ALGAL EXCRETION OF 14C-LABELED COMPOUNDS AND MICROBIAL INTERACTIONS IN CYANIDIUM CALDARIUM MATS1

Acid spring effluents are often covered with mats of the eucaryotic phycocyanin-containing alga. Cyanidium caldarium. The primary bacterial component of such mats is an acidophilic strain of Bacillus coagulans, and the primary fungal component is Dactylaria gallopava. Because of the limited species diversity, C. caldarium mats appeared to be an excellent system for studying algal excretion and various microbial interactions in nature. From 2 to 6% of the NaH¹⁴CO₃ taken up by natural or laboratory populations of the alga was excreted as ¹⁴C-labeled materials. The maximum excretion occurred at temperature, light, and pH values optimum for NaH¹⁴CO₃ uptake. However, when excretion was expressed as a percentage of NaH14 CO₃ uptake, a higher percentage of the radioactivity was excreted at nonoptimal conditions for NaH¹⁴CO₃ uptake. Fungal biomass was directly proportional to algal density, but bacterial numbers varied widely and did not correlate with algal numbers. The bacterial and fungal components could be grown in mixed culture with either growing C. caldarium cultures or in an extract prepared, by healing algal cells.     

Two Steps of Gas Exchange in Leaf Photosynthesis

Photosynthesis and transpiration of excised leaves of Taraxacum officinale L. and a few other species of plants were measured, using an open gas analysis system. The rates of CO₂ uptake and transpiration increased in two steps upon illumination of stomata-bearing epidermis of these leaves at a light intensity of 50 mW × cm⁻². Abscisic acid inhibited only the second step of gas exchange. Illumination of the astomatous epidermis of hypostomatous leaves caused only the first step of gas exchange. These data indicate that the first and second steps arise from cuticular and stomatal gas exchange, respectively. The rate of the cuticular photosynthesis in a Taraxacum leaf reached saturation at a light intensity of 5 mW × cm⁻², and the rates of the stomatal photosynthesis and transpiration reached saturation at a higher intensity of 35 mW × cm⁻². The cuticular photosynthesis of a Taraxacum leaf was 18% of the stomatal photosynthesis at 50 mW × cm⁻² and 270% at 5 mW × cm⁻². The other species of leaves showed the same trend. The importance of cuticular CO₂ uptake in leaf photosynthesis, especially under low light intensity was stressed from these data.     

INORGANIC CARBON AND ACETATE ASSIMILATION IN BOTRYOCOCCUS BRAUNII(CHLOROPHYTA)1

Assimilation of ¹⁴CO₂ or ¹⁴C-acetate by the hydrocarbon producing alga Botryococcus braunii Kützing was investigated to determine the allocation of incorporated ¹⁴C among early metabolites of photosynthesis and secondary metabolites. When the cells were exposed to NaH¹⁴CO₃ for 10 sec, over 90% of incorporated ¹⁴C was detected in phosphoglycerate, suggesting that this alga assimilates inorganic carbon by the C-3 pathway. The distribution pattern of ¹⁴C in the number of metabolites revealed that organic acids, neutral sugars and amino acids were first labelled with ¹⁴C, and, after lag periods of a few minutes, lipids including hydrocarbon were increasingly labelled. Addition of 5 mM acetate to the culture medium did not affect the growth of this alga but enhanced cellular respiration. The incorporation of ¹⁴CO₂ into the lipid fraction was stimulated, but net photosynthesis was inhibited by the addition of acetate. ¹⁴C-acetate was incorporated into lipids at a very low rate in comparison with the rate of ¹⁴CO₂ incorporation.     

