Environmental factors controlling the time of flower-opening in Pharbitis nil

Pharbitis nil, strain Violet, subjected to various photoperiods(24-hr cycle at 24?C) bloomed about 10 hr after light-off whenthe light period was 10 hr or longer, and about 20 hr afterlight-on when the light period was shorter. The higher the temperature(20–30?C) during the dark period, the later the time offlower-opening, with the temperature during the last half ofthe dark period having a stronger effect than that during thefirst half. In continuous dark or light, flower buds of Pharbitis openedabout every 24 hr at all temperatures tested between 20 and28?C, which suggests the participation of a circadian rhythmin determining the time of flower-opening. A light pulse given6–12 or 28–36 hr after the onset of the dark periodgreatly advanced the phase of this rhythm (8–10 hr). Phasedelay of this rhythm could not be obtained by light pulses givenat any time. (Received September 29, 1979; )     

Promotion of sink activity of developing rose shoots by light

Holding young rose shoots (Rosa hybrida cv. Marimba) in darkness while the rest of the plant was in light reduced the amount of ¹⁴C assimilates recovered from the darkened shoot by half. Relative specific activity of the shoot tip grown in light was 13.5 times greater than that of the darkened one. The flower bud at the shoot tip degenerated in darkness and died. Shoots 2 to 3 centimeters long, after flower initiation, were most sensitive to the dark treatment. The degeneration is a gradual and reversible process in the first 8 days of darkness, followed by irreversible damage and atrophy. Darkening enhanced the ability of the young leaves to compete for the available assimilates over that of the darkened shoot tip. The enhancement of the mobilizing ability of the shoot tip by light is independent of photosynthesis since spraying with 3-(3,4-dichlorophenyl)-1,1-dimethylurea or holding shoots in a CO₂-free atmosphere did not diminish the promoting effect of light on flower bud development or assimilate import. The possibility that light exerts its effect by photoproduction of ATP was also excluded inasmuch as no differences were found in ATP levels of shoot tips held in darkness and those held in light.     

The action of skeleton photoperiods on flowering in Lemna perpusilla

The effects of 24 hr cycle skeleton photoperiodic schedulesinvolving two short light pulses on flowering in Lemna perpusillahave been studied. Simulation of complete photoperiods by correspondingskeletal ones is nearly perfect for all photoperiods up to 8hr and is unstable for periods of 9 to 13 hr. A jump in theresponse phase appears when skeleton photoperiods ranging from12 to 13hr are given. For all skeleton photoperiods longer than14 hr the phase is entrained so that it agrees with that givenby skeleton photoperiods of complemental lengths. That is, askeleton photoperiod of 18 hr is equivalent to that of 6 (=24–18) hr. Simulation is largely related to whether thesecond pulse is locked on to "dawn" or to "sunset" dependingon when it falls during the dark period following the firstpulse. The inductive action of skeleton photoperiods that gives unstableentrainment depends on the length of a preliminary dark periodgiven before the plant receives the first pulse, since in theseskeleton schedules the sensitive zone to the second pulse shiftswith the length of the preliminary darkness. Thus, we tentatively conclude that the circadian oscillationin L. perpusilla involves an entrainment mechanism and thatphotoperiodic induction is contingent on the coincidence oflight and a specific inductive phase in oscillation. (Received September 18, 1968; )     

Diurnal change of light-dependent uridine incorporation into RNA in a long-day duckweed, Lemna gibba G3

Light-dependent incorporation during subjective day and nightof radioactive uridine into RNA of a long-day duckweed, Lemmagibba G3, was examined. When the dark treatment was startedfrom the subjective night phase, the activity of uridine incorporationdropped approximately by half only after the very subjectivenight phase had passed or with the commencement of the subsequentsubjective day phase. However, when the dark treatment was startedfrom the subjective day phase, the incorporating activity promptlybegan to decrease and the inhibition increased with the lengthof the dark period until a final steady level (also at ca. 50%of the initial level) was reached after 24 hr of darkness. Thesetwo phases of different light sensitivities recurred daily undercontrol of the physiological clock and the rhythm was resetby a light-on signal. The lowered incorporating activity dueto the darkened day phase was recovered completely by a 12-hror even 15-min white light period perturbing the succeedingnight phase. That the incorporation of uridine in every RNAspecies, especially in chloroplast ribosomal RNA, was loweredby dark treatment of the day and night phases, was disclosedby MAK column chromatography and acrylamide gel electrophoresis. (Received August 21, 1974; )     

