Transmembrane Ferricyanide Reduction and Membrane Properties in the Euryhaline Charophyte Lamprothamnium papulosum

The euryhaline charophyte Lamprothamnium papulosum has the abilityto reduce the extracellular electron acceptor ferricyanide (Fe³⁺Cy).Addition of 0.5 mol m^–3 Fe³⁺Cy stimulated H⁺-efflux ata rate of 0.8 H⁺/Fe³⁺Cy-reduced and increased K⁺-efflux intoa potassium-free medium at a rate of 0.66 K⁺/Fe³⁺Cy-reduced.0.5 mol m^–3 Fe³⁺Cy-induced maximum membrane depolarizationfor cells with resting potentials more negative than the diffusionpotential. The peak value of Fe³⁺Cy-induced depolarizationswas similar to the potential obtained by poisoning the electrogenicpump with DCCD. The value of maximum depolarization was determinedby (K⁺)₀. E_m tended to more positive values with increasing(K⁺)₀. Depolarizations coincided with a decrease in membraneresistance (R_m) from a resting value of 1.5 m² to 0.2 m² inthe depolarized state. Depolarization increased the sensitivityof the membrane potential (E_m) to (K⁺)₀. The resting potentialwas only slightly changed when (K⁺)₀ was increased from 3 to15 mol m^–3. The Fe³⁺ Cy-induced depolarized Em changedin a Nernstian fashion when (K⁺)₀ was increased. It is concludedthat Fe³⁺Cy reduction causes a net depolarization current flowacross the plasmalemma. The depolarization shifts the membranefrom a hyperpolarized pump dominated state into a depolarizedK⁺ diffusion state. Key words: Ferricyanide reduction, membrane potential, Lamprothamnium     

Membrane Potentials in Excitable Cells of Aldrovanda vesiculosa Trap-Lobes

The resting membrane potential in excitable cells of Aldrovandatrap-lobes is composed of diffusion and electrogenic potentials.The diffusion potential, about –100 mV in artificial pondwater, was determined from the external K⁺ and Na⁺ concentrations.The permeability ratio, P_Na/P_K of the membrane was estimatedto be about 0.3. The electrogenic potential hyperpolarized themembrane to about –140 mV. The peak value of the actionpotential increased by +26 mV with a tenfold increase in theexternal Ca²⁺ concentration. The action potential was blockedby an application of the Ca²⁺ chelater or the Ca channel blocker,LaCl₃. Cells showed additional Ca²⁺ influx (7.8 pmole/cm² impulse)during membrane excitation. These facts suggest that the transientincrease in Ca²⁺ influx causes the action potential presentin cells of Aldrovanda trap-lobes. ¹ Present address: Jerry Lewis Neuromuscular Research Center,School of Medicine, University of California Los Angeles, LosAngeles, CA90024, U.S.A. ² Present address: Biological Laboratory, Kyoritsu Women's University,Hachioji 193, Japan. (Received September 21, 1983; Accepted September 7, 1984)     

Modeling cell volume regulation in nonexcitable cells: the roles of the Na+ pump and of cotransport systems

The purpose of this study is to contribute to understanding therole ofNa⁺-K⁺-ATPaseand of ionic cotransporters in the regulation of cell volume, byemploying a model that describes the rates of change of theintracellular concentrations ofNa⁺,K⁺, andCl, of the cell volume, andof the membrane potential. In most previous models of dynamic cellularphenomena,Na⁺-K⁺-ATPaseis incorporated via phenomenological formulations; the enzyme isincorporated here via an explicit kinetic scheme. Another feature ofthe present model is the capability to perform short-term cell volumeregulation mediated by cotransporters of KCl and NaCl. The model isemployed to perform numerical simulations for a "typical" nonpolarized animal cell. Basically, the results are consistent withthe view that the Na⁺ pump mainlyplays a long-term role in the maintenance of the electrochemicalgradients of Na⁺ andK⁺ and that short-term cell volumeregulation is achieved via passive transport, exemplified in this caseby the cotransport of KCl and NaCl.

