Effects of Photoperiod on Germination of Seeds of Talinum triangulare (Jacq.) Willd

Seed germination in Talinum triangulare as affected by photoperiod,with or without previous incubation in the dark in water at25 or 4 °C, was studied. The time course and quantity ofseed germination in photoperiods of 1 h and above were similarwith or without dark pretreatment, but the time to half maximumgermination was reduced from 12 days in non-dark pretreatedseeds to 4 days in seeds given 20 days in the dark at 25°C.A photoperiod of 0·25 h gave a lower rate and total germinationthan photoperiods of 1 h and above. Un-pretreated seeds required17 cycles of 24 h photoperiod for maximum germination as comparedwith 7 or less cycles if the seeds received more than 10 daysdark pretreatment at 25 °C. Both the rate and total germinationin light increased as the length of dark pretreatment at 25°C was increased from zero to 30 days. Incubation of theseeds in water in the dark at 4 °C for 5 to 30 days priorto illumination at 21 °C, reduced both the rate and quantityof seed germination in light as compared with those similarlyincubated in the dark at 25 °C. However, previous incubationin the dark for 30 days at 4 °C partially substituted forthe light requirement. The possible mechanism of breakage ofseed dormancy in Talinumis discussed in relation to these andother findings. Talinum triangulare (Jacq.), Willd, light, photoperiod, seed germination     

The Effects of {delta}-Aminolevulinic Acid and Inhibitors of RNA and Protein Synthesis on Phytochrome Mediated Chlorophyll Accumulation in Sorghum bicolor

In 5-d-old etiolated seedlings of Sorghum bicolor, 12 h of darknessafter 5 min in red light eliminated a lag before the accumulationof chlorophylls in subsequent continuous white light. Increasingthe dark period to 24 h and 36 h, increased the rate of chlorophyllaccumulation in the later stages of greening. Exogenous -aminolevulinicacid neither completely removed the lag, nor increased the rateof chlorophyll accumulation. Cycloheximide (25 µg ml^–1)and 6-methyl purine (5.0 µg ml^–1), given continuouslyor only until the 12 h dark period following the red light irradiation,restored the lag and decreased the rate of chlorophyll accumulation.D-threo-chloramphenicol (400µg ml^–1) also decreasedthe rate of chlorophyll accumulation but did not restore thelag. Addition of these inhibitors even 12 h after red lightirradiation decreased the rate of chlorophyll accumulation.Rifampicin (Rifamycin SV, 400 µg ml^–1) did not havesuch effects. Key words: Chlorophylls, Phytochrome, -Aminolevulinic acid, Sorghum bicolor     

H+ Transport across the Plasmalemma and Tonoplast of Nitellopsis obtusa during Excitation

Measurements of intra- and extracellular pH during the excitationof Nitellopsis obtusa were carried out with antimony microelectrodesat conditions of dark adaptation and of continuous illumination.The pH of the vacuolar sap of both dark-adapted and illuminatedcells increased during cell excitation by 0·1–0·15units. H⁺ ions which had entered the cytoplasm during excitationin dark-adapted cells were extruded back into the vacuole acrossthe tonoplast. After cell excitation in the light H⁺ ions wereextruded from the cytoplasm also into the external medium probablyacross the light-stimulated active H⁺-channels. Protoplasmicstreaming ceased during excitation in the dark for 1–3min, and during excitation in the light—for 5–20s.     

