Photosynthetic Electron Transport During Senescence of the Primary Leaves of Phaseolus vulgaris L.: III. KINETICS OF CHLOROPHYLL FLUORESCENCE EMISSION FROM INTACT LEAVES

The kinetics of 685 nm chlorophyll fluorescence emission weremeasured at 20 °C following illumination of primary leavesof P. vulgaris. During foliar senescence, a large reductionwas observed in the maximal level of fluorescence emission (P)of the induction curve, normalized with respect to the minimallevel (O), and in the time taken to reach P. This suggests thatfewer plastoquinone (PQ) molecules were able to accept electronsfrom each photosystem two (PS II) reaction centre in older leaves.Measurements of fluorescence emission at 77 °K indicatedthat the primary photochemical quantum yield of the PS II reactioncentres remained constant during senescence. The redox stateof the PQ pool was estimated throughout the induction curveat 20 °C. In both mature and senescent leaves PQ was highlyreduced at P. There followed a reoxidation of PQ in the matureleaves, but in the old leaves the PQ pool remained reduced.This indicates that the rate of electron flow from PQ to photosystemone (PS I) decreased considerably during senescence. Fluorescencewas quenched from P to a steady state level (T) in leaves ofall ages, and this was associated with a redistribution of excitationin favour of PS I. Since, in senescent leaves, changes in theredox state of PQ were absent, it is suggested that quenchingresulted from the generation of proton and ion gradients acrossthe thylakoid membranes, and the synthesis of ATP.     

Chlorophyll Fluorescence and Photon Yield of Oxygen Evolution in Iron-Deficient Sugar Beet (Beta vulgaris L.) Leaves

The response of sugar beet (Beta vulgaris L.) leaves to iron deficiency can be described as consisting of two phases. In the first phase, leaves may lose a large part of their chlorophyll while maintaining a roughly constant efficiency of photosystem II photochemistry; ratios of variable to maximum fluorescence decreased by only 6%, and photon yields of oxygen evolution decreased by 30% when chlorophyll decreased by 70%. In the second phase, when chlorophyll decreased below a threshold level, iron deficiency caused major decreases in the efficiency of photosystem II photochemistry and in the photon yield of oxygen evolution. These decreases in photosystem II photochemical efficiency were found both in plants dark-adapted for 30 minutes and in plants dark-adapted overnight, indicating that photochemical efficiency cannot be repaired in that time scale. Decreases in photosystem II photochemical efficiency and in the photon yield of oxygen evolution were similar when measurements were made (a) with light absorbed by carotenoids and chlorophylls and (b) with light absorbed only by chlorophylls. Leaves of iron-deficient plants exhibited a room temperature fluorescence induction curve with a characteristic intermediate peak I that increases with deficiency symptoms.     

Effect of cadmium on photosystem II activity in <Emphasis Type="Italic">Chlamydomonas reinhardtii</Emphasis>: alteration of O–J–I–P fluorescence transients indicating the change of apparent activation energies within photosystem II

In this study, we evaluated how cadmium inhibitory effect on photosystem II and I electron transport may affect light energy conversion into electron transport by photosystem II. To induce cadmium effect on the photosynthetic apparatus, we exposed Chlamydomonas reinhardtii 24 h to 0–4.62 μM Cd²⁺. By evaluating the half time of fluorescence transients O–J–I–P at different temperatures (20–30°C), we were able to determine the photosystem II apparent activation energies for different reduction steps of photosystem II, indicated by the O–J–I–P fluorescence transients. The decrease of the apparent activation energies for PSII electron transport was found to be strongly related to the cadmium-induced inhibition of photosynthetic electron transport. We found a strong correlation between the photosystem II apparent activation energies and photosystem II oxygen evolution rate and photosystem I activity. Different levels of cadmium inhibition at photosystem II water-splitting system and photosystem I activity showed that photosystem II apparent activation energies are strongly dependent to photosystem II donor and acceptor sides. Therefore, the oxido-reduction state of whole photosystem II and I electron transport chain affects the conversion of light energy from antenna complex to photosystem II electron transport.     

