Role of Peripheral Innervation in P-Chloroamphetamine-Induced Ejaculation in Anesthetized Rats

doi:10.2164/jandrol.05163

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Role of Peripheral Innervation in P-Chloroamphetamine–Induced Ejaculation in Anesthetized Rats

PIERRE CLÉMENT^*, HOSSEIN K. KIA^*, STEPHANE DROUPY, JACQUES BERNABE^*, LAURENT ALEXANDRE^*, PIERRE DENYS AND FRANÇOIS GIULIANO^*^,

From the ^* Pelvipharm Laboratories, Campus CNRS, Gif-sur-Yvette, France; Groupe de Recherche en Urologie, UPRES, Medical University of Paris-South, Le Kremlin-Bicêtre Cedex, France; and Neuro-Urology Unit, Department of Neurological Rehabilitation, Raymond Poincaré Hospital, Garches, France.

Correspondence to: Dr François Giuliano, Neuro-Urology Unit, Department of Neurological Rehabilitation, Raymond Poincaré Hospital, 104 bd Raymond Poincaré, 92380 Garches, France (e-mail: giuliano{at}cyber-sante.org).

Received for publication September 12, 2005; accepted for publication December 19, 2005.

Abstract

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Abstract
Materials and Methods
Results
Discussion
References

The occurrence of ejaculation, which consists of 2 distinctphases (emission and expulsion), requires a tight coordinationof peripheral autonomic and somatic nerves. However, some aspectsof the mechanism of ejaculation are not clearly defined. Toclarify this issue, we used the p-chloroamphetamine (PCA)-inducedejaculation model in anesthetized rats and investigated theeffects of selective peripheral nerves lesions on seminal vesicleand bulbospongiosus (BS) muscle activities as representing physiologicalmarkers of emission and expulsion phases, respectively. In intactrats, ejaculation induced with PCA (intraperitoneal 5 mg/kg)correlated with coordinated increases in seminal vesicle pressure(SVP) and BS electromyographic activity. PCA-induced ejaculationwas still observed in rats with bilateral lesion of hypogastricnerves (HNx), lumbar paravertebral sympathetic chain (LSCx),or dorsal nerves of the penis (DNPx). Conversely, bilateralsection of pelvic nerves (PNx) or L6-S1 dorsal roots (DRx) abolished PCA-induced ejaculation. The amplitude of SVP increases inducedby PCA was reduced in PNx, HNx, and LSCx rats, whereas it wasunchanged in DRx and DNPx rats. The time interval between SVPincreases and BS muscle contractions induced by PCA was comparablein the different neural lesion groups. In conclusion, PCA initiatesboth emission and expulsion independently from each other.In this model, afferents conveyed by the pelvic nerves appearto be unnecessary for occurrence of BS muscle contractionsbut are essential for a complete ejaculatory response.

Key words: Seminal vesicle, bulbospongiosus muscles, sympathetic nerves, parasympathetic nerves, sensory afferents

Ejaculation is a complex physiological process that resultsin the expulsion of the seminal fluid from urethra at the meatus(for review, see Giuliano and Clément, 2005). Ejaculationconsists of 2 distinct successive phases: 1) emission phase(ie, secretion of the various components of sperm by seminal vesicles [SVs], prostate, and ampullary vas deferentia contentsinto the prostatic urethra [Gil-Vernet et al, 1994; Bohlen et al, 2000])and 2) expulsion phase (ie, forceful propulsion of sperm fromthe prostatic urethra to the urethral meatus caused by rhythmic contractions of perineal striated muscles, with a primary rolefor the bulbospongiosus [BS] muscles [Gerstenberg et al, 1990]).It is largely assumed that expulsion is triggered by pressurebuild-up in the prostatic urethra, a concept referred to asthe prostatic pressure chamber (Jannini et al, 2002). Afferentsoriginating in penile glans and reaching the lumbosacral spinalcord via the dorsal nerve of the penis and then the pudendalnerve play a crucial role in the ejaculatory process (Johnson and Hubscher, 1998). The occurrence of ejaculation requires coordination of neuralperipheral autonomic and somatic efferent inputs after appropriatecentral and peripheral stimuli (DeGroat and Booth, 1993; McKenna, 1998).The detailed mechanisms of the peripheral neural control of ejaculation are poorly understood. Recently, supraspinal nucleiinvolved in ejaculation have been identified by using the immediateearly gene c-fos protein pattern of expression in rats (forreview, see Coolen et al, 2004). These nuclei include themedial amygdala, the bed nucleus of the stria terminalis, andthe medial portion of the parvocellular subparafascicular nucleus.In addition, a spinal ejaculation generator has been identifiedin lamina VII and X in the L3-L4 spinal segments of rats (Truit and Coolen, 2002).