CO2 uptake patterns depend on water current velocity and shoot morphology in submerged stream macrophytes

1. The influence of current velocity on the pattern of photosynthetic CO₂ uptake in three species of submerged stream macrophytes was described by analysing the grain density in autoradiographs of leaves exposed to ¹⁴CO₂. 2. In Elodea canadensis, the CO₂ uptake was approximately two‐fold higher near the leaf periphery compared with the midrib section at high current velocity, whereas at low current velocity the area of relatively high CO₂ uptake expanded from the leaf periphery towards the midrib and basal sections of the leaves. 3. In Potamogeton crispus and Callitriche stagnalis the CO₂ uptake was uniform throughout the leaves at low current velocity, whereas at high current velocity the CO₂ uptake appeared to increase randomly in some areas of the leaves. 4. The relationship between the photosynthetic CO₂ uptake pattern and the dynamics of flow surrounding submerged shoots at low and high current velocity is discussed in relation to shoot morphology. In E. canadensis, thick diffusive boundary layers may develop between leaves because of screening effects at high current velocity. Increased diffusion path for CO₂ may contribute to inhibitory effects on photosynthesis in this species.     

TRANSPORT OF CARBON AMONG CONNECTED RAMETS OF EICHHORNIA CRASSIPES (PONTEDERIACEAE) AT NORMAL AND HIGH LEVELS OF CO2

The floating, stoloniferous plant, Eichhornia crassipes, has high rates of productivity and rapidly invades new sites. Because the transport of carbon among connected ramets is known to increase the growth of clonal plants, we asked whether there is intraclonal carbon transport in E. crassipes. Because net photosynthesis of E. crassipes is significantly higher at high levels of atmospheric CO₂, we also asked if high CO₂ can change patterns of carbon transport in ways that might modify clonal growth. We exposed individual ramets within groups of connected ramets to ¹⁴CO₂ for 15–45 min and measured the distribution of ¹⁴C in the group after 4 days of growth at 350, 700, 1,400, or 2,800 μ1 1^−-1 CO₂. At 350 μ1 1^−-1 CO₂, a parent ramet exported approximately 10% of the ¹⁴C that it assimilated to its first rooted offspring ramet. The offspring exported a similar percentage of the ^l4C it assimilated toward the parent; two-thirds of this ¹⁴C was retained by the parent, and one-third moved into new offspring of the parent. In all ramets, imported carbon moved into leaves as well as roots. At the higher levels of CO₂, the percentage of assimilated carbon exported from a parent ramet to the leaf blades of its first offspring was lower by half. High CO₂ had little other effect on carbon transport. E. crassipes maintains bidirectional transport of carbon between ramets even under uniform and favorable environmental conditions and when external CO₂ levels are very high.     

Advanced radiogasometric method for the determination of the rates of photorespiratory and respiratory decarboxylations of primary and stored photosynthates under steady-state photosynthesis

An advanced radiogasometric method for the study of plant leaf CO₂ exchange is presented. The method enables determination of the rates of CO₂ fixation, photorespiration and respiration in the light under steady‐state photosynthesis and discrimination between primary and stored photosynthates as substrates of photorespiratory and respiratory decarboxylations. The method is based on the analysis of the time curves of ¹⁴CO₂ evolution from labeled primary and stored photosynthates in leaves previously exposed to ¹⁴CO₂. The molar rates of different decarboxylation reactions are calculated from the initial slopes of the curves taking into account the specific radioactivity of CO₂ fed to leaves and/or evolved from leaves. To estimate the contribution of primary and stored photosynthates, the measurements of ¹⁴CO₂ evolution are performed after feeding plant leaves for different periods with ¹⁴CO₂. Photorespiration and respiration are distinguished on the basis of data obtained from measurements of ¹⁴CO₂ evolution under normal (210 ml l⁻¹) and low (15 ml l⁻¹) concentrations of oxygen. A principally new method for the determination of the rate of intracellular refixation of respiratory CO₂ has been developed. The method is based on the measurements of ¹⁴CO₂ evolution from leaves into the medium of very high concentrations (30 ml l⁻¹) of ¹²CO₂, where the probability of refixation of ¹⁴CO₂ evolved inside the cell is close to zero. The results obtained were comparable with the data derived from parallel refixation measurements by means of gasometric methods. As an example of application, the data on CO₂ exchange in leaves of two contrasting groups of C₃‐species, differing in the ability of starch accumulation, are presented.     