     

Expression and localization of rat NBC4c in liver and renal uroepithelium

Previous studies provided functional evidence for electrogenic Na⁺-HCO₃^– cotransport in hepatocytes and in intrahepatic bile duct cholangiocytes. The molecular identity of the transporters mediating electrogenic sodium-bicarbonate cotransport in the liver is currently unknown. Of the known electrogenic Na⁺-HCO₃^– cotransporters (NBC1 and NBC4), we previously showed that NBC4 mRNA is highly expressed in the liver. In the present study, we performed RT-PCR, immunoblotting, and immunohistochemistry to characterize the expression pattern of NBC4 in rat liver and kidney. For immunodetection, a polyclonal antibody against rat NBC4 was generated and affinity purified. Of the known human NBC4 variants, only the rat NBC4c ortholog was detected by RT-PCR in rat liver, and the molecular mass of the NBC4c protein was 145 kDa. NBC4c protein was expressed in hepatocytes and in the cholangiocytes lining the intrahepatic bile ducts. In hepatocytes, NBC4c was localized to the basolateral plasma membrane, whereas intrahepatic cholangiocytes stained apically. The NBC1 electrogenic sodium cotransporter variants kNBC1 and pNBC1 were not detected by immunoblotting and immunohistochemistry in rat liver. The pattern of localization of NBC4c in the liver suggests that the cotransporter plays a role in mediating Na⁺-HCO₃^– cotransport in hepatocytes and intrahepatic cholangiocytes. Unlike the liver, the rat kidney expressed electrogenic sodium-bicarbonate cotransporter proteins kNBC1 and NBC4c. In kidney, NBC4c also had a molecular mass of 145 kDa and was immunolocalized to uroepithelial cells lining the renal pelvis, where the cotransporter may play an important role in protecting the renal parenchyma from alterations in urine pH. bicarbonate; transport; electrogenic     

Electrical properties of intact pollen grains of Lilium longiflorum: characteristics of the non-germinatingpollen grain

As a first step to characterizing membrane function during theprocess of germination in pollen, the transport characteristicsof Lilium longiflorum Thunbpollen were examined in the quiescentgrains.Membrane voltages were recorded, and conventional voltage-clampmeasurements were carried out with double-barrelled microelectrodes.The resting membrane voltage (V_m) was found to depend on theexternal K⁺; concentration and generally followed the equilibriumpotential for K^plus; (E_k). In some cells a more negative V_mwas measured indicating the presence of an electrogenic pump.The presence of a pump current was also detected by a depolarizationof the plasma membrane after inhibition of ATP synthesis byaddition of CN^– and SHAM. Besides this pump, two othercurrent components were found in the plasma membrane of ungerminatedpollen grains: an outward potassium current (l_k,out) and aninward K+ current (l_k,in). Outward K⁺ currents were detectedat membrane voltages more positive than the resting voltageand were blocked by externally applied TEA⁺ and Ba²⁺. The voltageat which l_k,out was first detected shifted in parallel withthe equilibrium potential for K⁺. By contrast, activation ofl_k,in was less affected by the external K⁺ concentration, exceptthat the magnitude of the inward current increased with K⁺ concentration.The detected current components may be involved in initiationof osmotic water influx for germination by allowing a K⁺ influxafter the membrane voltage has been driven more negative thanE_k by an electrogenic pump. Key words: Pollen, germination, potassium channel, proton pump, voltage-clamp     

Gastric parietal cell secretory membrane contains PKA- and acid-activated Kir2.1 K+ channels