Determination of Nitrate Reductase Activity in Barley Leaves and Roots

The inactivation of nitrate reductase in the leaves and rootsof barley (Hordeum vulgare L. cv. Mazurka) during and afterextracting was investigated. At 0 °C in the absence of casein,25 per cent of ‘total’. i.e. maximal in vitro, nitratereductase activity was lost during the 2 min extraction process,followed by a slower loss of activity while the extract wasstored in ice. Activity was maintained by adding a minimum of1 per cent casein to the extraction medium containing 0·1M phosphate (pH 7·5), 1 mM EDTA and 1 mM dithiothreitol.Nitrate reductase was stable for several hours in these extracts,but declined in a first order manner in the absence of dithiothreitol.Casein also prevented the initial loss while making root extracts,but had less effect during storage. Using casein and thiols, nitrate reductase activity in light,(as product of maximal in vitro rates and wt g^–1) in leaveswas 98 per cent of the total activity in 31-day-old plants grownwith full nutrient in water culture and 60-day-old field-grownplants receiving no fertilizer. Field-grown plants, however,exhibited only 17 per cent of the activity of culture-grownplants. Nitrate reductase in leaves of barley plants grown in waterculture had a diurnal rhythm. During the first 3 h of the lightperiod, activity increased to 1·3 x the ‘dark’value. This was followed by a temporary decrease and then byanother increase to a maximum of 1·7 x the ‘dark’value, occurring about 8 h after illumination. Activity thendecreased during the rest of the light period and in darkness. Hordeum vulgare L., barley, nitrate reductase     

Androgenic Stimulating Factors in the Anther and Isolated Pollen Grain Culture of Datura innoxia Mill

Flower buds, anthers, and/or pollen grains collected at thetime of first haploid mitosis and 1–2 d before or afterthis division were submitted to different treatments beforeculturing anthers or isolated pollen grains. In the case ofanther culture, the percentages of androgenic anthem were notedat the end of 2, 3, 4, and 5 weeks of culture. Statistical studiesof the results thus obtained showed that some factors were highlyeffective in favouring androgenesis. The best results were obtained1–2 d after the first haploid mitosis with anther's centrifugedat 40 g for 5 min after cold treatment of the flower buds (48h at 3 °C); these treatments increased the percentage ofandrogenic pollen grains 12-fold. In case of isolated pollengrains, a system of culture particularly favourable for inductionand development of androgenic embryos was found. This systemincluded a cold treatment of the flower buds (48 h at 3 °C),the centrifugation of the isolated pollen grains (120 g for15 min), and culturing them for 20 d in the dark and then incontinuous light.     

Flowering in Pisum: the Effect of Genotype, Plant Age, Photoperiod, and Number of Inductive Cycles

The genotypes If e Sn hr, Lf e Sn hr, and If e Sn Hr requirefewer inductive cycles as they age. It is suggested that thisresults from a decrease in the activity of the Sn gene in theleaves as they age, resulting in a higher ratio of promoterto inhibitor. Gene Lf does not affect the rate of this agingbut it does increase the number of inductive cycles requiredfor flower induction over the first 5 weeks of growth. The geneHr has no effect until week 4 but thereafter causes a reductionin the effect of age on the Sn gene. The genotype If e Sn Hrcan be induced by a single inductive cycle (32 h of light) fora relatively long period. The length of dark period required for the expression of theSn gene is shown to be less than 4 h providing a relativelylong photoperiod precedes the dark period. It appears that noper manent induction of tissue by photoperiods favourable toflowering occurs in peas. The critical photoperiod for plantsof genotype if e Sn Hr is shown to be between 12 and 14 h atl7·5 °C and the usefulness of the term ‘criticalphotoperiod’ is discussed with respect to quantitativelong-day plants.     

Geotropic Responses and Pod Development in Gynophore Explants of Peanut (Arachis hypogaea L.) Cultured In Vitro

Peanut gynophore explants cultured in vitro on a defined mediumshow a positive geotropic response in both light and dark whenplanted either horizontally, or vertically with the tip pointingupwards. The growth following the initial curvature dependedon age of the gynophores and on the levels of growth substancesin the medium. In the dark and in presence of 0·01–0·1p.p.m. kinetin, naphthalene acetic acid at concentrations of0·1 p.p.m. and lower promoted gynophore elongation. Athigher concentrations elongation was promoted to a lesser extentin younger explants, caused enlargement of the ovary and formationof pods. Young explants generally elongated more than olderones and pod formation took place inside the medium, while inolder ones it took place above the medium. In the light, theinitial positive geotropic response was followed by elongationbut without any enlargement of the ovary. Decapitation of gynophores1·5–2·0 mm below their tip, removing theovary but leaving most of the intercalary meristem, had no effecton the geotropic response and elongation. The initial geotropicresponse and elongations of explants in vitro was not dependenton the presence of the ovary but on the meristem proximal toit. Changes in growth substances balance during gynophore developmentseem to affect geotropic response, elongation and pod formationin the peanut.     

