Diadenosine Polyphosphates Directly Relax Porcine Coronary Arterial Smooth Muscle

Assistant Professor of Medicine (Clinician-Educator)

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Vol. 283, Issue 2, 548-556, 1997

Diadenosine Polyphosphates Directly Relax Porcine Coronary Arterial Smooth Muscle¹

Rieko Sumiyoshi, Junji Nishimura, Junya Kawasaki, Sei Kobayashi, Shosuke Takahashi² and Hideo Kanaide

Division of Molecular Cardiology, Research Institute of Angiocardiology, Faculty of Medicine, Kyushu University, Fukuoka 812-82, Japan

	Abstract

Top Abstract Introduction Materials & Methods Results Discussion References

By use of front-surface fluorometry and fura-2-loaded medial strips of the porcine coronary artery, cytosolic Ca⁺⁺ concentration ([Ca⁺⁺]_i) and force development were monitored simultaneously to determinethe mechanisms of vasorelaxation induced by the diadenosine polyphosphates(AP_nA) diadenosine 5 $'$ ,5 $'''$ -P¹,P⁴-tetraphosphate (AP₄A) and diadenosine 5 $'$ ,5 $'''$ -P¹,P⁵-pentaphosphate (AP₅A). AP_nA concentration-dependently inhibitedthe sustained elevations of [Ca⁺⁺]_i and force induced by U-46619, a thromboxane A₂ analog, in thepresence of extracellular Ca⁺⁺. AP_nA shifted the [Ca⁺⁺]_i-force relation curves of contractions induced by various concentrationsof high K⁺ to the right. The AP₄A-induced decreases in [Ca⁺⁺]_i and force were largely attenuated by tetrabutylammonium. TheAP₄A-induced decreases in force were attenuated by 4-aminopyridineand charybdotoxin. The AP₅A-induced decreases in [Ca⁺⁺]_i and force were attenuated by tetrabutylammonium, 4-aminopyridineand charybdotoxin. In the absence of extracellular Ca⁺⁺, AP_nA did not inhibit the transient elevations of [Ca⁺⁺]_i induced by histamine or caffeine. Both AP₄A and AP₅A increasedintracellular cAMP content. We thus conclude that AP₄A and AP₅Arelax the porcine coronary artery by decreasing [Ca⁺⁺]_i, possibly through the activation of K⁺ channels, but not through inhibition of intracellular Ca⁺⁺ release and by decreasing the Ca⁺⁺ sensitivity of the contractile machinery. These effects wereconsidered to be mediated by cAMP.

	Introduction

Top Abstract Introduction Materials & Methods Results Discussion References

Diadenosine polyphosphates such as AP₄A and AP₅A have received considerable attention because of their multiple biologicalactivities. These compounds are present in various types of cells,including platelets (Flodgaard and Klenow, 1982), chromaffin cells(Rodriguez del Castillo et al., 1988) and neural tissue (Pintoret al., 1992), and are implicated primarily in platelet functions(Flodgaard and Klenow, 1982; Luthje and Ogilvie, 1983; Zamecniket al., 1992) and neurotransmission (Baxi and Vishwanatha, 1995).

In recent years, interest in AP_nA in vasomotor activity has been renewed. Busse et al. (1988) first described AP₄A inducedendothelium-independent vasoconstriction in rabbit mesentericarteries. Subsequent studies also indicated that AP₄A elicitsincreases in perfusion pressure of rat portal vein (Busshardtet al., 1989) and that AP₄A also induces the vasoconstrictor responsesmediated by P_2X-purinergic receptors (Ralevic et al., 1995). AP₅Awas recently reported to be a novel vasoconstrictor agent isolatedfrom human platelets (Schluter et al., 1994). These authors reportedthat AP₅A induced increases in perfusion pressure of the vasculturein isolated perfused rat kidney and aorta. AP₅A-induced vasoconstrictionhas also been documented in both the rat mesenteric artery (Ralevicet al., 1995) and human umbilical artery (Davies et al., 1995).

AP₄A also induces endothelium-dependent vasodilation in rabbit mesenteric arteries (Busse et al., 1988), and endothelium-dependentand -independent decreases in rabbit coronary perfusion pressure(Pohl et al., 1991). Intravenous administration of AP₄A to a dogproduced a dose-dependent decrease in mean arterial pressure (Kikutaet al., 1994), which thus indicates that AP₄A may induce, eitherdirectly or indirectly, relaxation rather than constriction ofvascular smooth muscle in vivo. However, the cellular mechanismfor AP_nA-induced vasorelaxation has yet to be investigated extensively.In the present study, we determined the mechanism underlying thevasorelaxing effects of AP₄A and AP₅A on porcine coronary smoothmuscle cells by use of the simultaneous measurements of [Ca⁺⁺]_i and force. We obtained evidence that AP₄A and AP₅A reduce [Ca⁺⁺]_i by modulating the function of K⁺ channels and decreasing the Ca⁺⁺ sensitivity of the contractile machinery and, as a result, inducevasorelaxation. These effects were thought to be mediated by theincrease in the cellular cAMP content.

