REDUCED NEAR-UV SENSITIVITY IN Phycomyces MUTANTS AFFECTED IN THE BIOSYNTHESIS OF 6,7-DIMETHYL-8-RIBITYLLUMAZINE

Riboflavin-requiring mutants of Phycomyces blakesleeanus with defects in the genes ribA, ribB, ribC and ribD were analyzed with respect to their contents of flavins, 6,7-dimethyl-8-ribityllu-mazine (DMRL) and pterins as well as their phototropic sensitivity. Strains were grown on minimal medium enriched with 10^?6M riboflavin (RB), and the concentrations of the respective pigments in sporangiophores were determined by HPLC. In strains A607 ribC401 and A641 ribC402 madA7 a loss of DMRL correlated with a loss of near-UV sensitivity. In general terms, the results suggest the participation of DMRL in photoreception, which does not necessarily imply DMRL as a photoreceptor chromophore. In more specific terms, the result could be understood on the basis of a UV/blue-light photoreceptor, which includes besides a flavin also a lumazine-like chromophore. Mutants C318 ribA I and C323 ribA4 accumulated DMRL, the immediate precursor of RB, as well as biopterin and neopterin. Mutant C322 ribB contained normal amounts of DMRL and pterins. Mutant C324 ribD5 had reduced amounts of neopterin and biopterin. The fact that some of the RB-requiring mutants displayed abnormal amounts of pterins indicates a common regulation for the flavin and the pterin pathway.     

PTERIN- AND FLAVIN-LIKE FLUORESCENCE ASSOCIATED WITH ISOLATED FLAGELLA OF Euglena gracilis

Fluorescence excitation- and emission spectra indicate the presence of pterin(s) and flavin(s) in isolated flagella of the phytoflagellate Euglena gracilis. These compounds appear to bind at least in part non-covalently to the molecular framework of the paraflagellar body, which is the presumed photoreceptor organelle and which is attached to the isolated flagella. A compound with pterin-like fluorescence excitation and emission spectrum could he extracted with methanol from isolated flagella and could he recovered on thin-layer silica gels. Besides the previously assumed photoreceptor function of flavins, our results suggest also a role for pterins in the photosensory transduction chain of Euglena gracilis.     

DETECTION OF PTERINS IN Phycomyces SPORANGIOPHORES*

Differential fluorometry with sodium dithionite showed pterin-like signals in extracts of Phycomyces sporangiophores. After iodine oxidation, pterin, biopterin and neopterin could be separated. The concentrations determined for these three pterins exceed the calculated minimal concentration of 3 times 10^?7M for the photoreceptor.     

PHOTOCONTROL OF HYPOCOTYL ELONGATION IN LIGHT-GROWN Cucumis sativus L. PHOTOSYNTHETIC REQUIREMENT FOR A FLUENCE RATE DEPENDENT PHYTOCHROME RESPONSE

We investigated the role of photosynthesis in the photocontrol of extension growth of the hypocotyl of light-grown Cucumis sativus L. Previous work [Gaba and Black (1985b) Plant Physiol. 79 , 1011] demonstrated that the inhibition of cucumber hypocotyl elongation is a fluence rate dependent response in red light. However, the relative contributions of phytochrome and photosynthesis to the photon flux dependent inhibition response were not clear. Here we have shown that photoperception by the foliar cotyledons as well as the hypocotyl itself are responsible for fluence rate dependence in red light. The inhibitor of photosynthesis diuron [3-(3,4-dichlorophenyl)-1, 1-dimethylurea] reduced both the magnitude of inhibition and the fluence rate dependency in red light, indicating an involvement of photosynthesis. Furthermore, the growth of non-pigmented seedlings (treated with the herbicide norflurazon) was less inhibited by red light, with no fluence rate dependency. In particular, inhibition due to cotyledon photoperception was completely lost in non-pigmented (norflurazon-treated) plants, and much reduced by diuron treatment. Hypocotyl-perceived red light inhibition was only slightly reduced by treatment with norflurazon and diuron. Photosynthesis was compared directly to photo-inhibition of growth: the photon flux response curve of oxygen evolution of green Cucumis cotyledons was distinctly different from that of hypocotyl inhibition. In conclusion, photosynthesis is an essential requirement for the cotyledon-perceived inhibition, but the response itself is not due to photosynthesis.     