The anatomical structures involved in ejaculation (ie, the seminaltract, including the accessory sex glands as well as the bladderneck) are innervated by efferent neural fibers originatingin the pelvic plexus, which represents a peripheral crossroadsite relaying 1) sympathetic (traveling through hypogastricnerve and paravertebral sympathetic chain) and 2) parasympathetic (traveling through pelvic nerve) components (Janig and McLachlan, 1987). Together with the pudendal nerve, which conveys motor outputsto pelvic striated muscles, these nerves ensure the peripheralcontrol of the 2 phases of ejaculation. The pharmacology ofejaculation has been mostly studied with the aid of behavioralexperiments in rats (for review, see Coolen et al, 2004). Themain reason is because of the lack of suitable models in whichfully developed ejaculatory responses can be easily and reliablyelicited in anesthetized animals.

P-chloroamphetamine (PCA) is an amphetamine derivative thatliberates catecholamines and serotonin from monoaminergic nerveterminals. Systemic administration of PCA has been reportedto induce ejaculation in both conscious (Humphries et al, 1981;Rènyi, 1985) and anesthetized (Yonezawa et al, 2000)rats. Pharmacological data indicate that serotonin plays theprimary role in mediating the effect of PCA on ejaculation,whereas noradrenaline is of secondary importance (Rènyi, 1985).The site of action for PCA to induce ejaculation is not clearlyidentified, though it seems not to include supraspinal sitesbecause PCA-induced ejaculation has been reported in rats afteracute spinal transection at the T8 level (Yonezawa et al, 2000).Theoretically, the possible targets for PCA to provoke ejaculationmay thus be the spinal cord or at the periphery, the postganglionicneurons of the efferent pathways commanding the physiological events leading to ejaculation, the smooth muscle fibers ofthe seminal tract, the terminals of primary afferent fibersinvolved in the ejaculatory reflex, or a combination of 2 ormore of these elements.

To better understand the proejaculatory mechanism of actionof PCA, we performed selective lesions of efferent and afferentnerves supplying anatomical structures participating in ejaculation.Increases in intra-SV pressure (SVP), in which secretions represent50%–80% of total ejaculate volume, and contractile activityof BS muscles were measured as physiological markers of emissionand expulsion phases of ejaculation, respectively. The datacollected in such an integrative physiological approach aimto provide new insights to examine in a more critical lightthe current concept of the peripheral neurophysiology of ejaculation.

Materials and Methods

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Abstract
Materials and Methods
Results
Discussion
References

All animal experiments were carried out in accordance with theEuropean Community Council Directive (86/609/EEC) on the useof laboratory animals. All efforts were made to minimize animalsuffering and to reduce the number of animals used.

Animal Preparation

Thirty-six adult male Wistar rats (Janvier, Le Genest-St-Isle,France) weighing 200–300 g were used in the study. Theywere separated randomly into 6 groups of 6 rats depending onthe acute neural lesion they underwent. Rats were anaesthetizedwith isoflurane (1.5%–2%; Sigma, Saint-Quentin Fallavier,France) and their body temperature was maintained at 37°Cwith a homeothermic blanket. The trachea was cannulated toprevent aspiration of saliva. The carotid artery was catheterizedwith polyethylene tube (0.50 mm) filled with heparinized saline(50 IU/mL) to record mean arterial pressure via a pressuretransducer (EM750, Elcomatic, Glasgow, United Kingdom). For measuring intra-SVP, a suprapubic midline incision was performedand a polyethylene catheter (0.50 mm), filled with mineraloil, was inserted into 1 SV through the apex and connectedto a pressure transducer. A pair of stainless steel electrodes(32 gauge) was placed within the BS muscle exposed via a perinealincision for recording electrical activity (BS-EMG). The electricalsignal from the BS muscle was amplified (DP-301, Warner Instrument Corp, Hamden, Conn) (gain, 10 000; low pass, 10 kHz; high pass,300 Hz) before being digitized. During the experiment, thesurgical area was filled with warm (37°C) mineral oil toprevent dehydration.