	Materials and Methods

Top Abstract Introduction Materials & Methods Results Discussion References

Tissue preparation. Left circumflex coronary arteries (2-3 cm from the origin) were isolated from fresh porcine hearts at a local slaughterhouseimmediately after the animals had been sacrificed. The tissuespecimens were placed in ice-cold normal PSS and brought to thelaboratory. After the segments were cut open longitudinally, theadventitia was trimmed away. The inner surfaces of the arterieswere rubbed with cotton swabs to remove the endothelium. Eachspecimen was cut into similar sized strips (1 × 5 × 0.1 mm). Completeremoval of the endothelium was confirmed by the lack of any relaxingresponse of the strips to 1 µM bradykinin.

Fura-2 loading. Coronary arterial media strips were loaded with Ca⁺⁺ indicator dye, fura-2, by incubating them in oxygenated (a mixture of 95%O₂ and 5% CO₂) Dulbecco's modified Eagle's medium containing 25µM fura-2/AM (an acetoxymethyl ester form of fura-2) and 5% fetalbovine serum for 4 hr at 37°C. After loading with fura-2, medialstrips were incubated in normal PSS for at least 1 hr at 37°Cbefore starting the measurement, to remove the dye in the extracellularspace and for purposes of equilibration. Loading the medial stripswith fura-2 per se did not affect the contractility, as describedpreviously (Abe et al., 1990; Hirano et al., 1990).

Front-surface fluorometry. Changes in the fluorescence intensity of the fura-2-Ca⁺⁺ complex were monitored simultaneously with the force development, bya front-surface fluorometer specifically designed for fura-2 fluorometry(CAM-OF3, Japan Spectroscopic Co., Tokyo, Japan), as describedpreviously (Ushio-Fukai et al., 1993). The ratio of the fluorescence(500 nm) intensities at alternating 340-nm and 380-nm excitationwavelengths was monitored. The fluorescence ratio was expressedas a percentage, by assigning the values at rest in normal (5.9mM K⁺) and 118 mM K⁺ PSS to be 0% and 100%, respectively. The absolute values of [Ca⁺⁺]_i of vascular strips were calculated according to the methodof Grynkiewicz et al. (1985) with the K_d (apparent dissociationconstant) of the fura-2-Ca⁺⁺ complex of 225 nM (at 37°C). The absolute values of [Ca⁺⁺]_i for 0% and 100% levels were determined in separate measurementsand were 108 ± 27 nM (n = 10) and 715 ± 103 nM (n = 10), respectively.The obtained [Ca⁺⁺]_i values are considered to be an approximation to the true [Ca⁺⁺]_i value, and the calibration of the absolute levels of [Ca⁺⁺]_i at the end of experiments is likely to be uncertain (Miyagiet al., 1995). Therefore, a statistical analysis of the [Ca⁺⁺]_i signal was performed with use of the percent fluorescence ratio.

Measurement of force development. Coronary arterial media strips were mounted vertically in a quartz organ bath, and the isometric tension was measured, asdescribed previously (Ushio-Fukai et al., 1993). The strips werestimulated with 118 mM K⁺ PSS every 15 min during the fura-2 equilibration period (1 hr),and then the resting tension was increased in a stepwise mannerto obtain the maximal tension development. The appropriate restingtension level obtained by this procedure was about 300 mg. Atthe beginning of each protocol, the responsiveness of each stripto 118 mM K⁺ PSS was recorded. The developed force was expressed in a percentage,by assigning the values at rest in normal PSS (5.9 mM K⁺) to be 0%, and those at steady state of contraction in 118 mMK⁺ PSS to be 100%.

Assay of cAMP and cGMP. The content of cAMP and cGMP in porcine coronary artery were assayed as described previously (Abe et al., 1994). After incubationof vascular strips with oxygenated (95% O₂ and 5% CO₂) normalPSS containing 10 µM AP₄A or AP₅A for 15 min at 37°C, the reactionwas stopped by replacing the solution with ice-cold perchloricacid (6%). The strips were then homogenized in perchloric acid.The homogenate was centrifuged at 1500 × g for 15 min. The supernatantwas used to measure the cAMP and cGMP content by using radioimmunoassaykits (Yamasa, Tokyo, Japan). cAMP and cGMP levels were expressedas nanomoles or picomoles per milligram of wet weight of tissue(nmol or pmol/mg tissue).