Phototaxis in the ciliated protozoan Ophryoglena flava: dose-effect curves and action spectrum determination

The sensitivity of positive phototactic orientation of cells of the ciliated protozoan Ophryoglena flava has been measured for white light, broad-band blue and red light, and narrow-band monochromatic light, using a laboratory-developed computer aided system. The white-light fluence rate-response curve shows that there is no negative phototaxis in the fluence rate range investigated (0-15 W/m2) and no adaptation phenomena; it is very well fitted by a hyperbolic function; the fluence rate curves under broad band blue and red light (full width at half maximum, FWHM= 100 nm) can be fitted by the same model. The saturation level is, within experimental errors, the same for the three curves, indicating that there are no chromaticity effects and that if there is more than one photoreceptor pigment, they act independently of each other. The fluence rate-response curves determined under narrow band monochromatic light (FWHM = 10 nm) can also be fitted by the same model and show, within experimental errors, the same saturation level. An action spectrum for positive phototaxis at 10-nm intervals has been calculated from fluence rate-response curves: it shows three maxima, at 420, 540 and 590 nm. This action spectrum is significantly different from the ones for photomotile responses in Blepharisma japonicum, Stentor coeruleus and Chlamydodon mnemosyne, whereas it resembles the ones of Paramecium bursaria and Fabrea salina.     

A PHOTORECEPTOR SYSTEM REGULATING in vivo AND in vitro PHOSPHORYLATION OF A PEA PLASMA MEMBRANE PROTEIN*

Abstract— We have continued to characterize the blue light-regulated phosphorylation of a 120 kDa pea plasma membrane protein thought to be involved in sensory transduction for phototropism (Short and Briggs, 1990, Plant Physiol. 92 , 179–185). By incubating pea stem sections in ³²P-phosphate, we show that the 120 kDa protein is phosphorylated in vivo only after blue light irradiation and that the photosensitive fluence range matches that for phototropism. Blue light induces phosphorylation of the protein in vitro as well, but the fluences required to elicit the response are at least 30-fold higher. Triton solubilization of the plasma membrane vesicles does not further alter the fluence-response relationship. Very little turnover was detected over 20 min phosphorylation time courses or by pulse-chase experiments on unirradiated, blue light pulse-irradiated, or continuously irradiated membranes. Experiments with a dark period intervening between irradiation and addition of adenosine triphosphate show the light-induced change to persist for several minutes at 30°c. Agents that disrupt the normal photochemistry of flavins preferentially inhibit the light-induced enhancement of phosphorylation, suggesting a flavin chromophore. However, exogenous free flavins do not affect the sensitivity of the response. Staphylococcus aureus V-8 proteolysis of the phosphorylated protein from membranes subjected to a range of fluences before phosphorylation shows that the radiolabel on each of three peptides increases in proportion to the phosphorylation level of the undigested polypeptide. These studies may be valuable for assessing the nature of the photoreceptor and for unravelling the early sensory transduction steps in phototropism.     

Lipofuscin and A2E Accumulate with Age in the Retinal Pigment Epithelium of Nrl−/− Mice†

Lipofuscin is a fluorescent material with significant phototoxic potential that accumulates with age in the retinal pigment epithelium (RPE) of the eye. It is thought to be a factor in retinal degeneration diseases. The most extensively characterized lipofuscin component, N‐retinylidene‐N‐retinylethanolamine (A2E), has been proposed to be a byproduct of reactions involving the visual pigment chromophore. To examine the impact of the visual pigment and photoreceptor cell type on lipofuscin accumulation, we analyzed the RPE from Nrl^?/? mice of various ages for lipofuscin fluorescence and A2E levels. The photoreceptor cells of the Nrl^?/? retina contain only cone‐like pigments, and produce cone‐like responses to photostimulation. The cone‐like nature of these cells was confirmed by the presence of RPE65. Lipofuscin was measured with fluorescence imaging, whereas A2E was quantified by UV/VIS absorbance spectroscopy coupled to HPLC. The identity of A2E was corroborated with tandem mass spectrometry. Lipofuscin and A2E accumulated with age, albeit to lower levels compared with wild type mice. The emission spectra of RPE lipofuscin granules from Nrl^?/? mice were similar to those from wild type mice, with λ_maxca 610 nm. These results demonstrate that cone visual pigments can contribute to the production of lipofuscin and A2E.     

