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Department of Urology-Urodynamics, Erasmus University Rotterdam, 3000 DR Rotterdam, The Netherlands
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ABSTRACT |
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 TOP
 ABSTRACT
 INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES
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In this study we measured urethral pressure changes in response to efferent pudendal nerve stimulation in rats. All other neural pathways to the urethra were transected, and the urethra was continuously perfused. We found fast twitch-like contractions, superimposed on a slow relaxation. The amplitude of the twitches was independent of the stimulation frequency below 26 Hz, whereas the relaxation depended highly on this frequency. The twitches were caused by striated urethral muscles, and the relaxation was caused by smooth muscles. Both were mediated by acetylcholine. We calculated the effective urethral relaxation as the absolute relaxation multiplied by the time fraction between the twitches. Maximum effective relaxation occurred at 8-10 Hz, exactly the frequency of spontaneous oscillations during bladder voiding in rats. Although the oscillatory sphincter contractions in rats during voiding may be needed in other mechanisms for efficient voiding, our data suggest that they may be a side effect of the actual purpose: urethral relaxation.
rat; urethral oscillations; nitric oxide; acetylcholine
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INTRODUCTION |
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TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES
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DYNAMIC PROPERTIES of the lower urinary tract have been extensively studied over the years, and mechanical models have been developed (12, 42). More recently, attention has been paid to the innervation of the pelvic organs (1, 17, 26, 38), and the activity in the innervating nerves is being incorporated in these models (18, 19, 25, 29, 39). The extended models may enable differentiation between myogenic and neurogenic causes for dysfunction of the lower urinary tract or may improve the clinical use of neurostimulation as a treatment for lower urinary tract dysfunction in patients with spinal cord injury.
Most studies on lower urinary tract innervation have been done in animals, mostly rats. Like humans, rats have three major nerves that innervate the pelvic organs: the (predominantly sympathetic) hypogastric nerve, the (predominantly parasympathetic) pelvic nerve, and the (predominantly somatic) pudendal nerve. The sympathetic system is assumed to be active during urine storage, whereas the parasympathetic system controls bladder voiding. Despite the many similarities, there are some major differences between the human and the rat urinary system; one of the most striking is the oscillatory contractions of the external urethral sphincter (EUS) during voiding in rats (3, 6, 22, 24, 28, 40). The oscillations occur more often and are stronger in male rats than in female rats (22). The rat's normal pattern of bladder-EUS coordination has some superficial similarities to the dyssynergic pattern observed in humans with spinal cord injury. However, unlike the spinalized human, the rat is able to void quite successfully, and knowledge of the differences between the rat and human mechanism of bladder-EUS coordination has therefore been suggested to be of use in evaluating micturition problems in patients with spinal cord injuries (16).
The reason for the sphincter contractions in the rat, which occur at a rate of 6-10 per second (24, 28, 40), has been a subject of discussion for years. A pumplike function (22), a mechanism to sustain a high level of bladder afferents and therefore bladder contraction (16), and a mechanism necessary for territory marking (40) have been suggested. However, none of these explanations seems very satisfactory. Furthermore, it remains unclear why the oscillations occur at the specific frequency range of 6-10 Hz.
In this study, we investigated the relationship between efferent pudendal nerve activity and urethral resistance, as well as some of the major neurotransmitters involved. Urethral oscillations normally occurring during voiding contractions (6-10 Hz) were simulated by pudendal nerve stimulation at 2-70 Hz. We distinguished smooth muscle and striated muscle responses to pudendal stimulation. We will introduce a third explanation for the urethral oscillations, taking into account the frequency of the oscillations during spontaneous bladder voiding.
