Plasmalemma Voltage Noise in Chara corallina

Voltage noise analysis is applied to plasmalemma ion transport in Chara corallina. There is a component in the noise power spectrum that is probably associated with current fluctuations within passive transport channels, and another component that may be associated either with fluctuations in the number of open channels, or with active transport. The data allow the calculation of time constants that may be attributable to molecular level events in these transport processes.     

The Uptake of Sugars by Chara corallina

The influx of several monosaccharides into Chara corallina wasstudied under varying conditions of temperature, in the presenceof inhibitors, and by the use of competition experiments. Itwas found that the mechanism of transport was stereospecific,and the complex interactions between the sugars were characteristicof a carrier-mediated system. There is reason to believe thatthe carrier involved in this system has a narrower range ofaffinities than is usually attributed to a sugar carrier, forglucose and fructose appear to have different sites of entry,though each can influence the uptake of the other. In additionthe carrier system is situated in the plasmalemma and maintainedby metabolic energy.     

Plasmalemma Transport of HCO3- and OH- in Chara corallina: Non-antiporter Systems

An experimental system was designed to test the obligate couplingbetween HCO₃^– and OH^– fluxes (i. e. a ‘Mitchell-type’antiporter) proposed by Lucas and Smith (1973). The resultsof these experiments demonstrated categorically that the OH^–efflux process can function in the absence of exogenous HCO₃^–at the actual OH^– efflux site. Hence, the obligate couplinghypothesis is invalid. It is proposed that HCO₃^– and OH^–are transported across the plasmalemma ‘independently’,on quite distinct carriers. It is possible, therefore, thatthese fluxes contribute towards determining the electrical propertiesof this membrane when the bathing solution pH value is 6.5.It was also found that HCO₃^– can be transported acrossthe dark segment of a partly illuminated cell. The observedrates were always much less than those obtained in the illuminatedcell segment. The significance of this result is discussed.     

Plasmalemma transport of OH- in Chara corallina: dynamics of activation and deactivation.

The light-mediated, time-dependent rise in the pH value at the center of an alkaline band was analyzed using the methods of numerical analysis. From this analysis an expression of the time-dependent build-up of OH- efflux was obtained for these bands. This information can now be employed to determine whether the light-activated transport of OH- and HCO3- influences the electrical properties of the plasmalemma. The dark-induced deactivation of OH- transport was also characterized, revealing a transition from efflux to a transient influx phase during deactivation. Numerical analysis of the steady-state OH- diffusion pattern, established along the surface of an alkaline band, revealed that the OH- efflux width was wider than previously envisaged. It was also found the OH- sink regions exist on either side of the efflux zone. These, and other characteristics revealed by the numerical analysis, enabled us to extend the OH- transport model proposed by Lucas (J. Exp. Bot. 1975, 26:347).     

The Apparent Induction of Nitrate Uptake by Chara corallina Cells following Pretreatment with or without Nitrate and Chlorate

Nitrate provision has been found to regulate the capacity forChara corallina cells to take up nitrate. When nitrate was suppliedto N sufficient cells maximum nitrate uptake was reached after8 h. Prolonged treatment of the cells in the absence of N alsoresulted in the apparent ability of these cells to take up nitrate.Chlorate was found to substitute partially for nitrate in the‘induction’ step. The effects on nitrate reductionwere separated from those on nitrate uptake by experiments usingtungstate. Tungstate pretreatment had no effect on NO^–₃uptake ‘induced’ by N starvation, but inhibitedNO^–₃ uptake associated with NO^–₃ pretreatment. Chloridepretreatment similarly had no effect on NO^–₃ uptake ‘induced’by N deprivation, but inhibited NO^–₃ uptake followingNO^–₃ pretreatment. The data suggest that there are atleast two mechanisms responsible for the ‘induction’of nitrate uptake by Chara cells, one associated with NO^–₃reduction and ‘induced’ by CIO^–₃ or NO^–₃and one associated with N deprivation. Key words: Nitrate, Chlorate, Chara corallina, Induction     