Control of the Entry into S Phase by Phytochrome and Blue Light Receptor in the First Cell Cycle of Fern Spores

Phytochrome- and a blue light receptor-dependent pathway antagonisticallyregulate the first mitosis in spores of the fern Adiantum capillus-venerisL. This study focused on determining which phase(s) of the cellcycle is positively regulated by phytochrome and negativelyregulated by a blue light receptor in germinating spores. Incorporationof the radioactivity of ³H-thymidine into the acid-insolublematerial prepared from the spores indicated that phytochromein the PFR form induced the entry into S phase of the firstcell cycle in the spores 20-28 h after irradiation with redlight. Blue light treatment before or after red light treatmenttotally prevented the P_FR-induced DNA synthesis. Brief irradiationwith red, far-red or blue light showed no effects on mitosisif the irradiation was given 28 h after the red light induction,during S and M phases. These results indicate that phytochromeand a blue light receptor regulate the entry into S phase duringthe first cell cycle of fern spores. ( Accepted July 10, 1997)     

Photoperiodic requirements for flowering of the long-day duckweed, Lemna gibba G3

The min-LD estimation by the log. flower number vs. the cultureperiod curve provides a unique method of judging whether a givenphotoperiodic schedule is a long day or not for Lemna gibbaG3. Duckweeds in M-sucrose medium are exposed to the test scheduleat 26°C on either the first or second day of a continuouslight culture. If the min-LD (48 hr for control cultures) isnot changed, the inserted schedule is considered to have functionedas a long day. If, however, the min-LD is extended by 24 hr,the inserted schedule is judged to have functioned as a shortday. Examinations using this method of orderly designed light-darkschedules disclosed two critical phases in the light requirement;the initial and terminal 1 hr portions (designated the L1- andL2-phases) of the subjective day. Thus, a given day became along or short day when both the L1- and L2-phases were illuminatedor when either or both of the two phases were darkened. Thecritical daylength (11.5 hr) was just long enough to cover boththe L1- and L2-phases and the inductive phase (L2-phase) waslocated at the end of the subjective day. (Received June 9, 1975; )     

THE RHYTHMICAL CHANGE IN SENSITIVITY OF A LONG-DAY DUCKWEED, LEMNA GIBBA G3, TO DARK-BREAK

1. Effect of varied lengths of darkness given before continuousillumination, and that of dark-break of continuous light asa function of the time of its application, on the flower formationin a long-day duckweed, Lemna gibba G3, were studied. The results obtained suggested a rhythmic change in sensitivityto darkness, i.e., a cycle of 36 hr-period consisting of 12hr of sensitivity and the following 24 hr of insensitivity.The inhibition by darkness (12–36 hr) given before thestart of, or by dark-break (12, 24 hr) inserted in, the inductionperiod involved an extension of the induction period, but nota slow-down of the rate of flower formation. The dark-breakgiven after the induction period, however, suppressed the rateof flower production in proportion to the length of the darkness. 2. The inhibition of flowering by darkness given in the darksensitivephase was cancelled by a relatively brief light period insertedin the darkness. 3. Relation between the rhythm and the length of induction periodwas discussed. (Received August 13, 1965; )     

Floral Inhibition of Biloxi Soybean During a 72-hour Cycle

The inhibitory effect of light interruptions given during the photophobe phases of a 72-hour cycle was studied with Biloxi soybean [Glycine max (L.) Merr.]. The basic 72-hour cycle consisted of 8 hours of light followed by 64 hours of darkness and was repeated 7 times. Supplementary white light treatments given at the twenty-fourth and/or forty-eighth hour of the cycle (photophil phases) promoted the flowering levels of the controls and kept light treatments given at the most inhibitory points from inhibiting flowering completely. Such supplementary light treatments did not affect the time of maximum sensitivity to light interruptions. When 30-minute light breaks were used, maximum inhibition occurred at the 16-, 43-, and 63-hour points. The duration of the light breaks affected the time of maximum inhibition when given during the second photophobe phase. The time of maximum inhibition occurred earlier with 4-hour light breaks than with either 3-minute or 2-hour light interruptions.