Drugs and solutions. The composition of normal PSS for fura-2 studies was as follows (mM): NaCl, 123; KCl, 4.7; NaHCO₃, 15.5; KH₂PO₄, 1.2; MgCl₂,1.2; CaCl₂, 1.25; D-glucose, 11.5. The Ca⁺⁺-free solution (Ca⁺⁺-free PSS) contained 2 mM EGTA instead of 1.25 mM CaCl₂. HighK⁺ PSS was prepared by replacing NaCl with equimolar KCl. PSS wasbubbled with a mixture of 95% O₂ and 5% CO₂, and the resultingpH was 7.4. Fura-2/AM was purchased from Dojindo Laboratories(Kumamoto, Japan). AP₄A, AP₅A and bovine serum albumin were purchasedfrom Sigma Chemical Co. (St. Louis, MO). Bradykinin, ChTX andapamin were purchased from the Peptide Institute, Inc. (Osaka,Japan). U46619 was purchased from Funakoshi (Tokyo, Japan). Caffeinewas obtained from Katayama Chemical (Osaka, Japan). Kits for radioimmunoassayof cAMP and cGMP were purchased from Yamasa (Tokyo, Japan). Allother chemicals were obtained from Wako (Osaka, Japan).

Data analysis. The values are expressed as the mean ± S.E.M. Student's t-test was used to determine statistical significance between twogroups, and analysis of variance was used to determine the dose-dependenteffect of AP_nA on [Ca⁺⁺]_i and force. The number of experiments corresponds to the numberof the animals used. The IC₅₀ values, the concentrations thatdecreased the fluorescence ratio and force to 50% of the maximumresponse, were determined based on the concentration-responsecurve fitted according to a four-parameter logistic model (DeLeanet al., 1978). The significance of the shift of the [Ca⁺⁺]_i-force relation curve was determined by an analysis of covariance.A value of P < .05 was considered to have statistical significance.All data were collected by a computerized data acquisition system(MacLab: Analog Digital Instruments, Castle Hill, Australia; andMacintosh: Apple Computer, Cupertino, CA).

	Results

Top Abstract Introduction Materials & Methods Results Discussion References

Effects of AP₄A and AP₅A on the [Ca⁺⁺]_i and force induced by U46619. Figure 1, a and b, shows representative recordings of the effects of cumulative application of AP₄A (0.01-10 µM) and AP₅A(0.01-10 µM), respectively, on the [Ca⁺⁺]_i and force induced by 60 nM U46619, a thromboxane A₂ analog.When the bathing medium was changed from normal PSS (5.9 mM K⁺) to 118 mM K⁺ PSS, both [Ca⁺⁺]_i and force rapidly increased and reached the plateau phaseswithin 10 to 15 min. The values at the resting and plateau phaseswere designated to be 0% and 100% for both [Ca⁺⁺]_i and force. The application of 60 nM U46619 induced a rapidincrease in [Ca⁺⁺]_i, which reached a peak level in 5 min and thereafter decreasedto a plateau level within 10 min (60.52 ± 0.97%, n = 20). Theforce also rapidly increased and reached a plateau level within10 min (95.27 ± 1.01%, n = 20). The applications of AP₄A and AP₅Aduring the U46619-induced sustained contraction caused concentration-dependentdecreases in [Ca⁺⁺]_i and force of the coronary strips. Figure 1, c and d, showsa summary of the results obtained from seven and nine independentexperiments performed in a manner similar to that shown in fig.1, a and b. The cumulative application of AP₄A and AP₅A causeddecreases in [Ca⁺⁺]_i and force (P < .05 by an analysis of variance) in a concentration-dependentmanner. The IC₅₀ values for [Ca⁺⁺]_i and force were 1.14 ± 0.29 µM and 1.03 ± 0.16 µM for AP₄A (n= 7) and 0.82 ± 0.09 µM and 1.74 ± 0.34 µM for AP₅A (n = 9), respectively.There was no significant difference in these IC₅₀ values betweenAP₄A and AP₅A.

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Fig. 1. Effects of AP₄A and AP₅A on the changes in [Ca⁺⁺]_i and force induced by U46619 in the porcine coronary artery without endothelium.Panels a and b, representative recordings showing the effectsof AP₄A (a) and AP₅A (b) on the coronary artery precontractedby U46619. Various concentrations of AP₄A or AP₅A (0.01-10 µM)were cumulatively applied during the steady state contractioninduced by 60 nM U46619. Panels c and d, concentration-responsecurves for changes in [Ca⁺⁺]_i (c) and force (d) obtained by the cumulative addition of AP₄A( $open circle$ , n = 7) or AP₅A ( $square$ : n = 9) during 60 nM U46619-induced contraction.Vertical bars represent S.E.M.

