Effects of Calmodulin Inhibitors and Blue Light on Rhythmic Movement of Robinia pseudoacacia Leaflets

Abstract— The effect of several calmodulin (CAM) antagonists, blue light and an intracellular calcium inhibitor, on the circadian rhythm of Robinia pseudoacacia leaflet movement has been studied. The CAM antagonists, chlorpromazine (CPZ), trifluoperazine (TFP), calmidazolium and N -(6-aminohexyI)-5-chloro-1-naphthalenesulfonamide (W₇) shifted the phase of the circadian rhythmic movement while W₅, an inactive analogue of W₇, had no effect. Two hour pulses of calmidazolium (10–50 μ M ) gave rise to a phase-response curve with maximum advances (up to 9 h) at circadian time (CT) 6 and maximum delays (up to 7 h) at CT 22. No effect was found on transition from subjective day to subjective night and vice versa. The TFP (10–50 μ M ), applied as 2 h pulses during the circadian cycle, shifted the phase of the circadian leaflet movement and also produced maximum advances in the middle of subjective day. Two hour blue light pulses shifted the phase of leaflet rhythmic movement. The phase-response curve obtained showed maximum advances (up to 5 h) in the middle of subjective day and maximum delays on transition from subjective day to subjective night. Two hour pulses of 50 μ M 8-(diethylamino)octyl 3,4,5-trimethoxybenzoate hypochloride (TMB-8), an intracellular calcium inhibitor, caused the same type of phase-response curve, with maximum advances and delays occurring at the same time as those produced by blue light. These results indicate that CAM might be involved in controlling the circadian oscillator that drives Robinia leaflet movement. The relationship between CAM and calcium with red and blue light is discussed.     

TEMPERATURE-SENSITIVITY OF LIGHT-INDUCED PHASE SHIFTING OF THE CIRCADIAN CLOCK OF NEUROSPORA

Two new mutants of Neurospora craasa , designated hth-1 and hth-2 , have been isolated which allow clear expression of the circadian conidiation rhythm at high temperature (36°C). Both strains showed single-gene segregation and produced similar phenotypes but mapped to different genetic loci. These mutants allowed an analysis of the effect of temperature on (1) light-induced phase-shifting of the circadian rhythm, (2) period length of rhythm, and (3) growth rate. The amplitude of the phase response curve to light was drastically reduced as the temperature was increased from 25°C to 34°C. Phase advances were decreased more than phase delays. As previously reported (Sargent et al. , 1966), the period length of the rhythm is temperature-compensated below 30°C ( Q ₁₀˜ 1) but not well-compensated above 30°C ( Q ₁₀ 1.3–1.7). The decrease in amplitude of the light phase response curve occurred in both temperature ranges. Furthermore, the Q ₁₀ value was lowered by addition of yeast extract in the high temperature range but not in the low range. Q ₁₀ values for growth rate also differed in these strains both in the low temperature range (25–30°C) and the high temperature range (30–34°C).     

CIRCADIAN PHASE OF SPARROWS: CONTROL BY LIGHT AND DARK

Abstract— Sparrows ( Passer domesticus ) are day-active birds which exhibit circadian rhythms of perch-hopping activity. The phases of sparrow's circadian rhythms were studied following single 4 h light pulses, single 4 h dark pulses, doublet treatments of light and dark pulses, and a 10 h light pulse.
The sparrows exhibited a phase response curve to 4 h light pulses with maximum phase advances (3.8 h) at CT20 and maximum phase delays(–1.3 h) at CT16. The sparrows also displayed a phase response curve to dark pulses with maximum phase advances (2.2 h) at CT16 and maximum phase delays at CTO(–0.7 h).
The remaining pulses were imposed during the subjective dark-time. The 10 h pulse beginning 1 h after lights-out produced a 2.2 h phase shift. The doublet of 2 h pulses that were the "skeleton" of the 10 h pulse produced a 2.5 h phase shift. The early 2 h pulse, applied by itself resulted in a -0.4 h delay; the late 2 h pulse applied singly produced a 3.1 h advance. When an early 3 h dark pulse was imposed together with a late light pulse, the phase was advanced 3.6 h; singly the pulses produced 1.8 h and 2.7 h advances.     