FORTY YEARS OF BLUE-LIGHT RESEARCH AND NO ANNIVERSARY

The status of near- UV/blue-light research is described and critically assessed. It is argued that the generally accepted proposition of flavins acting as near- UV/blue-light photoreceptors is reasonable, but that also other pigments, specifically pteridines and pterins, should be considered. In view of the fact that a receptor assay, applicable to any organism and near-UV/blue-light reaction, is not yet at hand, caution appears to be indicated as to what one can accept as a reasonable “criterion” for the involvement of any proposed photoreceptor pigment.     

ARE THERE SEVERAL PHOTORECEPTORS INVOLVED IN PHOTOTROPISM OF Phycomyces blakesleeunus? KINETIC STUDIES OF DICHROMATIC IRRADIATION*

Abstract— Photogeotropic equilibrium angles were measured for Phycomyces blakesleeanus wild type firstly by means of dichromatic fluence rate response curves using simultaneous irradiation with near threshold 450 nm reference light (constant at 1.2 × 10^?8 W m^?2) and variable fluence rates of test light (498–630 nm) from the same side. These curves showed minima for test light fluence rates that were close to the photogeotropic threshold for these wavelengths. Secondly, the time course of this inhibitory effect was studied with both the inductive reference 450 nm light (2 × 10^?-⁷ W m^?2) and the test light (606 or 450 nm) given as light pulses of 2 s duration (2 s light/48 s dark periods for 6 h). The dark period between the onset of the inductive reference light and test light pulses was varied between 0 and 48 s. No inhibitory effects were observed for simultaneous pulses; however, inhibitory effects were demonstrated for delay times of 2 s and 20 s for 606 nm as well as 450 nm test light. If the test light pulses were given immediately before the inductive reference light, only 606 nm test light was effective in producing a significant inhibitory effect. The results are discussed with regard to a multichromophoric photoreceptor system and to the wavelength dependence of the effects observed. The data and conclusions favor a photoreceptor system with at least two separate chromophoric absorptions of the blue light receptor type, one acting positively, the other acting inhibitorily, and at least one other photoreceptor of presumably minor influence.     

All‐Trans Retinal Mediates Light‐Induced Oxidation in Single Living Rod Photoreceptors†

All‐trans retinal is a potent photosensitizer that is released in photoreceptor outer segments by the photoactivated visual pigment following the detection of light. Photoreceptor outer segments also contain high concentrations of polyunsaturated fatty acids, and are thus particularly susceptible to oxidative damage such as that initiated by light via a photosensitizer. Upon its release, all‐trans retinal is reduced within the outer segment to all‐trans retinol, through a reaction requiring metabolic input in the form of NADPH. The phototoxic potential of physiologically generated all‐trans retinal was examined in single living rod photoreceptors obtained from frog (Rana pipiens) retinas. Light‐induced oxidation was measured with fluorescence imaging using an oxidation‐sensitive indicator dye from the shift in fluorescence between the intact and oxidized forms. Light‐induced oxidation was highest in metabolically compromised rod outer segments following photoactivation of the visual pigment rhodopsin, and after a time interval, sufficiently long to ensure the release of all‐trans retinal. Furthermore, light‐induced oxidation increased with the concentration of exogenously added all‐trans retinal. The results show that the all‐trans retinal generated during the detection of light can mediate light‐induced oxidation. Its removal through reduction to all‐trans retinol protects photoreceptor outer segments against light‐induced oxidative damage.     