Bilateral Nerve Transections

Pelvic nerves were freed from the surrounding connective tissueon the lateral aspect of the prostate and sectioned 5 mm posteriorto the major pelvic ganglion (PNx group). Hypogastric nerveswere located leaving the inferior mesenteric ganglion and travelingclose to the common iliac vessels. The nerves were then bilaterallysectioned 3 mm proximal to the major pelvic ganglion (HNx group).The lumbar sympathetic chain was identified behind the aortaand vena cava by a transperitoneal approach. Both trunks ofthe lumbar paravertebral sympathetic chain were sectioned atthe L4-L5 level of the spinal cord, with the superior renalartery used as an anatomical landmark (LSCx group). For sectionof L6-S1 dorsal roots, an L1-L2 laminectomy was performed.Dorsal and ventral roots were then separated, and dorsal rootswere sectioned bilaterally close to the entry zone (DRx group).For section of the dorsal nerves of the penis, the prepucewas circumcised and the penis was denuded of skin. Dorsal nervesof the penis were then freed from connective tissue and bilaterallysectioned at the penile crus (DNPx group). Figure 1 summarizesall the neural lesions performed.

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Figure 1. Diagram showing the sites of the neural lesions (unilateral) performed bilaterally in the study. Double-headed arrows indicate lesions; BS, bulbospongiosus muscles; DNP, dorsal nerve of the penis; DRG, dorsal root ganglion; HN, hypogastric nerve; PudN, pudendal nerve; PN, pelvic nerve; PP, pelvic plexus; and SV, seminal vesicle.

Drug

PCA was obtained from Sigma and dissolved in saline at a concentrationof 5 mg/mL. A volume of 1 mL/kg rat body weight was droppedin the peritoneal cavity after a 10-minute baseline periodwas obtained. SVP and BS-EMG were monitored for 30 minutesafter administration of PCA.

Data Analysis

Ejaculations (ie, expulsions of seminal plugs, associated withSVP rises together with synchronized BS muscle contractions)were enumerated for 30 minutes after PCA administration. Hereafter,the term ejaculation refers to expulsion of the plug. The latencyfor the first ejaculation to occur after intraperitoneal (i.p.)administration of PCA was determined. In absence of ejaculation,latency values were not determined.

For SVP, the maximal amplitude was quantified. For BS-EMG, thearea under the curve (AUC) of the square value of the electricalsignal was integrated. The time interval separating the beginningof the SVP rise and the first BS-EMG organized activity wasalso calculated. The time interval might reflect the synchronizationbetween emission and expulsion phases.

Statistical Analysis

Data were expressed as means ± SE. Statistical comparisonsof the different experimental groups were performed by 1-wayanalysis of variance (ANOVA) followed by Student-Newman-Keulspost hoc test when applicable (ANOVA with P < .05). Intergroupcomparisons of proportion of SVP increases coordinated withBS muscle contractions were performed by Fisher exact test.

Results

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Abstract
Materials and Methods
Results
Discussion
References

Intact Group

PCA i.p. administration resulted in ejaculation in 4 of 6 ratswithin the 30 minutes after treatment (Table). The mean numberof ejaculations in this control group was 1.4 ± 0.5with the latency for the first plug to occur of 7.5 ±0.9 minutes.

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Effect of the different transections on ejaculation in anesthetized rats ${dagger}$

Monitoring of SVP revealed 2 patterns of change elicited byPCA treatment (Figure 2). First, a gradual SVP increase occurredimmediately after PCA i.p. administration, reaching a maximumof 6.8 ± 1.3 mm Hg within 4 minutes after injection.This tonic increase in SVP baseline then slowly declined topretreatment value (2.3 ± 0.4 mm Hg). Second, phasicSVP increases in the form of brief peaks were observed beginningwithin 5–10 minutes after treatment and reaching a maximalamplitude of 13.4 ± 3.8 mm Hg (Figure 3A).