MULTIPLE ACTION OF FAR-RED LIGHT IN PHOTOPERIODIC INDUCTION and CIRCADIAN RHYTHMICITY

Abstract— It is generally accepted that phytochrome influences the photoperiodic induction of flowering through its interaction with the circadian clock mechanism. We have attempted to separate the effects of phytochrome on the clock mechanism from those that mediate flowering directly by examining a number of responses that are unrelated to flowering but are also regulated by the circadian clock. Gas exchange measurements of both CO₂ and H₂0 vapor were monitored under light conditions (200 μmol m ² s⁻¹) where the addition of far-red energy is required for the maximal promotion of flowering. In addition, photosynthetic capacity and maximal transpiration rates were measured in plants grown under continuous dim (20 μmol m⁻² S⁻') light, with or without supplemental far-red, by exposing them briefly to saturating fluxes (1000 μmol m⁻² s^-l) of light. Net CO₂ fixation was very weakly rhythmic in plants grown under both high and low light and this weak oscillation was completely suppressed by far-red light. Far-red also suppressed the rhythm in transpiration under high light, but the rhythm was immediately reinstated when the far-red light was removed. The phase of this rhythm was also reset with the next peak always occurring15–18 h after the far-red was turned off. When grown under dim light, the transpiration rhythm was not suppressed and the amplitude of the oscillation was more than doubled. Far-red light appears to interact with the rhythm in transpiration in a manner suggesting that the stomatal rhythm may be coupled to the same clock oscillator that regulates the flowering rhythm.     

PHOTOPHYSIOLOGY OF TURION GERMINATION IN Spirodela polyrhiza (L.) SCHLEIDEN–V. DEMONSTRATION OF A CALCIUM-REQUIRING PHASE DURING PHYTOCHROME-MEDIATED GERMINATION

Abstract— Etiolated turions of Spirodela polyrhiza are positively photoblastic and show a phytochrome-mediated low fiuence germination response. The far-red light (FR) reversibility decreased with the delay of FR irradiation (lag phase 1.06 ± 0.03 days after red light irradiation; half-maximal response 1.9 days). The action of the far-red-absorbing form of phytochrome (Pfr) was only realized by a germination response if exogenously applied Ca²+ was present. Calcium step-down (from 1 mM to 0.9 μ M Ca²+) and Ca²+ step-up (from 0.9 μ M to 1 m M Ca²+) experiments were carried out to determine the Ca²+-sensitive phase. There was no time gap between the two phases determined by the step-down and step-up experiments but a clear coincidence of both curves. Pulse treatments (24 h) with Ca²+ (1 m M ) showed the upper part of this common curve to represent the most Ca²+-sensitive phase. The Ca²+-sensitive phase was within the Pfr-requiring phase. After reversion of Pfr by FR pulses there was only a negligible response to the high Ca²+-concentration, independent of the delay between the red light (R) and FR pulses. These results are compatible with the assumption of Ca²+ acting as a second messenger of Pfr. However, the Ca²+-insensitivity in the first 12 h after the R pulse points against this hypothesis.     

IN VIVO CHLOROPHYLL a FLUORESCENCE TRANSIENTS AND THE CIRCADIAN RHYTHM OF PHOTOSYNTHESIS IN GONYAULAX POLYEDRA

Abstract— The intensity of chlorophyll a fluorescence during the early part of fluorescence induction at O , initial fluorescence, and P, peak fluorescence, was higher during the day phase of the circadian cycle than during the night phase in continuous light (LL) conditions and was positively correlated with the rate of oxygen evolution. The circadian rhythm in fluorescence in LL persisted in the presence of 10μM 3–(3,4-dichlorophenyl)-1,1-dimethylurea (DCMU), which blocks electron flow from photo-system (PS) II in photosynthesis. The rhythmic changes in fluorescence intensity are consistent with a lower rate constant for radiationless transitions during the day phase than during the night phase of the circadian rhythmicity. The circadian changes in the intensity of fluorescence were abolished at 77K, which may indicate the importance of structural changes in membranes in circadian oscillations.     