Our objective was to identify and localize a K⁺ channel involved in gastric HCl secretion at the parietal cell secretory membrane and to characterize and compare the functional properties of native and recombinant gastric K⁺ channels. RT-PCR showed that mRNA for Kir2.1 was abundant in rabbit gastric mucosa with lesser amounts of Kir4.1 and Kir7.1, relative to -actin. Kir2.1 mRNA was localized to parietal cells of rabbit gastric glands by in situ RT-PCR. Resting and stimulated gastric vesicles contained Kir2.1 by Western blot analysis at 50 kDa as observed with in vitro translation. Immunoconfocal microscopy showed that Kir2.1 was present in parietal cells, where it colocalized with H⁺-K⁺-ATPase and ClC-2 Cl^- channels. Function of native K⁺ channels in rabbit resting and stimulated gastric mucosal vesicles was studied by reconstitution into planar lipid bilayers. Native gastric K⁺ channels exhibited a linear current-voltage relationship and a single-channel slope conductance of 11 pS in 400 mM K₂SO₄. Channel open probability (P_o) in stimulated vesicles was high, and that of resting vesicles was low. Reduction of extracellular pH plus PKA treatment increased resting channel P_o to 0.5 as measured in stimulated vesicles. Full-length rabbit Kir2.1 was cloned. When stably expressed in Chinese hamster ovary (CHO) cells, it was activated by reduced extracellular pH and forskolin/IBMX with no effects observed in nontransfected CHO cells. Cation selectivity was K⁺ = Rb⁺ >> Na⁺ = Cs⁺ = Li⁺ = NMDG⁺. These findings strongly suggest that the Kir2.1 K⁺ channel may be involved in regulated gastric acid secretion at the parietal cell secretory membrane. H⁺-K⁺-ATPase; hydrogen chloride secretion; parietal cell K⁺ channel     

Ca2+ transients activate calcineurin/NFATc1 and initiate fast-to-slow transformation in a primary skeletal muscle culture

The calcineurin-mediated signal transduction via nuclear factor of activated T cells (NFATc1) is involved in upregulating slow myosin heavy chain (MHC) gene expression during fast-to-slow transformation of skeletal muscle cells. This study aims to investigate the Ca²⁺ signal necessary to activate the calcineurin-NFATc1 cascade in skeletal muscle. Electrostimulation of primary myocytes from rabbit for 24 h induced a distinct fast-to-slow transformation at the MHC mRNA level and a full activation of the calcineurin-NFATc1 pathway, although resting Ca²⁺ concentration ([Ca²⁺]_i) remained unaltered at 70 nM. During activation, the calcium transients of these myocytes reach a peak concentration of 500 nM. Although 70 nM [Ca²⁺]_i does not activate calcineurin-NFAT, we show by the use of Ca²⁺ ionophore that the system is fully activated when [Ca²⁺]_i is 150 nM in a sustained manner. We conclude that the calcineurin signal transduction pathway and the slow MHC gene in cultured skeletal muscle cells are activated by repetition of the rapid high-amplitude calcium transients that are associated with excitation-contraction coupling rather than by a sustained elevation of resting Ca²⁺ concentration. muscle plasticity; NFATc1; resting calcium concentration     

Potassium Transport Across the Membranes of Chara: I. THE RELATIONSHIP BETWEEN RADIOACTIVE TRACER INFLUX AND ELECTRICAL CONDUCTANCE

Smith, J. R., Smith, F. A. and Walker, N. A. 1987. Potassiumtransport across the membrane of Chara. I. The relationshipbetween radioactive tracer influx and electrical conductance.—J.exp. Bot. 38:731–751. The ⁴²K influx () and the electrical conductance (G_m) were measured simultaneously for the ‘membrane’of internodal cells of Chara australis as a function of theexternal [KCl] (K?. In bathing solutions of pH = 5?0, progressively increased from 20?5to 430?60 nmol m^–2 s^–1 and G_m increased from 0?36?0?02to 3?8?0?8 S m^–2 when K? was increased from 0?1 to 10mol m^–3. The resting membrane potential difference (p.d.)was approximately -135 mV for low K? and approached the expectedNernst equilibrium p.d. for K⁺ ions when K? > 1?0 mol m^–3.Measurements of ³⁶Cl influx suggested that the ⁴²K influx waspredominantly electrogenic. The equivalent Goldman permeabilityto K⁺ ions (P_k) was approximately 20–30 nm s^–1 anddid not vary significantly with increasing K?. The equivalentconductance attributable to the electrogenic transport of K⁺ ions was calculated from assuming passive, independent diffusionof K⁺ ions and the ratio was found to be typically close to one. It was also found that themagnitudes of and G_m measuredsimultaneously for each individual cell were also well correlatedfor K? 1?0 mol m^–3, and that the slope of the line ofbest fit was close to one. For each K? it was found that theconductance not attributable to K⁺ translocation and presumablyassociated primarily with the transport of protons or theirequivalents was typically 0?2–0?5 Sm^–2. For K? >1?0 mol m^–3 the results indicated that the transport ofK⁺ ions was essentially independent, i.e. there was no evidencefor flux interactions. The results also indicated that the equivalentconductance derived from the measured ⁴²K influx could usefullyindicate the fraction of the electrical conductance attributableto the translocation of K⁺ ions. Key words: Potassium, conductance, influx     