Sulfhydryl Group Involvement in Plasmalemma Transport of HCO(3) and OH in Chara corallina

The effect of the sulfhydryl reagents (—SH) p-chloromercuribenzene-sulfonic acid (PCMBS), N-ethylmaleimide (NEM), and inorganic mercury on H¹⁴CO₃⁻ assimilation in Chara corallina is reported. Commercial grade PCMBS caused severe inhibition of H¹⁴CO₃⁻ assimilation. Results obtained using purified PCMBS (stock solution passed through a chelating resin) indicated that inhibition observed using unpurified PCMBS was due predominantly to the presence of inorganic mercury (as a contaminant). The inhibitory role of inorganic mercury was verified using HgCl₂. This chemical caused a dramatic inhibition of H¹⁴CO₃⁻ assimilation, while it had little effect on cellular ¹⁴CO₂ fixation. Reversal of the Hg²⁺ inhibition of H¹⁴CO₃⁻ assimilation (in presence of 1.0 millimolar dithioerythritol) was extremely slow, requiring 2 to 3 hours for the reestablishment of control rates. This slow recovery may reflect de novo synthesis of transport proteins.     

Effect of Sulfhydryl Reagents on the Biophysical Properties of the Plasmalemma of Chara corallina

The administration of the sulfhydryl reagent N-ethyl-maleimide (NEM) to internodal cells of Chara corallina caused alterations in the biophysical properties of the plasmalemma, as measured with electrophysiological and radioactive tracer techniques. The membrane potential depolarized to, or near, the calculated Nernst potential for potassium (E_K) after 30 seconds' exposure to 0.1 millimolar NEM. During this time, the ATP level did not decrease below the control value, and the specific membrane resistance did not increase; only upon further exposure to NEM did the resistance approach the value observed in the dark. In the depolarized state, the membrane potential responded to changes in the external potassium concentration in the manner of a K⁺-electrode, but it retained it's relative insensitivity to external sodium.     

Plasmalemma Transport of HCO-3 and OH- in Chara corallina: Inhibitory Effect of Ammonium Sulphate

The influence of (NH₄)₂SO₄ on ¹⁴C assimilation and cyclosisin internodal cells of Chara corallina was investigated. Severeinhibition of ¹⁴C assimilation was found at pH values above7·0, this inhibition being correlated with the exogenouslevel of NH3 rather than NH⁺₄. Cyclosis was also affected athigher concentrations of (NH₄)₂SO₄. This effect was similarlycorrelated with exogenous levels of NH₃. ¹⁴C assimilation was inhibited non-competitively by (NH₄)₂SO₄,the apparent Km being increased from 0·55 to 1·5mM. The results suggest that the site(s) of inhibition is locatedat the plasmalemma, rather than at the chloroplasts. (Evidencein support of in vivo uncoupling of photophosphorylation, bylow concentrations of (NH₄)₂SO₄, was not obtained). Significant perturbation of the OH^– efflux pattern wasobserved as the level of (NH₄)₂SO₄ was increased. Induced migrationof efflux sites indicates that NH₃ may interfere with the cellularmechanism that controls OH^– transport. Using a cell-segmentisolating chamber it was shown that (NH₄)₂SO₄ inhibited OH^–efflux rather than HCO^–₃ transport. This inhibitory effectwas readily reversible. These data are discussed in terms of a possible relationshipbetween the observe NH₄)²SO₄ stimulation of ³⁶Cl^– influxand the effect of this compound on ¹⁴C assimilation.     

