An Analysis of Osterhout and Hill's Salt Bridge Experiments in Characeae Internode

Conduction of action potentials in Chara internodal cells wasblocked at a 5%-urethane treated region. The action potentialscould be propagated beyond this region when an electric bridgewas built across it with a low enough resistance that the actioncurrent across it could depolarize the membrane at the distaljunction of the bridge up to the threshold level. After recoveryof propagation, the configuration of the action current flowingthrough the bridge changed from monophasic to diphasic. Coursesof the monophasic action current and the depolarizing potentialof the resting membrane were in parallel with the course ofaction potential, although they were slightly out of phase witheach other. The magnitudes of the current and depolarizing potentialagreed well with those estimated using a simplified equivalentcircuit of the bridge arrangement or with those observed usingan electric model circuit. ¹Present address: Department of Physiology, Tohoku UniversitySchool of Dentistry, Seiryo-machi, Sendai 980, Japan. ²Present address: Biology Laboratory, Kyoritsu Women's University,Hachioji, Tokyo 193, Japan. (Received December 18, 1985; Accepted March 26, 1986)     

Chloride Electrochemical Potentials and Membrane Resistances in Nitella translucens

The chloride electrochemical potential difference between theinside of cells of Nitella translucens and the bathing mediumhas been measured by a direct electrical method employing Ag/AgClelectrodes. The membrane potential has been measured by meansof conventional salt bridge microelectrodes. These data havebeen used to calculate the internal chloride concentration ofthe cells; the mean value obtained was 39 mM. This chlorideelectrochemical potential difference has been short-circuitedthus causing an outward (depolarizing) electric current to flowthrough the cell membrane. The resulting membrane depolarizationhas been measured at two points along the length of the cellenabling the membrane resistance and space constant to be deduced;the respective values obtained were 24.8 Kcm² and 3.0 cm. Itis suggested that these experiments lend additional supportto the hypothesis that during the action potential in the Characeaethere occurs a transient increase in the chloride conductanceof the plasmalemma.     

Cellular Structure and Light Absorbtion in Leaves of Frithia pulchra (Mesembryanthemaceae)

In order to quantify the structural differences between celltypes of leaves from a ‘ window’ plant, an ultrastructuralmorphometric analysis was made of the epidermal, window andchlorenchyma tissues of Frithia pulchra. Epidermal cells arethe largest cells found in Frithia leaves and are characterizedby the presence of a thick outer tangential cell wall and numerousvacuolar inclusions. Epidermal tissue has an optical densityof 0.30. The transparent window tissue (i.e. optical density= 0.08) has a uniform ultrastructure throughout the length ofthe leaf. The vacuome comprises aproximately 97 per cent ofthe protoplasmic volume of window cells. Chlorenchyma cellspossess thin cell walls and are surrounded by numerous intercellularspaces. Cells of the apical chlorenchyma tissue possess approximately30 plastids per cell. These chloroplasts have an average individualvolume of 220 µm². Cells of the basal chlorenchyma tissuecontain chloroplasts that are five to six times smaller andmore numerous than those in cells of the apical chlorenchyma.The increased volume of chloroplasts in the apical comparedwith basal chlorenchyma cells (i.e. 31.4 and 20.2 per cent ofthe protoplasm, respectively) is positively correlated withtheir optical densities of 1.46 and 0.97, respectively. Frithia pulchra, stereology, leaf, light absorption, window plant     

Temporal Relationship between Action Potential and Ca2+ Transient in Characean Cells

Temporal relationship between the action potential and the changein cytosolic Ca²⁺ concentration was investigated in cells offour species of Characeae, Chara corallina, Nitellopsis obtusa,Nitella flexilis and Nitella axilliformis. The Ca²⁺ transientwas detected by light emission from Ca²⁺-sensitive photoproteinaequorin injected into the cytoplasm. Action potential was triggeredby an outward or sometimes inward electric current pulse of20–50 ms in most cases. In all species the action potentialstarted at almost the same time as the time at which the lightemission from aequorin began to increase. Also the peak of actionpotential almost coincided with that of light emission, whichis in contrast with the slower Ca²⁺ transient in Chara reportedby Thiel et al. [(1997) J. Exp. Bot. 48: 609]. A discussionwas made on the origin of Ca²⁺ transient and the ionic processesduring membrane excitation. (Received July 2, 1998; Accepted October 5, 1998)     

