Rationale for the Combination of PGE1 and S-Nitroso-glutathione to Induce Relaxation of Human Penile Smooth Muscle

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Vol. 295, Issue 2, 586-593, November 2000

Rationale for the Combination of PGE₁ and S-Nitroso-glutathione to Induce Relaxation of Human Penile Smooth Muscle¹

Javier Angulo, Pedro Cuevas, Ignacio Moncada, Antonio Martín-Morales, Antonio Allona, Argentina Fernández, Sonia Gabancho, Peter Ney and Iñigo Sáenz de Tejada

Fundación para la Investigación y el Desarrollo en Andrología, Madrid, Spain (J.A., I.M., A.M.-M., A.A., S.G., I.S.d.T.); Departmento de Investigación, Hospital Ramón y Cajal, Madrid, Spain (P.C., A.F.); and Corporate Development, Schwarz-Pharma, Monheim, Germany (P.N.)

	Abstract

Top Abstract Introduction Experimental Procedures Results Discussion References

Many men with erectile dysfunction have been successfully treated with intracavernosal injection of prostaglandin E₁ (PGE₁)but this treatment is ineffective in 30 to 40% of patients. Thegoals of this study were to characterize PGE₁-induced relaxationof isolated human penile smooth muscle (penile arteries and trabecularstrips), correlating this in vitro response with the clinicalresponse to this drug, and to evaluate the effects of the combinationof PGE₁ with S-nitrosoglutathione (SNO-Glu) on relaxation of isolatedhuman penile smooth muscle. Large variability in the EC₅₀ andmaximal relaxation induced by PGE₁ was observed between tissuesof different patients. Patients with poor clinical response tointracavernosal alprostadil (PGE₁) had significantly larger EC₅₀values and smaller maximal relaxation compared with patients withpartial or complete clinical response to this drug. SNO-Glu consistentlyproduced complete or near complete relaxation of human corpuscavernosum strips and penile arteries, even when the tissue respondedpoorly to PGE₁. In trabecular strips, the combination of PGE₁and SNO-Glu in a 1:100 ratio demonstrated a synergistic relaxationeffect. The combination of PGE₁ and SNO-Glu simultaneously increasedthe levels of both cAMP and cGMP in human corpus cavernosum tissue.Our results suggest that the clinical effectiveness of intracavernosaladministration of PGE₁ is related to the variability of the relaxationresponses of human trabecular tissue and penile arteries to thisdrug. The synergistic interaction of PGE₁ and SNO-Glu makes thiscombination an effective method to cause penile smooth musclerelaxation, a necessary step to initiate and maintain penileerection.

	Introduction

Top Abstract Introduction Experimental Procedures Results Discussion References

Intracavernosal prostaglandin E₁ (PGE₁) has been extensively used as a therapeutic agent for the treatment of erectile dysfunction(Buvat et al., 1996, 1998; Linet and Ogring, 1996). Although somesuccess has been obtained, a considerable number of patients (about30-40%) have not responded to treatment with PGE₁ (Porst, 1996).The reason for the lack of response to PGE₁ in refractory patientsis not known, but could depend on many factors (number of receptors,transduction mechanisms, metabolism, tissue structure, etc.).Indeed, it has not been demonstrated that the efficacy in theclinical response to PGE₁ correlates with the relaxation of humanpenile smooth muscle (arterial and trabecular) to thisdrug.

