Effects of estradiol on phenylephrine contractility associated with intracellular calcium release in rat aorta

The ability of estradiol to affect phenylephrine-induced contraction and the subsequent increase in resting tone, associated with capacitative Ca²⁺ entry across the plasma membrane, was evaluated in rat aortic rings incubated in Ca²⁺-free solution. The incubation with estradiol (1–100 nM, 5 min) inhibited both the phenylephrine-induced contraction and the IRT. Neither cycloheximide (1 µM; inhibitor of protein synthesis) nor tamoxifen (1 µM; blocker of estrogenic receptors) modified the effects of estradiol. Estradiol (100 µM) also blocked the contractile response to serotonin (10 µM) but not to caffeine (10 mM). In addition, estradiol (100 µM) inhibited the contractile responses to cyclopiazonic acid (1 µM; selective Ca²⁺-ATPase inhibitor) associated with capacitative Ca²⁺ influx through non-L-type Ca²⁺ channels. Finally, estradiol inhibited the Ca²⁺-induced increases in intracellular free Ca²⁺ (after pretreatment with phenylephrine) in cultured rat aorta smooth muscle cells incubated in Ca²⁺-free solution. In conclusion, estradiol interfered in a concentration-dependent manner with Ca²⁺-dependent contractile effects mediated by the stimuli of ₁-adrenergic and serotonergic receptors and inhibited the capacitative Ca²⁺ influx through both L-type and non-L-type Ca²⁺ channels. Such effects are in essence nongenomic and not mediated by the intracellular estrogenic receptor. estrogen; ₁-adrenergic agonists     

Diaphragm disuse reduces Ca2+ uptake capacity of sarcoplasmic reticulum

Howell, Sandra, Wen-Zhi Zhan, and Gary C. Sieck.Diaphragm disuse reduces Ca²⁺uptake capacity of sarcoplasmic reticulum. J. Appl.Physiol. 82(1): 164-171, 1997.Chronic phrenictetrodotoxin (TTX) blockade and phrenic denervation (Dnv) of hamsterdiaphragm result in decreased maximum specific tension, prolongedcontraction time, and improved fatigue resistance (W. Z. Zhan and G. C. Sieck. J. Appl. Physiol. 72:1445-1453, 1992). An underlying increased relative contribution oftype I fibers to total muscle mass appears to be consistent with, butdoes not completely account for, changes in contractile and fatigueproperties. The present study was designed to evaluate a potential rolefor altered cellular Ca²⁺metabolism in the adaptive response of the diaphragm to chronic disuse.An analytic method based on simulation and modeling of long-term⁴⁵Ca²⁺efflux data was used to estimateCa²⁺ contents (nmolCa²⁺/g wet wt tissue) and exchangefluxes (nmolCa^{2+ ·} min^{1 ·} g¹)for extracellular and intracellular compartments in the in vitro hamster hemidiaphragm after prolonged disuse. Three groups were compared: control (Con, n = 5),phrenic TTX blockade (TTX, n = 5), andphrenic denervation (Dnv, n = 5).Experimental muscles were loaded with⁴⁵Ca²⁺for 1 h, and efflux data were collected for 8 h by using a flow-through tissue chamber. Compartmental analysis of efflux data estimated thatthe Ca²⁺ contents andCa²⁺ exchange fluxes of thelargest and slowest intracellular compartment (putative longitudinalreticulum) were reduced by ~50% in TTX and Dnv muscle groupscompared with Con. In addition, the kinetic model predicted significantdecreases in total intracellularCa²⁺ and total diaphragmCa²⁺ in TTX and Dnv muscles. Weconclude that the data support the hypothesis that the capac- ity ofthe sarcoplasmic reticulum for Ca²⁺ sequestration is reduced inchronic diaphragm disuse. The impact of this effect on diaphragmcontractile and fatigue properties is discussed.