Effects of AP₄A and AP₅A on the [Ca⁺⁺]_i and force and the [Ca⁺⁺]_i-force relation (the sensitivity of the contractile machinery) induced by high K⁺ depolarization. Figure 2 shows the representative recordings of the effects of 10 µM AP₄A (fig. 2, a-e) and AP₅A (fig. 2, f-j), respectively,on the [Ca⁺⁺]_i and force induced by high K⁺ depolarization (20, 30, 40, 60 and 118 mM). The extent of theAP₄A- and AP₅A-induced decrease in force during the high K⁺ depolarization was much greater than that expected from the extentof reduction of [Ca⁺⁺]_i. This effect can be typically seen in figure 2, c, d, e, h,i and j, where AP₄A (panels c, d and e) or AP₅A (panels h, i andj) induced relaxation with little or no reduction of [Ca⁺⁺]_i. These observations indicated that AP₄A and AP₅A might decreasethe Ca⁺⁺ sensitivity of the contractile machinery. To further analyzethe AP₄A- and AP₅A-induced change in the Ca⁺⁺ sensitivity, the [Ca⁺⁺]_i (abscissa)-force (ordinate) relation curves were constructedwith the data points obtained from several experiments done ina manner similar to shown in figure 2. As shown in figure 3, AP₄A(panel a) and AP₅A (panel b) shifted the [Ca⁺⁺]_i-force relation curves to the right (P < .05 by an analysisof covariance), which indicated that the reduction of force wasmuch greater than that expected from the given reduction in [Ca⁺⁺]_i levels (the decrease in Ca⁺⁺ sensitivity). AP₄A and AP₅A increased the ratio (%) values atwhich force was reduced by 50%, from 62.4 ± 6.2% to 76.3 ± 1.7%(AP₄A); from 59.9 ± 8.7% to 77.1 ± 1.2% (AP₅A).

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Fig. 2. Representative recordings showing the effects of 10 µM AP₄A or AP₅A on the elevations of [Ca⁺⁺]_i and force induced by various concentrations of extracellularK⁺. AP₄A (a-e) or AP₅A (f-j) was applied 15 min after the applicationof various concentration of K⁺ PSS as shown in each panel. Response of ratio and force to 118mM K⁺ was recorded before each experiment, as a control, and was designatedto be 100% (indicated by C).

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Fig. 3. Effects of AP₄A or AP₅A on the [Ca⁺⁺]_i-force relationship of the steady state contractions induced by various concentrationsof extracellular K⁺. Each point was obtained by the same protocol as that shown infigure 2. The [Ca⁺⁺]_i (abscissa)-force (ordinate) relationships of high K⁺-induced contractions (5.9, 20, 30, 40, 60 and 118 mM, as indicatedby the number shown in the figure) were obtained in the absence( $diamond$ , n = 4-8 for AP₄A and n = 4-6 for AP₅A) or presence ( $open circle$ , n =4-8 for AP₄A and n = 4-6 for AP₅A) of 10 µM AP₄A (a) or 10 µMAP₅A (b). The arrow tails and heads indicate the levels just beforeand 15 min after the application of AP₄A or AP₅A, respectively.The data are expressed as the means ± S.E.M.

Differential effects of AP₄A and AP₅A on the contractions induced by high K⁺ depolarization to those by U46619. As shown in figure 1, 10 µM AP₄A or AP₅A almost completely inhibited the increases in [Ca⁺⁺]_i and force induced by U46619, whereas 10 µM AP₄A or AP₅A hadlittle effect on the increases in [Ca⁺⁺]_i and force induced by high K⁺ depolarization (fig. 2, a-j) These observations indicated thatthe increase in [Ca⁺⁺]_i induced by high K⁺ depolarization is more resistant to inhibition by AP₄A or AP₅A.To further characterize this, we made a new figure (fig. 4) usingparts of the data points shown in figure 1, c and d, and figure3, a and b. At comparable [Ca⁺⁺]_i (30 mM K⁺ depolarization vs. 60 nM U46619) and force (60 mM K⁺ depolarization vs. 60 nM U46619) levels, both AP₄A and AP₅A inducedsmaller decreases in the [Ca⁺⁺]_i and force in the contractions induced by K⁺ depolarization than those induced by U46619 (fig. 4). These resultssuggest that the AP₄A- and AP₅A-induced decrease in [Ca⁺⁺]_i is caused, at least in part, by membrane hyperpolarization.

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Fig. 4. Comparison of AP₄A- or AP₅A-induced reductions of [Ca⁺⁺]_i and force during the activation by U46619 to those during high K⁺ depolarization. A comparison of the [Ca⁺⁺]_i level (a) was performed at the contractions between 60 nM U46619and 30 mM K⁺ depolarization, whereas a comparison of the force level (b) wasperformed at the contractions between 60 nM U46619 and 60 mM K⁺-depolarization. This is because the levels of increases in [Ca⁺⁺]_i and force induced by 60 nM U-46619 were comparable to the increasein [Ca⁺⁺]_i level induced by 30 mM K⁺-depolarization and to the increase in force level induced by60 mM K⁺-depolarization, respectively. The corresponding data points weretaken from fig. 1, c and d, and figure 3. Each column representsthe levels of [Ca⁺⁺]_i or force just before ( $square$ ) and after the application of eitherAP₄A (

) or AP₅A (

). The data are expressed as the means ± S.E.M.***; P < .001; n.s., difference not significant.