Role of HERG-like K+ currents in opossum esophageal circular smooth muscle

An inwardlyrectifying K⁺ conductance closelyresembling the human ether-a-go-go-related gene (HERG) current wasidentified in single smooth muscle cells of opossum esophageal circularmuscle. When cells were voltage clamped at 0 mV, in isotonicK⁺ solution (140 mM), stephyperpolarizations to 120 mV in 10-mV increments resulted inlarge inward currents that activated rapidly and then declined slowly(inactivated) during the test pulse in a time- and voltage- dependentfashion. The HERG K⁺ channelblockers E-4031 (1 µM), cisapride (1 µM), andLa³⁺ (100 µM) strongly inhibitedthese currents as did millimolar concentrations ofBa²⁺. Immunoflourescence stainingwith anti-HERG antibody in single cells resulted in punctate stainingat the sarcolemma. At membrane potentials near the resting membranepotential (50 to 70 mV), thisK⁺ conductance did not inactivatecompletely. In conventional microelectrode recordings, both E-4031 andcisapride depolarized tissue strips by 10 mV and also induced phasiccontractions. In combination, these results provide direct experimentalevidence for expression of HERG-likeK⁺ currents in gastrointestinalsmooth muscle cells and suggest that HERG plays an important role inmodulating the resting membrane potential.

     

Pharmacological and biophysical isolation of K+ currents encoded by ether-a-go-go-related genes in murine hepatic portal vein smooth muscle cells

Previous studies have shown that murine portal vein myocytes express ether-à-go-go related genes (ERGs) and exhibit distinctive currents when recorded under symmetrical K⁺ conditions. The aim of the present study was to characterize ERG channel currents evoked from a negative holding potential under conditions more pertinent to a physiological scenario to assess the possible functional impact of this conductance. Currents were recorded with ruptured or perforated patch variants of the whole cell technique from a holding potential of –60 mV. Application of three structurally distinct and selective ERG channel blockers, E-4031, dofetilide, and the peptide toxin BeKM-1, all inhibited a significant proportion of the outward current and abolished inward currents with distinctive "hooked" kinetics recorded on repolarization. Dofetilide-sensitive currents at negative potentials evoked by depolarization to +40 mV had a voltage-dependent time to peak and rate of decay characteristic of ERG channels. Application of the novel ERG channel activator PD-118057 (1–10 µM) markedly enhanced the hooked inward currents evoked by membrane depolarization and hyperpolarized the resting membrane potential recorded by current clamp and the perforated patch configuration by 20 mV. In contrast, ERG channel blockade by dofetilide (1 µM) depolarized the resting membrane potential by 8 mV. These data are the first record of ERG channel currents in smooth muscle cells under quasi-physiological conditions that suggest that ERG channels contribute to the resting membrane potential in these cells. vascular smooth muscle; voltage-dependent K⁺ current; membrane excitability     

Electrophysiological Evidence for an Electrogenic Proton Pump and the Proton Symport of Glucose in the Marine Fungus Dendryphiella salina