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MATERIALS AND METHODS |
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TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES
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Surgery
Sixteen male Wistar rats (444 ± 47 g) were anesthetized with urethan (1.2 g/kg ip) (23) and placed on a heated pad. A dorsal incision was made on the left side of the spine, just below S3, to access the pudendal nerve. Two trimel-coated silver wires were twisted around the nerve (the undivided efferent and afferent branch) (26) at a distance of ~2 mm. The wound was then closed, and the animal was turned over on its back.An abdominal midline incision was made to access the urethra. The right side pelvic and hypogastric nerves were transected. The left side pelvic and hypogastric nerves were freed from the underlying tissue and marked with sutures. Warm saline kept the abdomen moist during surgery. The animal was placed in a frame with a heated ground plate, and the abdominal wall was tied to the frame to create a basin. During the measurements, this basin was filled with warm paraffin oil.
Experimental Setup
A 20-gauge angiocatheter was inserted through the bladder into the urethra. Through this needle, the pressure at the entrance of the urethra (Pura) was measured with the use of a disposable pressure transducer and a Statham SP-1400 blood pressure monitor. Furthermore, the needle was used to pump saline through the urethra with a Harvard Apparatus (Millis, MA) infusion pump at a flow rate (Q) of 0.5 ml/min. The bladder was emptied and tied to prevent leakage from the urethra to the bladder and high bladder pressures.A bipolar platinum-iridium electrode that consisted of two metal hooks at a distance of ~0.5 mm was lowered into the paraffin oil basin. Either the pelvic or the hypogastric nerve was guided over the electrode, which was used for stimulation. The silver wires around the pudendal nerve provided another stimulation electrode. A Hameg programmable function generator, HM-8130, generated the stimulation signals. The pressure signal was read into a personal computer at sample rates of 200 or 1,000 Hz, with the use of specially developed software driving a PCL 818 analog-to-digital converter. The stimulation signal was also sampled, at a rate of 25 kHz.
Measurement Conditions
Measurements were done under two conditions: 1) with intact left pelvic and hypogastric nerves and 2) with bilaterally transected pelvic and hypogastric nerves.Intact left pelvic and hypogastric nerves. After transection of the right side pelvic and hypogastric nerves, in eight rats we electrically stimulated the left side pudendal nerve (frequency 2-70 Hz, amplitude 0.4-3.5 V, pulse width 50 µs) and measured the change in urethral pressure. Because the pudendal nerve electrode was very close to the sciatic nerve, pudendal stimulation also induced hindleg movement, which restricted the maximum stimulation amplitude. In four rats we measured the effect of hypogastric nerve stimulation on Pura.
Bilaterally transected pelvic and hypogastric nerves.
After exclusion of central reflexes by bilateral transection of the
pelvic and hypogastric nerves, there were only pudendal efferent
pathways to the urethra (see Fig. 1). The
pudendal nerve was stimulated again (at maximum amplitude with only
minor hindleg movement), and urethral pressure was measured. In seven
rats, we determined the frequency dependence of the urethral pressure response to pudendal nerve stimulation by varying the stimulation frequency
(fstim) between
2 and 20 Hz (5 rats) or between 1 and 70 Hz (4 rats). In two of these
rats both protocols were applied.
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-nitro-L-arginine methyl ester
[L-NAME; 50 mg/ml
(n = 2) or 100 mg/ml
(n = 3); 0.2 ml] administration.
These series of measurements were done at
fstim of 15 Hz.
First, three control measurements were done, and then a drug was
administered. If both drugs were given in the same animal, we allowed
at least 1 h in between administrations.
Measurements
Under both conditions (bilaterally transected pelvic and hypogastric nerves), electrical stimulation of the pudendal nerve had a dual effect: fast twitch-like contractions were superimposed on a slow relaxation (see Fig. 2). The recorded urethral pressure was analyzed in blocks with a length equal to the stimulus period. The blocks were synchronized to the stimulation signal, which was recorded for this purpose. In each block, the maximum (Pmax) and baseline pressures (P'0) during pudendal stimulation were determined. P'0 was defined as the mean pressure in the block after exclusion of the first twitch and the subsequent pressure undershoot (see Fig. 2). Before stimulation and at the end of the measurements, P'0 equaled the urethral pressure necessary to maintain a flow rate of 0.5 ml/min without nerve stimulation (P0, see Fig. 2). P'0 described the relaxant response. An exponential function was fitted to P'0 to determine the time constant of relaxation,
relax.