Spectral Dependence of Night-break Effect on Photoperiodic Floral Induction in Lemna paucicostata 441

A single dark period of longer than 8 hr induced flowering inLemna paucicostata 441 cultured in E medium. Monochromatic lightsof 450, 550, 650 and 750 nm with a half-power bandwidth of 9nm given for 10 min at the 8th hour of a 14-hr dark period inhibitedflowering. The fluence rates required for 50% inhibition were10, 0.5, 0.1 and 3 µmol m^–2. sec^–1, respectively.When applied between the 4th and the 10th hour of the dark period,lights of 450, 550 and 650 nm were inhibitory showing a maximumeffect at the 8th hour. But 750-nm light completely inhibitedflowering when applied at any time during the first 8 hr ofthe dark period. The inhibitory effect of 750-nm light givenat the beginning of the dark period was totally reversed bya subsequent exposure to 650-nm light, and the fluence-responsecurves for the effect of 750-nm light given at the 0, 4th and8th hour were essentially the same. This suggests that the presenceof P_FR is crucial for the floral initiation throughout the first8 hr of the inductive dark period. The role of phytochrome inthe photoperiodic flower induction of L. paucicostata is discussed. (Received January 4, 1982; Accepted March 19, 1982)     

A Comparative Study of Germination Responses to High Irradiance Light

Seeds of 19 native British herbaceous species (14 grasses andfive forbs) were exposed to white light at three photon fluencerates: high (19–2 mol m^–2 d^–1), medium (9·6mol m^–1 d^–1) and low (2·3 mol m^–2 d^–2) These photon doses have been found by previous workers to inhibitgermination in several species. High and low photon doses wereapplied only as continuous light, but the medium dose was appliedas both continuous light and as a 12 h light/12 h dark photoperiod.All four treatments, plus a dark control, were carried out at15 °C; the high and low doses were also applied with a dailyalternation of 10/20 °C. The majority of species (15) fell into one of two groups. Inseven species germination was relatively high and consistentacross all treatments, including darkness; in the other eightspp germination was inhibited only in darkness. Mostly thesedata confirmed published results for the same species In contrast in Agrostis capillaris and A. stolonifera germinationwas high only at alternating temperatures, irrespective of photondose, but was also slightly promoted by a constant temperaturecombined with light/dark alternations. Only in Bromus sterilisand B. ereclus was germination inhibited by light, in B. erectusat all photon doses and in B. sterilis only at the highest photondose These results suggest that inhibition of germination by highirradiance light is not widespread among native British species Aira caryophyllea, Arrenatherum elatius, Festuca ovina, F. rubra, Hordeum murinum, Milhim effusum, Silene dioica, Achillea millefolium, Brachypodium syhaticum, Digitalis purpurea, Holcus lanatus, Leucanlhemum vulgare, Phleum pratense, Poa trivialis, Taraxacum officinale, Agrostis capillaris, A. stolonifera, Bromus erectus, B. sterilis, seed, dormancy, germination, light, High irradiance reaction, alternating temperatures, photoperiod     

Export, Mobilization, and Respiration of Assimilates in Uniculm Barley during Light and Darkness

The respiratory losses and the pattern of carbon supply froma leaf of unicuim barley were examined during a complete diurnalperiod using a steady state ¹⁴C-labelling technique. After a delay of c. 1 h a portion of the ¹⁴C exported from acontinuously assimilating leaf was lost in respiration in thelight. This respiratory loss amounted to c. 20% of the total¹⁴C fixed. A further 28% of the total ¹⁴C fixed was respiredduring the dark period. In the light, carbon was fixed at a rate of c. 8·9 mgC dm^{–2 h–1} and exported from the leaf at ^c. 5·3mg C dm^{–2 h–1}. Dark export averaged ^c. 31% of theday-time rate. Carbohydrate was stored in the leaf during the day and was almostcompletely remobilized during the dark. Sucrose, the major reservecarbohydrate, was exported first whilst the starch level remainedconstant. After some 9 h of darkness, sucrose declined to alow level and starch remobilization began.     

