Kaohsiung Medical University Institutional Repository:Item 310902000/18627

Effect of castration on male rabbit lower urinary tract tissue

enzymes

Yung-Shun Juan Æ Bulent Onal Æ Samuel Broadaway Æ Julia Cosgrove Æ Robert E. Leggett Æ Catherine Whitbeck Æ Elise De Æ Rebekah Sokol Æ Robert M. Levin

Received: 25 September 2006 / Accepted: 19 January 2007 / Published online: 9 February 2007

Springer Science+Business Media B.V. 2007

Abstract Objectives The influence of testosterone on the prostate and corpus cavernosum have been stu-died extensively. However, the influence of testoster-one on the lower urinary tract (bladder and urethra) have not been investigated to any great extent. The aim of this study was to determine whether androgen deprivation alters lower urinary tract metabo-lism.Methods A total of 16 rabbits were divided into four groups of four rabbits each. Each rabbit in groups 1–3 underwent surgical bilateral castration for duration of 1, 2 , and 4 weeks, and group 4 underwent sham operations. Sections of bladder body and base wall and mucosa, urethra and corpora were isolated, frozen, and stored under liquid nitrogen. The

activ-ities of citrate synthase-thapsigargin sensitive Ca2+ ATPase (Sarco/Endoplasmic Reticulum Ca2+ ATPase [SERCA]), and choline acetyl-transferase were ex-amined as markers for mitochondrial function, sar-coplasmic reticular calcium storage and release, and cholinergic nerve function, respectively.Results The activity of SR function indicator, Ca2+ ATPase was significantly higher in the control corpora than in the control bladder or urethra. Castration resulted in decreased activity in the mitochondria specific en-zyme, citrate synthase, the activity of which was greatest in the urethra and lowest in the corpora. Cholinergic nerve density indicator, choline acetyl-transferase activity was greatest in the bladder body and lowest in the urethra.Conclusions Our data in-dicate that (1) significant differences exist in the ac-tivities of all three enzymes in the various organs associated with the lower urinary tract; and (2) that castration results in significant alterations in the ac-tivities of all three enzymes in the bladder body, base, urethra, and corpora.

Keywords Castration
Rabbit
Bladder

Mitochondria
Atpase
Choline acetyl transferase

Introduction

Bladder dysfunction secondary to benign prostatic hyperplasia (BPH) is a common consequence in the aging male. The frequent urinary symptoms include the storage symptoms of urgency, frequency and nocturia and the voiding symptoms of incomplete emptying, intermittency, weak stream, and voiding with straining. It is well-known that prostate enlargement is androgen

R. E. Leggett
C. Whitbeck
R. M. Levin

Stratton Veterans Affairs Medical Center, Albany, NY, USA

S. Broadaway
J. Cosgrove
R. E. Leggett
C. Whitbeck
R. M. Levin (&)

Albany College of Pharmacy, 106 New Scotland Avenue, Albany, NY 12208, USA

e-mail: [email protected] E. De
R. M. Levin

Albany Medical College, Albany, NY, USA Y.-S. Juan

Kaohsiung Municipal Hsiao-Kang Hospital, Kaohsiung, Taiwan

B. Onal

University of Istanbul Cerrahpasa School of Medicine, Istanbul, Turkey

R. Sokol

Albany Academy for Girls, Albany, NY, USA DOI 10.1007/s11010-007-9415-8

dependent, and the effect of prostate enlargement in-duced partial bladder outlet obstruction is extensively studied in many animal models [1–3]. Clinically, the a-blocker and anti-androgen medications are widely used as treatments for BPH and lower urinary tract syn-dromes (LUTS) in the aging males. However, the im-pact of androgen on lower urinary tract function and biochemistry is not well-known. In clinical practice, the size of the prostate does not always correlate with the severity of urinary symptoms. Some men with greatly enlarged glands may have little obstruction and few symptoms while others with prostate glands less en-larged have more outlet blockage and severe problems. By immunohistochemical methods, it has been proved that estrogen receptor and androgen receptor are widely distributed in the bladder, proximal urethra and autonomic ganglia of the prostatic plexus, suggesting the importance of sex hormone in regulating lower urinary tract function [4].