Three-minute red light interruptions produced essentially the same effect as 3-minute white light interruptions. Such treatments inhibited flowering completely in the first photophobe phase, inhibited flowering to only a small degree in the second photophobe phase, and inhibited flowering to an intermediate degree in the third photophobe phase. Far-red light interruptions strongly inhibited flowering in the first photophobe phase, especially when given early in the dark period. Three minutes of supplementary white light given at the twenty-fourth or forty-eighth hour of the cycle partially overcame the inhibitory effect of far-red light. Four hours of supplementary white light at these times completely overcame the far-red inhibition.

     

Effects of indoleacetic, p-chlorophenoxyisobutyric and 2,4,6-trichlorophenoxyacetic acids on three phases of rooting in Azukia cuttings

In adventitious root formation of disbudded epicotyl cuttingstaken from light-grown, 5-day-old Azukia angularis seedlings,indoleacetic acid (IAA), 1 x 10^–4 M, applied during thefirst day showed no effect, but enhanced the effect of IAA,1 x 10^–4 M, applied during the second day. Treatment duringthe second day promoted rooting by about 70%, and a combinationof treatments for the first and second days promoted rootingsome 200%. p-Chlorophenoxyisobutyric acid (PCIB), 3 x 10^–4M, and2,4,6-trichlorophenoxyacetic acid (2,4,6-T), 2 x 10^–44M, applied the first day also enhanced the effect of IAA, 2x 10^–4 M, applied the second day. When applied the second day, PCIB, 2 x 10^–4M, increasedthe number of root primordia or clusters of small cells, butnot die number of protruded roots. Formation of the cell clusterwas inhibited by 2,4,6-T, 3 x 10^–4M, applied the secondday. Rooting processes in Azukia cuttings seem to include at leastthree phases: the first phase is induced not only by IAA butalso by PCIB or 2,4,6-T, the second phase is induced by IAAor PCIB and the diird phase depends specifically on IAA. (Received October 28, 1970; )     

Inhibition of Flower Induction by Some Inhibitors of Protease in the Short-day Plant Lemna paucicostata 6746 and the Long-day Plant Lemna gibba G3

Four inhibitors of proteases, namely, bestatin, diisopropylfluorophosphate, elastatinal and p-toluenesulfonyl-L-lysinechloromethyl ketone hydrochloride, were examined for their effectson flowering of a short-day plant Lemna paucicostata 6746 anda long-day plant Lemna gibba G3. Each of the inhibitors greatlyinhibited the flowering of Lemna paucicostata 6746 that is normallyinduced by nitrogen deficiency. Bestatin or elastatinal givenonly during the first half of the culture period inhibited theflowering more clearly than when each was given during the latterhalf, suggesting that they inhibited the inductive process(es)involved in flowering rather than development of flower buds.Bestatin or elastatinal greatly inhibited the flowering of Lemnapaucicostata 6746 induced by photoperiodic stimulus, ferricyanideand continuous far-red light. Simultaneous application of thesetwo inhibitors was more effective in the inhibition of photoperiodicallyinduced and ferricyanide-induced flowering than was each inhibitoralone. They also completely inhibited the photoperiodic floweringof Lemna gibba G3. These results suggest that the inductionor activation of some proteases, probably followed by the degradationof some protein(s), is necessary for the induction of floweringin both these plants. (Received November 21, 1989; Accepted February 19, 1990)     