Photo-induced H+ Transport between Chloroplasts and the Cytoplasm in a Protoplasmic Droplet of Characeae

Svintitskikh, V. A., Andrianov, V. K. and Bulychev, A. A. 1985.Photo-induced H⁺ transport between chloroplasts and the cytoplasmin a protoplasmic droplet of Characeae.—J. exp. Bot. 36:1414–1429. The effects of light on the membrane potential and cytoplasmicpH of isolated droplets of protoplasm from Nitella have beenstudied using microcapillary electrodes and pH-sensitive antimonymicro-electrodes. Illumination of chloroplast-containing dropletscaused a change of the membrane potential with a concomitantacidification of both the cytoplasm and the outer medium, butit had no effect on the electrical resistance of the surfacemembrane. Treatment of protoplasmic droplets with uncouplers(NH₄Cl and CCCP) resulted in a complete inhibition of the light-inducedacidification of the cytoplasm, whereas the energy transferinhibitor DCCD had no effect. A correlation between the formationof a pH gradient across the thylakoid membrane and the acidificationof the cytoplasm was explicable in terms of the assumption ofrestricted spatial communication between the intra-thylakoidvolume and the cytoplasm in intact chloroplast. The photo-inducedacidification of the boundary layer of an external medium wasmarkedly stimulated under the action of inhibitors of H⁺-ATPaseDCCD and DES. These findings suggest that the active extrusionof H⁺ from the cytoplasm into the external medium is not drivenby an ATPase, although H+-conducting channels of membrane ATPaseprovide a pathway for a passive diffusion of protons from outsideinto the cytoplasm Key words: Transport of protons, protoplasmic droplet, intact chloroplasts, Characeae     

Studies on Mechanoperception in Characean Cells: Pharmacological Analysis

The mechanisms for generating receptor potentials and actionpotentials upon mechanical stimulation were studied in internodalcells of Chara. Receptor potentials and the subsequent actionpotentials could be generated even when the electrogenic protonpump was inhibited, indicating that the proton pump does notplay a central role in generating receptor potentials and actionpotentials. The involvement of Ca²⁺ and/or Cl^– channelsin both receptor and action potentials was suggested, basedon the equilibrium potentials of these ions across the plasmamembrane. Inhibitors of the Ca²⁺ channel, Cl^– channeland stretch-activated channel could not inhibit generation ofthe receptor potential. These findings suggested that the channelsinvolved in generating the receptor potential are insensitiveto these channel inhibitors, although all inhibitors significantlyinhibited the action potential. (Received July 26, 1996; Accepted November 19, 1996)     

Action of Mono- and Difluorodinitrobenzene on Induced Electrical Modifications by External pH Changes in Nitella

The action of mono- (FNB) or difluorodinitrobenzene (DFNB) onion permeability is mainly attributed to its interactionwithamino groups of the membrane by dinitrophenylation. Nitella cells were dimtrophenylated at pH 7.3 and the membranepotential and electrical resistance were then measured in acidicor basic solutions. No matter what the pH value was, FNB andDFNB induced a depolarization of the membrane potential andcaused a diminution of resistance. However these effects ofFNB and DFNB were more drastic at alkaline pH and in the presenceof a weak concentration of potassium. Neither the addition of0.1 mM calcium nor the substitution of chlorides by nitratesmodified the DFNB effect. These results are compatible withthe assumption that the DFNB binding to the membrane leads toan augmentation of the negative charges of the membrane bringingabout an increased cation conductance and a modification ofthe affinity of a K⁺/H⁺exchange pump. The transient responseof the membrane potential at the time of dinitrophenylationwas used to roughly estimate the total density of amino groupsof the membrane of Nitella.     