Electron donor pool of photosystem II in Tris-washed chloroplasts in a study of low temperature delayed fluorescence

Transient time courses ("induction") and the intensity of thedelayed fluorescence of chlorophyll a (measured between 0.1and 3.9 msec after a 0.9 msec excitation period) were studiedwith a phosphoroscope at temperatures between 40 and –170°Cin Tris-washed chloroplasts. Tris-washing of chloroplasts changed the temperature dependenciesof the induction and the intensity of the delayed fluorescence.From the analysis of the induction each photosystem II reactioncenter appears to be linked to a donor pool which can supplyone electron to the acceptor pool in Tris-washed chloroplasts. An artificial electron donor, diphenylcarbazide affected thedelayed fluorescence above –100°C evidence that electronsare donated to photosystem II in at least two different ways. An electron transport inhibitor, 3-(3',4'-dichlorophenyl)-l,l-dimethylurea,changed the induction of the delayed fluorescence at temperaturesabove –60°C. The temperature dependence of the electron transport in thevicinity of photosystem II was characterized from these results. (Received May 27, 1980; )     

Temperature-Dependent Modulation of the Photoinhibition-Sensitivity of Photosystem II in Solanum tuberosum Leaves

High temperature (38°C) dramatically exacerbated the photoinhibitionof photosystem II in 23°C-grown potato leaves. This workshows the existence of an adaptive mechanism that cancels thesynergism between heat and strong light and markedly enhancesthe resistance of photosystem II to photodamage. Photoinhibition-resistanceof photosystem II was triggered by exposing leaves in weak lightto moderately elevated, non-injurious temperatures in the range32–38°C and was established within about 20 min, thusproviding a rapid process of photosynthetic adaptation to simultaneousincrease in temperature and light intensity. The reversal at23°C occurred on a much longer time scale of several hours.Temperature-induced increase in PSII photoresistance did notrequire de novo protein synthesis, as judged from its insensitivityto cycloheximide and chloramphenicol, and was not accompaniedwith any apparent change in the antenna size of photosystemII. From the presented chlorophyll fluorescence data, one canpostulate that temperature-dependent regulation of the photoinhibition-sensitivityof photosystem II could primarily involve a change in the PSIIreaction center, the nature of which remains to be established. (Received January 27, 1994; Accepted April 18, 1994)     

The Growth and Development of Maize (Zea mays L.) at Five Temperatures

The objectives of this work were to measure growth and developmentrates over a range of temperatures and to identify processeswhich may limit vegetative yield of maize (Zea mays L.). Twosingle cross Corn Belt Dent maize hybrids were grown from sowingin a diurnal temperature regime of 16/6 °C day/night andin constant temperature environments of 16, 20, 24 and 28 °C.The 16/6 °C environment was close to the minimum for sustainedgrowth and 28 °C was near the optimum. Entire plants wereharvested at stages with 4, 6, 7 and 8 mature leaves in alltemperature treatments except 20 °C in which the final twoharvests were carried out at 9 and 10 mature leaves. Mean totalleaf number varied between 19.5 and 16.0 with the maximum occurringat 16/6 °C. Although harvests were carried out at comparableleaf numbers, and hence at similar developmental stages, thetime interval between sowing and harvest decreased considerablyas temperatures increased. The relative rates of dry weight and leaf area accumulationwith time increased with a Q₁₀ of 2.4 between 16 and 28 °C,while leaf appearance rate increased with a Q₁₀ of 2.9 overthe same range; both rates were highest at 28 °C. Althoughdry matter partitioning to the shoots increased with temperature,the area of individual leaves varied in a systematic patternwhich resulted in maximum leaf area, leaf area duration andconsequently dry weight being realized at 20 °C for anygiven stage of development. Zea mays, corn, low temperature stress, temperature response, growth, development     

Inhibition of the Chloroplast Photochemical Reactions by Treatment of Wheat Seedlings with Low Concentrations of Cadmium: Analysis of Electron Transport Activities and Changes in Fluorescence Yield