     

Effects of PKCalpha activation on Ca2+ pump and KCa channel in deoxygenated sickle cells

We have previously shown that a pretreatment with phorbol12-myristate 13-acetate (PMA), an activator of protein kinase C (PKC),reduced deoxygenation-induced K⁺loss and Ca²⁺ uptake and preventedcell dehydration in sickle anemia red blood cells (SS cells) (H. Fathallah, E. Coezy, R.-S. De Neef, M.-D. Hardy-Dessources, and F. Giraud. Blood 86: 1999-2007,1995). The present study explores the detailed mechanism of thisPMA-induced inhibition. The main findings are, first, the detection ofPKC and PKC in normal red blood cells and the demonstration that both isoforms are expressed at higher levels in SS cells. The -isoform only is translocated to the membrane and activated by PMAand by elevation of cytosolicCa²⁺. Second, PMA is demonstratedto activate Ca²⁺ efflux indeoxygenated SS cells by a direct stimulation of the Ca²⁺ pump. PMA, moreover, inhibitsdeoxygenation-induced, charybdotoxin-sensitive K⁺ efflux in SS cells. Thisinhibition is partly indirect and explained by the reduceddeoxygenation-induced rise in cytosolicCa²⁺ resulting fromCa²⁺ pump stimulation. However, asignificant inhibition of theCa²⁺-activatedK⁺ channels(K_Ca channels) by PMA can also bedemonstrated when the channels are activated byCa²⁺ plus ionophore, underconditions in which the Ca²⁺ pumpis operating near its maximal extrusion rate, but swamped byCa²⁺ plus ionophore. The data thussuggest a PKC-mediated phosphorylation both of theCa²⁺ pump and of theK_Ca channel or an auxiliaryprotein.

     

Contractile activity is required for sarcomeric assembly in phenylephrine-induced cardiac myocyte hypertrophy

Agonist-inducedhypertrophy of cultured neonatal rat ventricular myocytes (NRVM) hasbeen attributed to biochemical signals generated during receptoractivation. However, NRVM hypertrophy can also be induced byspontaneous or electrically stimulated contractile activity in theabsence of exogenous neurohormonal stimuli. Using single-cell imagingof fura 2-loaded myocytes, we found that low-density, noncontractingNRVM begin to generate intracellularCa²⁺ concentration([Ca²⁺]_i)transients and contractile activity within minutes of exposure to the₁-adrenergic agonistphenylephrine (PE; 50 µM). However, NRVM pretreated with verapamiland then stimulated with PE failed to elicit[Ca²⁺]_itransients and beating. We therefore examined whether PE-induced [Ca²⁺]_itransients and contractile activity were required to elicit specificaspects of the hypertrophic phenotype. PE treatment (48-72 h)increased cell size, total protein content, total protein-to-DNA ratio,and myosin heavy chain (MHC) isoenzyme content. PE also stimulatedsarcomeric protein assembly and prolonged MHC half-life. However,blockade of voltage-gated L-typeCa²⁺ channels with verapamil,diltiazem, or nifedipine (10 µM) blocked PE-induced total protein andMHC accumulation and prevented the time-dependent assembly ofmyofibrillar proteins into sarcomeres. Inhibition of actin-myosincross-bridge cycling with 2,3-butanedione monoxime (7.5 mM) alsoprevented PE-induced total protein and MHC accumulation, indicatingthat mechanical activity, rather than[Ca²⁺]_itransients per se, was required. In contrast, blockade of[Ca²⁺]_itransients and contractile activity did not prevent the PE-induced increase in cell surface area, activation of the mitogen-activated protein kinases ERK1 and ERK2, or upregulation of atrial natriuretic factor gene expression. Thus contractile activity is required to elicitsome but not all aspects of the the hypertrophic phenotype induced by₁-adrenergic receptoractivation.