In the rabbit bladder outlet obstruction study, bladder dysfunction is mainly mediated by three cel-lular processes, including (1) progressive denervation, (2) cellular mitochondria malfunction, and (3) dysre-gulation of intracellular calcium storage and release from the sarcoplasmic reticulum (SR) [3]. Biomarkers for these three functions are calcium ATPase for cal-cium regulation; citrate synthase for mitochondrial function, and choline acetyl-transferase for cholinergic innervation. The aim of this study is to determine whether androgen deprivation alters the activities of these biomarkers in the various organs of the lower urinary tract, namely, bladder body, bladder base muscle and mucosa, urethra and corpora.

Materials and methods

These studies were approved by the Institutional Animal Care and Use Committee of the Stratton Af-fairs Medical Center, Albany, NY.

Animal preparation

A total of 16 adult male rabbits were divided into four groups of 4 rabbits each. Each rabbit was anesthetized with isoflorane (1–3%). The rabbits in groups 1–3 were bilaterally castrated through two small incisions, which were then closed with 3–0 silk. The rabbits in group 4 were sham operated.

The rabbits in groups 1–3 were anesthetized at 1, 2, and 4 weeks following castration. The following tissues were surgically excised, frozen in liquid nitrogen and stored at –70C until analyzed: bladder body muscle

and mucosa; bladder base muscle and mucosa, urethra, and corpus cavernosum. The mucosa of the urethra could not be separated from the muscle. The rabbits were euthanized immediately following surgery. The rabbits in group 4 were anesthetized one rabbit with group 1, two rabbits with group 2, and one rabbit with group 3. Tissues were removed as described above and the rabbits euthanized. The sham rabbits showed no significant differences and were combined into one group.

Mitochondrial function

Citrate synthase (CS) assay [5]

Frozen tissue samples are homogenized in ice-cold Tris buffer (50 mM, pH 7.6) at 50 mg/ml and cen-trifuged at 2500g for 10 min to remove the cell membranes and nuclei. A sample aliquot (100 ll) of supernate is added to a 0.5 cm cuvette, along with 1.0 ml 0.05 M Tris buffer (pH 7.6), 50 ll 0.2–10 mM oxaloacetate (substrate), 30 ll 12.3 mM acetyl-coen-zyme A, 100 ll 1 mM 5,5¢- dithiobis-2-nitrobenzoic acid (DTNB), and 100 ll 10% Triton X-100. The free coenzyme-A generated by CS activity reacts with DTNB to form a colored compound that is quantified at 412 nm. Absorbance is recorded every 30 s for 6 min (reaching steady state), using a Hitachi spectrophotometer. Protein concentration is deter-mined using the Lowry method. Citrate synthase activity is given as nmoles Coenzyme-A generated per min. per mg protein.

Sarcoplasmic reticulum (SR) function

Ca2+ ATPase Activity [6]

SR function is evaluated by measuring thapsigargin-sensitive calcium ATPase activity (SERCA) activity. Frozen tissue samples are homogenized at 10 mg/ml in ice-cold Tris buffer (50 mM, pH 7.4) and centrifuged at 2,500g for 10 min to remove the cell membranes and nuclei. Aliquots of particulate preparations are incu-bated at 37C in TRIS buffer with 4 mM ATP (sub-strate) and CaCl2(1 mM). The reaction system for a typical assay designed to measure ATPase activity is as follows: 75 mM TRIS, 0.25–4 mM ATP, 4 mM MgCl2, 100 ul tissue extract (pH 7.4; total volume 2.0 ml). At the end of the incubation (e.g. 30 min) the reaction is stopped by adding 1 ml 12.5% TCA. Reaction tubes are centrifuged at 1,000g for 20 min to remove protein precipitates, and inorganic phosphate is determined. Inorganic phosphate present in the ATP reagent and in

the tissue extracts is measured initially, and then sub-tracted from total inorganic phosphate. Results are expressed as lmol phosphate/mg protein/min. Thapsi-gargin inhibition is assessed by incubating the reaction system in the absence and presence of 10 lM thapsi-gargin; % inhibition of activity is calculated.