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The pressure amplitude of the fast contraction
(Ptwitch) was calculated as the
mean value of Pmax 
P'0 during stimulation. The
pressure amplitude of the slow relaxation
(Prelax) was calculated as the
difference between P0 and the
minimum value of P'0.
In each rat Ptwitch was expressed in decibels [= 20 · log(amplitude)], and the responses were plotted on a logarithmic frequency axis (2). For each rat the horizontal part of the graph was shifted to 0 (normalization), and all graphs were averaged. A two-parameter model (cutoff frequency and slope) was fitted to the data. To evaluate the effect of the tested drugs, we had to distinguish between the decay with time that was always observed in the urethral pressure responses to pudendal nerve stimulation and the effect caused by the drug itself. We assumed that both drugs did not have any effect on Pura after more than 30 min. The decay with time was estimated from the first three measurements (controls) and the measurements done more than 30 min after drug administration by fitting a straight line to these data. Urethral pressures measured within 30 min after drug administration were corrected using this line.
Materials
Drugs used were atropine (Pharmachemie BV) and L-NAME (Sigma), both dissolved in saline (0.9% NaCl), and urethan (Sigma), which was dissolved in water.Experiments were carried out as outlined in the Erasmus University of Rotterdam Guidelines for the Care and Use of Laboratory Animals, which in general follow the National Institutes of Health Guide for the Care and Use of Laboratory Animals. All data are presented as means ± SD.
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RESULTS |
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TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES
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In 16 rats, we measured urethral responses to electrical stimulation of
the pudendal nerve. At a perfusion rate of 0.5 ml/min we measured a
pressure loss of ~1 hPa in the connecting tubing. Pudendal nerve
stimulation had a dual effect: fast twitch-like contractions on each
stimulus pulse were superimposed on a slow relaxation (Fig. 2). The
amplitude of the fast contractions
(Ptwitch), the amplitude of the
relaxation (Prelax), and the
pressure necessary for urethral perfusion
(P0) were measured. Stimulation
of the hypogastric nerve (15-30 V) induced slow urethral
contraction without twitches (
P = 6 ± 3 hPa) in three of four
rats. In one rat we measured no effect.
To exclude the possible effects of afferent pudendal stimulation,
either the stimulated pudendal nerve was transected centrally to the
stimulation electrode (Fig. 1, transection
3; 1 rat), or the bilateral pelvic and hypogastric
nerves were transected (Fig. 1, transections
1 and 2; 12 rats).
After transection, again twitches superimposed on slow relaxation were
observed. Figure 3 shows an example of the
development of Pmax,
Pmin, and
P'0 before, during, and after
pudendal nerve stimulation. P0,
Prelax, and Ptwitch were determined. In all
rats, Prelax and
Ptwitch increased with the
stimulation amplitude. In two rats, pudendal nerve stimulation hardly
had any effect, probably because of insufficient stimulation amplitude.
In these rats, the amplitude could not be increased further because of
violent hindleg movement; therefore, they were excluded from further
analysis. P0 did not change after
pelvic nerve transection (P0 = 0 ± 10%, 0.9 ± 5.4 hPa) and was slightly but
significantly reduced after hypogastric nerve transection (P0 = 6 ± 4%,
3.2 ± 2.1 hPa; paired
t-test:
P = 0.02). Transection of both nerves
had no significant effect on P0
(P0 = 4 ± 11%, 1.7 ± 5.2 hPa; paired
t-test:
P > 0.2). Statistical tests were applied to absolute pressure changes. The average
P0 in all rats was 51 ± 18 hPa. Transection of the hypogastric and pelvic nerves had
no influence on Ptwitch.
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In four rats we determined the frequency dependence of
Ptwitch. We stimulated the
pudendal nerve at frequencies between 1 and 70 Hz and plotted the
frequency responses as in a Bode diagram. The amplitude of the twitches
(Ptwitch) was found to be
independent of the stimulation frequency up to 26 Hz (Fig.