14C-Studies on Apple Trees. VI. The Influence of the Fruit on the Photosynthesis of the Leaves, and the Relative Photosynthetic Yields of Fruits and Leaves

When paired samples of either intact or detached apple shoots with and without fruits were exposed simultaneuosly to ¹⁴CO₂, the uptake of ¹⁴CO₂ of leaf area was found to be greater in the fruit-bearing shoots, often by a factor of 1.5 or more, although the difference tends to be slight or even non-existent when the experiments follow shortly after a previous dark period. The uptake of ¹⁴CO₂ by photosynthesis in the skin of detached fruits is very slight compared to the simultaneous uptake of ¹⁴CO₂ by the leaves from the same spur, and can hence contribute only slightly to the development of the fruit compared with the supply of assimilates taking place from the leaves to the fruit.     

PHOTOSYNTHESIS AND CALCIFICATION BY EMILIANIA HUXLEYI (PRYMNESIOPHYCEAE) AS A FUNCTION OF INORGANIC CARBON SPECIES

To test the possibility of inorganic carbon limitation of the marine unicellular alga Emiliania huxleyi (Lohmann) Hay and Mohler, its carbon acquisition was measured as a function of the different chemical species of inorganic carbon present in the medium. Because these different species are interdependent and covary in any experiment in which the speciation is changed, a set of experiments was performed to produce a multidimensional carbon uptake scheme for photosynthesis and calcification. This scheme shows that CO₂ that is used for photosynthesis comes from two sources. The CO₂ in seawater supports a modest rate of photosynthesis. The HCO is the major substrate for photosynthesis by intracellular production of CO₂ (HCO+ H⁺→ CO₂+ H₂O → CH₂O + O₂). This use of HCO is possible because of the simultaneous calcification using a second HCO, which provides the required proton (HCO+ Ca²⁺→ CaCO₃+ H⁺). The HCO is the only substrate for calcification. By distinguishing the two sources of CO₂ used in photosynthesis, it was shown that E. huxleyi has a K_½ for external CO₂ of “only” 1.9 ± 0.5 μM (and a V_max of 2.4 ± 0.1 pmol·cell⁻¹·d⁻¹). Thus, in seawater that is in equilibrium with the atmosphere ([CO₂]= 14 μM, [HCO]= 1920 μM, at fCO₂= 360 μatm, pH = 8, T = 15° C), photosynthesis is 90% saturated with external CO₂. Under the same conditions, the rate of photosynthesis is doubled by the calcification route of CO₂ supply (from 2.1 to 4.5 pmol·cell⁻¹·d⁻¹). However, photosynthesis is not fully saturated, as calcification has a K_½ for HCO of 3256 ± 1402 μM and a V_max of 6.4 ± 1.8 pmol·cell⁻¹·d⁻¹. The H⁺ that is produced during calcification is used with an efficiency of 0.97 ± 0.08, leading to the conclusion that it is used intracellularly. A maximum efficiency of 0.88 can be expected, as NO uptake generates a H⁺ sink (OH⁻ source) for the cell. The success of E. huxleyi as a coccolithophorid may be related to the efficient coupling between H⁺ generation in calcification and CO₂ fixation in photosynthesis.     

Photosynthetic Uptake of Free CO2, by the Roots of Lobelia dortmanna

Lobelia dortmanna L. is probably unable to utilize HCO₃^?and uses only free CO₂ for photosynthesis as shown by the Winkler method. A ¹⁴C technique was used to show that if CO₂ is added to the water around roots, photosynthesis increases 3–5 times more than when the corresponding amount of CO₂ is added to the water surroundings the leaves. As the CO₂ content in lakes where Lobelia grows is very limited, Lobelia must absorb CO₂ from the sediment, and the carbon dioxide will have to diffuse from the roots up into the leaves through the intercellular system of the plant. In conjunction with Lobelia's CO₂ uptake from the sediment O₂ is liberated. The plant, therefore, acts as an oxygen pump, which oxidizes the sediment down to a depth of 20 cm.     