INHIBITION OF LIGHT-DEPENDENT PHOTOMORPHOGENESIS OF SPORANGIOPHORES FROM Phycomyces blakesleeanus BY APPLICATION OF PTERIDINE BIOSYNTHESIS INHIBITORS*†

Abstract— In the zygomycete Phycomyces blakesleeanus the morphogenesis of both macrosporangiophores and microsporangiophores is under separate control of different blue-light photoreceptors. Blue light represses microphorogenesis and enhances macrophorogenesis. Both, flavins and pterins are discussed as possible components of these blue-light photoreceptors. 2,4-Diamino-6-hydroxypyrimidine (DAHP) was shown to be an inhibitor of GTP-cyclohydrolase I, the initial enzyme of pteridine biosynthesis, in vitro and in vivo in Phycomyces. When grown on agar plates containing 5 mM of DAHP, Phycomyces shows a 6.0-fold reduction of light-dependent enhancement of macrophorogenesis, and microphorogenesis was 3.1 times less repressed when compared with controls grown without DAHP. This implies a participation of pteridines in blue-light photoreception in both phenomena, with greater influence on macrophorogenesis enhancement than on microphorogenesis repression.     

PHYTOCHROME ACTION AT HIGH PHOTON FLUENCE RATES: RAPID EXTENSION RATE RESPONSES OF LIGHT-GROWN MUSTARD TO VARIATIONS INFLUENCE RATE and RED: FAR-RED RATIO*

Abstract— Extension growth rate of light-grown mustard (Sinapis alba L.) seedlings was monitored continuously using a sensitive linear displacement transducer system. When high fluence rates (ca 2 mmol m^?2 s^_1) of mixed red and far-red light were presented to the growing internodes from fibre optic probes, fluctuations in extension rate occurred during the first 30 min. High red: far-red ratios (R: FR) caused growth deceleration, whilst low R: FR caused transitory growth acceleration. These changes in extension rate were not exactly as predicted from the proportions of Pr (the red-absorbing form of phytochrome) and Pfr (the far-red absorbing form of phytochrome) calculated to be established by the light sources. Nevertheless, the data demonstrate that phytochrome is able to control extension growth at fiuence rates approaching those of summer sunlight, thereby providing the capacity to sense the presence of neighbouring vegetation before shading seriously compromises photosynthesis. Varying fiuence rate over two orders of magnitude whilst maintaining R: FR constant evoked transient fluctuations in extension rate. At high R: FR, a 100-fold step down in fiuence rate led, after a lag of ca 10 min, to a transient (i.e. 20 min) deceleration of extension that was followed by a marked transient (i.e. 20 min) acceleration. After a 100-fold step up in fiuence rate, a transient (i.e. 20 min) acceleration only was observed, beginning after a lag of ca 10 min. When R: FR was low, neither a step-down nor a step-up in fluence rate resulted in appreciable fluctuations in extension rate. The data are discussed in relation to the possible role played by the accumulation of photoconversion intermediates using a simple computer model for simulating active phytochrome concentrations at high fluence rates. The possibility that the mechanism for the photoperception of light quality by phytochrome may be capable of rapid adaptation to fluence rate fluctuations is proposed.     

Retinal Photodamage Mediated by All‐trans‐retinal†

Accumulation of all‐trans‐retinal (all‐trans‐RAL), reactive vitamin A aldehyde, is one of the key factors in initiating retinal photodamage. This photodamage is characterized by progressive retinal cell death evoked by light exposure in both an acute and chronic fashion. Photoactivated rhodopsin releases all‐trans‐RAL, which is subsequently transported by ATP‐binding cassette transporter 4 and reduced to all‐trans‐retinol by all‐trans‐retinol dehydrogenases located in photoreceptor cells. Any interruptions in the clearing of all‐trans‐RAL in the photoreceptors can cause an accumulation of this reactive aldehyde and its toxic condensation products. This accumulation may result in the manifestation of retinal dystrophy including human retinal degenerative diseases such as Stargardt’s disease and age‐related macular degeneration. Herein, we discuss the mechanisms of all‐trans‐RAL clearance in photoreceptor cells by sequential enzymatic reactions, the visual (retinoid) cycle, and potential molecular pathways of retinal photodamage. We also review recent imaging technologies to monitor retinal health status as well as novel therapeutic strategies preventing all‐trans‐RAL‐associated retinal photodamage.     