4). Beyond this frequency, the amplitude of
Ptwitch decreased because there
was no longer complete relaxation between two consecutive twitches. In
all rats, the relaxation
(Prelax) depended highly on the
stimulation frequency. In five rats we quantified this frequency
dependence (Fig. 5). To avoid interference
of the contractions with Prelax, these measurements were done up to 20 Hz only. For analysis each measurement was divided into blocks with a length equal to the stimulus
period. P'0 described the
relaxant response during stimulation (see MATERIALS
AND METHODS and Fig. 3). Fitting an exponential
function to the relaxation showed a time constant of 3 ± 1 s (Fig.
3). The absolute values of Prelax
were stimulation amplitude dependent, and the hindleg movement limited
the maximum stimulation amplitude. Still, considerable urethral
pressure decreases of ~30 hPa could be observed. On average,
Prelax increased by 70% after
bilateral transection of the pelvic and hypogastric nerves. However,
this increase was not significant (P = 0.3, paired t-test).
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On average a twitch-like contraction lasted 31 ± 4 ms and had
an amplitude of 23 ± 15 hPa. The twitch amplitude
(Ptwitch) depended highly on the
stimulation voltage. In contrast to
Ptwitch, the twitch width
did not depend on the stimulation amplitude. In three rats we
varied the stimulation amplitude and determined the ratio,
Ptwitch/Prelax.
At very low stimulation intensities only slight twitches were observed;
at higher voltages Prelax appeared
to increase linearly with Ptwitch
(see Fig. 6). We found that
Ptwitch/Prelax ~ 3.
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We investigated the neurotransmitters involved in the pudendus-induced urethral relaxation by administration of the nitric oxide synthase (NOS) inhibitor L-NAME and the muscarinic receptor antagonist atropine.
Over the course of the experiments (56 ± 9 min), the effects of pudendal nerve stimulation (Prelax and Ptwitch) generally decreased. A straight line was fitted to the first three (control) values of Prelax and the values measured more than 30 min after drug administration. The slope of this line was used as an estimate for the decrease of Prelax with time and was used to correct for this time effect (mean slope, 0.14 ± 0.10 hPa/min).
Intravenous administration of
L-NAME reduced
Prelax in four of five rats by
30% on average and had no significant influence on
Ptwitch
(Ptwitch was 0.7 ± 3.9 hPa;
paired t-test:
P = 0.74). Intravenous administration
of atropine reduced Prelax in all
rats by 40% (n = 4) and did not
affect Ptwitch. An example of the
effect of both drugs is shown in Fig. 7.
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DISCUSSION |
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|
TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES
|
|---|
In this study we measured urethral pressure (Pura) in response to pudendal nerve stimulation. To allow urethral pressure measurement, the urethra was perfused at a constant flow rate (0.5 ml/min). At this flow rate the urethral pressure was 51 ± 18 hPa, which is in agreement with an earlier study (Pura ~ 56 ± 22 hPa) (19).
The rat urinary sphincter has been shown to receive both autonomic and somatic input (43). The somatic input is conducted through the pudendal nerve (26), whereas the autonomic input is generally assumed to be provided via the major pelvic ganglion (7). The pudendal nerve anatomy allows a clear distinction between an efferent and an afferent trunk (26), the afferent trunk contributing ~84% to the total number of fibers (13). Although the pudendal nerve is generally considered somatic, the efferent trunk appears to contain ~25% sympathetic fibers. The other 75% are parasympathetic or somatic motor fibers. Only 12% of the efferent fibers are myelinated and are suggested to be somatic motor fibers (13).
After the initial transection of the right pelvic and hypogastric nerve, there were four possible neural pathways to control urethral pressure: left pelvicus, left hypogastricus, and left or right pudendus. As in the experiments done by Kihara and de Groat (15), electrical stimulation of the hypogastric nerve increased Pura. In their experiments, the central pathway was transected. Therefore, the increased urethral pressure had to be caused by efferent hypogastric nerve stimulation. It is thus probable that the hypogastric nerve provides an excitatory (adrenergic) input to the smooth muscle of the proximal urethra. Fraser et al. (11) showed that electrical stimulation of parasympathetic pathways in the anesthetized rat produces urethral smooth muscle relaxation sensitive to NOS inhibition.