Effects of K⁺ channel blockers on AP₄A- and AP₅A-induced decreases in the [Ca⁺⁺]_i and force. To determine whether or not K⁺ channels are involved in the relaxation induced by AP_nA, we examined the effect of various K⁺ channel blockers on AP₄A- and AP₅A-induced decreases in [Ca⁺⁺]_i and force. The following K⁺ channel blockers were examined: 1 mM TBA (nonspecific K⁺ channel blocker), 100 nM ChTX (large conductance Ca⁺⁺-activated K⁺ channel blocker), 30 µM 4-AP (voltage-dependent K⁺ channel blocker), 3 µM glibenclamide (ATP-sensitive K⁺ channel blocker) and 1 µM apamin (small conductance Ca⁺⁺-activated K⁺ channel blocker). These K⁺ channel blockers were applied 10 min before and during the applicationof 60 nM U46619. We chose the highest concentrations of K⁺ channel blockers that do not directly affect U46619-induced increasesin [Ca⁺⁺]_i and force (Kawasaki et al., 1997). As shown in figure 5, aand b, TBA partially inhibited the AP₄A-induced decrease in [Ca⁺⁺]_i (P < .05 by an analysis of covariance) and TBA, ChTX and 4-APpartially inhibited the AP₄A-induced decrease in force (P < .05by an analysis of covariance). As shown in figure 5, c and d,TBA, ChTX and 4-AP partially inhibited the AP₅A-induced decreasein [Ca⁺⁺]_i and force (P < .05 by an analysis of covariance). Glibenclamideand apamin had no significant blocking effect on the decreasesin [Ca⁺⁺]_i and force induced by AP₄A or AP₅A (data not shown).

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Fig. 5. Effects of various types of K⁺ channel blockers on the decreases in [Ca⁺⁺]_i and force induced by various concentrations of AP₄A or AP₅A.The concentration-response curves for AP₄A (a and b) or AP₅A (cand d) were constructed in the same manner as in figure 1, c andd, in the absence ( $open circle$ ; n = 7 for AP₄A, n = 9 for AP₅A) or presenceof 1 mM TBA ( $bullet$ ; n = 4), 100 nM ChTX ( $black-diamond$ ; n = 7) or 30 µM 4-AP,( $triangle$ ; n = 7 for AP₄A, n = 5 for AP₅A). Vertical bars represent S.E.M.

Effects of AP₄A and AP₅A on the elevation of [Ca⁺⁺]_i and force induced by histamine and caffeine in the absence of extracellular Ca⁺⁺. Figure 6a shows representative time courses of the changes in [Ca⁺⁺]_i and force induced by histamine in Ca⁺⁺-free PSS containing 2 mM EGTA. When vascular strips were exposedto Ca⁺⁺-free PSS, [Ca⁺⁺]_i gradually declined to reach a steady state ( $-$ 21.60 ± 2.18%,n = 8), whereas the force remained unchanged. The applicationof 10 µM histamine after a 10-min incubation in Ca⁺⁺-free PSS caused transient elevations of [Ca⁺⁺]_i (22.51 ± 2.76%, n = 8) and force (48.04 ± 1.75%, n = 8) withpeaks at 15 s and 30 s, respectively. As shown in figure 6, band c, pretreatment with AP₄A or AP₅A for 10 min did not affectthe transient elevations of [Ca⁺⁺]_i induced by histamine. However, AP₄A and AP₅A did inhibit thetransient elevations of force induced by histamine. Figure 6dsummarizes the results obtained from eight independent experiments.

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Fig. 6. Effects of AP₄A or AP₅A on elevations of [Ca⁺⁺]_i and force induced by histamine or caffeine in Ca⁺⁺-free PSS containing 2 mM EGTA. Panels a, b and c: The representativerecordings of changes in [Ca⁺⁺]_i and force induced by 10 µM histamine in Ca⁺⁺-free PSS, in the absence (a) or presence of 10 µM AP₄A (b) or10 µM AP₅A (c). Panel d is a summary of the results obtained fromexperiments performed in the same manner as in panels a, b andc. The [Ca⁺⁺]_i and force development induced by the application of 10 µM histamineor 20 mM caffeine in the absence ( $square$ ; n = 8 for histamine and n= 5 for caffeine) or presence of AP₄A (

; n = 8 for histamineand n = 5 for caffeine) or AP₅A (

; n = 8 for histamine and n= 5 for caffeine). The bottom and top of each column indicatethe [Ca⁺⁺]_i and force just before and at the peak levels obtained by theapplication of histamine or caffeine, respectively. The data areexpressed as the means ± S.E.M. shown as vertical bars. **; P< .01; ***; P < .001; n.s., difference not significant.

