-inducedacidification was not. Light caused a hyperpoianzation of themembrane potential in epidermal strips, and stimulated ⁸⁶Rb⁺uptake by epidermal protoplasts. These results show that phytochromeand an additional blue light-photoreceptor function in isolatedepidermal cells to promote proton efflux, hyperpolarization,and cation uptake. Key words: Pisum sativum, light-induced acidification, ion transport, epidermis, photoreceptor     

Abscission: Response to Red and Far-Red Light

Craker, L. E., Zhao, S. Y. and Decoteau, D. R. 1987. Abscission:response to red and far-red light.—J. exp. Bot. 38: 883–888. The dose-response and time relationship of red and far-red lightin the inhibition and promotion, respectively, of dark-inducedleaf abscission was quantified using cuttings of coleus (ColeusBlumei Benth.). A continuous photon flux of approximately 15nM m^–2 s^–1 of red light was sufficient to preventleaf abscission. Abscission was promoted by exposure to a photonflux of approximately 10 nM m^–2 s^–1 of far-red lightThe inhibition of abscission by red light could be reversedby treatment with far-red and the promotion of abscission byfar-red light could be reversed by treatment with red lightThe data were consistent with a phytochrome receptor systemlocated in the leaves that controlled the presence of an abscission-inhibitingsubstance in the abscission zones. Key words: Abscission, Coleus Blumei, far-red light red light     

The appearance of glutamine synthetase in turions of Spirodela polyrhiza (L.) Schleiden as regulated by blueand red light, nitrate and ammonium

Control by light and nitrogen (nitrate and ammonium) of theappearance of glutamine synthetase (GS; EC 6.3.1.2 [EC] ) in turionsof Spirodela polyrhiza (L.) Schleiden, strain SJ, was investigatedduring the pregermination period, i.e. up to 48 h after onsetof light. Immediately after transfer from after-ripening conditions(5C, darkness, D) to germination conditions (25C), GS activitydid not respond to light or nitrate. After 72 h in D (25C)activity increased in continuous light. Therefore, the regulatoryrole of light, nitrate and ammonium in the process of appearanceof GS was mainly studied between 72 and 120 h after transferfrom after-ripening to germination conditions (phase II of thepre-germination process). The inducing effect of red light ismediated by the photoreceptor phytochrome: the effect of long-termcontinuous red light (6 or 24 h) can be reversed, at least inpart, by a subsequent far-red light pulse (‘end of day’Irradiation). Blue light is more effective than red light ininducing the appearance of GS. Therefore, a specific blue lighteffect has to be assumed. This represents a novel mode of lightaction in regulating the level of the ammonium assimilatingenzyme in an angiosperm system. lmmunoblots showed that (i)increase in the enzymatic activity is caused by de novo synthesisof the enzyme protein, (ii) two different subunits (38 and 42kDa) contribute to the total activity which must be attributedto two different isofornis. In accordance with results fromother higher plants, the 38 kDa subunit (presumably relatedto the cytosolic isoform) did not increase in the presence oflight, whereas the 42 kDa subunit (presumably related to theplastidic isoform) was induced. The maximal enzyme level wasreached only in the presence of both light (blue light) andnitrate. Light induction was also observed in the presence ofammonium; however, GS activity was decreased, when comparedto nitrate-treated turions. Comparison of these results withprevious observations suggest that the influence of light andnitrate on the germination response and regulation of the nitrate/ammoniumassimilation pathway in turions appear to be unrelated phenomena. Key words: blue light, germination, glutamine synthetase, phytochrome, Spirodela polyrhiza, turion     

Phytochrome regulation of nitrate reductase in wheat

In excised wheat leaves, the activity of nitrate reductase was enhanced by a brief pulse of red light and this increase was reversed by far-red light irradiation. Even under continuous far-red light, nitrate reductase activity increased by 258% after 18 h. When leaves were kept in distilled water during exposure to red light and then transferred to potassium nitrate, there was no difference in endogenous nitrate concentration. The nitrate reductase activity was the same whether leaves were floated in potassium nitrate or in distilled water during irradiation. Partial to complete inhibition of enzyme activity was observed when leaves were incubated in actinomycin-D and cycloheximide respectively, following 4 h of red light irradiation.In vitro irradiation of extract had no significant effect on nitrate reductase activity