Plasmalemma Chloride Transport in Chara corallina: Inhibition by 4,4'-Diisothiocyano-2,2'-Disulfonic Acid Stilbene

Chloride transport, presumably via a Cl⁻-2H⁺ co-transport system, was investigated in Chara corallina. At pH 6.5, the control influx (3.1 picomoles per centimeter² per second) was stimulated 4-fold by an 18-hour Cl⁻ starvation. The stimulated influx was inhibited to 4.7 picomoles per centimeter² per second after a 60-minute pre-exposure to 0.5 millimolar 4,4′-diisothiocyano-2,2′-disulfonic acid stilbene (DIDS). This compares with a nonsignificant inhibition of the control under similar conditions. At 2 millimolar DIDS, both stimulated and control influx were inhibited to values of 1.1 and 2.2 picomoles per centimeter² per second, respectively; in all cases, DIDS inhibition was reversible. Over the pH range 4.8 to 8.5, the control and DIDS-inhibited influx showed only slight pH sensitivity; in contrast, the stimulated flux was strongly pH dependent (pH 6.5 optimum). Inasmuch as changes in pH alter membrane potential, N-ethylmaleimide was used to depolarize the membrane; this had no effect on Cl⁻ influx. A transient depolarization of the membrane (about 20 millivolts) was observed on restoration of Cl⁻ to starved cells. The membrane also depolarized transiently when starved cells were exposed to 0.5 millimolar DIDS, but the depolarization associated with Cl⁻ restoration was inhibited by a 40-minute pretreatment with DIDS. Exposure of control cells to DIDS caused only a small hyperpolarization (about 7 millivolts). DIDS may have blocked Cl⁻ influx by inhibiting the putative plasmalemma H⁺-translocating ATPase. Histochemical studies on intact cells revealed no observable effect of DIDS on plasmalemma ATPase activity. However, DIDS application after fixation resulted in complete inhibition of ATPase activity.

The differential sensitivity of the stimulated and control flux to inhibition by DIDS may reflect an alteration of transport upon stimulation, but could also result from differences in pretreatment. The stimulated cells were pretreated with DIDS in the absence of Cl⁻, in contrast to the presence of Cl⁻ during pretreatment of controls. The differential effect could result from competition between Cl⁻ and DIDS for a common binding site. Our histochemical ATPase results indicate that Cl⁻ transport and membrane ATPase are separate systems, and the latter is only inhibited by DIDS from the inside of the cell.

     

HCO(3) Influx Across the Plasmalemma of Chara corallina: Divalent Cation Requirement

An absolute requirement for divalent cations is reported for H(14)CO(3) (-) influx in Chara corallina. Effective substitution of eluted Ca(2+) by Mg(2+) and Sr(2+) was observed, but Mn(2+) was completely ineffective in restoring H(14)CO(3) (-) transport activity. Similarly, La(3+) could not substitute for Ca(2+) in this system. Low concentrations of ethylenediaminetetraacetate (0.01 to 0.06 mm) significantly enhanced the rate at which H(14)CO(3) (-) transport capacity was lost.Examination of the response of OH(-) efflux, during Ca(2+)-free treatment, indicated that the cellular control over OH(-) efflux remained unaffected until membrane integrity became severely affected. This conclusion was supported by the response of OH(-) efflux to 10 mm K(+). Therefore, assimilation of H(14)CO(3) (-) is not rate-limited by an effect of Ca(2+) elution on the OH(-) transport system. Kinetic experiments indicated that Ca(2+) removal from the membrane resulted in noncompetitive inhibition of H(14)CO(3) (-) assimilation; the apparent Michaelis constant remained unaltered over a wide range of conditions. An hypothesis is presented which suggests that membrane integrity is necessary for HCO(3) (-) transport to occur, but Ca(2+) (Mg(2+), Sr(2+)), per se, must be bound to the transport complex before activity is established.     