     

Stretch-induced Ca(2+) release via an IP(3)-insensitive Ca(2+) channel

Various mechanicalstimuli increase the intracellular Ca²⁺ concentration([Ca²⁺]_i) in vascular smooth muscle cells(VSMC). A part of the increase in [Ca²⁺]_i isdue to the release of Ca²⁺ from intracellular stores. Wehave investigated the effect of mechanical stimulation produced bycyclical stretch on the release of Ca²⁺ from theintracellular stores. Permeabilized VSMC loaded with ⁴⁵Ca²⁺ were subjected to 7.5% average (15%maximal) cyclical stretch. This resulted in an increase in⁴⁵Ca²⁺ rate constant by 0.126 ± 0.0035. Inhibition of inositol 1,4,5-trisphosphate (IP₃),ryanodine, and nicotinic acid adenine dinucleotide phosphate channels(NAADP) with 50 µg/ml heparin, 50 µM ruthenium red, and 25 µMthio-NADP, respectively, did not block the increase in⁴⁵Ca²⁺ efflux in response to cyclical stretch.However, 10 µM lanthanum, 10 µM gadolinium, and 10 µMcytochalasin D but not 10 µM nocodazole inhibited the increase in⁴⁵Ca²⁺ efflux. This supports the existence of anovel stretch-sensitive intracellular Ca²⁺ store in VSMCthat is distinct from the IP₃-, ryanodine-, and NAADP-sensitive stores.

     

Maitotoxin and P2Z/P2X7 purinergic receptor stimulation activate a common cytolytic pore

The effects ofmaitotoxin (MTX) on plasmalemma permeability are similar to thosecaused by stimulation of P2Z/P2X₇ionotropic receptors, suggesting that1) MTX directly activatesP2Z/P2X₇ receptors or2) MTX andP2Z/P2X₇ receptor stimulationactivate a common cytolytic pore. To distinguish between these twopossibilities, the effect of MTX was examined in1) THP-1 monocytic cells before andafter treatment with lipopolysaccharide and interferon-, a maneuverknown to upregulate P2Z/P2X₇receptor, 2) wild-type HEK cells andHEK cells stably expressing theP2Z/P2X₇ receptor, and3) BW5147.3 lymphoma cells, a cellline that expresses functional P2Z/P2X₇ channels that are poorlylinked to pore formation. In control THP-1 monocytes, addition of MTXproduced a biphasic increase in the cytosolic freeCa²⁺ concentration([Ca²⁺]_i);the initial increase reflects MTX-inducedCa²⁺ influx, whereas the secondphase correlates in time with the appearance of large pores and theuptake of ethidium. MTX produced comparable increases in[Ca²⁺]_iand ethidium uptake in THP-1 monocytes overexpressing theP2Z/P2X₇ receptor. In bothwild-type HEK and HEK cells stably expressing theP2Z/P2X₇ receptor, MTX-inducedincreases in[Ca²⁺]_iand ethidium uptake were virtually identical. The response of BW5147.3cells to concentrations of MTX that produced large increases in[Ca²⁺]_ihad no effect on ethidium uptake. In both THP-1 and HEK cells, MTX- andBz-ATP-induced pores activate with similar kinetics and exhibit similarsize exclusion. Last, MTX-induced pore formation, but not channelactivation, is greatly attenuated by reducing the temperature to22°C, a characteristic shared by theP2Z/P2X₇-induced pore. Together,the results demonstrate that, although MTX activates channels that aredistinct from those activated byP2Z/P2X₇ receptor stimulation, thecytolytic/oncotic pores activated by MTX- and Bz-ATP are indistinguishable.

     

Evidence for Ca(2+)-permeable AMPA receptors in the olfactory bulb

-Amino-3-hydroxy-5-methyl-4-isoxazolepropionic acid (AMPA) receptors (AMPARs), a subtype of glutamate receptor, contribute to olfactory processing in the olfactory bulb (OB). These ion channels consist of various combinations of the subunits GluR1–GluR4, which bestow certain properties. For example, AMPARs that lack GluR2 are highly permeable to Ca²⁺ and generate inwardly rectifying currents. Because increased intracellular Ca²⁺ could trigger a host of Ca²⁺-dependent odor-encoding processes, we used whole cell recording as well as histological and immunocytochemical (ICC) techniques to investigate whether AMPARs on rat OB neurons flux Ca²⁺. Application of 1-naphthylacetyl spermine (NAS), a selective antagonist of Ca²⁺-permeable AMPARs (CP-AMPARs), inhibited AMPAR-mediated currents in subsets of interneurons and principal cells in cultures and slices. The addition of spermine to the electrode yielded inwardly rectifying current-voltage plots in some cells. In OB slices, olfactory nerve stimulation elicited excitatory responses in juxtaglomerular and mitral cells. Bath application of NAS with D,L-2-amino-5-phosphonovaleric acid (AP5) to isolate AMPARs suppressed the amplitudes of these synaptic responses compared with responses obtained using AP5 alone. Co²⁺ staining, which involves the kainate-stimulated influx of Co²⁺ through CP-AMPARs, produced diverse patterns of labeling in cultures and slices as did ICC techniques used with a GluR2-selective antibody. These results suggest that subsets of OB neurons express CP-AMPARs, including functional CP-AMPARs at synapses. Ca²⁺ entry into cells via these receptors could influence odor encoding by modulating K⁺ channels, N-methyl-D-aspartate receptors, and Ca²⁺-binding proteins, or it could facilitate synaptic vesicle fusion. GluR2; polyamines; cobalt; glutamate receptor; olfaction     