The effect of treatment of wheat plants with Cd²⁺ ions on thephotochemical activity of the primary leaves was examined. Threeday-old etiolated seedlings were treated with Cd²⁺ ions for24 h in dark, and after this treatment the plants were grownin the light until the primary leaves were fully developed.Cd²⁺ ions (30–120 µM) induced a significant decreasein activities of both photosystem II and photosystem I. Theextent of the decrease in PS II activity was much greater thanthat in the PS I activity. Analysis of changes in the fluorescenceyield of chlorophyll also indicated that Cd²⁺ ions drasticallyaffect the photochemistry of photosystem II. Cd²⁺ ions induceddecrease in the rates of photoreduction of 2,6-dichlorophenolindophenol even in the presence of the exogenous electron donor,hydroxylamine, both in Tris-treated and untreated chloroplasts.This result suggests that the site of inhibition is near thesite of donation of electrons by hydroxylamine. Treatment withCd²⁺ ions impairs the electron transport system on the reducingside of PS II. The decrease in the fluorescence yield of Chi is less than that in the evolution of O₂ mediated by oxidizedphenylenediamine. This difference may be a result of inhibitionon the reducing side of PS II. In addition to inhibition onthe reducing side, Cd²⁺ ions may affect the oxidizing side ofPS II. A comparative study of the rates of evolution of O₂ withp-benzoquinone and dichloro-p-benzoquinone as electron acceptorswas performed since the halogenated benzoquinones have beenshown to accept electrons from both active and inactive centersof photosystem II while some of the benzoquinones accept electronsonly from active centers. The results suggest that Cd²⁺ ionsinduced a marginal increase in the number of inactive reactioncenters in PS II. Analysis of light-saturation-kinetics of theevolution of O₂ catalysed by PS II indicates a reduction inthe size of the antennae as well as in the concentration ofthe active (-type) reaction centers of PS II. Thus, the Cd²⁺-inducedeffects on the photochemistry of PS II involve changes on thereducing side of PS II as well as possible changes in the sizesof the populations of active and inactive centers. Thus, short-termexposure to Cd²⁺ ions during establishment of seedlings hasa severely detrimental effect on photochemical activities inchloroplasts. (Received October 17, 1990; Accepted July 3, 1991)     

Modifications in photosystem II photochemistry in senescent leaves of maize plants

Analyses of CO2 exchange and chlorophyll fluorescence were carried out to assess photosynthetic performance during senescence of maize leaves. Senescent leaves displayed a significant decrease in CO2 assimilatory capacity accompanied by a decrease in stomatal conductance and an increase in intercellular CO2 concentration. The analyses of fluorescence quenching under steady-state photosynthesis showed that senescence resulted in an increase in non-photochemical quenching and a decrease in photo-chemical quenching. It also resulted in a decrease in the efficiency of excitation energy capture by open PSII reaction centres and the quantum yield of PSII electron transport, but had very little effect on the maximal efficiency of PSII photochemistry. The results determined from the fast fluorescence induction kinetics indicated an increase in the proportion of QB-non-reducing PSII reaction centres and a decrease in the rate of QA reduction in senescent leaves. Theoretical analyses of fluorescence parameters under steady-state photosynthesis suggest that the increase in the non-photochemical quenching was due to an increase in the rate constant to thermal dissipation of excitation energy by PSII and that the decrease in the quantum yield of PSII electron transport was associated with a decrease in the rate constant of PSII photochemistry. Based on these results, it is suggested that the decrease in the quantum yield of PSII electron transport in senescent leaves was down-regulated by an increase in the proportion of QB-non-reducing PSII reaction centres and in the non-photochemical quenching. The photosynthetic electron transport would thus match the decreased demand for ATP and NADPH in carbon assimilation which was inhibited significantly in senescent leaves.Key words: Chlorophyll fluorescence, gas exchange, maize (Zea mays L.), photochemical and non-photochemical quenching, photosystem II photochemistry.      