Cholinergic nerve density

Choline acetyl-transferase (ChAT) activity [7]

Frozen tissue samples are homogenized in ice-cold phosphate buffer (50 mM, pH 7.4) containing 10 mM EDTA and centrifuged at 20,000g for 30 min to re-move the cell membranes, mitochondria, and nuclei. Aliquots are incubated at 37C for 10 and 20 min with 200 l1 of reaction mixture consisting of 0.2–10 mM acetyl -coenzyme A (acetyl-CoA) (substrate), 0.2 mM 3

H-acetyl-CoA (200 mCi/mmol), 8 mM choline, 50 mM sodium phosphate, 0.3 M NaCl, 20 mM EDTA, and 96 nM physostigmine. After incubation, each solution is diluted with 5 m1 of 0.01 M sodium phosphate and the reaction stopped with 2 ml of ace-tonitrile containing 5 mg/ml tetraphenylboron. Then, the contents of each reaction tube are transferred to a 20 ml scintillation vial and 10 ml of Betamax scintil-lation fluid are added slowly to each vial. The vials are shaken lightly. Samples stand for 1 h while the phases separate, extracting acetylcholine (3H-Ach) into the Betamax phase, while 3H-acetyl-CoA stays in the aqueous phase. The aqueous phase is removed and3 H-ACh is measured using scintillation spectroscopy. ChAT activity is reported as fmoles Acetyl-Co-A generated per min per mg protein/30 min.

Data analysis

All values are presented as mean ± SEM. Analysis was performed by Analyses of Variance and Bonferonni

test for individual differences. A P < 0.05 was required for statistical significance.

Results

Bladder weight: Bladder weight decreased progres-sively, after 2 weeks of castration reached statistical significance compared to the control (sham) group. The weights (in grams) for the groups were: 3.0+/–1.0 (control) 2.5+/–0.4 (1 Wk castrated); 2.1+/–0.36* (2 wk castrated); and 2.2+/–0.18* (4 wk castrated). * = sig-nificantly different from control, P < 0.05.

The basal activities of the three enzymes are pre-sented in Table1. The calcium ATPase activity of the corpora was significantly greater than all other tissues; whereas the corpora had the lowest citrate synthase activity. The citrate synthase activity of the mucosa of the bladder body and base were significantly greater than the activities of the bladder body and base muscle. The ChaT activity of the urethra was significantly lower than the activities of the bladder body and base. Interestingly, the corpora had a surprisingly high activity of ChAT.

Effect of castration

Calcium ATPase activity

Figure 1shows the effect of castration on Ca2+ATPase activity. The activity of the bladder body mucosa was significantly greater than the activity than bladder body muscle layer. The activities of body muscle increased by 2 weeks following castration and remained elevated at 4 weeks. The body mucosa significantly decreased at 1 week following castration and increased to control activity by 4 weeks. For the bladder base, the activity decreased progressively at 1 and 2 weeks following castration. By 4 weeks, the activity of the base muscle increased to control values, whereas the activity of the

Table 1 Basal activities of calcium ATPase, citrate synthase, and choline acetyltransferase in lower urinary tract tissues obtained from control male rabbits

Ca2+ATPase lmolPi/mg protein

Citrate Synthase nmol Co-A/min/mg protein

ChAT fmol Acetyl C0-A / 30 min Body muscle 2.8 ± 0.5 129 ± 19 743 ± 110 Body mucosa 6.9 ± 1.0* _{261 ± 39}* Base muscle 8.3 ± 1.0+ _{175 ± 26}+ _{550 ± 100} Base mucosa 7.5 ± 1.2 263 ± 39* Urethra 6.2 ± 0.9 342 ± 51x 388 ± 80a Corpora 23.0 ± 4.0x 44 ± 6x 469 ± 48

* = significantly different from muscle; + = bladder base significantly different from body;a= significantly different from bladder body and base; x = significantly different from all other tissues, P < 0.05. ChAT was not performed on mucosa

base mucosa was still significantly lower than that of the muscle. Castration had no effect on the calcium ATPase activity of the urethra, whereas the activity of the corpora decreased significantly by 1 week follow-ing castration to 20% of control activity and remained low throughout the 4-week study.

Citrate synthase activity

Figure2 presents the effect of castration on citrate synthase activity. The citrate synthase activity of the bladder body and base, muscle and mucosa decreased over the first week following castration, remained low at 2 weeks and then returned toward control values by 4 weeks following castration. The citrate synthase activities of the urethra and corpora progressively decreased over the course of the 4 weeks study such that at 4 weeks following castration the activity of the urethra was approximately 1/3 of the control values

and the activity of the corpora fell below detectable levels.