After subsequent transection of the left pelvic and hypogastric nerves only pudendal efferents controlled urethral resistance.
The first (rostral) half of the proximal urethra consists of three layers of smooth muscle, which receive mainly adrenergic innervation. In the innermost layer, cholinergic innervation has been described as well (43). In the second half, a single layer of smooth muscle cells is surrounded by a layer of mixed smooth and striated muscle cells and a layer of striated muscle. Both adrenergic and cholinergic nerves have been found in these layers. Ganglion cells have been described between the striated muscle layer and smooth muscular coat (43).
In our study, after bilateral transection of the pelvic and hypogastric
nerves, electrical stimulation of the pudendus induced fast twitch-like
contractions upon each stimulus pulse superimposed on a slow
relaxation. At low stimulation frequencies (
20 Hz) the pressure
reached a stable level P'0
before the next twitch contraction. The fast pressure undershoot
(Pmin, Fig. 2). was considered to
be an artefact caused by the sudden stop of moving fluid in a flexible
chamber. This point of view is supported by the fact that
P'0 at the end of stimulation
(and not Pmin) equals the
urethral pressure immediately after stimulation (Fig. 2). Thus
P'0 described the relaxant
response. We determined the time constant of this relaxation
(relax = 3 ± 1 s). Other studies have shown that bladder smooth muscle contracts with a time
constant of ~3.1 ± 1.1 s (41) or ~3.4 s (18). We therefore concluded that the slow decrease in urethral pressure was caused by
smooth muscle relaxation.
Ptwitch was not frequency dependent up to 26 Hz, which corresponds to a time constant of ~40 ms, 80 times faster than the smooth muscle time constant. Skeletal muscles have been shown to follow frequencies up to 2 Hz (32). However, this latter study concerned load-moving skeletal muscle, which decreased the maximum frequency. Isometric twitch contraction in the soleus muscle of mice was shown to have a contraction time of 21 ms (21), even less than the 31 ms measured in our study. We concluded that the twitches in our study were caused by striated muscle contractions. Because all other neural pathways to the urethra had been transected, both the smooth muscle relaxation and the striated muscle contraction must have been induced by efferent pudendal nerve firing [caused either directly by efferent stimulation or indirectly via the pudendo-pudendal reflex (27)].
Transection of the left hypogastric and pelvic nerve had no influence on the tonic urethral pressure. Similar results were obtained by Kakizaki et al. (14) after ganglionic blockade. Tonic urethral resistance is probably not neurally regulated by the pelvic or hypogastric nerve.
In our study, the effect of hypogastric and pelvic nerve transection on Prelax was probably underestimated because there was always a spontaneous decay with time, which was not compensated for. Thus a possible increase is masked by a decrease with time. Yet, we still measured a Prelax that tended to increase after hypogastric and pelvic nerve transection, although not significantly.
If Prelax increased after bilateral transection of the hypogastric and pelvic nerves, what may have caused this increase?
Stimulation of pudendal afferent fibers (originating in sex organs) has been shown to have an inhibitory effect on the bladder (9, 20). Inhibition of the micturition reflex may include an excitatory reflex (sympathetic adrenergic or parasympathetic cholinergic) to the urethral smooth muscle. The most probable pathway would be the sympathetic system because this is generally accepted to be active during the urine storage phase (8). Furthermore, far more adrenergic nerves than cholinergic nerves were found in the proximal urethra (43). Stimulation of the hypogastric nerve induced increased urethral resistance (15). Thus, before transection of the pelvic and hypogastric nerves, the relaxant effect of pudendal nerve stimulation may have been masked by a central reflex via the hypogastric nerve that induced contraction of urethral smooth muscle.