Figure 6d also summarizes the changes in [Ca⁺⁺]_i and force induced by caffeine in Ca⁺⁺-free PSS containing 2 mM EGTA. The protocol for caffeine wassimilar to that for histamine (fig. 6, a-c). The application of20 mM caffeine after a 10-min incubation in Ca⁺⁺-free PSS induced transient elevations of [Ca⁺⁺]_i (35.82 ± 1,95%, n = 5) and force (11.80 ± 0.83%, n = 5) withpeaks at 30 s and 22 s, respectively. It is noteworthy that the[Ca⁺⁺]_i levels induced by 20 mM caffeine were significantly greaterthan those by 10 µM histamine (P < .01), whereas the forces inducedby the former were smaller than those by the latter (P < .01)(fig. 6d). A pretreatment with AP₄A and AP₅A for 10 min did notaffect the transient elevations of [Ca⁺⁺]_i and force induced by caffeine.

Effects of AP₄A and AP₅A on cellular cAMP and cGMP contents. Figure 7 shows effects of AP₄A and AP₅A on the levels of cellular cAMP and cGMP contents of the porcine coronary artery innormal PSS. The cellular cAMP and cGMP contents were 0.21 ± 0.03nmol/mg tissue (n = 14) and 2.04 ± 0.51 pmol/mg tissue (n = 14)at resting level (5.9 mM K⁺ PSS), respectively. When the vascular strips were exposed to10 µM AP₄A and AP₅A for 15 min in normal PSS, the intracellularcAMP levels significantly increased to 0.31 ± 0.03 nmol/mg tissue(n = 14) and 0.32 ± 0.04 nmol/mg tissue (n = 14; vs. control,P < .05 for both, by student's t test), respectively (fig. 7a).Neither AP₄A nor AP₅A induced any change in the intracellularcGMP levels (1.99 ± 0.34 and 2.38 ± 0.44 pmol/mg tissue) (fig.7b).

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Fig. 7. Effects of AP₄A or AP₅A on the tissue contents of cAMP and cGMP in the porcine coronary arterial smooth muscle. The contentsof cAMP (a) and cGMP (b) were determined by radioimmunoassay.Each column represents the levels of cAMP or cGMP in the absence( $square$ ; n = 14 for both) or presence of 10 µM AP₄A (

; n = 14 forboth) or 10 µM AP₅A (

; n = 14 for both). The data are expressedas the means ± S.E.M. shown as vertical bars. *; P < .05, n.s.,difference not significant.

	Discussion

Top Abstract Introduction Materials & Methods Results Discussion References

The present study investigated the mechanisms underlying the AP₄A- and AP₅A-induced direct relaxation of the porcine coronaryartery without endothelium. The results obtained indicate thatAP₄A and AP₅A induce relaxation of the porcine coronary arteryby decreasing [Ca⁺⁺]_i (fig. 1), which may be partially caused by the opening of K⁺ channels (fig. 5), and also by decreasing the Ca⁺⁺ sensitivity of the contractile machinery (fig. 3). These effectswere thought to be mediated by cAMP, because AP₄A and AP₅A increasedthe cellular cAMP content (fig. 7). In addition, AP₄A and AP₅Ahad no effect on the intracellular Ca⁺⁺ release mechanism (fig. 6).

The relaxing effect of AP₄A on the coronary artery has already been described previously. Pohl et al. (1991) first reportedthat AP₄A induces endothelium-dependent and -independent decreasesin rabbit coronary perfusion pressure. Nakae et al. (1996) alsoreported AP₄A-induced coronary vasodilation in the porcine. However,the AP₅A-induced vasorelaxation apparently has not been describedpreviously. The results obtained in the present study indicatethat AP₄A- and AP₅A-induced relaxation of the coronary arteryis accompanied by a reduction of [Ca⁺⁺]_i. This mechanism could be clearly seen when precontraction wasinduced by U46619 (fig. 1). However, when precontraction was inducedby 60 mM or 118 mM K⁺ depolarization, the reduction of [Ca⁺⁺]_i was less obvious, although the reduction of force could stillbe detected (fig. 2). This result indicates that reduction of[Ca⁺⁺]_i is not the sole mechanism for the AP₄A- or AP₅A-induced coronaryvasorelaxation.