A POSSIBLE CONTROL BY A PHYTOCHROME-LIKE PHOTORECEPTOR OF CHLOROPHYLL SYNTHESIS IN THE GREEN ALGA Ulva rigida

Chlorophyll synthesis is stimulated by red light pulses in the green alga Ulva rigida C. Aghard. Chlorophyll synthesis in darkness is greater after longer red light pulses (30 min) than after shorter red light pulses (5 min). Chlorophyll synthesis was higher after red light pulses of 14 Wm_-2 fluence rate than after those of 7 Wm_-2. The effect of red light showed some far-red reversibility. The reversion by far-red light was higher after red light pulses of 4 min than after those of 30 min. These results indicate the existence of a rapid induction of chlorophyll synthesis during the red light pulses and a fast escape from photoreversibility. The percentage of reversion is also affected by the fluence rate of the light pulses. The reversion was reduced by about 15% when the photon fluence rate was increased from 7 to 14 Wm_-2. Reversion was also observed when red and far-red light pulses were applied successively. Thus, phytochrome or a phytochrome-like photoreceptor could be involved in the induction of chlorophyll synthesis in Ulva rigida.     

BIOPHYSICAL AND BIOCHEMICAL ASPECTS OF PHENGODID (RAILROAD-WORM) BIOLUMINESCENCE

In studies of the bioluminescence of 11 species of phengodid collected in central and southeast Brazil, we have found that: (1) their lateral lanterns emit light in the yellow-green region (λ_max= 540–580 nm) and the head lantern color is shifted to the red region ( λ_max= 565–620 nm), (2) the luciferins of both types of lanterns are identical to that of lampyrids and elaterids and (3) the luciferase physicochemical properties are also similar to those of lampyrids and elaterids (optimum pH ca 8.1; K_m(ATP) = 260–370 μM , Kμ(luciferin) = 170–400 μM; molecular weight ca 60 kDa; apparent activation energy of in vitro bioluminescence ca 58 kJ/mol). Thus the bioluminescence system of phengodids appears to be essentially the same as that of lampyrids and elaterids. The different bioluminescence colors of the lanterns of Phrixothrix species (λ_head= 600–620 nm; λ_lateral= 535–565 nm) and other phengodid species are probably elicited by the presence of luciferase isoenzymes, as occurs in the case of elaterid prothoracic and abdominal lanterns.     

PHOTOREVERSIBLE Ca2+-DEPENDENT AGGREGATION OF PURIFIED PHYTOCHROME FROM ETIOLATED PEA AND RYE SEEDLINGS

The aggregation of phytochrome purified from etiolated pea ( Pisum satirum cv. Alaska) and rye ( Secale cereale cv. Cougar) tissues was investigated by centrifugation and turbidimetry. Purified pea phytochrome (A₆₆₉/A₂₈₀= 0.88), if irradiated with red light, became precipitable in the presence of CaCl₂. The precipitation upon red-light irradiation was optimal at a Ca^2- or Mg²⁺ concentration of 10–20 m M , was greater at increased phytochrome concentration or lower pH values, and was inhibited by 0.1 M KG. The precipitated phytochrome slowly became soluble after far-red light exposure.
Turbidity of pea phytochrome solutions after red-light irradiation also increased rapidly in the presence of either Ca²⁺ or Mg²⁺. Far-red light exposure after the red light cancelled the turbidity increase. Rye phytochrome showed less turbidity increase than pea phytochrome and occurred only in the presence of Ca²⁺. Partially degraded pea phytochrome produced by endogenous proteases in the extract did not show the turbidity increase. Undegraded pea phytochrome also associated with microsomal fractions under conditions similar to those described above, but the partially degraded phytochrome did not.     