CELL WALL POTENTIAL IN NITELLA

In the process of inserting a microelectrode into the vacuoleof Nitella three potential levels were recorded. The first onewas at a water phase outside the cell wall, the second one inthe cell wall and the third one across the plasmalemma. Thefirst potential was variable with the distance from the surfaceof the cell wall. When the external solution was 10^–4M KCl, the second potential level was –90 mv and the thirdone –170 mv against an external reference electrode. Thesepotentials were less negative (more negative) with the increase(decrease) of the external KCl concentration and varied to someextent among samples. The vacuolar potential measured againstthe cell wall phase was, therefore, –80 mv inside negativeto outside. A large potential change such as action potentialwas observed only across the plasmalemma. An overshoot of theaction potential of Nitella flexilis was observed very often,when the vacuolar potential was measured against the cell wallphase. This work was supported by a Research Grant from the Ministryof Education of Japan. Part of this work was performed whenR. NAGAI was a Yukawa Research Grant fellow.     

An Analysis of Ultrastructural Changes during Oosphere-initial Development in Oogonia from Ca2+-sufficient and Ca2+-deficient cultures of Saprolegnia terrestris Cookson ex Seymour

The central vacuole system of oogonia of Saprolegnia terrestrisfrom Ca²⁺-sufficient cultures was fully enlarged prior to theformation of oosphere initials, which did not involve cleavagevesicles. In oogonia with fully-enlarged central vacuole systems,subsidiary vacuoles at the periphery of the system sometimescontained dense bodies, and dense-body profiles were sometimespresent within sections of the central vacuole system itself.As the central vacuole system enlarged, volume densities ofdense-body vesicles, peripheral vacuoles, lipid bodies and thecytoplasmic matrix decreased relative to total oogonial volume(peripheral protoplasm volume plus central vacuole volume),while the volume density of nuclei increased and that of mitochondriaremained constant. Relative to the peripheral protoplasm only,volume densities of dense-body vesicles, lipid bodies and mitochondriaincreased and volume densities of peripheral vacuoles and ofthe cytoplasmic matrix decreased, while the volume density ofnuclei increased during central vacuole enlargement but subsequentlydecreased during formation of oosphere initials. Under conditionsof Ca²⁺ deficiency, the volume densities of mitochondria andof the cytoplasmic matrix were significantly increased, whilethat of lipid bodies was significantly decreased, at early stagesof oogonial development; the volume densities of other organelleswere not significantly altered at any stage. Saprolegnia terrestris, oogonia, development, calcium, ultrastructure, stereology     

Effects of cations on the sugar receptor-site of the blowfly, Phormia

1) Ca^{+ +} (1 to 10 mM) lowered the binding affinity of sugarreceptor-site for sucrose in the labellar sugar receptor ofthe blowfly, Phormia regina, without changing the maximum-responseamplitude. It also elevated the values of the Hill coefficient(n_H) in some degrees. 2) Other divalent cations such as Mg^{+ +}, Ba^{+ +} or Cd^{+ +} alsoshowed almost the same property as above. The sequence of theeffect is as follows: Ba^{+ +}, Mg^{+ +} x Ca^{+ +} x Cd^{+ +}. Trivalentcation, La^{+ + +} (1 mM), changed the value of n_H from 1 (La^{++ +}-free) to 2. 3) On the contrary, the action of monovalent cations such asK⁺ or Na⁺, of which ionic strength was made the same as thatof the divalents hardly suppressed the response. 4) The results obtained do not support the hypothesis, at leaston the sugar receptor of the fly, that the receptor potentialis attributable to a change of the surface potential (zeta potential)as is proposed for the frog sugar receptor.     