Calcium sparks in smooth muscle

Local intracellular Ca²⁺transients, termed Ca²⁺ sparks, are caused by thecoordinated opening of a cluster of ryanodine-sensitive Ca²⁺ release channels in the sarcoplasmic reticulum ofsmooth muscle cells. Ca²⁺ sparks are activated byCa²⁺ entry through dihydropyridine-sensitivevoltage-dependent Ca²⁺ channels, although the precisemechanisms of communication of Ca²⁺ entry toCa²⁺ spark activation are not clear in smooth muscle.Ca²⁺ sparks act as a positive-feedback element to increasesmooth muscle contractility, directly by contributing to the globalcytoplasmic Ca²⁺ concentration([Ca²⁺]) and indirectly by increasingCa²⁺ entry through membrane potential depolarization,caused by activation of Ca²⁺ spark-activatedCl channels. Ca²⁺ sparks also have aprofound negative-feedback effect on contractility by decreasingCa²⁺ entry through membrane potential hyperpolarization,caused by activation of large-conductance, Ca²⁺-sensitiveK⁺ channels. In this review, the roles of Ca²⁺sparks in positive- and negative-feedback regulation of smooth musclefunction are explored. We also propose that frequency and amplitudemodulation of Ca²⁺ sparks by contractile and relaxantagents is an important mechanism to regulate smooth muscle function.

     

Regulation of the cardiac L-type Ca2+ channel by the actin-binding proteins alpha-actinin and dystrophin

Theactin-binding proteins dystrophin and -actinin are members of afamily of actin-binding proteins that may link the cytoskeleton tomembrane proteins such as ion channels. Previous work demonstrated thatthe activity of Ca²⁺ channels can be regulated by agentsthat disrupt or stabilize the cytoskeleton. In the present study, weemployed immunohistochemical and electrophysiological techniques toinvestigate the potential regulation of cardiac L-type Ca²⁺channel activity by dystrophin and -actinin in cardiac myocytes andin heterologous cells. Both actin-binding proteins were found tocolocalize with the Ca²⁺ channel in mouse cardiac myocytesand to modulate channel function. Inactivation of the Ca²⁺channel in cardiac myocytes from mice lacking dystrophin(mdx mice) was reduced compared with that in wild-typemyocytes, voltage dependence of activation was shifted by 5 mV to morepositive potentials, and stimulation by the -adrenergic pathway andthe dihydropyridine agonist BAY K 8644 was increased. Furthermore, heterologous coexpression of the Ca²⁺ channel with muscle,but not nonmuscle, forms of -actinin was also found to reduceinactivation. As might be predicted from a reduction ofCa²⁺ channel inactivation, a prolonging of the mouseelectrocardiogram QT was observed in mdx mice. These resultssuggest a combined role for dystrophin and -actinin in regulatingthe activity of the cardiac L-type Ca²⁺ channel and apotential mechanism for cardiac dysfunction in Duchenne and Beckermuscular dystrophies.

