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This Article Abstract Full Text (PDF) All Versions of this Article: 576/3/689    most recent jphysiol.2006.116657v1 Services Email this article to a friend Similar articles in this journal Similar articles in PubMed Alert me to new issues of the journal Download to citation manager Citing Articles Citing Articles via HighWire Citing Articles via Google Scholar Google Scholar Articles by McHale, N. G. Articles by Ward, S. M. Search for Related Content PubMed PubMed Citation Articles by McHale, N. G. Articles by Ward, S. M. Related Collections Perspectives

¹ Smooth Muscle Research Centre, Dundalk Institute of Technology, Dundalk, Co. Louth, Ireland
² Department of Physiology and Cell Biology University of Nevada, Reno, NV 89557-0271, USA

	Abstract

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ICC are found in both the upper and lower urinary tract. They are not found in the ureter itself but are confined to the lamina propria of the renal pelvis and pelvi-calyceal junction. They do not appear to have a primary pacemaker role (this is ascribed to atypical smooth muscle cells in the same location) but rather conduct and amplify the pacemaker signals generated by the atypical smooth muscle cells. In the bladder, ICC are widely distributed in the sub-urothelial region, in the lamina propria and at the margins of the detrusor smooth muscle bundles. Again they appear not to have a pacemaking role and such evidence as there is would suggest that they have a role in the modulation of signal transduction. The strongest evidence that ICC in the urinary tract act as pacemakers comes from studies of those in the urethra. Isolated ICC show regular spontaneous depolarizations in current clamp which resemble very closely the slow waves recorded from intact tissue. In voltage clamp they show abundant calcium-activated chloride current and spontaneous transient inward currents which can be blocked by chloride channel blockers. However, their role in the modulation of urethral tone has yet to be fully elucidated.

(Received 7 July 2006; accepted after revision 15 August 2006; first published online 17 August 2006)
Corresponding author N. McHale, Smooth Muscle Research Centre, Regional Development Centre, Dundalk Institute of Technology, Dundalk, Co. Louth, Ireland. Email: noel.mchale{at}dkit.ie

	Introduction

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The urinary tract has some affinity with the lower gastrointestinal tract in that it could be viewed as the fluid waste disposal system by analogy with the solid waste disposal system that is the lower gastrointestinal tract. Thus the kidney decides how much fluid and solute to retain and what to reject. The rejected fluid must then be propelled by the ureter to the storage depot (the bladder) where it is retained until it can be emptied when a suitable occasion presents itself. Thus the ureter must be capable of efficient peristalsis which is responsive to the rate of urine production. The bladder must be sufficiently compliant to accommodate an adequate volume increase without intravesicular pressure rising to a level where it would inhibit urine flow from the kidney. Lastly the urethra is the guardian of continence and as such makes the final decision as to whether urine is voided or retained in the bladder. What these organs have in common is that, underlying their apparently very different functions, they all have a basic spontaneous electrical rhythm. In the case of the ureter the role of a pacemaker is rather obvious in that it initiates the propulsion of fluid from the renal calyx to the bladder by means of well-coordinated peristaltic waves that have their site of origin in the renal pelvis. It is less obvious why the bladder, which acts as a storage organ most of the time, and the urethra, which remains tonically contracted most of the time, should have any need for spontaneous electrical rhythm. Nevertheless it has been known for a long time that activity recorded using external (Orbeli & Brucke, 1910; Prosser et al. 1955) or intracellular electrodes (Ursillo, 1961; Kuriyama et al. 1967; Creed, 1971; Creed et al. 1983; Hashitani et al. 1996; Bradley et al. 2004) shows rhythmic firing of action potential complexes in all three organs. The purpose of the present review is to explore the origins of this electrical activity and in particular the possible role of ICC or ICC-like cells in its generation or modulation.

Ureter

Electrical activity appears to arise in the most proximal calyceal regions of the renal pelvis. This is not accompanied by a significant contraction since this region is only weakly contractile due to the paucity of smooth muscle cells. It is only when the impulse is conducted to the ureter proper that it initiates a vigorous contraction that is propagated to the uretero-vesical junction as a peristaltic wave. The source of the electrical impulse has been extensively studied by Lang and colleagues (Lang et al. 1998, 2001; Klemm et al. 1999) and is the subject of several reviews by these authors (Lang et al. 2002; Lang & Klemm, 2005). Using intracellular recording and by injecting neurobiotin they identified spindle-shaped ‘pacemaker’ cells in pelvi-calyceal junction and the proximal renal pelvis. These were approximately 160 µm in length and fired oscillations at a frequency of 8 min^–1. Their morphology was closer to that of smooth muscle cells than to typical ICC and they were described as atypical smooth muscle cells. These cells have not yet been studied in isolation in voltage clamp so their detailed electrophysiology and the nature of the pacemaking current have not been described. In the lamina propria of the renal pelvis and pelvi-calyceal junction a cell type similar to typical ICC was found. They fired ‘intermediate’ action potentials at a frequency of 3–4 min^–1. These cells were not regarded as the primary pacemaker but rather were thought responsible for conducting and amplifying pacemaker signals to initiate action potentials in smooth muscle cells. The observation that c-kit expression is up-regulated in the developing ureter prior to its ability to undergo unidirectional contractions (David et al. 2005) and that anti-c-kit antibodies inhibit peristaltic contractions would suggest that these cells, even if they are not the primary pacemakers, do play an important role in normal ureteral rhythmic activity.