Water channels in Chara corallina

Water relations parameters ofChara corallina inter-nodes weremeasured using the single cell pressure probe. The effect ofmercurials, which are recognized as non-specific water channelinhibitors, was examined. HgCl₂ concentrations greater than5 mmol m^–3 were found to inhibit hydraulic conductivity{Lp) close to 90%, whereas pCMPS was found to have no effecton Lp. The activation energy of water flow was increased significantlyfrom 21.0 kJ mol^–1 to 45.6 kJ mol^–1, following theapplication of HgCl₂. These results are in accordance with evidencefor Hg²⁺sensitive water channels in the plasma membrane of charophytes(Henzler and Steudle, 1995; Tazawa et al., 1996). The metaboliceffects must, however, be considered in view of the rapid inhibitionof respiration and the depolarization of the membrane potentialwith HgCl₂ concentrations lower than those found to affect Lp.It was possible to measure simultaneously water relations andmembrane PD, in order to examine the contribution of potassiumchannels to Lp. Cells were induced into a K⁺ permeable state.The K⁺ channels, assumed to be open, were subsequently blockedby various blockers. No significant difference in Lp was foundfor any of these treatments. Finally, the permeability of C.corallina membranes to ethanol was examined. HgCl₂ was foundto cause a decrease in reflection coefficient, coinciding witha decrease in Lp, but there was no change in the ethanol permeabilitycoefficient. This has been interpreted in terms of both thefrictional model and composite model of non-electrolyte membranetransport. Key words: Water channels, Chara, hydraulic, conductivity, membrane transport models, reflection coefficient     

Control of Intracellular pH in Chara corallina during Uptake of Weak Acid

Butyric acid was used to acidify the cytoplasm of cells of Characorallina in order to study the mechanisms that regulate intracellularpH. Butyric acid was found to enter the cell rapidly, predominantlyas the undissociated acid, and to dissociate in the cytoplasmto yield high concentrations of the butyrate anion. A rapidreduction in cytoplasmic pH was followed by partial recovery.The reductions in cytoplasmic pH resulting from butyrate accumulationwere small compared to the proton load calculated from the cytoplasmicbuffering capacity and intracellular dissociation of butyricacid. The cytoplasmic and vacuolar buffering capacities, calculatedfrom titration of cell extracts, were 17.9 and 0.5 mol m^–3per pH unit respectively. It was concluded that pH control in Chara during weak acid accumulationwas mainly due to membrane transport (active efflux) of protons.The factors which might determine the rate and extent of protonefflux, such as the energy supply and the availability of ionsfor charge balance, were examined. Butyrate strongly inhibitedphotosynthesis and caused a slight reduction in the rate ofrespiration. The mechanism of inhibition of photosynthesis isdiscussed in relation to the reported effects of weak acidson isolated chloroplasts. Key words: Cytoplasmic pH, weak acids, Chara     

Plasmalemma Transport of OH in Chara corallina: III. FURTHER STUDIES ON TRANSPORT SUBSTRATE AND DIRECTIONALITY

The identity of the plasmalemma-transported species that develops the alkaline bands of Chara corallina was investigated. The effect of fusicoccin on the rate of HCO₃⁻ assimilation, and on the time-dependent alkaline band pH buildup following low pH flushing, was found to be small, with no stimulatory effect. Computer simulation of the flushing experiments showed that in the experimental situation the alkaline band transport system was slowed down, rather than speeded up, by low pH flushing. A detailed theoretical examination of the maximum rate of proton production from water showed that measured alkaline band fluxes are too large to be explicable in terms of an H⁺ influx system. The experimental and theoretical results indicate that the plasmalemma transport of OH⁻ ions is responsible for the measured negative external electric potential and alkalinity flux which are associated with the alkaline band phenomenon. Consequently, HCO₃⁻ influx across the characean plasmalemma must be charge-balanced by the efflux of OH⁻ ions.     

Influence of Turgor Pressure Manipulation on Plasmalemma Transport of HCO(3) and OH in Chara corallina

A modified version of the osmotic shock technique was used to investigate HCO₃⁻ and OH⁻ transport in the alga Chara corallina. Cell turgor was brought close to zero and then restored. When turgor was reduced to near the plasmolytic point using an osmoticum, little effect was observed on H¹⁴CO₃⁻ assimilation and OH⁻ transport. However, when turgor was recovered in these cells, there was a large reduction in HCO₃⁻ and OH⁻ transport activity. In contrast, when cells were air-dried to zero turgor, and rewetted to restore turgor, no significant effect on OH⁻ transport was observed.     