Choline acetyl-transferase activity

The effect of castration on ChAT activity is presented in Fig.3. Castration had no significant effect on the ChAT activity of the bladder body, whereas the activities of the base and urethra were significantly reduced at both 2 and 4 weeks following castration. Surprisingly, the activity of the corpora increased at 1 and 2 weeks following castration and returned to control values by 4 weeks after castration.

Discussion

The basic function of bladder is to store urine in a low intravesical pressure and efficiently expel the urine

Fig. 1 Effect of castration on calcium ATP’ase (SERCA) Each bar is the mean ± SEM of four individual animals. * = signif-icantly different from muscle; x = signifsignif-icantly different from control, P < 0.05

Fig. 2 Effect of castration on citrate synthase. Each bar is the mean ± SEM of four individual animals. * = significantly differ-ent from muscle; x = significantly differdiffer-ent from control, P < 0.05

after the bladder is full. Lower urinary tract symptoms (LUTS), including frequency, urgency, and nocturia are major problems for the aging male population. It has been estimated that approximately 30% of men aged over 50 have mild to severe micturition problems. Bladder dysfunction, including smooth muscle hyper-plasia and contractile dysfunction in aging male was considered as a consequence of BPH. However, in aging men, the testosterone levels also declines as a result of both decrease in Leydig cell mass and alter-ation of the hypothalamic -pituitary-gonadal axis [8]. Secretion of the testosterone is regulated by a precise positive and negative biofeedback interaction in the hypothalamic-pituitary-gonadal axis. In addition, the testosterone can be converted to other hormones by several enzymes, to dihydrotestosterone (DHT) by 5a-reductase and to estrogen by aromatase. The action of the testosterone is mediated by the androgen receptor located in the cellular nucleus [9]. Comparing with the female menopause, the decline in testosterone in aging male occurs gradually and had few acute clinical manifestations. However, long-term androgen defi-ciency (as may occur during the treatment of andro-gen-sensitive prostate cancer) are characterized by decreased muscle mass and strength, increase fat mass, impaired cognitive function, and osteoporosis [10,11]. Despite androgens’ effect on central and peripheral nervous system which are well-known, the local effect of androgen on bladder and urethra has not been extensively studied [12–15]. Morita et al. reported that a1-adrenergic and muscarinic cholinergic receptor densities decreased significantly after castration and were not affected by estrogen administration [16].

b-Adrenergic receptors were not affected either by castration or estrogen administration [16].

The indicator of cholinergic innervation, choline acetyl-transferase activity, significantly decreased in bladder base and urethra after 2 weeks of castration. This finding can concur with the previous observation that a decrease in extracts of hypogastric ganglion ta-ken from castrated rats [12] and indicating the impor-tance of testosterone in maintaining cholinergic nerve function. A change in the cholinergic to adrenergic nerve ratio in the bladder base and urethra would be expected to enhance bladder emptying during mictu-rition, in that during cholinergic stimulation which is what generates tension in the bladder during micturi-tion would have a relatively lower contractile effect on the bladder base and urethra, thus reducing urethral resistance during micturition.

The choline acetyl-transferase activity in corpora increased after 1 week of castration and progressively returned to control level after 4 weeks. Testosterone enhances the erectile response of cavernous nerve stimulation. The sites of action for testosterone or its metabolites are situated on neurons rather than on penile erectile tissue. Postganglionic parasympathetic neurons seem to be the exact target for androgen ste-roids [17]. However, the exact cause of this phenome-non is still unclear and may need further experiment to investigate this observation.

Bladder contraction can be divided into phasic and tonic period, the phasic response depends on the adenosine triphosphate (ATP) concentration in the bladder wall, whereas the tonic phase requires mito-chondrial oxidative activity to generate energy [18]. Mitochondria also have a critical role in Ca2+buffering in bladder smooth muscle [19]. There are some evi-dences suggesting that low testosterone level may be associated with insulin resistance and decreased expression of genes involved in oxidative metabolism in mitochondria [20]. Mitochondrial function was evaluated by the mitochondrial marker enzyme citrate synthase. We observed that citrate synthase activity decreased significantly after castration in all of the lower urinary tract, including bladder body, base, urethra, and especially in corpora. However, interest-ingly, the citrate synthase activity of the bladder body and base returned toward control activity by 4 weeks following castration whereas in the urethra and copora, the citrate synthase activity continued to decrease. This would indicate that in regards to micturition, castration would significantly decrease high-energy phosphate generation for the urethra and corpora, which would decrease the ability of the urethra to sustain tension during bladder filling and might be significantly

in-Fig. 3 Effect of castration on choline acetyl transferase. Each bar is the mean ± SEM of four individual animals. * = signif-icantly different from control, P < 0.05

volved in the increased incidence of incontinence in aging men; especially following TURP or other pros-tatic surgery.