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Figure 2. Sample of simultaneous recordings of seminal vesicle pressure (SVP; top trace) and bulbospongiosus (BS) muscles EMG (bottom trace) after p-chloroamphetamine (PCA) administration in intact anesthetized rats. SVP and BS-EMG were monitored for 30 minutes after intraperitoneal administration of PCA (5 mg/kg). A magnification of the recording is displayed in the inset. Note that the brief increases in SVP start before contraction of the BS muscle and accordingly are not direct consequence of BS muscle contractions.

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Figure 3. Effect of selective nerve transections on seminal vesicle pressure (SVP) phasic increases (A) and area under the curve (AUC) of bulbospongiosus (BS) muscle contractions (B) induced by p-chloroamphetamine (PCA) intraperitoneal administration. Lesion of pelvic nerves (PNx), hypogastric nerves (HNx), and L4-L5 paravertebral sympathetic chain (LSCx) resulted in a dramatic decrease of SVP, whereas AUC of BS muscle contractions was not statistically modified. Lesion of L6-S1 dorsal roots (DRx) had no statistically significant effect on either SVP or AUC of BS muscle contractions. Statistics: analysis of variance and Bonferroni post hoc test. Asterisks indicate significant difference compared with intact group (^* P < .05; ^** P < .01).

Recording of BS-EMG revealed the occurrence of rhythmic andintense bursts of BS muscle contractions after i.p. administrationof PCA. For most of the time, phasic SVP increases were followedby BS muscle contractions in a mean time interval of 6.4 ±2.3 seconds (Figure 4). Some rare cases of uncoupled phasicSVP increase and BS muscle contractions were observed. The meanAUC value for BS bursts of contractions was 4.2 ± 0.8 10^-4 V.s (Figure 3B).

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Figure 4. Effect of selective nerve sections on time interval separating seminal vesicle pressure (SVP) phasic increase and bulbospongiosus (BS) muscle contractions after p-chloroamphetamine intraperitoneal administration. Neither lesion of pelvic nerves (PNx), hypogastric nerves (HNx), L4-L5 paravertebral sympathetic chain (LSCx), L6-S1 dorsal roots (DRx), nor dorsal nerves of the penis (DNPx) exerted a noticeable effect on time coordination of SV and BS muscle contractions.

Bilateral Section of the Pelvic Nerves

In the 6 rats in the PNx group, i.p. administration of PCA failedto induce ejaculation (Table).

Contractions of SV and BS muscles were still observed afteri.p. administration of PCA (Figure 5). In comparison withintact rats, the tonic increase in SVP was not significantlymodified in PNx rats (5.3 ± 0.7 mm Hg), whereas a significantreduction in the maximal amplitude of SVP peaks (phasic contractions)was observed (3.0 ± 0.5 mm Hg; ANOVA, P < .01; Bonferronitest, P < .05; Figure 3A).

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Figure 5. Sample of simultaneous recordings of seminal vesicle pressure (SVP; top trace) and bulbospongiosus (BS) muscle EMG (bottom trace) after p-chloroamphetamine intraperitoneal administration in rat with acute bilateral lesion of the pelvic nerves (LSCx), rat with acute bilateral lesion of the hypogastric nerves (HNx), rat with acute bilateral lesion of the lumbar paravertebral sympathetic chain (PNx), rat with acute bilateral lesion of the L6-S1 dorsal roots (DRx), and rat with acute bilateral lesion of the dorsal nerves of the penis (DNPx).

The time interval between SVP peaks and associated BS musclecontractions was not significantly modified in PNx rats (7.2± 1.4 seconds; Figure 4) compared with intact rats.Quantitative analysis of BS muscle contractions induced by i.p. administration of PCA revealed a decrease in AUC in PNx rats(-48% compared with intact rats), though this did not reachstatistical level of significance (Figure 3B).

Bilateral Section of the Hypogastric Nerves

Occurrence of PCA-induced ejaculation was observed in 2 of 6rats after acute bilateral section of hypogastric nerves (HNx) (Table). Overall, the mean number of ejaculations in thisgroup of rats was almost 5 times lower than in intact rats(ANOVA, P < .01; Bonferroni test, P < .05), though thelatency of the first plug was not markedly altered (Table).