In in vitro experiments done by others, electrical stimulation of
urethral tissue also induced both relaxation and contraction of smooth
muscle (14, 31, 34). The contraction was no longer observed after
supramaximal 
-adrenergic stimulation (31), which indicates that the
smooth muscle contraction upon electrical stimulation was mediated by
adrenergic pathways and therefore sympathetic.
Nonadrenergic, noncholinergic-mediated relaxation of urethral smooth muscle has been described (3, 31), whereas norepinephrine has been found to be the major excitatory transmitter (5). Parlani et al. (31) reported atropine-sensitive relaxation of urethral muscle strips on acetylcholine stimulation.
In our study, atropine reduced the smooth muscle relaxation by ~40% and had no influence on the striated muscle contractions. Thus the smooth muscle relaxation was at least partially mediated by cholinergic activation of muscarinic receptors. Acetylcholine had an excitatory effect on the urethral striated musculature, but this effect was not blocked by atropine because the contraction is mediated by nicotinic receptors (14, 22).
The smooth muscle relaxation in our study was also reduced (by ~30 %) after L-NAME administration. We therefore concluded that the relaxation was also (partially) mediated by nitric oxide (NO). Persson et al. (33) described a dense innervation of NOS-containing nerves in the pig urethra and suggested a possible corelease of NO and acetylcholine because a considerable overlapping of NOS immunoreactivity and acetylcholinesterase (AChE) staining was found. In a more recent paper, they (34) suggested that the function of cholinergic nerves in the rat urethra is mainly to release inhibitory NO and to evoke urethral relaxation.
NO might also be released on cholinergic stimulation from endothelium cells (30). In the urethra, this may seem unlikely because cholinergic fibers were mainly found in the outer layers (43), whereas endothelium cells are located on the inner side. However, Persson et al. (35) found AChE-positive terminals that ran in close association with the urothelium, with branches arborizing into it. NOS-immunoreactive nerves were also observed in the suburothelial stroma (35).
NO may also be released from ganglion cells that are found in the urethra (43). In the major pelvic ganglion coexistence of cholinergic and nitrergic nerves has been demonstrated (34). This mechanism may play a role, but if so, it is not the single pathway because it does not explain the reduced relaxation after atropine administration that we found. Atropine has no effect on the nicotinic receptors in ganglion cells. Possibly, acetylcholine (also) has a relaxant effect on urethral smooth muscle, which is not mediated by NO. This is emphasized by our finding that a muscarinic receptor blocking agent induces stronger reduction of the urethral relaxation than an NO synthase inhibitor. Moreover, it was shown that L-NAME may block muscarinic receptors, and thus even the urethral relaxation that was reduced after L-NAME administration may have been mediated by acetylcholine instead of NO (4).
However, either of these mechanisms implies an important role of acetylcholine in pudendal nerve-controlled urethral relaxation.
If acetylcholine has an inhibitory effect on urethral smooth muscle and an excitatory effect on urethral striated muscle, and these types of muscle cells intermingle rather freely in the rat urethra (43), the question arises: what is the predominant effect of acetylcholine release?
Our results show that the urethral relaxation is highly dependent on the frequency of pudendal nerve stimulation. The amplitude and the duration (~31 ms) of the striated muscle contractions, however, are independent of this stimulation frequency, up to 26 Hz. On average the amplitude of the contractions was three times larger than the amplitude of the relaxation. We concluded that during contraction of the striated muscles, the urethra was always closed. The relaxation was therefore only effective in the fraction of time when the striated muscles did not contract.
We calculated the effective urethral relaxation (EUR) as the urethral
smooth muscle relaxation multiplied by this fraction (1 0.031 · fstim).
The result is shown in Fig. 8. From other studies it is known that rats normally void at bladder pressures of
~40 hPa (40). Pura necessary for
perfusion at a flow rate as low as 0.5 ml/min generally exceeded this
pressure (~51 ± 18 hPa), and thus urethral relaxation is needed
to enable bladder emptying. Figure 8 shows that the EUR is maximum at
frequencies between ~7 and ~15 Hz, the frequency range of natural
urethral oscillations during voiding. In our measurements the absolute value of the maximum EUR was ~7 hPa, but this depended highly on the
stimulation amplitude and may be much larger if all nerves fire at
maximum frequency.