Consistant with previous studies, the bladder mu-cosa has a significantly higher activity than the muscle in both bladder body and bladder base. This goes along with the demonstrations that the mucosa has a signifi-cantly higher metabolic rate and high-energy phos-phate turnover than the muscle.

In rat animal studies, DHT treatment will increase micturition frequency and increase the incidence of unstable detrusor contractions [21, 22]. Smooth muscle contractile activity is regulated by intracellular Ca2+ concentration. The sarcoplasmic reticulum Ca2+-ATPase (SERCA), plasma membrane Ca2+ -AT-Pase (PMCA), and plasmalemmal Na+/Ca2+exchanger are responsible for lower intracellular Ca2+, which lead to smooth muscle relaxation [23]. By thapsigargin -sensitive Ca2+ATPase enzyme activity assays, we determined the SERCA activity in urinary bladder, urethra, and corpus cavernosum after castration.

Interestingly, the mucosa of the bladder body has a significantly higher SERCA activity than the muscle compartment, whereas in the bladder base, the activi-ties of the mucosa and muscle are approximately equal, and equal to the mucosa activity of the body. The SERCA activity of the urethral smooth muscle is approximately equal to the activity of the muscle of the bladder base. This may be related to the fact that during bladder filling (representing over 90 percent of the micturition cycle), both the urethra and bladder base are under tonic alpha adrenergic stimulation and must maintain active tension, whereas during bladder filling the bladder body is under beta adrenergic stim-ulation and maintains a relaxed state to allow for filling at low intravesical pressures. The activity of the cor-pora was surprisingly high. This may be related to the fact that during erection, the corpora smooth muscle needs to maintain a relaxed state and thus needs to have a well-defined calcium storage capacity, which would be directly related to the high SERCA activity. The SERCA activity in bladder body wall is signif-icantly increased after 2 weeks of castration, indicating that bladder will increase relaxation after castration. This phenomenon also demonstrates that the effect of testosterone in inhibiting smooth muscle contraction is calcium ion dependent. The SERCA activity signifi-cantly decreased after castration in corpus cavernosum, pointing out the importance of testosterone in corporal myocyte relaxation and related to erectile dysfunction after testosterone deficiency.

It is interesting to note that the four tissues studies responded very differently to castration. For the

bladder body, no change was seen in regard to choline acetyl transferase activity. For both citrate synthase and SERCA, whereas the activity fell immediately following castration, the activities returned toward normal by 4 weeks following castration for both mus-cle and mucosa. In regard to the bladder base, choline acetyl-transferase decreased throughout the castration period, whereas for both citrate synthase and SERCA the activities decreased immediately then recovered toward control by 4 weeks following castration. In re-gard to the urethra, the SERCA activity did not change following castration whereas both citrate synthase and choline acetyl-transferase decreased throughout the castration period. For the corpora tissue, the choline acetyl-transferase increased then returned to control activity by 4 weeks; whereas for both SERCA and citrate synthase the activities continually decreased throughout the castration period. One last point, even though the net activities of the bladder body and base muscle and mucosa had different activities, castration had very similar effects on both tissues.

Conclusions

Our data clearly demonstrate that castration (androgen deprivation) has significant short-term effects on three important enzymes involved with lower urinary tract muscle and mucosal function and are consistent with the known effects of testosterone and androgen deprivation on bladder, urethral, and corporal func-tion. Future studies will be directed at looking at the long-term effects of androgen deprivation.

Acknowledgements This material is based in part upon work supported by the Office of Research and Development, Department of Veterans Affairs and NIH grant RO-1-DK067114. Bulent Onal was supported in part by The Scientific & Technological Research Council of Turkey (TUBITAK).

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