Permeability of Lipophilic Cations

The permeability (P) of a lipophilic cation, triphenylmethylphosphonium(TPMP⁺) which is frequently used as a membrane potential probe,has been measured in Chara australis (Charophyceae). P_TPMP+across biological membranes is usually thought to be very highbut this is not the case across the plasmalemma of Chara. Thepermeability of TPMP⁺ across the plasmalemma was found to betypical of inorganic cations, about 1.0 nm s^–1. Estimateswere made of the permeability of lipophilic cations across someother cell membranes, based on previously published work. Thepermeability of TPMP⁺ across the plasma membranes of the redalga, Griffithsia monilis and the blue-green alga, Anabaenavariabilis was about 2–5 nm s^–1. The permeabilityof TPMP⁺ across the plasma membranes of eukaryotes and prokaryotesappears to be similar. The permeability of lipophilic cationsacross the cristae of isolated mitochondria are exceptionallyhigh, about 170 nm s^–1. TPMP⁺ did not behave as a thiamineanalogue in Chara, unlike in the case of yeast. The means ofentry of TPMP⁺ into the Chara cell, driven by the electrochemicalgradient across the plasmalemma, has not been identified. Thepresence of a second lipophilic cation probe, DDA⁺ (dibenzyldimethylammonium),caused a decrease in the uptake flux of TPMP⁺; this suggeststhat the two lipophilic cations compete for the same site atthe surface of the plasmalemma. Key words: Chara australis, TPMP⁺, Permeability, Lipophilic cation     

ADP-ribose gates the fertilization channel in ascidian oocytes

We report an ionchannel in the plasma membrane of unfertilized oocytes of the ascidianCiona intestinalis that is directly gated by the second messenger ADP-ribose. The ion channel is permeable to Ca²⁺ andNa⁺ and ischaracterized by a reversal potential between 0 and +20 mV and aunitary conductance of 140 pS. Preinjection of theCa²⁺ chelator1,2-bis(2-aminophenoxy)ethane-N,N,N',N'-tetraacetic acid (BAPTA) or antagonists of intracellularCa²⁺ release channels into oocytesdid not inhibit the ADP-ribose current, demonstrating that the channelis activated in a Ca²⁺-independentmanner. Both the fertilization current and the current induced by theinjection of nicotinamide nucleotides are blocked by nicotinamide,suggesting that the ADP-ribose channel is activated at fertilization ina nicotinamide-sensitive manner. These data suggest that ascidian spermtrigger the hydrolysis of nicotinamide nucleotides in the oocyte toADP-ribose and that this mechanism is responsible for the production ofthe fertilization current.

     

Demonstration of Voltage Dependency of Light-induced Potential Change in Chara

The electromotive force (E_m) of the plasma membrane of the tonoplast-freecell of Chara australis decreased when the electrogenic pumpwas stopped by removing ATP or Mg²⁺ from the cell. Such a cellshowed a rapid light-induced potential change (rLPC). Threefactors were considered to be responsible for the generationof rLPC; removal of Mg-ATP, stoppage of the electrogenic pumpand membrane depolarization per se. Tonoplast-free cells having enough Mg-ATP occasionally showedsmall E_m (–87— –116 mV) due to stoppage ofthe electrogenic pump. Since the rLPC was induced in such cells,removal of Mg-ATP cannot be the factor. Cells having large E_mdue to active pump activity also showed rLPC when the potentialdifference across the plasma membrane (V_m) was depolarized byan outward electric current; evidence that not the stoppageof the pump but membrane depolarization is a necessary conditionfor the generation of rLPC. In the rLPC Vm always changed in the negative direction. However,calculation of E_m revealed the existence of a reversal potential[ (E_m)rev] toward which E_m converged from either more negativeor more positive values. The (E_m)rev approximately coincidedwith the equilibrium potential for K⁺ across the plasma membrane.Intracellular anions occupying lower positions in the lyotropicseries inhibited rLPC. (Received February 9, 1981; Accepted May 16, 1981)     

Electrophysiological Techniques and the Magnitudes of the Membrane Potentials and Resistances of Nitella translucens