Oxygen effect on photosynthetic and glycolate pathways in young maize leaves

To study the effect of O₂ on the photosynthetic and glycolate pathways, maize leaves were exposed to ¹⁴CO₂ during steady-state photosynthesis in 21 or 1% O₂. At the two O₂ concentrations after a ¹⁴CO₂ pulse (4 seconds) followed by a ¹²CO₂ chase, there was a slight difference in CO₂ uptake and in the total amount of ¹⁴C fixed, but there were marked changes in ¹⁴C distribution especially in phosphoglycerate, ribulose bisphosphate, glycine, and serine. The kinetics of ¹⁴C incorporation into glycine and serine indicated that the glycolate pathway is inhibited at low O₂ concentrations. In 1% O₂, labeling of glycine was reduced by 90% and that of serine was reduced by 70%, relative to the control in 21% O₂. A similar effect has been observed in C₃ plants, except that, in maize leaves, only 5 to 6% of the total ¹⁴C fixed under 21% O₂ was found in glycolate pathway intermediates after 60 seconds chase. This figure is 20% in C₃ plants. Isonicotinyl hydrazide did not completely block the conversion of glycine to serine in 21% O₂, and the first carbon atom of serine was preferentially labeled during the first seconds of the chase. These results supported the hypothesis that the labeled serine not only derives from glycine but also could be formed from phosphoglycerate, labeled in the first carbon atom during the first seconds of photosynthesis.     

Transfer of Photosynthetically Produced Carbohydrate from Endosymbiotic Chlorellae to Paramecium bursaria*

Paramecium bursaria (Ehrenberg) and an endozoic zoochlorella Chlorella conductrix (Brandt) live in a symbiotic relationship. Uptake of NaH¹⁴CO₃ was studied to determine if carbohydrate products of photosynthesis are transferred to the host paramecium. Paramecium bursaria containing the algal symbionts took up NaH¹⁴CO₃ but those without the algal symbionts did not. Radioactive maltose, glucose, fructose and malate were identified from the ethanolic extract of paramecia. Transfer of materials from Paramecium to Chlorella and the transfer of other materials from Chlorella to Paramecium, led to the conclusion that this is a mutualistic relationship, both organisms benefiting from the relationship.     

Photosynthesis of Desiccating Leaves of Poplar

The relation between photosynthesis and water content was investigated using detached leaves of Populus euramericana (Dode) Guinier cv. Robusta. The time course of photosynthesis was measured at different light intensities, at different CO₂ contents of the air and at constant temperature during the desiccation of the leaves. The time course of decreasing water content was obtained from continuous measurement of water transpired from the leaves. A large reduction of light saturated (400 W × m⁻²) photosynthetic rates was observed with decreasing water contents between 78 and 64% (water potential between −14 and −24 atm (bar)). This reduction was much greater in air with 0.3 % CO₂ than in air with 5 % CO₂, indicating a significant influence of CO₂ diffusion resistance on rate of photosynthesis. The reduction of the rate of light and CO₂ saturated photosynthesis (at 400 W × m^–2 and 5% CO₂ in the air) is a measure of the inactivation of the photosynthetic enzyme system by desiccation. A proportional reduction of the light saturated and light limited rate of photosynthesis (for different H₂O contents) was found, when measured in air containing a saturating amount of CO₂ (5 %). The reduction of the light limited rate of photosynthesis (at 20 W × m⁻²) was the same at both CO₂ levels.     