In HNx rats, the tonic increase in SVP (6.4 ± 0.3 mmHg) induced by PCA i.p. administration was similar to thoseobserved in intact and PNx rats. By contrast, the maximal amplitudeof SVP peaks was drastically decreased (0.6 ± 0.2 mmHg; ANOVA, P < .01; Bonferroni test, P < .01) in comparisonwith intact rats (Figures 3A and 5).

The time interval between SVP and associated BS muscle contractionsin HNx rats was comparable with intact and PNx rats (7.2 ±0.9 seconds; Figure 4). Statistical analysis of the AUC ofBS muscle contractions did not reveal significant changes comparedwith intact and PNx rats (Figure 3B).

Bilateral Section of the Lumbar Paravertebral Sympathetic Chain

PCA i.p. administration induced ejaculation in 3 of 6 rats afteracute bilateral section of the paravertebral sympathetic chainat the L4-L5 level (LSCx) (Table). Both the mean number ofplugs and latency of the first plug were similar to the values obtained in intact rats (Table).

Section of LSC remained ineffective in impairing the tonic SVPincrease obtained after PCA administration (5.1 ± 0.5mm Hg). In comparison with intact rats, a strong reductionin the maximal amplitude of SVP peaks was evidenced in LSCxrats (1.2 ± 0.2 mm Hg; ANOVA, P < .01; Bonferronitest, P < .01; Figures 3A and 5).

The time interval between SVP and associated BS muscle contractions(5.2 ± 1.2 seconds) in LSCx rats was unchanged comparedwith those obtained in intact, PNx, and HNx rats (Figure 4).Analysis of the AUC of BS muscle contractions did not reveal any significant modification when compared with other groups (Figure 3B).

Bilateral Section of L6-S1 Dorsal Roots

PCA-induced ejaculation was abolished in the 6 rats in the DRxgroup (Table). Nevertheless, contractions of SV and BS muscleselicited by PCA i.p. administration were still present in DRxrats (Figure 5). Both tonic (5.5 ± 1.7 mm Hg) and phasic(14.7 ± 3.9 mm Hg) increases in SVP were unchanged incomparison with intact rats (Figure 3A).

SVP peaks observed in DRx rats after i.p. PCA administrationwere followed by BS muscle contractions in a mean time interval(5.8 ± 1.1 seconds) similar to the other experimentalgroups (Figure 4). The decrease (-64% compared with intactrats) in the AUC of BS muscle contractions recorded in DRxrats did not reach statistical significance (ANOVA, P = .09; Figure 3B).

Bilateral Section of the Dorsal Nerves of the Penis

All 6 rats in the DNPx group displayed ejaculation after PCAi.p. administration (Table). Both the mean number of plugsand latency of the first plug were similar to the values obtainedin intact rats (Table).

In comparison with intact rats, no significant changes in bothtonic (8.7 ± 0.6 mm Hg) and phasic (9.0 ± 1.6mm Hg) SVP increases were observed in DNPx rats (Figures 3Aand 5).

The time interval between SVP increases and BS muscle contractions(9.5 ± 0.5 seconds) was not different when comparedwith other groups (Figure 4). Bilateral lesion of the DNPremained without effect on AUC of BS muscle contractions (Figure 3B).

Discussion

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Abstract
Materials and Methods
Results
Discussion
References

This is the first study using a pharmacological model of ejaculationto describe the consequences of selective peripheral autonomicand sensory denervations on dynamical changes in physiologicalcomponents related to emission and expulsion phases of theejaculatory process.

Two types of changes in SVP—tonic and phasic increases—were observed after PCA i.p. administration to anesthetized rats.Whatever the neural lesion performed, the tonic increase remainedand was characterized by a low and progressive augmentationof SVP beginning immediately after i.p. administration of PCA.This was not associated with ejaculation, as this tonic increasein SVP was still evidenced in rats not ejaculating. We proposethat such a tonic increase, which likely reflects slow andweak sustained contraction of SV, is elicited by a direct actionof PCA on the SV smooth muscle fibers. Indeed, PCA is knownto release noradrenaline from adrenergic terminals, and noradrenergicinnervation of SV is well established (Dail, 1993). Accordingly,this tonic SV contraction may well be because of the releaseof noradrenaline within SV. In all groups of rats tested, thephasic increases in SVP were characterized by rapid augmentationof SVP in the form of peaks lasting between 15 and 25 seconds.Expulsion of a seminal plug was observed when phasic increasewas followed by an organized burst of BS muscle contractions starting between 5 and 9 seconds after the beginning of theSVP rise (ie, before SVP reaches its maximal amplitude). Thisobservation, together with the fact that SVP phasic increasesin HNx and LSCx rats were very low despite concomitant BS musclecontractions, clearly indicates that SVP variations measuredin our conditions were not attributed to BS muscle contractionsbut reflect intrinsic activity of the SV.