The mechanism other than the reduction of [Ca⁺⁺]_i for the AP₄A- or AP₅A-induced coronary vasorelaxation was explored in theexperiments shown in figures 2 and 3. As shown in figure 2, c,d, e, h, i and j, where AP₄A and AP₅A induced relaxation withlittle or no reduction of [Ca⁺⁺]_i. AP₄A and AP₅A shifted the [Ca⁺⁺]_i-force curve to the right during stimulation with high-K⁺ depolarization (fig. 3), which indicates that AP₄A and AP₅A decreasethe Ca⁺⁺ sensitivity of the contractile machinery. This mechanism alsoexplains the observation that AP₄A and AP₅A inhibited the developmentof force without affecting the transient increase in [Ca⁺⁺]_i induced by histamine in Ca⁺⁺-free medium (fig. 6). However, this is not case in the contractionsinduced by 20 mM caffeine in Ca⁺⁺-free medium (fig. 6d). Neither AP₄A nor AP₅A were able to inhibitthe caffeine-induced transient force development. In Ca⁺⁺-free medium without AP_nA, 20 mM caffeine induced a much smallerforce than 10 µM histamine, although the former induced a greater[Ca⁺⁺]_i elevation than the latter (fig. 6). We reported previouslythat caffeine increases cAMP, which markedly decreases Ca⁺⁺ sensitivity of the contractile machinery (Watanabe et al., 1992).The inability for AP₄A and AP₅A to decrease the caffeine-inducedcontraction could be explained by the saturation of the effectof cAMP on the reduction of the Ca⁺⁺ sensitivity, because the relaxing effect of AP₄A and AP₅A wasalso mediated by cAMP (fig. 7). We did not use permeabilized preparations,which could directly demonstrate the decrease in the Ca⁺⁺ sensitivity, because the solution used for permeabilized cellpreparations contains millimolar concentrations of ATP. Theseconditions may desensitize the purinergic and possibly adenosinereceptors, that are proposed to be involved in AP₄A- and AP₅A-inducedvasorelaxation (discussed later).

It is well known that contraction of vascular smooth muscle is regulated by agonist-mediated modulation of the [Ca⁺⁺]_i-force relation (= the Ca⁺⁺ sensitivity of the contractile machinery) as well as the changesin [Ca⁺⁺]_i (Somlyo and Somlyo, 1994). As to the candidate mediator forthe reduction of Ca⁺⁺ sensitivity, cAMP and cGMP have been shown to decrease the Ca⁺⁺ sensitivity of the smooth muscle contractile machinery (Nishimuraand van Breemen, 1989). We have also shown in a previous studythat nitroglycerine (Abe et al., 1990) and isoprenaline (Ushio-Fukaiet al., 1993) shift the [Ca⁺⁺]_i-force relation to the right in the porcine coronary artery.It thus seems likely that the decreases in Ca⁺⁺ sensitivity of the contractile machinery induced by AP₄A or AP₅Amay be mediated by cAMP or cGMP. In the present study we determinedthe second messenger for AP₄A- or AP₅A-induced vasorelaxation.As shown in figure 7, both AP₄A and AP₅A increased the cellularcontents of cAMP. These results also support the hypothesis thatAP₄A and AP₅A decrease the Ca⁺⁺ sensitivity of the contractile machinery.

The inhibitory effects of AP₄A or AP₅A on [Ca⁺⁺]_i and force were attenuated when the strips were precontracted by high K⁺ depolarization, as compared with those during U46619 stimulation(fig. 4). This observation evoked speculation that the reductionof [Ca⁺⁺]_i might involve membrane hyperpolarization mediated by the openingof K⁺ channels, because this mechanism is eliminated during high K⁺ depolarization. Recent evidence has suggested that vascular toneand membrane potential are regulated by several types of K⁺ channels, including Ca⁺⁺-activated K⁺ channels, voltage-dependent K⁺ channels and ATP-sensitive K⁺ channels (Nelson and Quayle, 1995). Therefore, we investigatedthe effects of selective blockers for these K⁺ channels on the AP₄A- and AP₅A-induced decrease in [Ca⁺⁺]_i and force during the stimulation with U46619. Comparative studieswith these selective K⁺ channel blockers, as shown in figure 5, suggest that the activationof large conductance Ca⁺⁺-activated K⁺ channels and voltage-dependent K⁺ channels may contribute to the decrease in [Ca⁺⁺]_i and force. It has been hypothesized that cAMP may decrease[Ca⁺⁺]_i by a hyperpolarization (Somlyo et al., 1970) probably by stimulationof Ca⁺⁺-activated K⁺ channel openings (Sadoshima et al., 1988). Thus, the presentresults that AP₄A and AP₅A significantly increased the intracellularcAMP levels (fig. 7) support the idea that AP₄A and AP₅A may inducemembrane hyperpolarization mediated by the opening of K⁺ channels. Our results do not support the notion that ATP-sensitiveK⁺ channels and small conductance Ca⁺⁺-activated K⁺ channels play a major role in the AP₄A- and AP₅A-induced vasorelaxationand decrease in [Ca⁺⁺]_i.

Another potential mechanism for the reduction of [Ca⁺⁺]_i, namely the inhibition of Ca⁺⁺ release from intracellular stores, was examined in the experimentsshown in figure 6. AP₄A and AP₅A did not inhibit the histamine-and caffeine-induced release of intracellular Ca⁺⁺ in the absence of extracellular Ca⁺⁺. These observations suggested that AP₄A and AP₅A do not affectintracellular Ca⁺⁺ release through inhibition of a receptor-coupled signal transductionpathway or through a direct effect on intracellular storage sites.