Photosynthesis and transpiration of tomato and CO2 fluxes in a greenhouse under changing environmental conditions in winter

Responses of tomato leaves in a greenhouse to light and CO₂ were examined at the transient stage at the end of winter, when both photoperiod and irradiance gradually increase. Additionally, CO₂ fluxes were calculated for a greenhouse without supplementary lighting and without CO₂ enrichment based on CO₂ sinks (plant photosynthesis) and CO₂ sources (plant and substrate respiration). In January, tomato leaves in the greenhouse showed low photosynthesis with a maximum assimilation of 6–8 μmol CO₂ m⁻² s⁻¹, a quantum yield of 0.06 μmol CO₂ μmol⁻¹ photosynthetic active radiation (PAR) and a low light compensation point of 26 μmol PAR m⁻² s⁻¹, a combination which classifies them as shade leaves. In February, tomato leaves increased their light compensation point to 39 μmol PAR m⁻² s⁻¹ and quantum yield to 0.08, the former indicating the adaptation to increased irradiance and photoperiod. These tomato leaves increased their transpiration from 0.4 to 0.9 in January to ∼2 mmol H₂O m⁻² s⁻¹ in February. Both photosynthesis and transpiration were primarily limited by light but neither by stomatal conductivity nor by CO₂. In January, light response of photosynthesis, dark respiration and transpiration were negligibly affected by increasing CO₂ concentrations from 600 to 900 ppm CO₂ under low light conditions, indicating no benefit of CO₂ enrichment unless light intensity increased. In February, tomato leaves were photoinhibited at inherent greenhouse CO₂ concentrations on the first sunny day; this photoinhibition was further enhanced by an increased CO₂ concentration of 1000 ppm. CO₂ fluxes in the greenhouse appeared strongly dependent on solar radiation. After exceeding the light compensation point in the morning, greenhouse CO₂ concentrations decreased by 58 or by 110 ppm CO₂ h⁻¹ on a sunny day in January or February and by 23 ppm on overcast days in both months. Calculated per overall tomato canopy, plant photosynthesis contributed 42–50% to the morning CO₂ depletion in the greenhouse. Dark respiration of tomato leaves was ∼2 μmol CO₂ m⁻² s⁻¹ in January and ∼3 μmol CO₂ m⁻² s⁻¹ in February. This dark respiration resulted in rises of 15 and 17 ppm CO₂ h⁻¹ at night in the greenhouse compartment and was identified as primary source of CO₂. Respiration of the substrate used to grow the plants, which produced 7.3 ppm CO₂ h⁻¹, was identified as secondary source of CO₂. The combined plant and substrate respiration resulted in peaks of up to 900 ppm CO₂ in the greenhouse before dawn.     

An in vivo analysis of the effect of SO2 fumigation on photosynthesis in Zea mays.

Fumigation of leaves with SO₂ can reduce the capacity for photosynthetic CO₂ uptake even in the absence of visible symptoms of damage. In vitro studies suggest that this invisible injury to intact leaves could be affected by damage to each of the main stages in the photosynthetic process. Reduced stomatal apertures may also reduce photosynthesis following SO₂ fumigation. The responses of CO₂ uptake by leaves to intercellular CO₂ concentration and to absorbed light provide information for quantitative separation of the in vivo contribution of the different stages of photosynthesis to reduction in overall rate. This study uses these techniques to examine the basis of reduction in CO₂ uptake in Zea mays cv. LG11 leaves following short-term fumigation with SO₂. Fumigation with 33 μmol m^–3 SO₂ for 30 min reduced light saturated CO₂ uptake by about one-third. An even greater reduction in light limited CO₂ uptake was observed and with no significant change in light absorptance this was attributed to a reduced quantum yield of photosynthesis. The light saturated CO₂ uptake rate and the stomatal conductance decreased in parallel. However, the relationship of CO₂ uptake to the intercellular CO₂ concentration suggested that the reduced stomatal conductance did not account for the reduced rate of CO₂ uptake following fumigation. Both the initial slope and plateau of this relationship were significantly reduced, suggesting that both carboxylation efficiency and capacity for regeneration of CO₂ acceptor were diminished by SO₂ fumigation. The operating intercellular CO₂ concentration indicated that both processes were co-limiting, before and after fumigation. The time required for induction of photosynthetic CO₂ uptake on illumination was approximately doubled following SO₂ fumigation, showing that fumigation impairs the ability of the photosynthetic apparatus to adapt to fluctuations in light level.     