The marine hyphomycete Dendryphiella salina (Suth.) Nicot &Pugh has a resting membrane potential of –250 mV (insidenegative). The respiratory inhibitors sodium azide and FCCPinduced a rapid but reversible depolarization of the membraneof at least 180 mV; sodium azide also caused alkalinizationof the medium. Vanadate brought about significant depolarizationbut this was not always reversible. EDTA induced depolarizationthough to a lesser extent. DIDS and SITS caused a depolarizationof around 30–70 mV which was readily reversible, N-ethylmaleimideirreversibly depolarized the membrane by 180–200 mV. Ouabainhad no effect. When external concentrations of H⁺ , K⁺ , Na⁺or Cl^– were changed singly, only changes in H⁺ affectedmembrane potential, with shifts decreasing with increasing pH.Glucose and 3-O-methyl glucose depolarized the membrane in aconcentration-dependent manner which was enhanced by starvationof the hyphae. Recovery occurred in the presence of the hexose.Glucose caused an alkalinization of the medium, with time characteristicssimilar to the membrane potential changes. It is concluded thatthere is an electrogenic proton pump and a proton—glucosesymporter in D. salina. The retention of proton-based transportsystems suggests a terrestrial origin for the fungus. Key words: Marine fungi, Dendryphiella salina, membrane potential, electrogenic proton pump, proton symport, hexose     

The Relationship between the Cell Electrical Potential Difference and Salt Uptake in the Roots of Helianthus annuus

The effect of ringing the stem on the electrical potential difference(PD) in the root cortical cells of H. annuus was studied. PDand salt transport were followed simultaneously. By ringingit was possible to separate the PD from K⁺, , and Cl^– uptake and H⁺ efflux. The uptake of phosphatehowever was found to be closely connected with a component ofthe PD. It was concluded that there is an electrogenic pumpfor phosphate in these roots which generates 60–80 mV.     

Heterologous expression of Na(+)-K(+)-ATPase in insect cells: intracellular distribution of pump subunits

TheNa⁺-K⁺-ATPase is a heterodimeric plasmamembrane protein responsible for cellular ionic homeostasis in nearlyall animal cells. It has been shown that some insect cells (e.g., HighFive cells) have no (or extremely low)Na⁺-K⁺-ATPase activity. We expressed sheepkidney Na⁺-K⁺-ATPase - and -subunitsindividually and together in High Five cells via the baculovirusexpression system. We used quantitative slot-blot analyses to determinethat the expressed Na⁺-K⁺-ATPase comprisesbetween 0.5% and 2% of the total membrane protein in these cells.Using a five-step sucrose gradient (0.8-2.0 M) to separate theendoplasmic reticulum, Golgi apparatus, and plasma membrane fractions,we observed functional Na⁺ pump molecules in each membranepool and characterized their properties. Nearly all of the expressedprotein functions normally, similar to that found in purified dogkidney enzyme preparations. Consequently, the measurements describedhere were not complicated by an abundance of nonfunctionalheterologously expressed enzyme. Specifically, ouabain-sensitive ATPaseactivity, [³H]ouabain binding, and cation dependencieswere measured for each fraction. The functional properties of theNa⁺-K⁺-ATPase were essentially unaltered afterassembly in the endoplasmic reticulum. In addition, we measuredouabain-sensitive ⁸⁶Rb⁺ uptake in whole cellsas a means to specifically evaluateNa⁺-K⁺-ATPase molecules that were properlyfolded and delivered to the plasma membrane. We could not measure anyouabain-sensitive activities when either the -subunit or -subunitwere expressed individually. Immunostaining of the separate membranefractions indicates that the -subunit, when expressed alone, isdegraded early in the protein maturation pathway (i.e., the endoplasmicreticulum) but that the -subunit is processed normally and deliveredto the plasma membrane. Thus it appears that only the -subunit hasan oligomeric requirement for maturation and trafficking to the plasma membrane. Furthermore, assembly of the - heterodimer within theendoplasmic reticulum apparently does not require a Na⁺pump-specific chaperone.