     

Essential role for extracellular Ca(2+) in JNK activation by mechanical stretch in bladder smooth muscle cells

Mechanicalstretch has been implicated in phenotypic changes as an adaptiveresponse to stretch stress physically loaded in bladder smooth musclecells (BSMCs). To investigate stretch-induced signaling, we examinedthe mitogen-activated protein kinase (MAPK) family using rat primaryBSMCs. When BSMCs were subjected to sustained mechanical stretch usingcollagen-coated silicon membranes, activation of c-JunNH₂-terminal kinase (JNK) was most relevant among three subsets of MAPK family members: the activity was elevated from 5 minafter stretch and peaked at 10 min with an 11-fold increase. Activationof p38 was weak compared with that of JNK, and ERK was notactivated at all. JNK activation by mechanical stretch was totallydependent on extracellular Ca²⁺ and inhibited byGd³⁺, a blocker of stretch-activated (SA) ion channels.Nifedipine and verapamil, inhibitors for voltage-dependentCa²⁺ channels, had no effect on this JNK activation.Moreover, none of the inhibitors pertussis toxin, genistein,wortmannin, or calphostin C affected stretch-induced JNK activation,indicating that G protein-coupled and tyrosine kinase receptors areunlikely to be involved in this JNK activation. On the other hand, W-7,a calmodulin inhibitor, and cyclosporin A, a calcineurin inhibitor,prevented JNK activation by stretch. These results suggest a novelpathway for stretch-induced activation of JNK in BSMCs: mechanicalstretch evokes Ca²⁺ influx via Gd³⁺-sensitiveSA Ca²⁺ channels, resulting in JNK activation underregulation in part by calmodulin and calcineurin.

     

Role of K(+) channel expression in polyamine-dependent intestinal epithelial cell migration

Polyamines are essential for cell migrationduring early mucosal restitution after wounding in the gastrointestinaltract. Activity of voltage-gated K⁺ channels (Kv) controlsmembrane potential (E_m) that regulates cytoplasmicfree Ca²⁺ concentration([Ca²⁺]_cyt) by governing thedriving force for Ca²⁺ influx. This study determinedwhether polyamines are required for the stimulation of cell migrationby altering K⁺ channel gene expression,E_m, and[Ca²⁺]_cyt in intestinal epithelialcells (IEC-6). The specific inhibitor of polyamine synthesis,-difluoromethylornithine (DFMO, 5 mM), depleted cellularpolyamines (putrescine, spermidine, and spermine), selectivelyinhibited Kv1.1 channel (a delayed-rectifier Kv channel) expression,and resulted in membrane depolarization. Because IEC-6 cells did notexpress voltage-gated Ca²⁺ channels, the depolarizedE_m in DFMO-treated cells decreased [Ca²⁺]_cyt as a result of reduceddriving force for Ca²⁺ influx through capacitativeCa²⁺ entry. Migration was reduced by 80% in thepolyamine-deficient cells. Exogenous spermidine not only reversed theeffects of DFMO on Kv1.1 channel expression, E_m,and [Ca²⁺]_cyt but also restoredcell migration to normal. Removal of extracellular Ca²⁺ orblockade of Kv channels (by 4-aminopyridine, 1-5 mM) significantly inhibited normal cell migration and prevented the restoration of cellmigration by exogenous spermidine in polyamine-deficient cells. Theseresults suggest that polyamine-dependent intestinal epithelial cellmigration may be due partially to an increase of Kv1.1 channelexpression. The subsequent membrane hyperpolarization raises[Ca²⁺]_cyt by increasing the drivingforce (the electrochemical gradient) for Ca²⁺ influx andthus stimulates cell migration.

     

The calcium-dependent activity of large-conductance, calcium-activated K+ channels is enhanced by Pyk2- and Hck-induced tyrosine phosphorylation