FUNCTIONAL ROLE OF CALCIUM IN PHOTORECEPTOR CELLS

Abstract— Ca-uptake by disc membranes prepared from frog rod photoreceptor outer segments was examined. Ca-uptake study revealed two affinity sites which were saturated with 10–⁵ M and 10–³ M of ATP. When disc membranes in 20 m M Tris-HCl buffer (pH 7.5) were stored at -20°C for 6 h, more than 95% of Ca-uptake activity was lost. Ca-uptake activity was, however, preserved if the disc membrane suspension was mixed with 1–10m M ATP and stored at -20°C. Furthermore the reactivation of Ca-uptake was observed if disc membranes, which had lost Ca-uptake ability by storing at 4°C for 3 h, were mixed with 10 m M ATP and then frozen at -20°C for 5 h or 28 h (ATP-induced ATP-dependent Ca-uptake). When the contents of ATP bound to disc membranes were measured during a brief aging at 37°C, the decrement of bound ATP content was correlated well with the decreasing of Ca-uptake activity. Carbonylcyanide m -chlorophenylhydrazone (CCCP), a conductor of protons, inhibited Ca-uptake activity and half maximal inhibition was achieved at 2 × 10–⁸ M. When 10–⁶ M of CCCP was added to the ⁴⁵Ca-accumulated disc membranes, rapid release of ⁴⁵Ca from the disc membranes was observed. These results suggest that ATP may play a role in the Ca-pump regulation in disc membranes and a [H⁺] gradient across disc membrane may be linked to Ca-uptake mechanism.     

PHOTOMORPHOGENESIS IN Penicillium isariaeforme: EXOGENOUS CALCIUM SUBSTITUTES FOR LIGHT

Abstract— Penicillium isariaeforme is a photomorphogenic fungus which produces upright bundles of conidia-bearing mycelia (called coremia) when grown on a defined medium in visible (450–500 nm) light. We found that exogenous Ca²⁺ ions could substitute for light. In the dark 1–2 m M Ca²⁺ triggered coremia formation. Dark induction of coremia was specific for Ca²⁺ in that it could not be duplicated by 50 m M Ba²⁺, Fe²⁺, Mg²⁺, Mn²⁺, Sr²⁺, or Zn²⁺. Additionally, light-induced coremia formation was inhibited by both KI (2.5 m M ) and phenylacetic acid (0.25 m M ).     

CONTROL BY PHYTOCHROME OF EXTENSION GROWTH and POLAROTROPISM IN CHLORONEMATA OF Funaria hygrometrica

Abstract— The photocontrol of extension growth and polarotropism has been investigated in chloronemata of the moss Funaria hygrometrica Hedw. When grown on a 12/12 h light/dark cycle, chloronemata show light-stimulated diurnal variations in elongation rate with no evidence of a circadian rhythm. Regulation of elongation by a low energy, photoreversible phytochrome mechanism was demonstrated by brief red (R) and far red (FR) irradiations given either at the end of the day (EOD) or 6 h later as a night break (NB). Night break irradiation with polarised R caused polarotropic reorientations of chloronemal growth also through a FR-reversible, low energy phytochrome mechanism. Such transformations of P_r to P_fr were accompanied by a 90° shift in the orientation of the phytochrome chromophore. Microbeam irradiation indicated that the phytochrome chromophores involved in both responses were predominantly, if not entirely, located in the tip of the apical chloronemal cell.     

MODE OF COACTION OF PHYTOCHROME AND BLUE LIGHT PHOTORECEPTOR IN CONTROL OF HYPOCOTYL ELONGATION

Abstract The rate of hypocotyl longitudinal growth in seedlings of Sesamum indicum L. is strongly inhibited by continuous blue light (cBL)† and slightly by continuous far-red light while continuous red light (cRL) or red light pulses are hardly effective from 60 h after sowing onwards. Between 36 and 60 h after sowing the growth rate responds to red light pulses the effect of which is fully reversible by long wavelength far-red light. When seedlings are kept in cBL for 3 days and then treated with red light hypocotyl growth rate responds strongly. However, RL effectiveness decreases with time after transfer from BL to RL. BL → darkness transfer experiments with different levels of P_fr established at the beginning of darkness show that after a BL pretreatment phytochrome (P_fr) alone is capable of fully controlling growth rate. When white light (WL) is given no BL effect is detectable in weak WL. Only high light fluxes maintain a typical BL growth rate. At medium WL fluxes elongation rate returns gradually to the dark rate. The simplest explanation of the data is that light absorbed by a separate BL photoreceptor is necessary to maintain responsivity to P_fr. With increasing age of the seedlings the requirement for BL increases strongly. On the other hand, brief light pulses—given to demonstrate photoreversibility of phytochrome—remain equally effective provided that responsivity to P_fr exists.     