Analysis of steady state photosynthesis in alfalfa leaves

A method for carrying out kinetic tracer studies of steady state photosynthesis in whole leaves has been developed. An apparatus that exposes whole leaves to ¹⁴CO₂ under steady state conditions, while allowing individual leaf samples to be removed as a function of time, has been constructed. Labeling data on the incorporation of ¹⁴C into Medicago sativa L. metabolite pools are reported. A carbon dioxide uptake rate of 79 micromoles ¹⁴CO₂ per milligram chlorophyll per hour was observed at a CO₂ level slightly below that of air. Several actively turning over pools of early and intermediate metabolites, including 3-phosphoglyceric acid, glycerate, citrate, and uridine diphosphoglucose, showed label saturation after approximately 10 to 20 minutes of photosynthesis with ¹⁴CO₂ under steady state conditions. Alanine labeling increased more rapidly at first, and then at a lower rate as saturation was approached. Sucrose was a major product of photosynthesis and label saturation of the sucrose pool was not observed. Labeled carbon appeared rapidly in secondary metabolites. The steady state apparatus used has numerous advantages, including leaf temperature control, protection against leaf dehydration, high illumination, known ¹⁴CO₂ specific radioactivity, and provision for control and adjustment of ¹⁴CO₂ concentration. The apparatus allows for experiments of long duration and for sufficient sample points to define clearly the metabolic steady state.     

Insights of carbon assimilation and allocation in young cork oak (Quercus suber L.) plants using Carbon-14

¹⁴C methods were applied to young, woody, branched and well-watered cork oak (Quercus suber L.) plants to determine carbon assimilation and its distribution among plant organs. Carbon assimilation rates by attached leaves clamped in a foliar ¹⁴CO₂ assimilation chamber containing 3.7 × 10⁴ Bq of a portable ventilated diffusion porometer were measured at different ¹⁴CO₂ pulse-labeling periods (15, 30, 45, 60 and 120 s) in summer. Allocation of recently fixed C by attached leaves within plants was evaluated 7 days after a 60-min of 5.6 MBq of ¹⁴CO₂ pulse-labeling in late winter. ¹⁴CO₂ pulse-labeling was separately induced on leaves of a lower branch, two opposite branches at the same lower level, a middle branch and a top branch. ¹⁴C activity incorporated into the plants was measured by liquid scintillation and autoradiography. Our results show the optimum ¹⁴CO₂ pulse-labeling period is between 15 and 30 s, which corresponds to 9.81 ± 0.15 and 9.16 ± 0.12 µmol m⁻² s⁻¹ C assimilation rates in summer, respectively. The investment of current assimilates ranged from 18 to 29% in leaves, 1 to 7% in lateral branches, 0 to 3% in the stem and over 65% in roots, in late winter. Roots displayed the greatest sink strength for the total ¹⁴C recovered by whole-plants. These results were expected because the trial was done in winter, when cork oak does not produce their leaves. Our results highlight the contribution of current assimilates for growth and maintenance of roots, in young woody plants under Mediterranean climate.     

Intermediates Of Photosynthesis in Acetabularia mediterranie Chloroplasts

The chloroplast fraction isolated from Acetabularia mediterranie was exposed to ¹⁴CO₂ as NaH¹⁴CO₃ in light and darkness, and soluble radioactive compounds were analyzed at frequent intervals. The behavior of Calvin cycle intermediates indicates that this cycle was responsible for much of the carbon fixation in the chloroplasts. However, a substantial part of recently fixed carbon was metabolized via glycolic and glyceric acids. Possible pathways for their metabolism are discussed. Some carboxylation of C₃ acids was suggested by the behavior of phosphoenolpyruvate and malate. A number of amino acids were formed. Small amounts of such compounds as citrate, succinate, and fumarate not usually associated with photosynthesis might have been derived from a low level of mitochondrial contamination. About one-third of the carbon fixed in light was present in acid-labile insoluble compounds other than polysaccharides or proteins. Dark fixation of CO₂ was very small compared with photosynthesis.     