The membrane resistance of internodal cells of Nitella translucensincreased by 50 per cent during the first 5 h after insertionof two microelectrodes into the vacuole even when precautionswere taken to eliminate external disturbances. The insertionof a third microelectrode into the cytoplasm did not affectthe resistance. In artificial pond water the final value forthe plasmalemma resistance was 112 k cm² and that for the tonoplastwas 6 k cm². The increase in the membrane potential after thefirst hour was less than 10 per cent. A recent suggestion that accurate measurements of the plasmalemmaresistance can be made with a microelectrode outside the plasmalemma,but in close contact with it, is criticized. Tests were made of the claim that leakage of current at thepoint where microelectrodes enter the cytoplasm gives rise toa local increase in current density at the tonoplast and henceleads to an overestimate of the tonoplast resistance. Valuesfor the tonoplast resistance obtained when the cytoplasmic microelectrodewas inserted through the plasmalemma were similar to those observedwhen it was pushed across the cell and inserted through thetonoplast at a point remote from the postulated current leakage.Furthermore, the tonoplast resistance stayed remarkably constantwhen the plasmalemma resistance varied in a way which wouldcause different proportions of the applied current to pass throughthe leak resistance and produce variations in the apparent tonoplastresistance. It is concluded that published values of the tonoplastresistance are not grossly inaccurate.     

Propagation of Action Potential over the Trap-lobes of Aldrovanda vesiculosa

In the trap-lobes of Aldrovanda vesiculosa, an action potentialwas generated in a cell located at the base of a sensory hairstanding on the margin of central portion of the paired lobes,which spread over this portion within about 40 msec. The electricalcoupling ratio for two adjacent cells in the middle layer ofthe lobes was 0.8. This showed that an action potential generatedin a cell of the trap-lobes must spread electrotonically toadjacent cells. An analysis of an equivalent circuit for thecell injected with current and its neighboring cells in themiddle layer of the lobes showed that the resistances of theplasmalemma, tonoplast and junction between two cells were 11.1,4.7 and 0.56 M, respectively. Numerous plasmodesmata in thejunctional walls of the cells were found by electron microscopy.The low resistance of the junction between cells must be dueto the presence of the plasmodesmata which allows an electrotonictransmission of action potential from cell to cell. (Received January 23, 1982; Accepted April 13, 1982)     

Estrogen modulates paracellular permeability of human endothelial cells by eNOS- and iNOS-related mechanisms

Estradiol had abiphasic effect on permeability across cultures of human umbilical veinendothelial cells (HUVEC): at nanomolar concentrations it decreased theHUVEC culture permeability, but at micromolar concentrations itincreased the permeability. The objective of the present study was totest the hypothesis that the changes in permeability were mediated bynitric oxide (NO)-related mechanisms. The results revealed dualmodulation of endothelial paracellular permeability by estrogen.1) An endothelial NO synthase (eNOS)-, NO-, and cGMP-related,Ca²⁺-dependent decrease inpermeability was activated by nanomolar concentrations of estradiol,resulting in enhanced Clinflux, increased cell size, and increases in the resistance of thelateral intercellular space(R_LIS) and inthe resistance of the tight junctions(R_TJ); theseeffects appeared to be limited by the ability of cells to generate cGMPin response to NO. 2) An inducibleNO synthase (iNOS)- and NO-related,Ca²⁺-independent increase inpermeability was activated by micromolar concentrations of estradiol,resulting in enhanced Clefflux, decreased cell size, and decreasedR_LIS andR_TJ. We conclude that the net effect on transendothelial permeability across HUVEC depends on the relative contributions of each of these two systems tothe total paracellular resistance.     