Stress Tolerance of Photosystem II in Vivo: Antagonistic Effects of Water, Heat, and Photoinhibition Stresses

The in vivo photochemical activity of photosystem II was inferred from modulated chlorophyll fluorescence and photoacoustic measurements in intact leaves of several plant species (Lycopersicon esculentum Mill., Solanum tuberosum L., Solanum nigrum L.) exposed to various environmental stresses (drought, heat, strong light) applied separately or in combination. Photosystem II was shown to be highly drought-resistant: even a drastic desiccation in air of detached leaf samples only marginally affected the quantum yield for photochemistry in photosystem II. However, water stress markedly modified the responses of photosystem II to superimposed constraints. The stability of photosystem II to heat was observed to increase strongly in leaves exposed to water stress conditions: heat treatments (e.g. 42°C in the dark), which caused a complete and irreversible inhibition of photosystem II in well-watered (tomato) leaves, resulted in a small and fully reversible reduction of the photochemical efficiency of photosystem II in drought-stressed leaves. In vivo photoacoustic data indicated that photosystem I was highly resistant to both heat and water stresses. When leaves were illuminated with intense white light at 25°C, photoinhibition damage of photosystem II was more pronounced in water-stressed leaves than in undesiccated controls. However, in nondehydrated leaves, photoinhibition of photosystem II was strongly temperature dependent, being drastically stimulated at high temperatures above 38 to 40°C. As a consequence, when exposed to strong light at high temperature, photosystem II photochemistry was significantly less inhibited in dehydrated leaves than in control well-hydrated leaves. Our results demonstrate the existence of a marked antagonism between physicochemical stresses, with water stress enhancing the resistance of photosystem II to constraints (heat, strong light at high temperature) that are usually associated with drought in the field.     

Carotenoids and fatty alcohols as non-ionic hydrophobic inhibitors of photochemical activities of chioroplasts

Carotenoids and fatty alcohols were added to intact spinachchloroplasts in suspension, and the effects of these reagentson the absorption spectrum and photochemical activities of chloroplastswere examined. The addition of lutein, ß-caroteneand neoxanthin transformed a chlorophyll a form (C684) havingan absorption maximum at 684 nm into C666, and the activityof photosystem II decreased parallel with this transformation.The activity of photosystem I was completely unaffected by theeffect of added carotenoids, whereas both cyclic and non-cyclicphotophosphorylations were inhibited by the additions. Theseeffects were reproducibly observed only with a "petroleum ether-soluble"fraction of each carotenoid, monomeric and less polymerizedforms, which are soluble in petroleum ether at –25°C;the "insoluble" fraction of more polymerized forms was ineffective.Comparative experiments with lutein, DCMU and CCCP as inhibitorsand the dependence of inhibition on light intensity suggestedthat the site of inhibition by carotenoids is on the water sideof photosystem II between its reaction center and the CCCP-inhibitingsite. Fatty alcohols with carbon atoms between 8 and 12 producedstronger but less specific effects on the spectrum and activities.At low concentrations the uncoupling of photophosphorylationoccurred and, in a middle concentration range, the activityof photosystem II decreased with the transformation of C684into C666 and with a change in carotenoid bands. At higher concentrations,where the enhanced activity of photosystem I decreased froma maximum to zero, the red band of chlorophyll a further changedin a complex manner and the absorption around 503 nm decreased.We, thus, deduced that C684 and some endogeneous carotenoidsare associated with photosystem II on its water side and thatadded carotenoids and fatty alcohols at lower concentrationschange their states, resulting in the inhibition of this photosystem. (Received December 20, 1971; )     

Temperature-Induced Changes of Variable Fluorescence-Yield in Intact Leaves

Variable fluorescence (F_v) of intact leaves was measured whenthe temperature was lowered at a rate of 1–2?C per mn,from 20?C to –20?C. The quantum flux density of the excitinglight was 1–2 µE m^–2 sec^–1 in orderto sensitize F only at 20?C. The fluorescence yield decreasedrapidly at the freezing point of the leaf and upon further coolingthe fluorescence yield increased again. F_m was obtained a fewdegrees below the freezing point. Repeated freeze-thaw cycles caused successively increased damageto the thylakoid membranes on either the oxidizing or the reducingside of photosystem II. An eventual loss of F_v over F_o was typicalfor damage on the water splitting side of photosystem II, whereasdamage after the primary electron acceptor Q of photosystemII was characterized by an invariable fluorescence yield atF_m over the temperature range examined. (Received January 18, 1982; Accepted June 12, 1982)     