Bladder

The bladder has two essential functions: it must store the urine that is continually produced by the kidney without its pressure rising above the kidney filtration pressure and it must be able to empty quickly when required. However, the bladder is not simply a compliant bag but is rather a spontaneously active muscular organ. After voiding, spontaneous contractions are minimal and filling occurs with little increase in pressure but against a background of small phasic increases in pressure. These rhythmic pressure oscillations are myogenic resulting from poorly coordinated contractions which arise at many different sites throughout the bladder. As filling proceeds the pressure waves increase in magnitude and eventually cause the urge to micturate. The bladder must at this point change from an ill-coordinated set of oscillators which provide background tone to a well-coordinated propulsive system capable of efficient emptying. How both of these functions are controlled is not yet fully understood but it is clear that there must be many pacemaking loci which generate the fundamental rhythmic activity. ICC would be obvious candidates for such a role and there is ample evidence of their presence in the sub-urothelial region, in the lamina propria and on the peripheries of the muscle bundles of the detrusor (Sui et al. 2002; Wiseman et al. 2003; Davidson & McCloskey, 2005). These authors all speculated that the different types of ICC (or myofibroblasts), which had been identified using morphological techniques, were potential pacemaker cells but they presented no convincing evidence in support of these speculations. In a careful study using microelectrodes and intracellular calcium imaging, Hashitani et al. (2004) could find no evidence of a pacemaking role for ICC in the guinea-pig bladder. The latter authors suggested that spontaneous excitation in the bladder might be initiated by detrusor smooth muscle cells themselves with the main role of ICC being to modulate the signal transmission. Clearly we are not yet in possession of enough detailed information to define the role of ICC in the bladder.

Urethra

The mechanism by which urinary continence is achieved is complex and has at least three components: (1) external pressure on the urethra due to contraction of the abdominal and pelvic muscles; (2) neurogenic tone due to sustained contraction of both smooth and striated muscle in response to excitation of cholinergic and noradrenergic nerves; and (3) myogenic tone due to sustained contraction of urethral smooth muscle. While all of these undoubtedly play a part, it is likely that contraction of striated muscle is more important in the increase in urethral tone that accompanies increases in bladder pressure secondary to coughing or other sudden increases in intra-abdominal pressure than in the long-term maintenance of tone. On the other hand, smooth muscle in the urethral wall is better adapted to this latter task since it can achieve it at relatively low energy cost.

There is no doubt that the smooth muscle of the urethra is capable of generating significant tone in the absence of neural input. We have recently demonstrated that an isolated cannulated rat urethra can maintain sufficient tone to limit flow from a reservoir (held at a constant pressure of 20 cmH₂O) to less than 25% of the flow encountered when the urethra is maximally dilated (Fig. 1). Under these conditions nerve and striated muscle contributions are likely to be minimal so tone is largely due to sustained contraction of the intramural smooth muscle. That this is so can be demonstrated by applying wortmanin (a myosin light chain kinase inhibitor) which has the effect of fully dilating the urethra within 30 min. Prior to wortmanin application, electrical field stimulation of the inhibitory nerves (0.3 ms pulse width at 0.5 Hz in the presence of atropine and guanethidine) caused a similar increase in flow.

View larger version (10K): [in this window] [in a new window]   Figure 1.  Flow through a cannulated rat urethra that is connected to a constant pressure reservoir of Krebs solution Under resting conditions flow was about 20% of maximum. Stimulation of the inhibitory nerves caused the urethra to relax and flow to exceed 80% of maximum. When 30 µM wortmanin was added, flow increased almost to the level seen when the inhibitory nerves were stimulated.