Collagen gel overlay induces two phases of apoptosis in MDCK cells

We previously demonstrated that collagen gel overlayinduced cell remodeling to form lumen and apoptosis inMadin-Darby canine kidney cells. In the present study, we establishedthat collagen gel overlay-induced apoptosis was initiated atareas exclusive of cell remodeling within 24 h (first phase) andextended into areas of cell remodeling within 48 h (second phase).Collagen gel overlay-induced apoptosis was accompanied byselective proteolysis of focal adhesion kinase (FAK), talin,p130^cas, and c-src. Upon collagen geloverlay, FAK was initially degraded into a 90-kDa product during thefirst phase and subsequently into a 80-kDa product during the secondphase. Collagen gel overlay-induced apoptosis of focal adhesioncomplex proteins and apoptosis of the first phase could beblocked only by a protease inhibitor cocktail. In addition, we foundthat both DEVD-fmk and ZVAD-fmk inhibited secondary proteolysis of FAK,but only ZVAD-fmk blocked collagen gel overlay-inducedapoptosis of the second phase. Finally, collagen geloverlay-induced apoptosis and proteolysis of focal adhesioncomplex proteins were completely inhibited by the combination ofprotease inhibitor cocktail and ZVAD-fmk. Taken together, collagen geloverlay induces two phases of apoptosis; the first phase is dependent on proteolysis of focal adhesion complex proteins, and thesecond phase on activation of caspases.

     

HYPERSENSITIVITY OF MELATONIN SUPPRESSION IN RESPONSE TO LIGHT IN PATIENTS WITH DELAYED SLEEP PHASE SYNDROME*

Patients with delayed sleep phase syndrome (DSPS) experiencea chronic mismatch between the usual daily schedule required by the individual'senvironment and their circadian sleep-wake pattern, resulting in major academic,work, and social problems. Although functional abnormalities of the circadianpacemaker system have been reported in patients with DSPS, the etiology ofDSPS has not been fully elucidated. One hypothesis proposed to explain whypatients with DSPS fail to synchronize their 24h sleep-wake cycle to theirenvironment is that they might have reduced sensitivity to environmental timecues, most notably light-dark cycles. Therefore, we compared the sensitivityof melatonin suppression in response to light in patients with DSPS and normalcontrol subjects. Fifteen patients with DSPS and age- and sex-matched healthycontrols were studied. As the melatonin secretion rhythm in patients withDSPS was expected to be delayed compared to the controls, the time of peakmelatonin secretion was determined in each subject in the first session. Inthe second session, each subject was exposed to light with an intensity of1000 lux for 2h beginning 2h prior to his or her peak melatonin secretion.Melatonin was measured by radioimmunoassay in saliva sampled every 30 minutesduring the period of light exposure. Suppression of the melatonin concentrationin saliva was dependent on duration of light exposure. In addition, the suppressiveeffect of light on the melatonin concentration was significantly greater inpatients with DSPS than in control subjects. The results suggest hypersensitivityto nighttime light exposure in patients with this syndrome. Our findings thereforesuggest that evening light restriction is important for preventing patientswith DSPS from developing a sleep phase delay. (ChronobiologyInternational, 18(2), 263–271, 2001)     

Measurement of the Critical Nyctoperiod by Lemna paucicostata 6746 Grown in Continuous Light

The short-day duckweed Lemna paucicostata 6746 could be inducedto flower in two days at 26C when continuous illumination forentrainment was followed by continuous darkness. This 48-h darkperiod or the minimum darkness requirement for floral inductionwas called the induction period. The length of the inductionperiod (IP) was routinely computed as the number of 24-h cyclesusing the equation of regression of flower number in logarithmon culture time. A light pulse given about 7 h after the startof the induction period increased the apparent IP value fromtwo to three, suggesting that the interrupted first day hadfunctioned as a noninductive day. A pulse given at any otherpart of the induction period did not modify the IP value. Thelight-sensitive part is probably the inducible phase, and thefirst 7-h period of darkness terminated by it seems to be thecritical nyctoperiod. These and relevant facts suggest thatthe light-off oscillator measures the critical night length,7 h. Either red or far-red irradiation at the inducible phase extendedthe IP value by one. No red/far-red photoreversibility was detected.As expected, however, red or far-red irradiation of any otherpart of the critical nyctoperiod could not modify the IP value. (Received February 8, 1985; Accepted May 14, 1985)     