Pfr PHYTOCHROME AND SUCROSE REQUIREMENT FOR RHYTHMIC LEAFLET MOVEMENT IN ALBIZZIA

Abstract— Albizzia leaflets open and close with a circadian periodicity without damping during extended dark periods if supplied with sucrose and irradiated with red each rhythmic cycle. In the absence of a carbohydrate source, the rhythm damps irrespective of phytochrome status and the differential effects of red and far-red light treatments tend to disappear after 2 or 3 cycles. The rhythm also damps if leaflets are exposed to red only once, or if they are exposed to far-red once or cyclically. Sucrose does not prevent such damping but affects the stable angle assumed; the rhythm damps in the closed position in the presence of sucrose, and in the partially open position in its absence. Sucrose appears to have two distinct effects; it interacts with P _fr to promote manifestation of the rhythm and it reduces the average angle, whether the P _fr level is low or high.     

STIMULATION OF THE SHIBATA SHIFT BY PHOTOCHROME IN THE COTYLEDONS OF THE MUSTARD SEEDLING SINAPIS ALBA L.

Abstract— In the cotyledons of the mustard seedling Sinapis alba L. the duration of the Shibata shift can be greatly shortened by a pretreatment with light pulses prior to the protochlorophyllide– chloro-phyllide a photoconversion. It was shown that the light pulses act through photochrome (P _fr ). Since reversibility of a red light pulse induction by a far-red light pulse is rapidly lost (within 2 min) it is concluded that at least the initial action of P_fr occurs rapidly in this response. On the other hand, the effect of a red light pulse on the rate of protochlorophyll regeneration in the mustard seedling cotyledons is fully reversible by a far-red light pulse for more than 5 min. It is concluded that control of protochlorophyll regeneration and control of the Shibata shift by phytochrome cannot be consequences of the same initial action of P_fr Apparently P_fr controls both phenomena independently.     

PHYTOCHROME- and BLUE PIGMENT-MEDIATED LEAF MOVEMENTS: EXPERIMENTAL APPROACH IN THE SIGNAL TRANSDUCTION

Abstract— Leaflet movements of Cassia fasciculata are induced by transferring leaves from light to darkness or from darkness to light. Phytochrome mediates the dark-induced closure whereas a blue and far red light absorbing pigment (cryptochrome?) is the photoreceptor triggering the light-induced opening. These movements are the result of reversible turgor variation driven by ionic migrations (H+, K+, Cl^?) in cortical parenchyma cells of motor organs (“pulvini”) localized at the leaflet base. Calcium plays a predominant role in the regulation of the movements as shown by the inhibitory effects of chelators (EDTA, EGTA), intracellular antagonist TMB-8 and by the promoting effect of ionophore A 23187. Compounds known as calcium channel blockers (LaCl₃, verapamil and nifedipine) inhibited whereas Bay K 8644, a calcium channel activator, promoted the phytochrome-mediated movement. In contrast, all these calcium channel modulators had no effect on the blue pigment-mediated movement. From these results, it is suggested that calcium is not mobilized in the same manner in the two types of movements: possibly from external stores in the phytochrome-mediated response and from internal stores in the blue pigment-mediated response. Calcium acts possibly through calmodulin as suggested by a modification in the kinetics of the movements induced by inhibitors of calmodulin action (trifluoperazine, R 24571, W-7). The unexpected promotion of the movements by these inhibitors shows that calmodulin action on the ion migrations is not simple and direct. Experimental observations suggested that regulation might be done through cAMP metabolism. db-cAMP promoted the movements. Compounds known either to activate adenylate cyclase (prostaglandins, forskolin) or to inhibit phosphodiesterase (imidazolidinones, ICI 58301) induced the same modifications as db-cAMP. By contrast, a phosphodiesterase activator (imidazole) inhibited the movements.     