PGE₁ promotes relaxation of penile arterial smooth muscle via prostacyclin (IP) receptors and of trabecular smooth musclethrough interaction with prostaglandin E (EP) receptors, withsome preliminary data supporting a key role for the EP₂ receptorsubtype (Andersson and Wagner, 1995; Sáenz de Tejada et al.,1998). IP and EP receptors, coupled to G-proteins, increase intracellularcAMP levels through adenylyl cyclase stimulation (Andersson andWagner, 1995). Penile smooth muscle relaxation; however, is notonly mediated by the cAMP pathway but also by the nitric oxide(NO)-cGMP pathway, which plays a fundamental role in the relaxationof human penile smooth muscle (Kim et al., 1991; Rajfer et al.,1992) and penile erection (Burnett et al., 1992; Trigo-Rocha etal., 1993). Activation of the cGMP pathway is brought about bythe endogenous generation of NO from lacunar and vascular endotheliaand nitrergic nerves. The existence of NO donors allows for pharmacologicalactivation of the cGMP pathway and facilitates penile erection(Truss et al., 1994; Martínez-Piñeiro et al., 1998). S-Nitrosothiolsare NO donor molecules, some of which are present in human plasmaand tissues in physiological conditions and one of these compounds,S-nitrosoglutathione (SNO-Glu) has been reported to induce vascular(MacAllister et al., 1995) and penile trabecular (Gupta et al.,1995) smooth muscle relaxation. In addition, promising, althoughpreliminary clinical data have shown that intracavernosal coadministrationof PGE₁ and the NO donor linsidomine chlorhydrate (SIN-1) producesbetter erectile responses than those obtained with either compoundindividually (Tordjman, 1993). The mechanism behind such possibleclinical benefit has not beendetermined.

The aim of the present study was to analyze the relaxant responses to PGE₁ in human corpus cavernosum and penile resistancearteries from impotent patients and to determine whether the clinicalresponse to PGE₁ would depend, at least in part, on the degreeof penile smooth muscle relaxation induced by this prostanoid.We also sought to evaluate possible synergistic effects of combiningPGE₁ and SNO-Glu to cause relaxation of penile smoothmuscle.

	Experimental Procedures

Top Abstract Introduction Experimental Procedures Results Discussion References

Human Corpus Cavernosum Tissues. Human corpus cavernosum specimens were obtained from impotent men at the time of penile prosthesis insertion. All experimentalprotocols were approved by the local ethics committee. Tissueswere maintained at 4-6°C in M-400 solution (composition per 100ml: 4.19 g of mannitol, 0.205 g of KH₂PO₄, 0.97 g of K₂HPO₄·3H₂O,0.112 g of KCl, 0.084 g of NaHCO₃, pH 7.4) until used, which rangedbetween 2 and 16 h after extraction (Simonsen et al., 1997).

Vascular Reactivity of Resistance Penile Arteries. Penile small arteries, helicine arteries (lumen diameter 150-400 µm), which are the terminal branches of deep penile arteries,were dissected by carefully removing the adhering trabecular tissue,and arterial ring segments (2 mm in length) were subsequentlymounted on two 40-µm wires on microvascular Halpern-Mulvany myographs(J.P. Trading, Aarhus, Denmark) for isometric tension recordings.The vessels were allowed to equilibrate for 30 min in physiologicalsalt solution (PSS) of the following composition: 119 mM NaCl,4.6 mM KCl, 1.5 mM CaCl₂, 1.2 mM MgCl₂, 24. 9 mM NaHCO₃, 11 mMglucose, 1.2 mM KH₂PO₄, and 0.027 mM EDTA at 37°C continuouslybubbled with 95% O₂, 5% CO₂ to maintain a pH of 7.4. Passive tensionand internal circumference of vascular segments when relaxed insitu under a transmural pressure of 100 mm Hg (L₁₀₀), were determined.The arteries were then set to an internal circumference equivalentto 90% of L₁₀₀, at which the force development was close to maximal(Mulvany and Halpern, 1977). The preparations were then exposedto 125 mM K⁺ (equimolar substitution of NaCl for KCl in PSS) and the contractileresponse was measured. The arteries were contracted with 1 µMnorepinephrine and relaxation responses were evaluated by cumulativeadditions of compounds to the chambers. Relaxant responses areexpressed as percentage of total relaxation (loss in tone) inducedby the addition of 0.1 mM papaverine HCl to the chambers at theend of the experiment. All data are expressed as mean ± S.E.