Recent results showing that large-conductance, calcium-activated K⁺ (BK_Ca) channels undergo direct tyrosine phosphorylation in the presence of c-Src tyrosine kinase have suggested the involvement of these channels in Src-mediated signaling pathways. Given the important role for c-Src in integrin-mediated signal transduction, we have examined the potential regulation of BK_Ca channels by proline-rich tyrosine kinase 2 (Pyk2), a calcium-sensitive tyrosine kinase activated upon integrin stimulation. Transient coexpression of murine BK_Ca channels with either wild-type Pyk2 or hematopoietic cell kinase (Hck), a Src-family kinase, led to an enhancement of BK_Ca channel activity over the range of 1–10 µM free calcium, whereas coexpression with catalytically inactive forms of either kinase did not significantly alter BK_Ca gating compared with channels expressed alone. In the presence of either wild-type Pyk2 or Hck, BK_Ca -subunits were found to undergo tyrosine phosphorylation, as determined by immunoprecipitation and Western blotting strategies. However, tyrosine phosphorylation of the BK_Ca -subunit was not detected for channels expressed alone or together with inactive forms of either Pyk2 or Hck. Interestingly, wild-type, but not inactive, Pyk2 was also present in BK_Ca channel immunoprecipitates, suggesting that Pyk2 may coassociate with the BK_Ca channel complex after phosphorylation. Collectively, the observed modulation and phosphorylation of BK_Ca channels by Pyk2 and a Src-family kinase may reflect a general cellular mechanism by which G protein-coupled receptor and/or integrin activation leads to the regulation of membrane ion channels. BK channels; tyrosine kinase; calcium; immunoprecipitation     

Ionic mechanism for contractile response to hyposmotic challenge in canine basilar arteries

A hyposmotic challenge elicited contraction of isolated canine basilar arteries. The contractile response was nearly abolished by the removal of extracellular Ca²⁺ and by the voltage-dependent Ca²⁺ channel (VDCC) blocker nicardipine, but it was unaffected by thapsigargin, which depletes intracellular Ca²⁺ stores. The contraction was also inhibited by Gd³⁺ and ruthenium red, cation channel blockers, and Cl^– channel blockers DIDS and niflumic acid. The reduction of extracellular Cl^– concentrations enhanced the hypotonically induced contraction. Patch-clamp analysis showed that a hyposmotic challenge activated outwardly rectifying whole cell currents in isolated canine basilar artery myocytes. The reversal potential of the current was shifted toward negative potentials by reductions in intracellular Cl^– concentration, indicating that the currents were carried by Cl^–. Moreover, the currents were abolished by 10 mM BAPTA in the pipette solution and by the removal of extracellular Ca²⁺. Taken together, these results suggest that a hyposmotic challenge activates cation channels, which presumably cause Ca²⁺ influx, thereby activating Ca²⁺-activated Cl^– channels. The subsequent membrane depolarization is likely to increase Ca²⁺ influx through VDCC and elicit contraction. stretch-activated cation channels; Ca²⁺-activated Cl^– channels; voltage-dependent Ca²⁺ channels; large-conductance Ca²⁺-activated K⁺ channels; gadolinium     

Transcaltachia (the Rapid Hormonal Stimulation of Intestinal Calcium Transport): A Component of Adaptation to Calcium Needs and Calcium Availability

Calcium is one of the key elements required for maintenanceand survival of life in animals with both endo- and exoskeletons.Because there is a wide variation in dietary calcium (dependentupon the local habitat) and dietary practices, and because thereis a changing physiological need throughout life (e.g., formammals, during growth, puberty, pregnancy, lactation, and menopause),it is essential that the process of intestinal calcium absorptionbe adaptable and responsive to both the dietary and physiologicalcircumstances. This article reviews the evidence that transcaltachia,or the rapid stimulation of intestinal Ca²⁺ transport by thesteroid hormone, l, 25(OH)₂-vitamin D₃, as studied in the chicken,meets many of the objectives of an adaptive intestinal calciumtransport process. Transcaltachia is studied in a perfused chickduodenum, where ⁴⁵Ca²⁺ is placed in the lumen and potentialagonists are perfused into the celiac artery; the transcaltachicreponse represents the stimulation within 4–8 min of thetransfer of ⁴⁵Ca²⁺ from the lumen to the vascular perfusate.l,25(OH)₂-vitamin D₃ stimulation of transcaltachia occurs vianongenomic mechanisms which involve a plasma membrane receptorfor the secosteroid and the coupled opening of voltage-gatedCa²⁺ channels on the basal lateral membrane of the intestinalepithelial cell and the activation of the second messengers,protein kinase C and cAMP.     