PHOSPHORUS LIMITATION AND CARBON METABOLISM IN A UNICELLULAR ALGA: INTERACTION BETWEEN GROWTH RATE AND THE MEASUREMENT OF NET AND GROSS PHOTOSYNTHESIS1

Chlamydomonas reinhardii Dangeard was grown in continuous culture under P limitation at a range of dilution rates. Carbon uptake measurements were performed using double isotope (¹²C/¹⁴C) techniques and the fluxes of carbon in the light and dark were analysed over the range of growth rates. ¹⁴C uptake was shown to be equal to gross photosynthesis only at maximum relative growth rates; at low relative growth rates ¹⁴C uptake approximated net photosynthesis. The altered pattern of C uptake was found to be due to the suppression of dark respiration in the light and the release of ¹⁴C0₂ from respiratory pathways at low relative growth rates. Metabolic channelling of ¹⁴C from photosynthetic pathways to respiratory pathways occurred at low growth rates as the specific activity of the respired CO₂ reached 45% of the input gas mixture. These data are discussed in the light of the controversy concerning the measurement of gross and net photosynthesis in natural populations and in the light of models of ¹⁴C uptake in single celled algae. Existing models are shown to be adequate for high relative growth rates but not for low relative growth rates under P limitation.     

Effect of nitrate infusion into the shoot apoplast on photosynthesis and assimilate transport in symplastic and apoplastic plants

The shoots of fireweed (Chamerion angustifolium (L.) Holub) and common flax (Linum usitatissimum L.) were infused with 50 mM KNO₃ solution to compare the influence of nitrate on photosynthesis and assimilate export from leaves in plants with the symplastic and apoplastic phloem loading, respectively. The infusion of nitrate in the shoots of both plant species lowered ¹⁴CO₂ fixation and enhanced the assimilate transport in the upward direction. Irrespective of the phloem loading type, the incorporation of ¹⁴C into sucrose decreased in nitrate-treated seedlings exposed to assimilation for short (3 min) periods. However, when shoots were sampled 3 h after ¹⁴CO₂ fixation, the content of ¹⁴C-labeled sucrose was higher in treated plants than in control seedlings infused with water. In fireweed, in contrast to flax, a similar temporal pattern was also characteristic for ¹⁴C incorporation into oligosaccharides. Within 3 h after nitrate infusion into the fireweed apoplast, the mitochondria and the cell vacuolar system underwent ultrastructural changes indicative of the increase in cytosolic osmotic pressure. At the same time, we observed accumulation of fibrillar inclusions in cell vacuoles of vascular bundles. It is concluded that the mechanisms of nitrate influence on photosynthesis and sugar export in leaves of symplastic and apoplastic plants are similar to a certain extent and involve the blocking of pores in phloem tubes, initiated by the NO-signaling system.     

THE UPTAKE OF GLUCOSE BY CHLAMYDOMONAS SP.12

The glucose uptake of a species of Chlamydomonas was studied at various concentrations of d -glucose plus glucose-1-¹⁴C (0.003–10.0 mg/liter) and at various light levels (0–220 ft-c). The alga grows at 4 C either in the light or in the dark with added glucose, cellobiose, maltose, or fructose. Uptake of glucose could be described by the Michaelis-Menten equation, and both the maximum velocity of uptake and the half-saturation constant increased when the cells were exposed to glucose in the dark. However, the high value of the half-saturation constant (5 mg glucose/liter) compared with the low levels of glucose in nature (5–10 μg/liter) makes it unlikely that a transport system is effective under natural conditions. Even if a total of 10.0 mg/liter of glucose plus other organic compounds were available as substrate, the rate of photosynthesis would still be more than 10 times higher (at 220 ft-c) than the rate of organic substrate uptake. Light had no effect on the total uptake of glucose but did reduce the percentage of ¹⁴CO₂ evolved from 61% of the total ¹⁴CO taken up in the dark to 0% at 220 ft-c. This decrease could be due to either preferential use of the ¹⁴CO₂ in photosynthesis or of the photosynthate in respiration.