Photosynthetic activity of far-red light in green plants

We have found that long-wavelength quanta up to 780 nm support oxygen evolution from the leaves of sunflower and bean. The far-red light excitations are supporting the photochemical activity of photosystem II, as is indicated by the increased chlorophyll fluorescence in response to the reduction of the photosystem II primary electron acceptor, Q_A. The results also demonstrate that the far-red photosystem II excitations are susceptible to non-photochemical quenching, although less than the red excitations. Uphill activation energies of 9.8 ± 0.5 kJ mol⁻¹ and 12.5 ± 0.7 kJ mol⁻¹ have been revealed in sunflower leaves for the 716 and 740 nm illumination, respectively, from the temperature dependencies of quantum yields, comparable to the corresponding energy gaps of 8.8 and 14.3 kJ mol⁻¹ between the 716 and 680 nm, and the 740 and 680 nm light quanta. Similarly, the non-photochemical quenching of far-red excitations is facilitated by temperature confirming thermal activation of the far-red quanta to the photosystem II core. The observations are discussed in terms of as yet undisclosed far-red forms of chlorophyll in the photosystem II antenna, reversed (uphill) spill-over of excitation from photosystem I antenna to the photosystem II antenna, as well as absorption from thermally populated vibrational sub-levels of photosystem II chlorophylls in the ground electronic state. From these three interpretations, our analysis favours the first one, i.e., the presence in intact plant leaves of a small number of far-red chlorophylls of photosystem II. Based on analogy with the well-known far-red spectral forms in photosystem I, it is likely that some kind of strongly coupled chlorophyll dimers/aggregates are involved. The similarity of the result for sunflower and bean proves that both the extreme long-wavelength oxygen evolution and the local quantum yield maximum are general properties of the plants.     

Temperature Dependent Alterations in the Pattern of Photochemical and Non-Photochemical Quenching and Associated Changes in the Photosystem II Conditions of the Leaves

The alterations in the PSII activity of leaves, subsequent toa mild or severe heat stress were characterized by monitoringthe Chl a fluorescence and thermoluminescence emission fromintact leaves. The Chl a fluorescence measurements were carriedout in leaves adapted to either ‘state I’ or ‘stateII’ since under these two conditions the photosyntheticapparatus is known to have distinctly different structure-functionrelationships. The pattern of Chl a fluorescence induction instate II-adapted leaves was different from that of state I-adaptedleaves due to the alterations in the extent of photochemical(q_Q) and non-photochemical (q_E) quenching during the time courseof induction. The pattern of changes in q_Q and q_E values wasalso altered by heat treatment depending on the severity ofheat stress; severe heat stress (47°C) suppressing theseparameters drastically. Mild heat treatment (42°C) did notaffect the ability of leaves to undergo state I to state IItransition whereas the severe heat stress totally abolishedsuch transition. The fluorescence and thermoluminescence characteristicsof the leaves that have been exposed to the severe heat stresssuggest that a large number of affected PSII units retain afunctional water-oxidizing complex at the donor side. (Received June 14, 1994; Accepted July 19, 1995)     

The photochemical and fluorescence properties of whole cells, spheroplasts and spheroplast particles from the blue-green alga Phormidium luridum.