Organ Chamber Studies. Strips of corpus cavernosum tissue (3 × 3 × 7 mm) were immersed in 8-ml organ chambers containing PSS, maintained at 37°C,and aerated with 95% O₂, 5% CO₂, pH 7.4. Each tissue strip wasincrementally stretched to optimal isometric tension, as determinedby the maximal contractile response to 1 µM phenylephrine (Kimet al., 1991; Azadzoi et al., 1992). Relaxant responses were evaluatedby adding increasing cumulative concentrations of compounds tostrips contracted with 0.5 µM phenylephrine. Relaxation responsesare expressed as percentage of total relaxation (loss in tone)induced by the addition of 0.1 mM papaverine HCl to the chambersat the end of the experiment. All data are expressed as mean ±S.E. In studies using a combination of relaxant compounds, a molarproportion of 1:100, PGE₁:SNO-Glu, was chosen based on the EC₅₀value for penile smooth muscle relaxation for each compoundindividually.

Measurement of Cyclic Nucleotides in Human Corpus Cavernosum Tissue. Corpus cavernosum strips were immersed in 8-ml organ chambers containing PSS, maintained at 37°C, and aerated with 95% O₂,5% CO₂, pH of 7.4. Each tissue strip was incrementally stretchedto optimal isometric tension, as determined by the maximal contractileresponse to 1 µM phenylephrine. Then each tissue was treated withthe phosphodiesterase inhibitors zaprinast (30 µM) and 3-isobutyl-1-methylxanthine(100 µM) and allowed to incubate for 15 min, after which timetissues were treated with drug or vehicle. Tissues were allowedto incubate for another 30 min and then immediately frozen inliquid nitrogen and stored at $-$ 80°C until extraction for the cyclicnucleotide assay. Tissues were extracted by homogenization in6% trichloroacetic acid followed by ether (H₂O-saturated) extractionand lyophilization. Cyclic nucleotides were determined by enzyme-linkedimmunosorbent assay using a kit from Cayman Chemical Co. (AnnArbor,MI).

Protein Determinations. Protein were determined using the Bio-Rad Protein Assay kit microtiter plate assay procedure (Bio-Rad, Hercules, CA) withBSA as thestandard.

Drugs and Materials. Phenylephrine, norepinephrine (arterenol), and zaprinast were obtained from Sigma Chemical Co. (St. Louis, MO). 3-Isobuytl-1-methylxanthinewas obtained from Research Biochemicals International (Natick,MA). PGE₁- $alpha$ -cyclodextrine was kindly provided by Schwarz-Pharma(Monheim, Germany). SNO-Glu was kindly provided by Nitromed Inc.(Bedford, MA). Drugs were dissolved in distilled water at thetime of theexperiment.

Statistical Evaluation. A total of 57 patients was included in the study of individual responses to PGE₁. We obtained penile resistance arteries from22 of them and trabecular tissue from 39 (both arteries and cavernosalstrips were collected from four patients). Individual EC₅₀ (concentrationrequired to obtain the half-maximum response induced by the compound)and maximum relaxations to PGE₁ werecalculated.

Patients were divided into two groups according to the clinical erectile response (poor and partial or complete) to PGE₁,as assessed by the degree of penile tumescence after intracavernosalinjection of alprostadil (PGE₁) determined by visual and physicalexamination of the penis by the attending physician. The comparisonof EC₅₀, maximum relaxation, and clinical response to alprostadilbetween both groups was done by Student's t test analysis, whichwas evaluated using StatView software (Abacus Concepts, Inc.,Cary, NC) for Applecomputers.

Evaluation of the effects of PGE₁ and SNO-Glu, alone or in combination, on penile smooth muscle relaxation and cyclic nucleotideaccumulation was performed in tissues from another group of 10patients (five for relaxation studies and five for cyclic nucleotidedeterminations). Complete concentration-response curves were obtainedand compared by a two-factor ANOVA statistical analysis usingStatView software for Apple computers. Statistical analysis oftissue cyclic nucleotide levels was performed by ANOVA followedby a Student-Newman-Keuls post hoc test using GraphPad (San Diego,CA) InStatsoftware.