Transnodal Transport of 14C in Nitella flexilis: I. TANDEM CELLS WITHOUT APPLIED PRESSURE GRADIENTS

Using NaH¹⁴CO₃ (0·01-0·03 mol m^–3) fed to5·0 mm of Nitella flexilis in artificial pond water at22–25°C, we have found that uptake in 5 min or in1 h varies with the streaming rate of the fed cell and is reducedby anoxia over the uptake position. We have also found thatthe %¹⁴C transported across the node between two internodalcells in tandem is highly sensitive to the streaming rate ineach cell, to the physiological state of the cells (summer versuswinter), to the method of feeding (5 min versus 1 h) and tocovering the node, particularly with winter cells or summercells preconditioned for 3 h in the dark and run in the dark.Transnodal transport by plasmodesmata is sensitive to anoxiaand seems to be at least partly active. Key words: Node, plasmodesmata, anoxia, active transport, influx     

The Diurnal Pattern of Nitrate Uptake and Reduction by Spinach (Spinacia oleracea L.)

Spinach plants were grown in bowls of aerated nutrient solutionin a controlled environment chamber for 24 h, and harvestedevery 3·5-5 h to record their growth, nitrate and wateruptake, and plant nitrate concentration. Twelve such experimentsare described, either with a 14/10 h dark/light regime, or continuouslight or darkness. The irradiance was either 110, 320, or 510µmol m^-2 s^-1 (PPFD). All these regimes began at the endof the light period of a 14/10 h dark/light regime (510 µmolm^-2 s^-1) lasting approximately 2 weeks. Nitrate uptake rate per g of dry weight of plant continued almostunabated at about 17 µmol h^-1 through the initial 14-hdark period, and then fell away sharply if the light was notrestored, but increased slightly when it was. With continuouslight at 510 µmol m^-2 s^-1, uptake rate rose steadily forthe first 24 h of light, and then fell sharply for about 6 h.Shoot nitrate concentration increased about three-fold in thedark phase, and declined in the light at a rate which was positivelyrelated to the irradiance. Root nitrate concentration was severaltimes higher than that of the shoot: its diurnal change wassmaller (relative to the mean) than that of the shoot. Nitratereduction occurred to a small extent in the dark, and increasedrapidly as soon as the lights came on, to remain at a roughlyconstant rate (related to the irradiance) throughout the lightphase. Dry matter increase in the light was related to irradiance,but with little increase above 320 µmol m^-2 s^-1. Respiratoryweight loss in the dark was not detectable. Rate of fresh weightincrease was approximately constant throughout light and darkperiods. The results compare quite well with the predictions of a simplesimulation model, based on the pump/leak principle.Copyright1994, 1999 Academic Press Spinacia oleracea, nitrate, uptake, reduction, influx, efflux, diurnal, regulation, model, simulation     