Studies in Stomatal Behaviour: III. THE SENSITIVITY OF STOMATA TO MECHANICAL SHOCK

If Pelargonium stomata, wide open under a porometer-cup, aresubjected to a mechanical shock and then darkened, subsequentclosure is markedly accelerated. The effect persists for atleast 18 hours and, provided a relatively lengthy dark periodquickly follows the shock, is unaffected by subsequent lightperiods. If, however, the shock is followed by a light periodof about 2 hours, subsequent closure is decelerated, and thisdeceleration similarly persists through subsequent dark periods.The effects can largely be explained on the basis of shock-inducedrespiratory changes, if it is postulated that photosynthesisinhibits respiration in chlorophyllous tissue. The effect ofthe shock is not instantaneous, the new pattern of behaviournot being discernible in either case until the stimulated tissuehas been exposed to light or darkness for perhaps an hour. Itappears that in occasional sensitive leaves such phenomena maybe induced by the slight shock involved in fitting a porometer-cup,and the conditions of light or darkness to which the cup issubjected immediately after fixing may then influence its subsequentbehaviour.     

Heart-Shaped Prothallia of the Fern Adiantum capillus-veneris L. Develop in the Polarization Plane of White Light

When red light-precultured filamentous protonemata of Adiantumcapillus-veneris were cultured under linearly polarized whitelight, heart-shaped prothallia developed in the plane parallelto the vibration plane of electrical vector of polarized light,and were directed toward the light source. When the polarizationplane was rotated during the culture, the prothallial wingstwisted correspondingly to develop in the new plane. Continualobservation of the early steps of prothallial development witha time-lapse video system revealed that the apical cell of protonemaafter the first transverse cell division became flattened inthe vibration plane of electrical vector of polarized light,and that the first longitudinal cell division, that is, thefirst step in the transition from one-dimensional to two-dimensionalgrowth, as well as the subsequent cell divisions, occurred perpendicularlyto the electrical vector. (Received February 20, 1986; Accepted May 7, 1986)     

An Endogenous Rhythm in the Rate of Carbon Dioxide Output of Bryophyllum: I. SOME PRELIMINARY EXPERIMENTS

A techinique is described for recording automatically, withthe aid of an infrared gas analyzer, the rate CO₂ output orabsorption by plant material under controlled conditions. An examination of the rate of CO₂ output by excised leaves of16 species of succulent plants in darkness and in a CO_-2-freeatmosphere revealed clearly defined rhythms in only Bryophyllumfedtschenkoi, B. daigremontianum and B. calycinum (pinnatum). Further investigation of the rhythm in leaves of B. fedtschenkoirevealed that: (1) daylength has no effect upon the period ofthe rhythm in subsequent darkness, the phase being set at thetime the lights are extinguished; (2) normal air suppressesthe rhythm; (3) removel of the epidermis and cutting the mesophyllinto pieces 1 cm² does not effect either the phase or periodof the rhythm; (4) continuous illumination at an intensity of3,000 lux inhibits the rhythm which restarts when the lightsare extinguished. The phase of the rhythm can be set at anytime of day according to the time at which the lights are extinguished.The time which elapses between the onset of darkness and thefirst peak decreases as the length of the light treatment isincreased. The endogenuous nature of the rhythm is fully established. Theresults are compared with of other researches.     