Determination of synergism for the combination of PGE₁ and SNO-Glu was performed according to the "isobole method" (Berenbaum,1989

). This method applies the equation d_a/D_a + d_b/D_b = 1 to definethe additive effects between two agents, A and B, where d_a andd_b are the concentrations of agents A and B in the combinationthat is needed to obtain a specified level of the effect (relaxation),and D_a and D_b are the single concentrations of the drugs requiredto achieve the same level of effect. Synergy is assumed when solvingthis equation gives a value less than unity. Applying this equation,we determined, in each patient, the theoretical concentrationsof the PGE₁ and SNO-Glu combination (always in a 1:100 M ratio)needed to obtain several specified levels of relaxation of trabecularsmooth muscle (10, 20, 40, 60, and 70%) when additive effectsbetween the two agents areassumed.

The following equation is the application of the isobole method described by Berenbaum (d_a/D_a + d_b/D_b = 1) to our model. Weused this equation to obtain the theoretical concentration ofPGE₁ in the combination ([SNO-Glu] is 100-fold higher) neededto obtain a specified level of relaxation when only additive effectsare present.

<FR><NU>[<UP>PGE<SUB>1</SUB></UP>]<UP> in the combination</UP></NU><DE>[<UP>PGE<SUB>1</SUB> alone</UP></DE></FR>+<FR><NU>100 · [<UP>PGE<SUB>1</SUB></UP>]<UP> in the combination</UP></NU><DE>[<UP>SNO-Glu</UP>]<UP> alone</UP></DE></FR>=1

Using these data we constructed a theoretical curve that was compared with the curve experimentally obtained with the combinationof PGE₁ and SNO-Glu. Comparison of these curves was performedby a two-factor ANOVA using StatViewsoftware.

	Results

Top Abstract Introduction Experimental Procedures Results Discussion References

Evaluation of Individual Responses to PGE₁ in Human Penile Smooth Muscle. Relaxations induced by PGE₁ were individually studied in strips of corpus cavernosum from 39 impotent patients and in penileresistance arteries from 22 patients (Fig. 1). Notable variabilitywas observed with respect to the relaxant responses produced byPGE₁ in trabecular smooth muscle from different patients, resultingin a range of several orders of magnitude in individual EC₅₀ values(mean 0.226 µM, standard deviation 0.418, range from 0.01 to 10µM) and variability in maximal relaxation (mean 83.5%, standarddeviation 12.0, range from <60 to 100%). Similar results wereobtained when PGE₁-induced relaxations were evaluated in individualpenile resistance arteries, showing variability in EC₅₀ values(mean 0.896 µM, standard deviation 1.097, range from 0.01 to 10µM), and more noteworthy in maximal relaxation (mean 73.3%, standarddeviation 23.2, range from 50 to 100%).

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Fig. 1. Individualized responses to PGE₁ (1 nM to 10 µM) in human corpus cavernosum strips (top) contracted with phenylephrine (1 µM) and human penile resistance arteries (bottom) contracted with norepinephrine (1 µM) from 39 and 22 impotent patients, respectively. Data are expressed as the percentage of total relaxation induced by 0.1 mM papaverine.

Analysis of the data showed a statistically significant correlation between the clinical effectiveness of PGE₁ and the magnitudeof the relaxations obtained in vitro with PGE₁. Lower EC₅₀ valuesfor PGE₁ and larger maximal relaxations were observed when corpuscavernosum strips or penile arteries originated from patientswith better clinical response to intracavernosal injection ofPGE₁ (Fig. 2).

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Fig. 2. EC₅₀ values for PGE₁ (top) and maximum relaxation responses to PGE₁ (bottom) obtained in human corpus cavernosum strips contracted with phenylephrine (1 µM) (left) and human resistance penile arteries contracted with norepinephrine (1 µM) (right). The tissues were divided into two groups depending on the patients clinical erectile response (poor, n = 20 and n = 14; partial or complete, n = 19 and n = 8 for trabecular tissue strips and penile arteries, respectively) to intracavernosal injection of alprostadil (PGE₁). EC₅₀ is defined as the concentration of PGE₁ (in µM) required to obtain half of the maximum response to this drug. Maximum relaxation data are expressed as the percentage of total relaxation induced by 0.1 mM papaverine. *P < .05 and **P < .01 between groups by two-tailed Student's t test.