     

pH of TGN and recycling endosomes of H+/K+-ATPase-transfected HEK-293 cells: implications for pH regulation in the secretory pathway

The influences of the gastric H⁺/K⁺ pump on organelle pH during trafficking to and from the plasma membrane were investigated using HEK-293 cells stably expressing the - and -subunits of human H⁺/K⁺-ATPase (H⁺/K⁺-, cells). The pH values of trans-Golgi network (pH_TGN) and recycling endosomes (pH_RE) were measured by transfecting H⁺/K⁺-, cells with the pH-sensitive GFP pHluorin fused to targeting sequences of either TGN38 or synaptobrevin, respectively. Immunofluorescence showed that H⁺/K⁺-ATPase was present in the plasma membrane, TGN, and RE. The pH_TGN was similar in both H⁺/K⁺-, cells (pH_TGN 6.36) and vector-transfected ("mock") cells (pH_TGN 6.34); pH_RE was also similar in H⁺/K⁺-, (pH_RE 6.40) and mock cells (pH_RE 6.37). SCH28080 (inhibits H⁺/K⁺-ATPase) caused TGN to alkalinize by 0.12 pH units; subsequent addition of bafilomycin (inhibits H⁺ v-ATPase) caused TGN to alkalinize from pH 6.4 up to a new steady-state pH_TGN of 7.0–7.5, close to pH_cytosol. Similar results were observed in RE. Thus H⁺/K⁺-ATPases that trafficked to the plasma membrane were active but had small effects to acidify the TGN and RE compared with H⁺ v-ATPase. Mathematical modeling predicted a large number of H⁺ v-ATPases (8,000) active in the TGN to balance a large, passive H⁺ leak (with P_H 10^–3 cm/s) via unidentified pathways out of the TGN. We propose that in the presence of this effective, though inefficient, buffer system in the Golgi and TGN, H⁺/K⁺-ATPases (estimated to be 4,000 active in the TGN) and other transporters have little effect on luminal pH as they traffic to the plasma membrane. pHluorin; H⁺ v-ATPase; trans-Golgi network; organelle pH; H⁺ permeability     

The Na(+)-K(+)-ATPase alpha2-subunit isoform modulates contractility in the perinatal mouse diaphragm

This study uses genetically altered mice to examine the contribution of the Na⁺-K⁺-ATPase ₂ catalytic subunit to resting potential, excitability, and contractility of the perinatal diaphragm. The ₂ protein is reduced by 38% in ₂-heterozygous and absent in ₂-knockout mice, and ₁-isoform is upregulated 1.9-fold in ₂-knockout. Resting potentials are depolarized by 0.8–4.0 mV in heterozygous and knockout mice. Action potential threshold, overshoot, and duration are normal. Spontaneous firing, a developmental function, is impaired in knockout diaphragm, but this does not compromise its ability to fire evoked action potential trains, the dominant mode of activation near birth. Maximum tetanic force, rate of activation, force-frequency and force-voltage relationships, and onset and magnitude of fatigue are not changed. The major phenotypic consequence of reduced ₂ content is that relaxation from contraction is 1.7-fold faster. This finding reveals a distinct cellular role of the ₂-isoform at a step after membrane excitation, which cannot be restored simply by increasing ₁ content. Na⁺/Ca²⁺ exchanger expression decreases in parallel with ₂-isoform, suggesting that Ca²⁺ extrusion is affected by the altered ₂ genotype. There are no major compensatory changes in expression of sarcoplasmic reticulum Ca²⁺-ATPase, phospholamban, or plasma membrane Ca²⁺-ATPase. These results demonstrate that the Na⁺-K⁺-ATPase ₁-isoform alone is able to maintain equilibrium K⁺ and Na⁺ gradients and to substitute for ₂-isoform in most cellular functions related to excitability and force. They further indicate that the ₂-isoform contributes significantly less at rest than expected from its proportional content but can modulate contractility during muscle contraction. Na⁺-K⁺-ATPase ₂ catalytic subunit; heterozygous mice; knockout mice; resting potential     