Emission of Volatiles From Brown Boronia Flowers: Some Comparative Observations

Extensive research has focused on the concentration of aglyconeswithin brown boronia (Boronia megastigma) flowers, however emissionof volatiles into the headspace above these flowers is not welldocumented. Using solid-phase microextraction (SPME) to trapvolatiles and GCMS analysis, we observed 23 volatiles in theheadspace above buds and flowers throughout flower maturation,above dissected floral organs and above whole plants held for36 h under either continuous light, continuous dark or 12 hlight:12 h dark:12 h light treatments. Fully-opened flowersemitted the most complex mixture of volatiles and in the greatestquantity, with a rapid decline in senescent flowers. Caryophyllene,humulene and bicyclogermacrene declined as flower buds matured;ß-ionone increased. From the individual floral organs,emission from the petaline anthers comprised 38% of total emissionsfrom the (calculated) ‘whole flower’, with 27% contributedby the petals and 10.5% by the stigma. Monoterpenes dominatedthe headspace from the calyx; dodecyl acetate, methyl jasmonateand (Z)-n-heptadec-8-ene were relatively predominant in emissionsfrom the androecium. ß-Ionone, the major floral volatilein brown boronia, dominated volatiles emitted from the stigma(87%). However, the relatively tiny petaline anthers, activein pollen production and high in carotenoids, contributed thegreatest overall amount of ß-ionone to emission fromthe whole flower. There were three different patterns in emissionof volatiles from plants in response to different light conditions:(1) emission patterns identical irrespective of light environment,with maximum emission in the ‘endogenous’ dark period,i.e. when the plant would normally have been in the dark (-pinene);(2) similar emission in all treatments, with an increase anddecline over a period of 26 h (5-acetoxy linalool, cyclic ß-ionone,dodecyl acetate and (Z)-n-heptadec-8-ene); and (3) emissionin all treatments but enhanced in the dark, with a 27.5 h periodin some cases (cyclic ß-ionone endoperoxide, dihydroß-ionone, ß-ionone, and ‘total volatiles’).Preliminary evidence is presented for endogenous control ofemission of a number of volatiles such as -pinene, with perhapsdiurnal control of others such as ß-ionone. Copyright2000 Annals of Botany Company Boronia megastigma, brown boronia, SPME, headspace, floral volatiles, ß-ionone     

Theoretical Basis of Protocols for Seed Storage III. Optimum Moisture Contents for Pea Seeds Stored at Different Temperatures

In previous work, we demonstrated that there was an optimummoisture level for seed storage at a given temperature (Vertucciand Roos, 1990), and suggested, using thermodynamic considerations,that the optimum moisture content increased as the storage temperaturedecreased (Vertucci and Roos, 1993b). In this paper, we presentdata from a two year study of aging rates in pea (Pisum sativum)seeds supporting the hypothesis that the optimum moisture contentfor storage varies with temperature. Seed viability and vigourwere monitored during storage under dark or lighted conditionsat relative humidities between 1 and 90%, and temperatures between-5 and 65°C. The optimum moisture content varied from 0·015g H₂O g^-1 d.wt at 65°C to 0·101 g H₂O g^-1 d.wt at15°C under dark conditions and from 0·057 at 35°Cto 0·092 g H₂O g^-1 d.wt at -5°C under lighted conditions.Our results suggest that optimum moisture contents cannot beconsidered independently of temperature. This conclusion hasimportant implications for 'ultra-dry' and cryopreservationtechnologies.Copyright 1994, 1999 Academic Press Seed storage, seed aging, seed longevity, water content, temperature, glass, desiccation damage, ultradry, Pisum sativum L., pea, cryopreservation     

The Influence of Donor Plant Genotype and Environment on Production of Multicellular Microspores in Cultured Anthers of Brassica napus ssp. oleifera