Relaxant Responses Induced by the Combination of SNO-Glu and PGE₁ on Human Penile Smooth Muscle. The nitrosothiol SNO-Glu produced consistent relaxations of human corpus cavernosum strips and penile resistance arteriesin a concentration-dependent manner. Administration of SNO-Glualways elicited a near-to-full relaxation of both penile smoothmuscle preparations even when tissue from the same patient respondedpoorly to PGE₁. Representative examples of this observation areshown in Fig. 3. The coadministration of PGE₁ and SNO-Glu in a1:100 proportion (PGE₁:SNO-Glu) caused concentration-dependentrelaxation of both trabecular and arterial smooth muscle.

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Fig. 3. Tracings of concentration-response curves to PGE₁ (0.1 nM to 10 µM) and SNO-Glu (10 nM to 1 mM) in human corpus cavernosum strips contracted with 1 µM phenylephrine (PE) (top) and penile resistance arteries contracted with 1 µM norepinephrine (NE) (bottom). Note the poor response to PGE₁ and full relaxation to SNO-Glu. Concentrations are expressed as the log of molarity. Concentration-response curves to PGE₁ and SNO-Glu were performed in parallel tissues from the same patient.

Figure 4 shows relaxation to PGE₁ alone compared with relaxation caused by the combination of PGE₁ and SNO-Glu plotted asonly PGE₁ concentrations. There was a significant shift to theleft of the PGE₁ concentration-response curve with the coadministrationof SNO-Glu. (In trabecular tissue, EC₅₀ for PGE₁ alone was 0.083± 0.05 µM versus 0.006 ± 0.001 µM for PGE₁ + SNO-Glu, P < .01;in penile arteries, EC₅₀ for PGE₁ alone was 0.402 ± 0.160 µM versus0.043 ± 0.023 µM for PGE₁ + SNO-Glu, P < .01. Maximum responsesfor PGE₁ in trabecular tissue were 71.0 ± 5.1% versus 95.2 ± 2.1%with the PGE₁ + SNO-Glu combination, P < .01; and 52.9 ± 13.9%versus 91.4 ± 2.6% for PGE₁ versus PGE₁ + SNO-Glu, respectively,P < .01 in penile arteries.)

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Fig. 4. Concentration-response curves to PGE₁ (0.1 nM to 10 µM) and to the combination of PGE₁ (0.1 nM to 10 µM) and SNO-Glu (PGE₁/SNO-Glu, in 1:100 M ratio) in human corpus cavernosum strips contracted with phenylephrine (1 µM) (top) and human penile resistance arteries contracted with norepinephrine (1 µM) (bottom). The concentration-response curve obtained with the combination of PGE₁ and SNO-Glu is plotted only as PGE₁ concentrations. Data are expressed as mean ± S.E. of the percentage of total relaxation induced by 0.1 mM papaverine. n indicates the number of patients from whom the tissues were collected for the experiments. Concentration-response curves to PGE₁ and to the combination of PGE₁ and SNO-Glu were carried out in parallel tissues from the same patients. *, two-factor ANOVA indicates significant differences (P < .01) between the concentration-response curve obtained with the combination of PGE₁ and SNO-Glu and that elicited by PGE₁ alone.

The relaxation response of the PGE₁ and SNO-Glu combination was also compared with the relaxation-response curve induced bySNO-Glu alone, but this time plotted as only the concentrationof SNO-Glu in the combination, as shown in Fig. 5. There was asignificant shift to the left of the SNO-Glu concentration-responsecurve with the coadministration of PGE₁ in trabecular tissue,but not in penile arteries. The EC₅₀ for SNO-Glu alone was 2.56± 1.3 µM versus 0.58 ± 0.16 µM for SNO-Glu + PGE₁ (P < .05) intrabecular tissue. Maximum responses were 94.4 ± 4.2% for SNO-Gluversus 95.2 ± 2.1% for SNO-Glu + PGE₁ and were not significantlydifferent from each other.