EFFECT OF BLUE LIGHT AND RED LIGHT ON THE CONTROL PEA LEAVES TO INCREASED FLUENCE RATES OF CHLOROPLAST ACCLIMATION OF LIGHT-GROWN PEA LEAVES TO INCREASED FLUENCE RATES

Abstract— We have investigated the possibility of the involvement of a blue light fluence-rate sensing photoreceptor in the light acclimation of chloroplast components in light-grown pea seedlings. Low lightgrown seedlings were acclimated for 2 days to either 20 or 200 μmol^m-2s-2 of white, blue-enriched, or broad-band red light. An increase in blue-enriched light fluence rate was more effective than that of red light in bringing about both inhibition of internode growth and the enhancement of the chlorophyll a/b ratio. Ribulose 1,5-bisphosphate carboxylase/oxygenase and cytochrome f protein levels, per unit cell, also increased more markedly (around two-fold) in response to an increase in blue light. The 23 kDa polypeptide of the oxygen-evolving complex and the light-harvesting chlorophyll d b protein of photosystem II apoprotein levels vaned under all wavelengths to a lesser extent, correlating with total protein levels or greening. These data are consistent with the hypothesis of a role for a blue photoreceptor in detecting low versus high fluence rate of light, and subsequently controlling the light acclimation responses. Nevertheless photosynthesis or other mechanisms of fluence-rate photoperception must also be involved.     

Spectral characteristics of the photoreceptor pigment of phototaxis in Dictyostelium discoideum

Abstract —A photoresponsive pigment, described previously as the photoreceptor pigment for phototaxis in Dictyostelium discoideum, was examined by low-temperature spectroscopy. The absorption spectrum of the purified pigment frozen in darkness indicates the reduced form of a high-spin heme protein, and the spectrum of the pigment frozen during irradiation (to freeze in the photoproduct) indicates the oxidized form of the heme protein. The light-induced absorbance changes measured at room temperature also indicate photooxidation of a heme pigment. The action spectrum for the light-induced absorbance change shows a primary peak at about 430 nm and a broad, less active maximum in the 550–580 nm region. The absorption spectrum of the reduced pigment and the action spectrum for its photooxidation are both similar to the action spectrum for phototaxis of the pseudoplasmodia of D. discoideum.     

PHOTORECEPTOR PROTEINS AND PIGMENTS IN THE PARAFLAGELLAR BODY OF THE FLAGELLATE Euglena gracilis

Abstract— –The presumed photoreceptor for phototaxis, the paraflagellar body, in the flagellate Euglena gracilis , was isolated still attached to the flagellum. After solubilization, fast protein liquid chromatography (FPLC) analysis yielded four major protein fractions with the chromophoric groups still attached. Fluorescence spectra showed that three fractions had excitation peaks at 380 nm and emission peaks around 450 nm indicative of pterins, while the fourth chromoprotein had a fluorescence emission at 520 nm and an excitation peak at 450 nm, indicative of a flavin. The separated proteins were analyzed by gel electrophoresis: the pterin binding proteins have apparent molecular masses between 27 000 and 31 600 and the flavin binding protein has an apparent molecular mass of 33 500.     

A novel prokaryotic UVB photoreceptor in the cyanobacterium Chlorogloeopsis PCC 6912

We present evidence for the presence and nature of a UVB-specific photoreceptor in the cyanobacterium Chlorogloeopsis PCC 6912. The photoreceptor mediates at least the photosensory induction of mycosporine-like amino acid (MAA) synthesis. Because MAA synthesis in this organism can also be induced under salt stress, we could distinguish between the photosensory and the purely biochemical requirements of MAA synthesis. Neither visible light nor UV radiation was necessary for the biosynthetic process, thus indicating that the UVB (280-320 nm) dependence of biosynthesis is based on a UV photosensory capacity of the organism. An action spectrum of the MAA synthesis showed a distinct peak at 310 nm tailing down into the UVA (320-400 nm) region with no detected activity above 340 nm. We found that radiation below 300 nm caused significant inhibition of synthesis of MAAs indicating that the action spectrum at these wavelengths may not have been satisfactorily resolved. We propose that a pterin is a good candidate for a photoreceptor chromophore as (1) reduced pterins present absorption spectra congruent with the action spectrum obtained; and (2) an inhibitor of the biosynthetic pathway of pterins and an antagonist of excited states of pterins, both depressed the photosensory efficiency of induction but not its chemosensory efficiency.     