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Thus the dominant effect of acetylcholine on urethral resistance depends on the frequency of release. An oscillatory release at 7-15 Hz induces maximum EUR. The frequency of sphincter oscillations during evoked voiding contractions in anesthetized animals is in the lower half of this frequency range with maximum EUR. This may be so because the lower frequencies require less metabolic activity, but it has also been described that the use of anesthetics lowers the oscillation frequency (28). Thus the oscillations during voiding occur at the frequency that maximizes urethral relaxation. Moreover, the oscillations are observed more frequently in male rats than in female rats. This may be explained by their higher need for urethral relaxation during voiding; male rat urethras are approximately four times longer than female rat urethras.
It is generally assumed that the striated urethral muscles are controlled by somatic motor fibers that are presumably myelinated (13) and that the smooth muscles receive unmyelinated parasympathetic innervation. Because myelinated nerve fibers show a lower stimulation threshold (37), it might be expected that only twitches at low stimulation amplitude would be found. From our measurements we could not determine such a threshold amplitude (Fig. 6). However, other studies showed that the stimulation threshold for unmyelinated fibers is one order of magnitude higher than the threshold for myelinated fibers (36). Thus we probably stimulated only myelinated fibers, and only the number of recruited myelinated fibers increased with increasing stimulation amplitude. Both the twitch amplitude and the relaxant amplitude increased. Inasmuch as it is unlikely that all muscle cells in the urethral wall receive direct innervation (10), there may be myelinated axons that have influence on both striated and smooth muscle cells.
The major argument for the theory that the oscillations are needed to
pump the urine through the urethra is the observation that blocking the
oscillations by either pudendal nerve transection (6) or administration
of d-tubocurarine (22) increases the residual urine in the bladder or completely abolishes effective voiding. However, pudendal nerve transection obviously abolishes both
the twitches and the slow relaxation, whereas
d-tubocurarine also blocks
ganglionic transmission, and ganglionic blockade has been shown
to abolish the oscillatory reflex (22). In both situations there
is no acetylcholine release and thus no effective urethral relaxation. Kakizaki et al. (14) showed that the striated
muscle contractions could be blocked by -bungarotoxin
while there still was smooth muscle relaxation (although masked by
adrenergic smooth muscle contraction).
In conclusion, urethral oscillation during bladder emptying in rats may have a function in territory marking, or it may pump urine through the urethra. In this study, we showed that the pudendal nerve induces urethral relaxation, which is, at least partially, mediated by acetylcholine. Acetylcholine also induces contraction of striated urethral muscle, and the overall effect on urethral resistance depended on the frequency of acetylcholine release. We therefore introduced the (frequency dependent) effective urethral relaxation that was maximum at the frequency of the spontaneous oscillations. Thus, although the oscillatory sphincter contractions in rats during voiding may be needed in other mechanisms for efficient voiding, they may very well be a side effect of the actual purpose of pudendal acetylcholine release: urethral relaxation.
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ACKNOWLEDGEMENTS |
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This study was supported by Dutch Kidney Foundation Grant C95.1429.
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FOOTNOTES |
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The costs of publication of this article were defrayed in part by the payment of page charges. The article must therefore be hereby marked "advertisement" in accordance with 18 U.S.C. §1734 solely to indicate this fact.
Address for reprint requests and other correspondence: J. le Feber, Dept. of Urology-Urodynamics, Room EE 1630, Erasmus Univ. Rotterdam, PO Box 1738, 3000 DR Rotterdam, The Netherlands (E-mail: lefeber{at}udn.fgg.eur.nl).
Received 9 February 1999; accepted in final form 30 June 1999.
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REFERENCES |
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TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES
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). Change over time of Pmax,
Pmin, and
P'0 are shown in
B [stimulation frequency
(fstim) = 15 Hz; for clarity, only one +, 
,
Mean Ptwitch (±SD). Fitted
line had 2 degrees of freedom: cutoff frequency and slope.