Intercellular Transport and Photosynthetic Differentiation in Chara corallina

Intercellular transport of ¹⁴C-labelled photoassimilates, bothin isolated upper shoots and in isolated internode-branchletcomplexes of Chara corallina, was measured. The isolated uppershoots were composed of a primary apex, two mature internodes,and three branchlet whorls. A 10 min loading of the isolatedupper shoot with H¹⁴CO₃^– resulted in a greater accumulationof ¹⁴C in the apical complex and branchlets than in the internodes,while a subsequent 50 min chase with unlabelled solution inthe light resulted in a greater accumulation of ¹⁴C in internodesthan in other parts of the shoot. In the isolated internode-branchlet complex, when the apex wasnot detached, the amount of ¹⁴C transported from branchletsto internodes was about fives times that transported from internodesto branchlets. Removal of the apex resulted in a decrease intransport from branchlets to internodes and an increase in transportin the opposite direction. In an attempt to explain the mechanism of the polar transportof photosynthetically fixed carbon between branchlets and internodes,photosynthetic activities of both types of cells were investigated.Detached branchlets have higher photosynthetic ¹⁴C-fixationactivities than those of internodes. Chlorophyll contents, measuredin terms of surface area, in internodes and branchlets werealmost identical. The ribulose-l,5-bisphosphate carboxylase(RuBPCase) activity of branchlets was 1.6 times that of internodes,and the rate of ferricyanide-dependent evolution of oxygen inbranchlets was 1.4 times that in internodes. Key words: Chara, internode, branchlet, polar transport, photosynthesis     

Plasmalemma Transport of OH- in Chara corallina: II. FURTHER ANALYSIS OF THE DIFFUSION SYSTEM ASSOCIATED WITH- OH EFFLUX

The dynamic and steady state aspects of the pH and electricpotential () profiles, that develop in the experimental mediumin association with the photosynthetic assimilation of exogenousHCO^–₃ by internodal cells of Chara corallina, were investigated.A theoretical treatment is presented which explains the originof the phenomenon. This theory was tested by comparing thepH and values generated by a numerical analysis model (whichsimulated the experimental system) against experimental data.Verification of our model indicates that the steady state ionicfluxes, associated with HCO^–3 assimilation (HCO^–₃,OH^–, and CO^23–, are not significantly influencedby the electric potential gradients. The main driving forcecausing the observed fluxes is the diffusion gradient associatedwith the respective ion. By simultaneous measurement of and pH, at the centre of analkaline band, a direct correlation was established betweenlight-activation and dark-deactivation of the OH^– transportsystem and the light-mediated changes in at the cell surface.In addition, under steady state conditions, an almost perfectcorrelation was observed between alkaline band pH centres andthe negative electric potential maxima. These data offer strongsupport for the hypothesis that OH^–efflux, in this system,is an electrogenic process. Based on our present analysis, the profile along the cell indicatesthat, in terms of the spatial aspect of HCO3^– transport,the rate of HCO^–₃ influx varies quite dramatically alongthe length of an internodal cell. This aspect is discussed interms of the cellular integration of OH^– and HCO^–₃transport in this species.     

HCO(3) Influx across the Plasmalemma of Chara corallina: Physiological and Biophysical Influence of 10 mm K

The effect of 10 mm K⁺ on the HCO₃⁻ influx in Chara corallina has been used to distinguish a Ca²⁺-dependent membrane integrity site from the HCO₃⁻ transport site which is also Ca²⁺-dependent (Lucas and Dainty, Plant Physiology 1977 60: 862-867).     

The Influence of Light Intensity on the Activation and Operation of the Hydroxyl Efflux System of Chara corallina

The interrelationships between light intensity and the activationof OH^– bands was investigated. The lag period prior toOH^– efflux activation was longer than the photosyntheticinduction period. It was found that this lag period dependedupon the light regime employed as well as the photosyntheticcapacity of the cell. The response of the cell to low light intensities revealed thatall OH^– bands were not of equal status. Below a criticallight intensity the cell did not develop any bands even afterprolonged illumination. An hypothesis is presented to accountfor these results, interms of total cell OH^– band activationand the regulation of the HCO₃^– and OH^– transportsystems. It is proposed that the electrical properties of theChara corallina plasmalemma, observed at high pH values, canbe explained on the basis of the hypothesis presented in thispaper