LASER PHOTOLYSIS OF 3-METHYLLUMIFLAVIN

Abstract— Using high-intensity actinic light, the chlorophyll a fluorescence transient from HCO^-₃-depleted chloroplasts shows a rapid initial rise (O → I) followed by a slow phase (I → P). In the presence of HCO^-₃, the O → I rise is delayed but the I → P phase is much more rapid. Using low-intensity actinic light, the chlorophyll a fluorescence transient from 3-(3,4-dichlorophenyl)-1,1 dimethylurea (DCMU)-treated chloroplasts is delayed in the presence of HCO^-₃. Bicarbonate increases the amount of delayed light emission from chloroplasts given 10 s illumination with weak blue light (0·4 W/m²). DCMU greatly increases the amount of delayed light seen in the presence of HCO^-₃ under these conditions but decreases the amount seen in the absence of HCO^-₃. It is suggested that HCO^-₃ may somehow form or stabilize, in the dark, a number of reaction centers corresponding to the S₁ state in the model of B. Forbush, B. Kok and M. McGloin ( Photochem. Photobiol. 14, 307–321, 1971).     

PHOTOREVERSIBLE CHANGES IN pH OF PEA PHYTOCHROME SOLUTIONS

Abstract— Photoinduced pH changes in unbuffered solutions of undegraded pea phytochrome were studied at 10_oC by using a glass electrode. Red light irradiation caused alkalinization of the solutions in the pH range 5.2–xs7.5 and acidification in pH 7.5–8.9. The pH changes were fully reversed by a subsequent irradiation with far-red light. The red and far-red light effects were repeatedly reversible. The solution of tryptic peptide of phytochrome (mol. wt 60000) showed similar photoreversible pH changes.     

SPECTRAL PROPERTIES,PHOTOTRANSFORMATION KINETICS AND PELLETABILITY OF PHYTOCHROME IN Pharbitis nil Chois*

Abstract— An examination has been made of the involvement of phytochrome in the circadian rhythm of flowering in Pharbitis nil Chois. The peak position of P_fr absorption changes with time after a red light pulse. The shortest absorption wavelength of P_fr occurs at the same time as flowering is inhibited by red light in dark grown, red light pretreated plants. Pelletable and supernatant phytochrome show a similar trend with lowest values found at the time of flower inhibition. Neither phototransformation kinetics nor intermediates of phytochrome which accumulate in white light show such a relationship to the circadian rhythm found in flowering of dark grown P. nil.     

PHOTODESTRUCTION OF BACTERIORHODOPSIN

Abstract— Suspensions of purple membrane fragments showed obvious signs of degradation after illumination with intense pulses of light from 10 ns frequency doubled Nd: YAG laser at 532 nm with intensity densities in excess of 1 MW/cm². Using controlled illumination, a small fraction of the bacteriorhodopsin protein molecules were randomly destroyed in samples with a low salt concentration (12.5 m M ) and pH = 7.9. Calculations using information from the changes in the optical absorbance spectrum and transient changes in the optical absorbance spectrum during the photocycle support a model where one protein molecule of the bacteriorhodopsin trimer is photodestroyed, the other two protein molecules switch to a blue state . In the blue state , the protein molecules have a red shifted absorption, with a peak near 600 nm. The blue state molecules show transient absorption changes at 656 nm that are similar to the native bacteriorhodopsin, except the O state is missing or altered. Additionally, the changes in curvature of the purple membrane fragments that occur during the photocycle of intact protein molecules are severely depressed. The addition of salts to the photodestroyed suspension can change the blue state molecules back to a state with an absorption maximum at 568 nm. The salt ions probably shield the other members of the trimer from the photodestroyed protein. In these reconstituted samples, the O state is observed at 656 nm; however, the membrane bending is not observed.