The photochemical activities and fluorescence properties of cells, spheroplasts and spheroplast particles from the blue-green alga Phormidium luridum were compared. The photochemical activities were measured in a whole range of wavelengths and expressed as quantum yield spectra (quantum yield vs. wavelength). The following reactions were measured. Photosynthesis (O2 evolution) in whole cells; Hill reaction (O2 evolution) with Fe(CN)63- and NADP as electron acceptors (Photosystem II and photosystem II + Photosystem I reactions); electron transfer from reduced 2,6-dichlorophenolindophenol to diquat (Photosystem I reaction). The fluorescence properties were emission spectra, quantum yield spectra and the induction pattern. On the basis of comparison between the quantum yield spectra and the pigments compositions the relative contribution of each pigment to each photosystem was estimated. In normal cells and spheroplasts it was found that Photosystem I (Photosystem II) contains about 90% (10%) of the chlorophyll a, 90% (10%) of the carotenoids and 15% (85%) of the phycocyanin. In spheroplast particles there is a reorganization of the pigments; they loose a certain fraction (about half) of the phycocyanin but the remaining phycocyanin attaches itself exclusively to Photosystem I (!). This is reflected by the loss of Photosystem II activity, a flat quantum yield vs. wavelength dependence and a loss of the fluorescence induction. The fluorescence quantum yield spectra conform qualitatively to the above conclusion. More quantitative estimation shows that only a fraction (20--40%) of the chlorophyll of Photosystem II is fluorescent. Total emission spectrum and the ratio of variable to constant fluorescence are in agreement with this conclusion. The fluorescence emission spectrum shows characteristic differences between the constant and variable components. The variable fluorescence comes exclusively from chlorophyll a; the constant fluorescence is contributed, in addition to chlorophyll a, by phycocyanine and an unidentified long wavelength component. The variable fluorescence does not change in the transition from whole cells to spheroplasts. However, the constant fluorescence increases considerably. This indicates the release of a small fraction of pigments from the photosynthetic photochemical apparatus which then become fluorescent.     

Studies on the Hill reaction of membrane fragments of blue-green algae V. A correlation between the solubilization of a photochemically active chromoprotein (ACP) and the inactivation of photosystem II activity in membrane fragments of Anabaena cylindrica

The relationship between a photochemically active chromoprotein(ACP) (cf. ref. 1) and photosystem II was investigated withmembrane fragments of Anabaena cylindrica, A. variabilis andP. boryaman. ACP was solubilized from membrane fragments of A. cylindricabut not from those of A. variabilis or P. boryanum, when themembrane fragments had been incubated in a dilute buffer andhad lost their Hill or photosystem II activity. In A. cylindrica,ACP-solubilization always occurred, independent of photosystemII inactivation, on incubation of the membrane fragments inmedia without PEG. However, the amount of ACP solubilizationaccompanying photosystem II inactivation was twice that withoutphotosystem II inactivation. The increase in ACP solubilizationaccompanying photosystem II inactivation. The kinetics resembledthose for the decrease in 695 nm fluorescence emitted by membranefragments at — 196?C (cf. 2). The ACP solubilized independent of photosystem II inactivationwas assumed to have been released during disruption of intactcells in the preparation of membrane fragments. The slow ACPsolubilization upon the inactivation of photosystem II was attributedto the pigment being bound to membranes. We assume that thephoto-reactive component of ACP, P690 (cf. 3, 4), is releasedfrom the membranes during photosystem II inactivation, and thatP690 is a component of photosystem II which emits the 695 nmfluorescence at — 196?C. (Received March 22, 1974; )     

Leaf Development in Lolium temulentum: Photosynthesis and Photosynthetic Proteins in Leaves Senescing under Different Irradiances

Changes in carbon fixation rate and the levels of photosyntheticproteins were measured in fourth leaves of Lolium temulentumgrown until full expansion at 360 µmol quanta m^–2s^–1 and subsequently at the same irradiance or shadedto 90 µmol m^–2 s^–1. Ribulose-1,5-bisphosphatecarboxylase/oxygenase (Rubisco), light-harvesting chlorophylla/b protein of photosystem II (LHCII), 65 kDa protein of photosystemI (PSI), cytochrome f (Cytf) and coupling factor 1 (CF₁) declinedsteadily in amount throughout senescence in unshaded leaves.In shaded leaves, however, the decrease in LHCII and the 65kDa protein was delayed until later in senescence whereas theamount of Cyt f protein decreased rapidly following transferto shade and was lower than that of unshaded leaves at the earlyand middle stages of senescence. Decreases in the Rubisco andCF₁ of shaded leaves occurred at slightly reduced rates comparedwith unshaded leaves. These results indicate that chloroplastproteins in fully-expanded leaves are controlled individually,in a direction appropriate to acclimate photosynthesis to agiven irradiance during senescence. (Received August 20, 1992; Accepted January 5, 1993)     

The higher resistance to chilling stress in adaxial side of <Emphasis Type="Italic">Rumex</Emphasis> K-1 leaves is accompanied with higher photochemical and non-photochemical quenching