In the rat, parasympathetic cell bodies of preganglionic neurons innervating the pelvic viscera are located in the parasympatheticnucleus of the sacral spinal cord (L6-S1 levels) and theiraxons run in the pelvic nerve en route to the pelvic plexus(Nadelhaft and Booth, 1984). Sympathetic preganglionic neuronsdestined to the pelvis originate from T13-L2 levels of thespinal cord. Some have axons conveyed to the inferior mesentericganglion and continue to travel distally in the hypogastricnerves (Nadelhaft and McKenna, 1987). The rest of the preganglionicsympathetic neurons to the pelvis travel caudally in the paravertebralsympathetic chain and reach pelvic plexus through the pelvicnerves (Giuliano et al, 1997). The classical view about theautonomic neural control of ejaculation is that sympatheticfibers to the pelvis conveyed by the hypogastric nerves control the tone of the smooth musculature of the seminal tract. Thistheory is partly confirmed by the current findings showinga dramatic decrease in PCA-induced SV phasic contractions afterbilateral lesion of the hypogastric nerves. In addition, wehave evidenced an essential role for the sympathetic fibers traveling in the lumbar paravertebral sympathetic chain inmediating PCA effect on phasic SV contractions. As mentionedabove, sympathetic fibers exiting the paravertebral sympatheticchain are conveyed by the pelvic nerves. Therefore, we proposethat a decrease in PCA-induced phasic SV contractions afteracute section of pelvic nerves is due to the lesion of thosesympathetic fibers originating from the lumbar paravertebralsympathetic chain and further conveyed by the pelvic nerves.These findings lead us to suggest that both the hypogastricand the paravertebral sympathetic outflows play a primordialrole in controlling the tone of the seminal tract. It is tobe noticed that disruption of only 1 of the sympathetic pathwayis sufficient to severely impair SV contractile activity inthe model of PCA-induced ejaculation. The latest observationlikely indicates that sympathetic fibers running in lumbar paravertebralsympathetic chain are not part of a redundant mechanism but exert by themselves an essential role in controlling SV contractibility.

Interestingly, bilateral section of pelvic nerves abolishedejaculation, whereas lesion of the lumbar paravertebral sympatheticchain (ie, of the sympathetic component of the pelvic nerves)did not. These observations led us to hypothesize that eitherlesion of efferent parasympathetic fibers or lesion of theafferents traveling in the pelvic nerves was responsible forthe complete abolition of PCA-induced ejaculation. In the rat,afferent fibers conveyed by the pelvic nerves enter the spinalcord via L6 and S1 dorsal roots (Nadelhaft and Booth, 1984). Disruption of L6-S1 dorsal roots suppressed PCA-induced ejaculation.This implies that recruitment of these afferent fibers passingthrough the pelvic nerves is crucial for ejaculation to occur,at least in our experimental conditions. Other afferents originatingin the glans penis travel along the dorsal nerve of the penisand are further conveyed through the pudendal nerve to reachthe spinal cord via L6-S1 dorsal roots (McKenna and Nadelhaft, 1986; Johnson and Halata, 1991). The role of these sensory fibersin ejaculation is well documented (for review, see Sonksen and Ohl, 2002), but their involvement in human premature ejaculation is thesubject of controversy. Some clinical data suggest the hyperexcitabilityof the glans penis and the dorsal nerve of the penis as a putativebasis for premature ejaculation (Xin et al, 1997), whereasother results indicate that sensory afferents are not responsiblefor human premature ejaculation (Paick et al, 1998; Perretti et al, 2003).The participation of this pathway in the proejaculatory effectof PCA is very unlikely, as shown in our study by the inefficacyof dorsal nerves of the penis lesion to impair PCA-inducedejaculation. Altogether, these data demonstrate that pelvicsensory afferents running in the pelvic nerves are essentialfor a complete ejaculatory response to occur in rats afteri.p. administration of PCA. Whether the necessary recruitmentof those afferents is peculiar to PCA experimental model orhas physiological relevance remains to be clarified.