Evidence for electrogenic active ion transport across the frog olfactory mucosa in vitro

We present the first electrophysiological evidence for electrogenicion transport across the frog olfactory mucosa in vitro. Whenthe isolated dorsal mucosa was placed in an Ussing chamber andbathed symmetrically in amphibian Ringer's, the ciliated sidebecame electronegative (V = –5.2 mV ± 0.7 mV).The resistance of the mucosal preparation was 148 ± 4 cm². The true short-circuit current was obtained as the intersectionof the I–V curve with the current axis after correctingfor the series solution resistance. The average value of theshort-circuit current was 35.9 µA/cm². The I–V relationwas linear over the applied potential range of ± 16mV.The magnitude of the specific resistance of the olfactory mucosais comparable to values reported for various actively transportingrespiratory and oral cavity epithelia. Because the geometricalarea of the aperture used to normalize both the short-circuitcurrent and the resistance undoubtedly underestimates the actualarea of the dorsal olfactory epithelium, the specific resistanceand the short-circuit current are probably underestimated andoverestimated, respectively. Therefore, the nominally low resistanceneed not imply a leaky epithelium. Substitution of NO₃^–for Cl^– caused the current to increase and the resistanceto decrease. These results suggest that cation absorption playsa role in the sign of the short-circuit current. The in vitropreparation responded to the odorant ethyl n-butyrate by givingan electro-olfactogram (EOG)-like voltage transient which wassuperimposed on the steady-state potential created by activeion transport. The significance of these results is discussedfrom the perspective of the peripheral events surrounding olfactorytransduction.     

ACTION POTENTIAL OF NITELLA INTERNODES

The ionic current during a non-propagating action potentialis analysed from the voltage clamp experiments. The shape ofthe action potential of the Nitella internode can be reconstructedfrom the data of the voltage clamp experiments. The N-shapedcurrent-voltage characteristics (I-V curve) of the Nitella membraneis not constant with time as it is in the tunnel diode, butdecays with time, converging finally into a delayed rectificationcurve. The temporal locus of the potential at which each I-Vcurve crosses the voltage axis coincides almost exactly withthe action potential. The membrane resistance which is calculatedfrom the slope of the I-V curve at each intersection with thevoltage axis also changes in parallel to the action potential.Such correlations are found in the Nitella not only in the pondwater, but also in high Na, high Ca or high Mg medium, wherethe shape of the action potential is modified in various ways.It is highly probable that the action potential is a locus ofthe change of the membrane potential so that the net membranecurrent may be maintained at zero after the transient modificationof the membrane structure by stimulation. (Received June 30, 1966; )     

Mechanisms of solute efflux from seed coats: whole-cell K+ currents in transfer cell protoplasts derived from coats of developing seeds of Vicia faba L.

In developing seed ofVicia faba L., solutes imported throughthe phloem of the coats move symplastically from the sieve elementsto a specialized set of cells (the thin-walled parenchyma transfercells) for release to the seed apoplast. Potassium (K⁺) is thepredominant cation released from the seed coats. To elucidatethe mechanisms of K⁺ efflux from seed coat to seed apoplast,whole-cell currents across the plasma membranes of protoplastsof thin-walled parenchyma transfer cells were measured usingthe whole-cell patch-clamp technique. Membrane depolarizationelicited a time-dependent and an instantaneous outward current.The reversal potential (E_R of the time-dependent outward currentwas close to the potassium equilibrium potential (E_K and itshifted in the same direction as E_K upon changing the externalK⁺ concentration, indicating that this current was largely carriedby an efflux of K⁺. The activation of the time-dependent outwardK⁺ current could be well fitted by two exponential componentsplus a constant. The instantaneous outward current could alsobe carried by K⁺ efflux as suggested by ion substitution experiments.These K⁺ outward rectifier currents elicited by membrane depolarizationare probably too small to represent the mechanism for the normalK⁺ efflux from seed coat cells. Membrane hyperpolarization morenegative than –80 mV activated a time-dependent inwardcurrent. K⁺ influx was responsible for the inward current asthe current reversed at membrane voltage close to E_K and shiftedin the same direction as E_K when external [K⁺] was varied. Activationof this K⁺inward rectifier current was well fitted with twoexponential components plus a constant. A regulating functionfor this current is suggested. Key words: Potassium outward rectifier, potassium inward rectifier, transfer cell protoplast, seed coat, Vicia faba L