Responses of two sides of Rumex K-1 leaves to chilling stress (5 °C, photon flux density of 100 μmol m⁻² s⁻¹) were studied by using gas exchange, chlorophyll (Chl) fluorescence, and spectrum reflectance techniques. The Chl and carotenoid contents in the two sides were not affected by chilling treatment, and both were higher in the adaxial side. The maximum quantum yield of photosystem (PS) 2 and fraction of functional PS1 in the abaxial side decreased more markedly than those in the adaxial side during the chilling treatment, indicating that the abaxial side was damaged more significantly than the adaxial side. Before chilling, there were no obvious differences in actual photochemical efficiency of PS2, photosynthesis, and photorespiration between two sides of the leaves. Under chilling stress, the actual photochemical efficiency of PS2, photosynthesis, and photorespiration all declined more significantly in the abaxial side, which was partly attributed to lower carboxylation efficiency in the abaxial side than that in the adaxial side. Non-photochemical quenching was higher in the adaxial side, though the de-epoxidation of xanthophyll cycle pigments’ pool on basis of Chl was higher in the abaxial side. Both the slower decrease in the photochemical quenching and the higher non-photochemical quenching may account for the higher resistance to chilling stress in the adaxial side of Rumex K-1 leaves.     

Stoichiometries of Photosystem I and Photosystem II in Rice Mutants Differently Deficient in Chlorophyll b

Stoichiometries of photosystem I (PSI) and photosystem II (PSII)reaction centers in a cultivar of rice, Norin No. 8, and threechlorophyll b-deficient mutants derived from the cultivar wereinvestigated. Quantitation of PSI by photooxidation of P-700and chromatographic assay of vitamin K₁ showed that, on thebasis of chlorophyll, the mutants have higher concentrationsof PSI than the wildtype rice. Greater increases were observedin the PSII contents measured by photoreduction of Q_A, bindingof a radioactive herbicide and atomic absorption spectroscopyof Mn. Consequently, the PSII to PSI ratio increased from 1.1–1.3in the wild-type rice to 1.8 in chlorina 2, which contains noChl b, and to 2.0–3.3 in chlorina 11 and chlorina 14,which have chlorophyll a/b ratios of 9 and 13, respectively.Measurement of oxygen evolution with saturating single-turnoverflashes revealed that, whereas at most 20% of PSII centers areinactive in oxygen evolution in the wildtype rice, the non-functionalPSII centers amount to about 50% in the three mutant strains.The fluorescence induction kinetics was also analyzed to estimateproportions of the inactive PSII in the mutants. The data obtainedsuggest that plants have an ability to adjust the stoichiometryof the two photosystems and the functional organization of PSIIin response to the genetically induced deficiency of chlorophyllb. (Received July 29, 1994; Accepted February 7, 1996)     

Characterization of chilling effects on photosynthetic performance of maize crops during early season growth using chlorophyll fluorescence

Changes in a range of chlorophyll fluorescence parameters weremonitored for leaves of crops of three Zea mays cultivars (MO17,CB3 and LG11) during early canopy development when large fluctuationsin air temperatures occur. Crops were sown on 1 May 1993 andmeasurements made between 17 May and 7 June. Measurements ofthe ratio of variable to maximal fluorescence of dark-adaptedleaves (Fv/Fm) and the quantum efficiency of photosystem IIphotochemistry (     

Leaf Extension in Zea mays: I. LEAF EXTENSION AND WATER POTENTIAL IN RELATION TO ROOT-ZONE AND AIR TEMPERATURES

The temperature of the roots and shoots of Zea mays plants werevaried independently of each other and the rates of leaf extensionand leaf water potentials were measured. Restrictions of leafextension occurred when root temperatures were lowered from35 to 0 °C, but leaf water potentials were lowered onlyat root temperatures below 5 °C. Similar changes in ratesof leaf extension were measured at air temperatures from 30to 5 °. Between 30 and 35 °C air temperature, in anunsaturated atmosphere, restrictions of leaf extension wereassociated with low leaf water potentials. It was concluded that, at root temperatures 5 to 35 °C,and shoot temperatures 5 to 30 °C, water stress was notthe main factor restricting the extension of Zea mays leaves.