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Fig. 5. Concentration-response curves to SNO-Glu (10 nM to 1 mM) and to the combination of PGE₁ and SNO-Glu (10 nM to 1 mM; PGE₁/SNO-Glu, in 1:100 M ratio) in human corpus cavernosum strips contracted with phenylephrine (1 µM) (top) and human penile resistance arteries contracted with norepinephrine (1 µM) (bottom). The concentration-response curve obtained with the combination of PGE₁ and SNO-Glu is plotted only as SNO-Glu concentrations. Data are expressed as mean ± S.E. of the percentage of total relaxation induced by 0.1 mM papaverine. n indicates the number of patients from whom the tissues were collected for the experiments. Concentration-response curves to SNO-Glu and to the combination of PGE₁ and SNO-Glu were carried out in parallel tissues from the same patients. *, two-factor ANOVA indicates significant differences (P < .01) between the concentration-response curve obtained with the combination of PGE₁ and SNO-Glu and that elicited by SNO-Glu alone in human corpus cavernosum strips.

The possible existence of synergism in the relaxation of penile smooth muscle between PGE₁ and SNO-Glu was analyzed from theresponses obtained with the drug combination in human penile trabecularand arterial smooth muscle. The actual experimental curve withthe concentrations of the PGE₁ and SNO-Glu combination neededto obtain several specified levels of relaxation (10, 20, 40,60, and 70%) was compared with the calculated theoretical curveassuming additive effects of both drugs (under Experimental Procedures).Significantly lower concentrations of the PGE₁ and SNO-Glu combinationwere required than those that would be expected if only additiveeffects occurred between both compounds. This suggests a synergisticinteraction between PGE₁ and SNO-Glu in the relaxation of trabecularsmooth muscle (Fig. 6, top). However, PGE₁ and SNO-Glu did notexert synergistic effects in causing relaxation of penile arterialsmooth muscle (Fig. 6, bottom).

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Fig. 6. Analysis of synergism of the relaxations elicited by the combination of PGE₁ and SNO-Glu in human corpus cavernosum strips (top) and penile resistance arteries (bottom). Starting from the responses obtained with the two compounds individually, the theoretical concentrations of the drugs in the combination required to achieve several specified levels of relaxation, when additive effects are assumed, were calculated and compared with those experimentally determined. Data are expressed as mean ± S.E. of the concentrations of PGE₁ (in nM) present in the combination (concentration of SNO-Glu is 100-fold higher). n indicates the number of patients from whom the tissues were collected for the determinations. Synergistic effects were observed in human trabecular smooth muscle (*P < .05 versus theoretical additive effects by two-factor ANOVA) but not in penile resistance arteries.

Effect of the Combination of PGE₁ and SNO-Glu on Cyclic Nucleotide Accumulation in Corpus Cavernosum Tissue. Tissue levels of cGMP were not significantly altered by incubation with PGE₁ (1 µM), but a remarkable increase was observedwhen treating the tissues with SNO-Glu (100 µM). Incubation oftrabecular tissues with the combination of PGE₁ and SNO-Glu induceda significant increase in cGMP content compared with control (Fig.7, top).

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Fig. 7. cGMP (top) and cAMP (bottom) tissue content of human corpus cavernosum after exposure to PGE₁ (1 µM), SNO-Glu (100 µM), or both. Data are expressed as mean ± S.E. of picomoles of cGMP or cAMP per milligram of tissue protein content. n indicates the number of patients from whom the tissues were collected for the determinations. *P < .05, **P < .01 versus control. (Student-Newman-Keuls post hoc test).

cAMP content was increased by incubation of tissues with PGE₁ (1 µM). Incubation of the strips with SNO-Glu (100 µM) did notmodify tissue cAMP levels and the combination of SNO-Glu + PGE₁produced an increase in cAMP content that was similar to thatobtained with PGE₁ alone (Fig. 7,bottom).