Calcium Control of the Sign of Phototaxis in Brown Algal Gametes of Mutimo cylindricus

Brown algal swarmers usually exhibit positive or negative phototaxis. Such behaviors influence the increasing or decreasing dispersal distance or colonization on the new substratum. We confirmed that the sign of phototaxis (negative or positive) in male gametes of Mutimo cylindricus was affected by extracellular Ca²⁺ influx through Ca²⁺ channels. Under the control condition (10^?2 m [Ca²⁺]), male gametes swimming with a helical rotation of their cell body mostly showed positive phototaxis. At 10^?3 m [Ca²⁺], more than half of the male gametes showed positive phototaxis, whereas the others showed negative phototaxis. From 10^?4–10^?5 m [Ca²⁺], the phototactic sign changed to negative. When these negative phototactic gametes were transferred back to the control condition, the phototactic sign reverted to positive. At 10^?6 m [Ca²⁺], some of male gametes showed negative phototaxis, but most showed no phototaxis or flagellar beating. Lanthanum, a Ca²⁺ channel blocker, affected the sign of phototaxis at 10^?4 m [La³⁺] under 10^?2 m [Ca²⁺], and male gametes mostly showed negative phototaxis. A further increase in [La³⁺] inhibited phototaxis and flagellar beating. These results pointed out the involvement of Ca²⁺ channels that were blocked by La³⁺ in phototaxis and flagellar beating.     

Biphasic fluence-response curves and derived action spectra for light-induced absorbance changes in Phycomyces mycelium

The photoresponses of Phycomyces, including phototropism and photocontrol of sporangiophore development, are mediated primarily by blue and UV light. Recent results on these two responses indicated a subsidiary role for green light. We have measured in vivo light-induced absorbance changes (LIAC) in mycelial samples of a caroteneless (carB) strain to compare the effectiveness of UV, blue, and green light. In the dual-wavelength kinetic mode of the spectrophotometer, measuring wavelengths of 445 and 470 nm were chosen, because green light produces substantial absorbance changes between these two wavelengths. Fluence-response curves were measured for 13 wavelengths between 365 and 530 nm, and for variable exposure times between 0.5 and 320 s. With one exception (365 nm), the curves were biphasic. The low fluence component was generally sigmoidal with an abrupt rise. The high fluence component failed to reach saturation for the fluences tested (less than 70 μmol m⁻² s⁻¹). Using the inferred threshold fluences of these two components as criterion effects, we obtained two action spectra. For the low fluence component, the action spectrum showed major peaks at 394, 450, and 530 nm and a minor peak at 416 nm. The high fluence component action spectrum showed very little sensitivity in the blue region. The major sensitivity was in the near UV, and a relatively small peak appeared in the green part of the spectrum at 507 nm. The biphasic character of the fluence-response curves suggests that two photosystems are responsible for the absorbance changes. The low fluence photosystem is sensitive mainly to blue and UV light and may thus represent a physiological blue-light photoreceptor. The high fluence photosystem is clearly not of this type. It (and perhaps the low fluence system as well) may mediate some of the subsidiary physiological effects of green light.     

FLUOROMETRIC EVIDENCE FOR FLAVINS IN ISOLATED EYESPOTS OF EUGLENA GRACILIS VAR. BACILLARIS

Abstract— Fluorometric evidence suggesting the presence of flavins in isolated eyespots of Euglena gracilis var. bacillaris is reported for the first time. Fluorescence spectra of eyespots and flavin standards show maxima at 540nm and 530nm, respectively. Excitation spectra show matching major peaks at 360–370 nm and at 450nm. The addition of riboflavin standard to eyespot samples increases fluorescence intensity without major corresponding shifts in wavelength maxima. Photolysis of eyespot samples in the presence of EDTA effects a decrease in the fluorescence intensity; the fluorescence is quantitatively restored to its initial value by bubbling the photolyzed solution with air. Preliminary quantitative data, obtained by fluorescence measurements, indicate the presence of ca. 5 × 10^-4μg flavin/ml eyespot sample. While flavins have been hypothesized to be components of the photoreceptor system, they have been reported previously only in the paraflagellar bodies of intact cells. Emission and excitation data obtained by us for eyespots are similar to those previously reported by other investigators for paraflagellar bodies, but our studies now suggest the presence of flavins also in Euglena eyespots.