The receptors responsible for the AP₄A- and AP₅A-induced coronary vasorelaxation were not explored in the present study. Ithas been reported that mammalian cells typically contain a specificAP₄A hydrolase that hydrolyzes AP₄A in an asymmetric fashion toyield AMP and ATP, which is converted to AMP and inorganic pyrophosphate;and dephosphorylation of AMP yields adenosine (Hankin et al.,1995; Luthje and Ogilvie, 1985, 1988; Ogilvie et al., 1989; Thorneet al., 1995). This enzyme also hydrolyzes higher homologs (e.g.,AP₅A in an asymmetric fashion to yield ADP and ATP) and is presumedto be involved in the regulation of the intracellular level ofsuch nucleotides (Guranowski and Sillero, 1992). Thus, it is possiblethat the application of AP₄A and AP₅A may produce adenosine, AMP,ADP and ATP, and stimulate such multiple receptors as nucleotidereceptors and adenosine receptors. This may also partly explainwhy AP₄A and AP₅A have a different functional effect (constrictionin some smooth muscle and relaxation in the other) at differentpotencies. For example, AP₅A was approximately 10 to 1000 timesmore potent than AP₄A for the contraction of guinea pig urinarybladder and vas deferens (Bo et al., 1994; Hoyle et al., 1995;Ralevic et al., 1995; Stone and Paton, 1989). For the vasoconstrictionof rat and rabbit mesenteric vessels, AP₅A was more potent thanAP₄A (Busse et al., 1988; Ralevic et al. 1995). On the other hand,there was no significant difference in the potency of AP₄A andAP₅A to induce relaxation of the guinea pig left atrium (Hoyleet al., 1996). We also observed almost equal potency for AP₄A-and AP₅A-induced coronary vasorelaxation. However, it is stillpossible that AP₄A and AP₅A might stimulate receptors as theirown form without degradation because it has been reported thatAP_nA can be considered as the long-lived substances (Busse etal., 1988; Hoyle et al., 1996; Pohl et al., 1991). In agreementwith this speculation, the specific and saturable membrane receptorsfor AP₄A have been reported to be present in brain, cardiac, liver,kidney, spleen and adipose tissue (Hilderman et al., 1991; Walkerand Hilderman, 1993).

In summary, we obtained evidence that AP₄A and AP₅A induce relaxation of the porcine coronary artery by decreasing [Ca⁺⁺]_i, which may be partially caused by the opening of K⁺ channels, and decreasing the Ca⁺⁺ sensitivity of the contractile machinery. These effects werethought to be mediated by cAMP. These substances may be naturallyoccurring coronary dilators.

	Acknowledgments

We thank B. Quinn for comments on this manuscript. We also thank K. Kajishima for her excellent secretarial services.

	Footnotes

Accepted for publication July 16, 1997.

Received for publication March 7, 1997.

¹ This study was supported in part by Grants-in-Aid for Developmental Scientific Research (no. 06557045), for General ScientificResearch (nos. 07407022, 07833008) and for Creative Basic ResearchStudies of Intracellular Signaling Network from the Ministry ofEducation, Science, Sports and Culture, Japan, and also by Grantsfrom Japan Research Foundation of Clinical Pharmacology and theVehicle Racing Commemorative Foundation.

² Department of Anesthesiology and Critical Care Medicine, Faculty of Medicine, Kyushu University, Fukuoka 812-82, Japan.

Send reprint requests to: Professor Hideo Kanaide, M.D., Ph.D.. Division of Molecular Cardiology, Research Institute of Angiocardiology, Faculty of Medicine, Kyushu University, 3-1-1 Maidashi, Higashi-ku, Fukuoka 812-82, Japan.

	Abbreviations

[Ca⁺⁺]_i, cytosolic Ca⁺⁺ concentration; AP_nA, diadenosine polyphosphates; AP₄A, 5 $'$ ,5 $'''$ -P¹,P⁴-tetraphosphate; AP₅A, diadenosine 5 $'$ ,5 $'''$ -P¹,P⁵-pentaphosphate; TBA, tetrabutylammonium; 4-AP, 4-aminopyridine; ChTX, charybdotoxin; cAMP, cyclic AMP (adenosine 3 $'$ ,5 $'$ -cyclic monophosphate); cGMP, cyclic GMP (guanosine 3 $'$ ,5 $'$ -cyclic monophosphate); PSS, physiological salt solution; EGTA, ethyleneglycol-bis( $beta$ -aminoethyl ether)-N,N,N $'$ ,N $'$ -tetraacetic acid.

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Diadenosine Polyphosphates Directly Relax Porcine Coronary Arterial Smooth Muscle1

Diadenosine Polyphosphates Directly Relax Porcine Coronary Arterial Smooth Muscle¹