Studies of the effects of genotype and pre-flowering environmentalconditions on the production of multicellular microspores wereundertaken th four highly inbred lines of Brassica napus sap.oleifera. These lines were first grown in shaded and unshadedenvironments at 20/15°C arid unshaded at 30/25°C ina daylight phytotron. Buds were harvested from half the plantswhen first visible in the rosette and later from the remainingplants at the time when the first flower opened. The frequencyof microspores at a specific stage of development varied widelywithin a relatively narrow range of bud lengths. Uninucleatemicrospores were not detected in anthers from buds less than1·5 m or greater than 3·0mm long, but were generallypresent in frequencies of greater than 50 per cent in anthersfrom buds which were between 2·0 and 2·5 mm inlength. However, the bud length at which the highest frequencyof uninucleate microspores was detected varied significantlybetween genotypes and between the environments in which theywere grown. Examination of the remaining anthers from each budafter a period in culture revealed that the proportion of microsporesdeveloping into multicellular units varied greatly with budlength, an increase in frequency of multicellular microsporesbeing associated with an increase in the frequency of uninucleatemicrospores in the uncultured anther. Genotypes differed, however,in respect of the relationship between uninucleate microsporefrequency and production of multicellular units. Although thefrequency of multicellular units was as high as 57 percent,further development was limited and the number of embryoldsformed was low in all cases (<10 per cent). The frequency of multicellular units in pollen samples frombuds of a length in which uninucleate microspore frequency washigh varied significantly with genotype, temperature and lightconditions under which donor plants were grown, and the stageof inflorescence development at which buds were removed. Underconditions most conducive to multicellular unit formation (20/15°C,unshaded), the maximum frequency of multicellular units foreach genotype in buds from young inflorescences ranged from11·5 to 56·5 per cent. Shading or exposure tothe higher temperature was associated with a marked reductionin production of multicellular units. Higher frequencies ofmulticellular units were generally detected in microspore samplesfrom younger inflorescences irrespective of genotype or environment. Two of the four inbred lines were selected for a second experimentin which responses to vernalization and photoperiod durationwere monitored. There was a significant reduction in the numberof leaf nodes formed prior to floral initiation in both genotypesfollowing exposure to vernalization and/or a longer photoperiod,the response to photoperiod being more pronounced. Exposureto 4 weeks vernalization was accompanied by a significant increasein the frequency of multicellular units in both genotypes, thefrequency being double that in unvernalized plants under thelonger photoperiod. By contrast, genotypes differed sharplyin their response to photoperiod. In TB 20, the frequency ofmulticellular units was unaffected by an increase in day lengthirrespective of whether seed had been vernalized or not. Onthe other hand, in TB 42 the frequency of multicellular unitswas substantially greater in the 24 h day than in the 12 h day,being 27·3 per cent vs 13·0 per cent in the caseof unvernalized plants and 66·7 per cent vs 18·2per cent in the case of vernalized plants. Brassica napus, anther culture, pollen embryogenesis, genotype-environment interaction     

Flower Opening in Asiatic Lily is a Rapid Process Controlled by Dark-light Cycling

In commerce, Asiatic lilies are picked in bud, each stem holdingseveral buds. We found flower opening was rapid, taking lessthan 4 h both on the stem and for excised buds. Opening wasalso strongly synchronous. For a 12 h day-night cycle, openingbegan late in the dark period, reaching a mid-point after 11h of darkness. This was equally true of buds that were excisedwhen nearly ready to open, and those with 3–4 d of developmentto complete. Reversing day and night reversed the time of opening,and red light was as effective as white light in providing ‘day’conditions. A 15 min light break during the night did not affectthe opening. Lengthening the night (8, 12, 16 h) and shorteningthe day delayed opening from 9, to 11, to 13 h after the startof darkness, respectively. In continuous light and continuousdark, synchronicity was lost. If opening flowers were held inextended darkness, two phases of opening could be discriminated.In a ‘dark phase’, petals opened to approx. 40°,and anthers remained intact. When such flowers were returnedto light, there was a ‘light phase’, where petalsopened further, became more pigmented and began to recurve,and the anthers dehisced, these events taking only 2–3h. The net result was that flowers became fully open and anthersdehisced approx. 2 h after dawn, regardless of daylength. Copyright2000 Annals of Botany Company Asiatic lily, Lilium hybrid, flower opening, timing, endogenous rhythm, synchronicity     

Effects of Temperature and Photoperiod on Phenological Development in Three Genotypes of Bambara Groundnut (Vigna subterranea)