Analysis of a Ca2+-activated K+ channel that mediates hyperpolarization via the thrombin receptor pathway

Dami human leukemia cells express G protein-coupled thrombinreceptors that operate through the phospholipase C pathway. When thesereceptors are activated by -thrombin or by thrombinreceptor-activating peptide, an elevation in cytosolicCa²⁺ concentration develops thatis accompanied by hyperpolarization of the plasma membrane. Thistransitory phase of hyperpolarization is primarily mediated by inwardlyrectifying, Ca²⁺-activatedK⁺ channels that have an inwardconductance of ~24 pS. In cell-attached patches the channels openwithin seconds after superfusion of the cell with thrombinreceptor-activating peptide. In inside-out patches, perfusion ofsubmicromolar Ca²⁺ onto thecytosolic surface of the membrane is sufficient to activate thechannels. In outside-out patches, channel opening can be blocked bynanomolar concentrations of charybdotoxin. The function of theseintermediate-sized inwardly rectifying,Ca²⁺-activatedK⁺ channels has not beenestablished; however, by analogy with other cell systems, they mayserve to regulate cell volume during cellular activation or to increasethe electromotive drive that sustains Na⁺ and/orCa²⁺ influx through ligand-gatedcation channels.

     

Contractile apparatus and sarcoplasmic reticulum function: effects of fatigue, recovery, and elevated Ca2+

Williams, Jay H. Contractile apparatus and sarcoplasmicreticulum function: effects of fatigue, recovery, and elevated Ca²⁺. J. Appl.Physiol. 83(2): 444-450, 1997.This investigationtested the notion that fatiguing stimulation induces intrinsic changes in the contractile apparatus and sarcoplasmic reticulum (SR) and thatthese changes are initiated by elevated intracellularCa²⁺ concentration([Ca²⁺]_i).Immediately after stimulation of frog semitendinosus muscle, contractile apparatus and SR function were measured. Despite a largedecline in tetanic force (P_o),maximal Ca²⁺-activated force(F_max) of the contractileapparatus was not significantly altered. However,Ca²⁺ sensitivity was increased. Inconjunction, the rate constant ofCa²⁺ uptake by the SR wasdiminished, and the caffeine sensitivity ofCa²⁺ release was decreased. Duringrecovery, P_o, contractileapparatus, and SR function each returned to near-initial levels.Exposure of skinned fibers to 0.5 µM freeCa²⁺ for 5 min depressed bothF_max andCa²⁺ sensitivity of thecontractile apparatus. In addition, caffeine sensitivity ofCa²⁺ release was diminished.Results suggest that fatigue induces intrinsic alterations incontractile apparatus and SR function. Changes in contractile apparatusfunction do not appear to be mediated by increased[Ca²⁺]_i.However, a portion of the change in SRCa²⁺ release seems to be due toelevated[Ca²⁺]_i.

     

Coupling strength between localized Ca(2+) transients and K(+) channels is regulated by protein kinase C

Localized Ca²⁺ transients resulting from inositoltrisphosphate (IP₃)-dependent Ca²⁺ releasecouple to spontaneous transient outward currents (STOCs) in murinecolonic myocytes. Confocal microscopy and whole cell patch-clamptechniques were used to investigate coupling between localizedCa²⁺ transients and STOCs. Colonic myocytes were loadedwith fluo 3. Reduction in external Ca²⁺([Ca²⁺]_o) reduced localized Ca²⁺transients but increased STOC amplitude and frequency. Simultaneous recordings of Ca²⁺ transients and STOCs showed increasedcoupling strength between Ca²⁺ transients and STOCs when[Ca²⁺]_o was reduced. Gd³⁺ (10 µM) did not affect Ca²⁺ transients but increased STOCamplitude and frequency. Similarly, an inhibitor of Ca²⁺influx,1-2-(4-methoxyphenyl)-2-[3-(4-methoxyphenyl)propoxy]ethyl-1H-imidazole (SKF-96365), increased STOC amplitude and frequency. A protein kinase C(PKC) inhibitor, GF-109203X, also increased the amplitude and frequencyof STOCs but had no effect on Ca²⁺ transients. Phorbol12-myristate 13-acetate (1 µM) reduced STOC amplitude and frequencybut did not affect Ca²⁺ transients. 4-Phorbol (1 µM)had no effect on STOCs or Ca²⁺ transients. Single channelstudies indicated that large-conductance Ca²⁺-activatedK⁺ (BK) channels were inhibited by aCa²⁺-dependent PKC. In summary 1)Ca²⁺ release from IP₃ receptor-operated storesactivates Ca²⁺-activated K⁺ channels;2) Ca²⁺ influx through nonselective cationchannels facilitates activation of PKC; and 3) PKC reducesthe Ca²⁺ sensitivity of BK channels, reducing the couplingstrength between localized Ca²⁺ transients and BK channels.