Uptake of Thallium, a Toxic Heavy-Metal, in the Cyanobacterium Synechococcus R-2 (Anacystis nidulans, S. Leopoliensis) PCC 7942

Uptake of the toxic heavy-metal, thallium, was studied in thecyanobacterium Synechococcus R-2 (PCC 7942) using clinicallyavailable ²⁰¹Tl ⁺. Thallium was found to distribute across theplasmalemma passively, and so the accumulation ratio of theion ([Tl⁺]_i/[Tl⁺]_o) could be used to calculate the apparentmembrane potential (­_i,o) of the cells (^ETI⁺_i,o = ­_i,o).The permeability of the plasmalemma to TI⁺ (^PTI⁺ 1 to 5 nms^–1)is higher than that of K⁺. Valinomycin does not increase thepermeability of TI⁺. Transient changes in the ­_i,o of cells,because of electrogenic transport of ions, could be detectedfrom its effects upon the uptake rate of TI⁺. HCO^–₃ hyperpolarizedSynechococcus cells, whereas NH⁺₄, CH₃NH⁺, and K⁺ led to depolarization.The use of TI⁺ as a reporter of ­_i,o has some inherent limitations.Tl⁺ is toxic at very low concentrations (inhibitory effectsare apparent after about 6 h at concentrations as low as 1 mmolm^–3). The rate of equilibration is slow (t_1/25 to 20 min).Equilibration of TI⁺ takes about 2 h, which limits its valueas a membrane potential probe. Large amounts of TI⁺ bind tothe surface of the cells making the method impracticable formeasuring accumulation ratios of less than about 10 (­_i,o)values smaller than about –60 mV). Cultures continuouslyexposed to Tl⁺ (10 mmol m^–3) eventually become TI⁺ resistantby actively extruding TI⁺ (µTI⁺_i,o= –3±0.2kJ mol^–1) and so thallium cannot be used as a ­_i,oprobe in such cells. (Received October 28, 1997; Accepted August 31, 1998)     

Palytoxin disrupts cardiac excitation-contraction coupling through interactions with P-type ion pumps

Palytoxin is a coral toxin that seriously impairs heart function, but its effects on excitation-contraction (E-C) coupling have remained elusive. Therefore, we studied the effects of palytoxin on mechanisms involved in atrial E-C coupling. In field-stimulated cat atrial myocytes, palytoxin caused elevation of diastolic intracellular Ca²⁺ concentration ([Ca²⁺]_i), a decrease in [Ca²⁺]_i transient amplitude, Ca²⁺ alternans followed by [Ca²⁺]_i waves, and failures of Ca²⁺ release. The decrease in [Ca²⁺]_i transient amplitude occurred despite high sarcoplasmic reticulum (SR) Ca²⁺ load. In voltage-clamped myocytes, palytoxin induced a current with a linear current-voltage relationship (reversal potential 5 mV) that was blocked by ouabain. Whole cell Ca²⁺ current and ryanodine receptor Ca²⁺ release channel function remained unaffected by the toxin. However, palytoxin significantly reduced Ca²⁺ pumping of isolated SR vesicles. In current-clamped myocytes stimulated at 1 Hz, palytoxin induced a depolarization of the resting membrane potential that was accompanied by delayed afterdepolarizations. No major changes of action potential configuration were observed. The results demonstrate that palytoxin interferes with the function of the sarcolemmal Na⁺-K⁺ pump and the SR Ca²⁺ pump. The suggested mode of palytoxin toxicity in the atrium involves the conversion of Na⁺-K⁺ pumps into nonselective cation channels as a primary event followed by depolarization, Na⁺ accumulation, and Ca²⁺ overload, which, in turn, causes arrhythmogenic [Ca²⁺]_i waves and delayed afterdepolarizations. atrial myocytes; intracellular calcium     

The Influence of Temperature on a K+-Channel and on a Carrier-Type Transporter in Nitella