	Discussion

Top Abstract Introduction Experimental Procedures Results Discussion References

In clinical trials, response rates in the range of 40 to 70% to intracavernosal injection of PGE₁ have been reported in patientssuffering from erectile dysfunction (Buvat et al., 1996, 1998;Linet and Ogring, 1996; Porst, 1996). This observation, supportedby extensive clinical experience, presents intracavernous injectionof PGE₁ as an efficacious treatment for impotence. However, aconsiderable number of patients do not respond to such treatmentfor unknown reasons. Furthermore, the dose of PGE₁ required toachieve satisfactory erections is markedly variable, ranging from0.5 to 20 µg (Linet and Ogring, 1996), with some patients needingdoses as high as 40 µg to obtain responses (Porst, 1996).

Analysis of in vitro responses to PGE₁ in penile arterial and trabecular tissues from impotent patients shows a great degreeof variability in the relaxation of human penile smooth muscleto this prostanoid. The variability of PGE₁-induced relaxationswas observed in human penile resistance arteries as well as corpuscavernosum strips and it affected both the sensitivity to PGE₁,obtaining EC₅₀ values separated by several orders of magnitude,and the maximum relaxation, which varied, especially in penilearteries, from less than 50% to complete relaxation (100%). Itis interesting to note that the in vitro response to PGE₁ in humanpenile tissues correlated with the clinical response to PGE₁ inthe patients from whom the tissue was obtained. Our results showthat poor responses to intracavernosal alprostadil are associatedwith diminished maximum response and increased EC₅₀ of the relaxationsto PGE₁ in vitro. These data suggest that a lack of clinical responseto PGE₁ may be, in many cases, due to the inability of this prostanoidto relax penile arterial and/or trabecular smooth muscle sufficiently.The mechanisms underlying reduced penile smooth muscle relaxationto PGE₁ are currentlyunknown.

The rationale for the use of a combination of PGE₁ with other drugs, for the treatment of erectile dysfunction, is to increasethe number of responding patients and to diminish the dose ofPGE₁ required to achieve adequate responses because this prostanoidmay cause penile pain. To date, the most widely used combinationtherapy includes PGE₁, papaverine, and phentolamine, which hasbeen shown to improve response rates (Padma-Nathan, 1990; McMahon,1991; von Heyden et al., 1993).

In the present study, we have investigated the possibility of combining the administration of PGE₁, which activates the cAMPpathway, with the activation of the NO/cGMP pathway, which playsa prominent role in the physiological mechanism of penile erection(Kim et al., 1991; Burnett et al., 1992; Rajfer et al., 1992;Trigo-Rocha et al., 1993). Pharmacological stimulation of cGMPproduction in penile smooth muscle can be achieved with NO donors,which are compounds that release NO but are more stable, allowingfor their use as therapeutic drugs. These NO donors have beenreported to relax penile smooth muscle (Sáenz de Tejada et al.,1989; Bush et al., 1992) and have been evaluated for the treatmentof erectile dysfunction as a potential alternative treatment toPGE₁ (Truss et al., 1994; Martínez-Piñeiro et al., 1998).