     

Stretch-induced activation of Ca(2+)-activated K(+) channels in mouse skeletal muscle fibers

High-conductanceCa²⁺-activatedK⁺(K_Ca) channels werestudied in mouse skeletal muscle fibers using thepatch-clamp technique. In inside-out patches, application of negativepressure to the patch induced a dose-dependent and reversibleactivation of K_Ca channels.Stretch-induced increase in channel activity was found to be of thesame magnitude in the presence and in the absence ofCa²⁺ in the pipette. Thedose-response relationships betweenK_Ca channel activity andintracellular Ca²⁺ and betweenK_Ca channel activity and membranepotential revealed that voltage andCa²⁺ sensitivity were not alteredby membrane stretch. In cell-attached patches, in the presence of highexternal Ca²⁺ concentration,stretch-induced activation was also observed. We conclude that membranestretch is a potential mode of regulation of skeletal muscleK_Ca channel activity and could beinvolved in the regulation of muscle excitability duringcontraction-relaxation cycles.

     

Involvement of stretch-activated cation channels in hypotonically induced insulin secretion in rat pancreatic beta-cells

In isolated rat pancreatic -cells, hypotonic stimulation elicited an increase in cytosolic Ca²⁺ concentration ([Ca²⁺]_c) at 2.8 mM glucose. The hypotonically induced [Ca²⁺]_c elevation was significantly suppressed by nicardipine, a voltage-dependent Ca²⁺ channel blocker, and by Gd³⁺, amiloride, 2-aminoethoxydiphenylborate, and ruthenium red, all cation channel blockers. In contrast, the [Ca²⁺]_c elevation was not inhibited by suramin, a P₂ purinoceptor antagonist. Whole cell patch-clamp analyses showed that hypotonic stimulation induced membrane depolarization of -cells and produced outwardly rectifying cation currents; Gd³⁺ inhibited both responses. Hypotonic stimulation also increased insulin secretion from isolated rat islets, and Gd³⁺ significantly suppressed this secretion. Together, these results suggest that osmotic cell swelling activates cation channels in rat pancreatic -cells, thereby causing membrane depolarization and subsequent activation of voltage-dependent Ca²⁺ channels and thus elevating insulin secretion. calcium ion; swelling; patch-clamp; gadolinium     

Stimulation of cardiac L-type calcium channels by extracellular ATP

The co-release of ATP with norepinephrine from sympatheticnerve terminals in the heart may augment adrenergic stimulation ofcardiac Ca²⁺ channel activity. To test for a possibledirect effect of extracellular ATP on L-type Ca²⁺ channels,single channels were reconstituted from porcine sarcolemma into planarlipid bilayers so that intracellular signaling pathways could becontrolled. Extracellular ATP (2-100 µM) increased the openprobability of the reconstituted channels, with a maximal increase of~2.6-fold and an EC₅₀ of 3.9 µM. The increase in open probability was due to an increase in channel availability and adecrease in channel inactivation rate. Other nucleotides displayed arank order of effectiveness of ATP > ,-methylene-ATP > 2-methylthio-ATP > UTP > adenosine5'-O-(3-thiotriphosphate) >> ADP; adenosine had no effect.Several antagonists of P2 receptors had no impact on the ATP-dependentincrease in open probability, indicating that receptor activation wasnot required. These results suggest that extracellular ATP and othernucleotides can stimulate the activity of cardiac L-typeCa²⁺ channels via a direct interaction with the channels.