Sergeant et al. (2000) reported that collagenase dispersal of strips of rabbit urethra yielded, in addition to normal spindle-shaped smooth muscle cells, a small proportion of branched cells which resembled the interstitial cells of Cajal dispersed from canine colon (Langton et al. 1989). These were clearly distinguishable from smooth muscle in their appearance under the phase contrast microscope, their immunohistochemistry and ultrastructure. They had abundant vimentin filaments but no myosin, a discontinuous basal lamina, sparse rough endoplasmic reticulum, many mitochondria and well-developed smooth endoplasmic reticulum. At the time it was reported that the cells were not c-kit positive but with improved procedures it has recently been demonstrated that they are. Figure 2 shows a whole mount preparation of rabbit proximal urethra stained with Kit antibody. ICC are evident as irregular elongated cells of about 80–100 µm in length between and surrounding the smooth muscle bundles (the latter are evident because of their weak autofluoresence). ICC generated spontaneous depolarizations, whereas isolated SMCs from the same preparation were electrically quiescent, but could respond to injection of depolarizing current by producing action potentials (Fig. 3, taken from Sergeant et al. 2000). Clues to the mechanisms underlying these different responses were provided by the results of voltage clamp studies, which showed that ICC possessed an abundance of Ca²⁺-activated chloride current (I_ClCa) whereas SMCs in comparison did not. Moreover, when ICC were held at –60 mV they generated spontaneous transient inward currents (STICs; Sergeant et al. 2000) which were notably similar to pacemaker currents recorded from ICC in the gastrointestinal tract (Thomsen et al. 1998; Koh et al. 1998). This property, coupled with other fundamental structural and morphological similarities, opens up the intriguing possibility that urethral interstitial cells serve a similar purpose and are therefore key determinants of urethral tone. Our hypothesis therefore is that tone in the urethra is initiated by the oscillatory release of calcium from intracellular stores in the interstitial cells. This, in turn, causes activation of calcium-activated chloride channels resulting in the spontaneous depolarizations referred to above. These, in turn, activate in an asynchronous fashion the smooth muscle bundles to which they are electrically coupled to produce a sustained tone. Recent experiments with the isolated cannulated urethra preparation lend some support to this idea (Fig. 4). Anthracene-9-carboxylic acid (which is known to block Ca²⁺-activated chloride channels and spontaneous depolarizations in the isolated interstitial cells) was almost as effective as wortmanin in relaxing urethral tone.

View larger version (95K): [in this window] [in a new window]   Figure 2.  Whole mount of rabbit urethra labelled with anti-Kit antibody ICC are evident as irregular elongated cells of about 80–100 µm in length between and surrounding the smooth muscle bundles (the latter are evident because of their weak autofluoresence).

View larger version (30K): [in this window] [in a new window]   Figure 3.  Contrasting electrical properties of interstitial and smooth muscle cells Interstitial cells showed regular ‘slow-wave’ depolarizations in current clamp (A) while smooth muscle cells were quiescent, although they could produce an action potential in response to depolarizing current (B). Under voltage clamp, interstitial cells exhibited both L-type calcium currents and calcium-activated chloride currents (C) while the smooth muscle cells showed only L-type calcium currents (D). E and F show summaries of the currents measured in 26 interstitial and 21 smooth muscle cells (redrawn from Sergeant et al. 2000).

View larger version (8K): [in this window] [in a new window]   Figure 4.  The effect of anthracene-9-carboxcylic acid on flow through the isolated urethra A-9-C (1 µM), like wortmanin, caused an increase in flow almost equal to the effect of stimulation of the inhibitory nerves.

The urinary tract shows evidence of rhythmical electrical and mechanical activity at all levels. The purpose of this is evident in the ureter where it is important for pumping urine but rather less so in the bladder and in the urethra. It would seem that the bladder's ability to expand in a controlled way is dependent on the tone generated by asynchronous firing of many pacemakers. Clearly if these pacemakers could then be coordinated (under neural influence) one has the basis of an efficient emptying system. The urethra, on the other hand, exists only to produce tone and this may also occur by asynchronous firing of many pacemakers.

	Footnotes

 
This report was presented at The Journal of Physiology Symposium on Involvement of interstitial cells of Cajal in the control of smooth muscle excitability, Okayama, Japan, 22 July 2006. It was commissioned by the Editorial Board and reflects the views of the authors.

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	Acknowledgements

 
The authors wish to acknowledge support from grant number 064212 from the Wellcome Trust and NIH RO1 DK68565. G.P.S. is in receipt of a Research Fellowship awarded by the Health Research Board, Ireland.

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This Article Abstract Full Text (PDF) All Versions of this Article: 576/3/689    most recent jphysiol.2006.116657v1 Services Email this article to a friend Similar articles in this journal Similar articles in PubMed Alert me to new issues of the journal Download to citation manager Citing Articles Citing Articles via HighWire Citing Articles via Google Scholar Google Scholar Articles by McHale, N. G. Articles by Ward, S. M. Search for Related Content PubMed PubMed Citation Articles by McHale, N. G. Articles by Ward, S. M. Related Collections Perspectives