Factorial combinations of four photoperiods (10, 11·33,12·66 and 16 h d^-1) and three mean diurnal temperatures(20·2, 24·1 and 28·1°C) were imposedon nodulated plants of three Nigerian bambara groundnut genotypes[Vigna subterranea (L.) Verdc., syn. Voandzeia subterranea (L.)Thouars] grown in glasshouses in The Netherlands. The photothermalresponse of the onset of flowering and the onset of poddingwere determined. The time from sowing to first flower (f) wasdetermined by noting the day on which the first open flowerappeared. The time from sowing to the onset of podding (p) wasestimated from linear regressions of pod dry weight againsttime from sowing. Developmental rates were derived from thereciprocals of f and p. In two genotypes, 'Ankpa 2' and 'Yola',flowering occurred irrespective of photoperiod and 1/f was controlledby temperature only, occurring sooner at 28·1 than at20·2°C. The third genotype, 'Ankpa 4', was sensitiveto temperature and photoperiod and f was increased by coolertemperatures and photoperiods > 12·66 h d^-1 at 20·2°Cand > 11·33 h d^-1 at 24·1 and 28·1°C.In contrast, p was affected by temperature and photoperiod inall three genotypes. In bambara groundnut photoperiod-sensitivitytherefore increases between the onset of flowering and the onsetof podding. The most photoperiod-sensitive genotype with respectto p was 'Ankpa 4', followed by 'Yola' and 'Ankpa 2'. Therewas also variation in temperature-sensitivity between the genotypesinvestigated. Evaluation of bambara groundnut genotypes foradaptation to different photothermal environments will thereforerequire screening for flowering and podding responses.Copyright1994, 1999 Academic Press Vigna subterranea (L.) Verdc., Voandzeia subterranea (L.) Thouars, bambara groundnut, phenology, photoperiod, daylength, temperature, flowering, podding     

Environmental Effects on the Diurnal Accumulation of 45Ca by Young Fruit and Leaves of Tomato Plants

Diurnal uptake and distribution of ⁴⁵Ca in young fruiting tomatoplants were assessed 12 or 24 h after ⁴⁵Ca was applied to thenutrient solution at the beginning of either the light (12 h)or the dark (12 h) period. During the experiment, the salinityof the nutrient solution (measured as electrical conductivity,EC) was either 2·5 or 17 mS cm^–1 and the relativehumidity (measured as vapour pressure deficit, VPD) was either0·2 or 0·6 kPa The uptake of ⁴⁵Ca by a tomato plant over 12 h was higher inthe light than in the dark but the difference was less at lowhumidity. More ⁴⁵Ca was transported from the roots to the shootin the light than in the dark. More than half of the ⁴⁵Ca inthe shoot was accumulated by the stem; the proportion of ⁴⁵Cain the stem was greater in the dark and was further enhancedby high humidity to more than 80% of the ⁴⁵Ca in the shoot.The accumulation of ⁴⁵Ca by the fruit truss in the dark wasgreater than in the light in all experimental conditions. Underlow humidity the accumulation of ⁴⁵Ca by young leaves was similarin both light and dark. In high humidity there was considerablyless accumulation of ⁴⁵Ca by the young leaves in the dark The uptake of ⁴⁵Ca continued over 24 h but the transport of⁴⁵Ca to individual organs in the second 12 h period was affectedby both light and humidity. Some of the ⁴⁵Ca accumulated byyoung leaves and fruit in the second period appears to havebeen derived from ⁴⁵Ca released from the xylem wall along thetransport pathway in the stem The roles of root pressure and transpiration in the diurnalaccumulation of calcium in young fruit and leaves are discussed Calcium, diurnal translocation, tomato, young fruit and leaves     

Temporal pattern of feeding response of Chaoborus larvae to starvation

The effect of starvation on the feeding rate of larval Chaoborus(Diptera. Chaoboridae) was investigated using Daphnia roseaas prey. The starvation period varied from 12 h to 22 days.The starved Chaoborus were individually incubated with 10 Daphniaunder controlled light and temperature conditions. Observationswere made on prey mortality every 2 h for the first 12 h andonce after 24 h. Feeding rates gradually increased to a maximumbetween 7–11 days of starvation. After this period, feedingrates declined to previous low levels. Generally, feeding rateswere significantly higher during the first 2–4 h of feeding.Thereafter, feeding rates were lower and exhibited no consistentpattems with length of feeding time.