Fisahn, J. and Hansen, U-P. 1986. The influence of temperatureon a K⁺ -channel and on a carrier type transporter in Nilella—J.exp. Bot. 37. 440–460. In Nitella, the effects of temperature on membrane potentialand on resistance consist of several components. The evaluationof their associated time-constants measured in linear(ized)temperature responses at a resting potential of–120 mVprovides an approach to their identification. For changes slowerthan c. 1 s, the temperature effect on membrane potential andresistance does not originate from temperature action on theinvolved transporter, but is mediated by signals from temperaturesensitive metabolic processes. In the case of potential, theseprocesses seem to be identical to those which also mediate thelight effect: pH-regulation, and two direct signals from photosynthesis,as indicated by the similarities of the related time-constants( respectively). The temperature effect on resistance displays only one time-constant of 40 sinmost experiments. The related process is unknown. The non-coincidenceof the time-constants of the effect on potential and on resistanceimplies the involvement of a carrier-type transporter (H+-pumpor cotransporter) in the effect on potential, and of a K+channelin the effect on resistance. The K+-channel is identified bythe reversal potential of the effect on membrane potential measuredin cells depolarized or hyperpolarized by an injected electricalcurrent Under these conditions the temperature effect on resistancedominates the effect on potential. Key words: H⁺-pump, K⁺-channel, kinetic analysis, Nitella, oscillation, pH-regulation, reversal, potential, temperature, time-constants     

Na(+)/Ca(2+) exchange and its role in intracellular Ca(2+) regulation in guinea pig detrusor smooth muscle

The role of Na⁺/Ca²⁺ exchange inregulating intracellular Ca²⁺ concentration([Ca²⁺]_i) in isolated smooth muscle cellsfrom the guinea pig urinary bladder was investigated. Incrementalreduction of extracellular Na⁺ concentration resulted in agraded rise of [Ca²⁺]_i; 50-100 µMstrophanthidin also increased [Ca²⁺]_i. Asmall outward current accompanied the rise of[Ca²⁺]_i in low-Na⁺ solutions(17.1 ± 1.8 pA in 29.4 mM Na⁺). The quantity ofCa²⁺ influx through the exchanger was estimated from thecharge carried by the outward current and was ~30 times that which isnecessary to account for the rise of [Ca²⁺]_i,after correction was made for intracellular Ca²⁺ buffering.Ca²⁺ influx through the exchanger was able to loadintracellular Ca²⁺ stores. It is concluded that the levelof resting [Ca²⁺]_i is not determined by theexchanger, and under resting conditions (membrane potential 50 to60 mV), there is little net flux through the exchanger. However, asmall rise of intracellular Na⁺ concentration would besufficient to generate significant net Ca²⁺ influx.

     

Activation of K+-Channel in Membrane Excitation of Nitella axilliformis

Two processes of the K⁺ channel activation in plasma membraneexcitation are suggested for Nitella axilliformis. One is relatedto the repolarizing process in the action potential and theother to the after-hyperpolarization (AH). Extra- and intracellulartetraethylammonium (TEA⁺) and extracellular Co²⁺ prolonged theaction potential, indicating involvement of K⁺ channel activationin the repolarizing process of the action potential. The following findings showed that AH is caused by K⁺ channelactivation. First, AH was inhibited by extracellular K⁺ andRb⁺ but not by Na⁺ and Li⁺. Second, it was not inhibited byintracellular TEA⁺ but by extracellular TEA⁺. Third, the membraneconductance increased during AH. Generation of AH was dependenton the level of the resting membrane potential [(E_m)_rest] whichis affected by the activity of the electrogenic H⁺ pump. AHwas generated, when (E_m)_rest was more positive than a criticalvalue, which was supposed to be the equilibrium potential forK⁺ across the plasma membrane. Since extracellular Ca²⁺ competed with extracellular TEA⁺ andCo²⁺ in prolonging the action potential, and sometimes in inhibitingAH, Ca²⁺ may be involved in the K⁺ channel activation. (Received June 11, 1983; Accepted September 21, 1983)