Our results show that SNO-Glu, a nitrosothiol present in plasma, is an effective relaxant of human penile resistance arteriesand human trabecular smooth muscle. When the tissues, primarilyarteries but also trabecular smooth muscle, relaxed poorly toPGE₁, SNO-Glu alone was able to induce a strong response (nearfull relaxation) in those tissues. The combination with SNO-Gluimproved the relaxations to PGE₁ in human penile arteries andin trabecular smooth muscle, causing a shift to the left of thePGE₁ concentration-response curve and a larger maximum relaxationcompared with PGE₁ alone. Although in penile arteries the combinationof PGE₁ and SNO-Glu did not improve the relaxation response toSNO-Glu alone, this combination did relax human trabecular smoothmuscle more efficiently than SNO-Glu or PGE₁ alone. Furthermore,a synergistic interaction between the two compounds was observedwhen given in combination to relax trabecular smooth muscle, asshown in the analysis of synergism using the isobole method (Berenbaum,1989). The constructed theoretical curve for the existence ofadditive effects between PGE₁ and SNO-Glu predicted significantlyhigher concentrations of both drugs than those experimentallydetermined to produce the same level of relaxation, confirmingthe existence of synergism. Based on these results, we proposethat the combination of PGE₁ and SNO-Glu has significant advantagesfor the relaxation of penile trabecular smooth muscle comparedwith the separate administration of thesedrugs.

Improved relaxant properties of the combination of PGE₁ and SNO-Glu are probably due to the ability of this treatment to triggerthe activity of the two essential pathways responsible of penilesmooth muscle relaxation (i.e., cAMP and cGMP pathways). The activationof both pathways was demonstrated in our experiments by the accumulationof both cyclic nucleotides in human cavernosal tissue after treatmentwith the combination. Potentiation of the NO/cGMP pathway withoral sildenafil together with local PGE₁ is used on occasionsin the clinical management of patients who are partial respondersto PGE₁.

The existence of synergism between NO and cAMP is not well recognized in human penile smooth muscle. Furthermore, other investigatorshave tested the effect of combining two other molecules, vasoactiveintestinal polypeptide and SIN-1, stimulants of cAMP and cGMP,respectively, in human corpus cavernosum and cavernous artery,reporting a lack of synergistic interaction (Hempelmann et al.,1995). The difference between the results of Hempelmann et al.(1995) and those of our study may be due to the specificity ofstimulating different receptor pathways. The combination of PGE₁with SIN-1 has been shown to be more effective to produce erectionsthan PGE₁ or SIN-1 individually, when evaluated in a clinicaltrial involving 50 impotent patients (Tordjman, 1993). Our studyprovides new information that may explain the mechanism underlyingthis clinical finding. The synergistic interaction of PGE₁ andSNO-Glu was specific to trabecular smooth muscle because it wasnot observed in penile arteries, despite the fact that these twotissues are anatomically related, and functionally key to theerectileprocess.

In summary, the present study characterizes the responses to PGE₁ in human trabecular smooth muscle and penile resistancearteries, which both show large variability in response to PGE₁.We found a correlation of the in vitro response with the clinicalerectile response that had not been previously reported. Theseresults may explain why some patients respond and others do notto intracavernosal PGE₁. This study also demonstrates that SNO-Gluconsistently relaxes penile smooth muscle whether it relaxes wellor not to PGE₁. This suggests that the clinical response to PGE₁may be limited in some patients by the specific lack of responseof penile smooth muscle to this prostanoid, while maintainingthe ability to relax in response to agents that activate alternativerelaxant pathways. We also found that a combination of PGE₁ andSNO-Glu has a synergistic interaction to relax penile trabecularsmooth muscle. Such a combination may have significant therapeuticadvantages in the treatment of male erectiledysfunction.

	Acknowledgments

We thank Dr. Gordon Letts (Nitromed Inc.) for kindly providing SNO-Glu. We also thank Fundación Futuro for administrativemanagement.

	Footnotes

Accepted for publication June 22, 2000.

Received for publication March 17, 2000.

¹ This study was partially supported by a grant from SchwarzPharma.

Send reprint requests to: Iñigo Sáenz de Tejada, M.D., Antonio Robles, 4-9 C, 28034 Madrid, Spain. E-mail: isaenz{at}ntserver.coronadoserv.com

	Abbreviations

PGE₁, prostaglandin E₁; NO, nitric oxide; SNO-Glu, S-nitrosoglutathione; SIN-1, linsidomine chlorohydrate; PSS, physiological salt solution.

	References

Top Abstract Introduction Experimental Procedures Results Discussion References

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