According to a generally accepted idea, though not stronglysubstantiated, the expulsion phase is a spinal cord reflexthat occurs as the ejaculatory process reaches a "point ofno return." The point of no return is described as the pressurebuild-up in the prostatic urethra caused by seminal emissionentering it, meaning that expulsion is dependent on the volumeof seminal secretions. This view is actually contradicted byseveral lines of clinical and experimental evidence (reviewedin Levin, 2005) showing the triggering of expulsion (ie, activationof rhythmic stereotyped contractions of pelvi-perineal striatedmuscles) in absence of seminal fluids within the prostaticurethra or after urethral anesthesia (Larsson and Swedin, 1971; Brindley, 1983; Gerstenberg et al, 1990; Holmes and Sachs, 1991; Gil-Vernet et al, 1994). The present study provides additionalarguments suggesting that the expulsion phase does not strictlydepend on urethral inputs: 1) In HNx and LSCx rats where SVPincreases were dramatically reduced, BS muscle contractionsas powerful as in intact rats still occurred. In these lesionedanimals, the contractions of BS muscles allowed seminal plugsto be expelled, with a mean weight 3 times lower than in intactrats (data not shown). 2) In PNx and L6-S1 DRx rats in whichafferents originating in urethra were disrupted, organized BSmuscle contractions were still observed, though they were lesspowerful compared with intact rats despite the lack of statisticaldifference. 3) Whatever the neural lesion performed, the timeinterval between SVP increases and bursts of BS muscle contractions,likely reflecting a kind of synchronization between emissionand expulsion phases, was very comparable with that determinedin intact rats. 4) Finally, bursts of BS muscle contractionswere shown to start whereas SV contractions were not at completion,suggesting the physiological superimposition of these 2 events,a phenomenon also reported in humans (Gil-Vernet et al, 1994). Altogether, these observations support what was concluded fromprevious physiological studies carried out in animals and humans(ie, formation of a urethral "pressure chamber" does not appearnecessary for pelvi-perineal striated muscles contractionsto occur [Holmes and Sachs, 1991; Gil-Vernet et al, 1994; Hermabessiere et al, 1999]).

The search for an anatomical structure for handling the ejaculationtrigger is a key issue. Recently, the selective lesion of agroup of spinal cells (namely, LSt cells) was found to completelydisrupt the ejaculatory behavior of male rats without affectingother aspects of sexual behavior (Truit and Coolen, 2002). Anatomical investigations have shown that LSt cells, locatedat L3-L4 spinal levels, send projections to pudendal motoneuronsinnervating the BS muscles (Newton, 1994; Xu et al, 2005)as well as to sympathetic and parasympathetic preganglionicneurons destined to the anatomical structures that are involvedin the emission phase of ejaculation (Truit and Coolen, 2002; Xu et al, 2005). In addition, localization of LSt cells inthe vicinity of spinal projections of penile afferents (McKenna and Nadelhaft, 1986)suggests that they may also integrate peripheral sensory information.As a whole, these data place LSt cells in a pivotal positionto ensure coordinated activation of spinal nuclei controllingejaculatory peripheral events. Whether those findings couldbe directly extrapolated to humans remains to be established.To date, no information has been published about the neurotransmittersinvolved in the modulation of LSt cells activity. Because PCAinduces a complete ejaculatory response in spinalized rats atthe T8 level (Yonezawa et al, 2000), we assume that this compoundmay act on LSt cells.

In conclusion, these results indicate that PCA systemicallyadministered to anesthetized rats initiates both emission andexpulsion phases of ejaculation independently from each other.In the PCA-induced ejaculation model, afferents conveyed bythe pelvic nerves appear unnecessary for occurrence of BS muscle contractions; however, they are of primary importance for acomplete ejaculatory response (ie, expulsion of seminal plug).Further pharmacological investigations targeting the spinalejaculation generator are mandatory to confirm our resultsand to draw a clearer picture of the spinal physiology and pharmacologyof ejaculation.

Acknowledgments

The authors wish to thank D. Roussel and S. Goyer for theirexcellent technical assistance.

References

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