Light-induced formation of fruit-bodies in a basidiomycete, Favolus arcularius (FR.) AMES

fruit-bodies in Favolus arcularius. The effect of light lastedfor about one day after transfer to darkness. The mycelium became sensitive to light about 2.5 days afterinoculation; i.e., at the beginning of the rapid growth phase.The site of fruiting was 2–5 mm inside the edge of colony(actively dividing zone) at the start of illumination. Whenone half of the plate culture was illuminated, fruiting wasrestricted to the illuminated half of the colony ; i.e., theeffect of light was localized. These results suggest that thecells sensitive to light are the actively dividing cells. Under a fixed light intensity, the total irradiation time requiredfor the initiation of fruiting was nearly constant, irrespectiveof the durations of pre-incubation in darkness and the dailyillumination period. With increasing light intensities, up toabout 500 lux, fruiting was promoted, however, a further increasein light intensity was inhibitory. (Received March 27, 1968; )     

Removal by chemicals of photoperiodic light requirements of Lemna gibba G3

Both the initial and the terminal 1 hr portions of the subjectiveday fraction, namely the L1- arid L2-phases, of a 24 hr daymust be illuminated in order for the day to be perceived asa long day in the min-LD determination by the long-day plant,Lemna gibba G3 (9). The light requirement of the L1-phase wassatisfied by a 10 min red light pulse given at the beginningof the phase. The red light effect was erased by a subsequent10 min far-red light, indicating phytochrome-mediated processesoccurring in the L1-phase. The light requirement of the L2-phasewas satisfied by blue or far-red light given during the terminal10 min period of the phase; there was no indication of phytochromeinvolvement. The light action on the L1-phase was replaced by10^–5 M of cyclic AMP or 10^–7 M of DL-isoproterenol.The isoproterenol action was antagonized by 10^–7 M ofDL-propranolol. Cyclic AMP (10^–5 M) combined with salicylicacid (10^–6 M), which can remove the light requirementof the L2-phase (10), rendered a completely dark day physiologicallyequivalent to a long day. Acetylcholine (10^–5 M) exertednyctomimetic action on the L1-phase of the second light day.The action of acetylcholine was antagonized by cyclic AMP (10^–5M). The L2-phase required no light in the presence of 10^–7M of DL-propranolol, and this propranolol action was not affectedby isoproterenol. These findings suggest changes in membranepermeability caused by the light given during the L1- and L2-phases. (Received July 7, 1976; )     

LIGHT- AND DARK-GROWTH IN LONG-DAY DUCKWEED, LEMNA GIBBA G3, AS AFFECTED BY KINETIN

Under short-day conditions the growth or the production of fronds in Lemna gibba G3 was stimulated by KIN (10^–5 M);the longer the nyctoperiod, the greater the stimulation was.Under long-day conditions KIN was slightly inhibitory for thefirst 2 days, but promotive thereafter. IAA (10^–5 M) reversedthe growth inhibition by KIN in long-days, and DCA (10^–4to 10^–6 M) and also CA (10^–4 to 10^–6 M), althoughless effectively, cancelled the growth promotion by KIN in short-days.DCA (10^–5 M) little altered the KIN inhibition in thefirst 2 days of light culture, nevertheless it alleviated strikinglythe KIN promotion in the subsequent illuminated days. These and relevant findings explained the above-described promotionand inhibition by KIN of the duckweed growth in terms of invivo level of a cofactor (probably auxin) which may be underthe regulative influence of photoperiodic conditions given.Moreover, some bearing of the above conclusion on floweringmechanism in this long-day duck-weed was suggested. (Received September 12, 1966; )     

Floral initiation in strawberry: Spectral evidence for the regulation of flowering by long-day inhibition

Summary Floral initiation in strawberry cv. Cambridge Favourite, a facultative short-day plant, was inhibited by a daylength extension with red light (R) during the second half of a 16-hour night but not during the first half, and by far-red light (FR) in the first half but not during the second. Mixed R plus FR light was inhibitory to flowering at both times. This change in sensitivity to R and FR light in the evening and morning resembles the pattern for flower induction in long-day plants but differs from the pattern for flower inhibition in several other short-day plants, examples of which are given. These experiments afford further support for the hypothesis that the control of flower initiation in strawberry depends on the production of a flower inhibitor by leaves exposed to long photoperiods.Abbreviations R red - FR far-red - SD short day - LD long day - SDP short-day plant - LDP long-day plant