Histologic and functional outcomes of small intestine submucosa-regenerated bladder tissue

All of the animals underwent urodynamic testing under anesthesia with 2% Phenobarbital (30 mg/kg) before cystoplasty. Cystometrograms (CMGs) were carried out with a 5 F double-lumen urodynamic catheter placed through the urethra and a continuous infusion (10 ml/min) of sterile saline via the catheter. The saline infusion was stopped at the first sign of overflow incontinence. Then the CMGs were repeated twice, the averaged maximal capacity was recorded. Bladder compliance was calculated as the change in volume divided by the change in pressure. The CMGs were repeated 4, 12, and 24 weeks after surgery with the same method. Data are expressed as the mean ± standard error of the mean.

The entire bladder was removed post-operatively after CMGs at 4, 12, and 24 weeks and placed in Krebs solution continually bubbled with 95% O₂ and 5% CO₂. This solution contained the following compounds in g/L: NaCl, 6.92; KCl, 0.35; KH₂PO₄, 0.16; MgSO₄.7H₂O, 0.29; NaHCO₃, 2.1; CaCl₂, 0.35; and glucose, 2.0. SIS-regenerated bladder strips (10 × 3 × 3 mm) and normal bladder strips (10 × 3 × 3 mm) from the same bladder were obtained. Silk ligatures were used to mount the strips vertically between two suspension clasps in organ bath chambers. The tissue was continually immersed in Krebs solution at 37°C. Tension on the strips was measured using a force-displacement transducer. Tension (1 g) was applied to the strips. The frequency and amplitude of the strip over 15 min was recorded. Data are expressed as the mean ± standard error of the mean.

As controls for each rabbit, a full thickness bladder fragment was excised distal from the grafted area. Formalin-fixed specimens from the grafted and normal areas of the bladder were embedded in paraffin. Five μm sections were cut and stained with hematoxylin and eosin (HE). A-actin (BIOSS Inc., Massachusetts, USA) was also used for immunohistochemical evaluation of smooth muscle regeneration. The main steps of immunohistochemistry methods:(1) Put the slide with paraffin section in drying oven 2 hours, 60°C. (2) Put it in xylene 15 min, 3 times. (3) Then in ethanol, from 100% to 95%, then 90%, 80%, 70%, each 5 min. (4) Wash with water one time, 5 min, then transform into PBS (0.01 M, pH 7.4), wash 5 min, 3 times. (5) Antigen retrieval: put the slide into citrate buffer (0.01 M, pH 6.0), keep the solution in boiling water for 10-15 min, cool down to room temperature (6) Wash with PBS (0.01 M, pH 7.4) 5 min, 3 times (7) Block endogenous peroxidase by 3% H2O2 for 30 min (8) Wash with PBS (0.01 M, pH 7.4) 5 min, 3 times (9) Incubation with blocking buffer (normal goat serum or 3% BSA) at 37°C for 20 min (10) Discarding the goat serum and droping the primary antibody A-actin (BIOSS Inc, USA) with diluted in PBS (0.01 M PBS, pH 7.4,1:100–500), incubating the sections overnight at 4°C (11) Wash with PBS (3X5 min) (12) Add secondary antibody, Goat Anti-rabbit IgG,(BIOSS Inc, USA) incubating the sections for 20 min at 37°C (13) Wash with PBS (3X5 min) (14) Add Avidin/HRP, incubating the sections for 20 min at 37°C (15) Wash with PBS (3X5 min) (16) Colouration with 3,3-diaminobenzidin (DAB), Observe by microscope, stop colouration with the distilled water at the right time (17) Dehydration in ethanol, from 70% to 80%, then 90%, 95%, 100%, each 5 min, then transform into xylene 10 min, 3 times (18) Cover with coverslip by neutral gums. The preparations were observed under a light microscope. For the convenience of analysis, the results were quantified as optical density (OD) values. Using analysis software (Leica Qwin, v2.3; Leica Inc. Solms, Germany) with the same parameters (exposure time, 22 ms; light intensity, 60%), the mean OD of A-actin was measured.

In this study, self-control was approached. Quantitative data were compared using t-tests. All statistical analyses used SPSS 13.0 (SPSS, Inc., Chicago, IL, USA).

All rabbits were euthanized. The outer and inner surfaces of the bladder, perivesical fat, kidneys, and ureters were evaluated macroscopically. The kidneys and ureters were grossly normal without evidence of hydronephrosis. There were no diverticula in any group. There was no extravasation or contractions in the graft regions. The material was degraded in groups B and C, but not degraded on the inner surface in group A. Regenerated tissue covered the outer surface of the region of the graft, which was indistinguishable from the normal host bladder at the outer and inner surfaces in group C (Figure 2b).

Continuation of host transitional epithelium in the region of the SIS graft was observed under light microscopy in all groups. Inflammatory cells infiltrated regenerated epithelium 4 weeks after surgery (group A; Figure 1c), and nearly disappeared 12 weeks post-operatively (group B). Detrusor was formed 12 weeks post-operatively (group B). These layers were indistinguishable from normal bladder 24 weeks post-operatively (group C).

Detrusor was present and well-visualized with A-actin staining. The detrusor component was scarce in group A, while the detrusor fiber was more evident in group B than in group A, but smaller in number and size compared with normal tissue (P = 0.001). There was no significant difference in the OD value of A-actin staining in group C and normal bladder (P = 0.759) (Figure 2).

Pre-operatively, the bladder capacities in groups A, B, and C were 40.30 ± 7.6, 55.7 ± 27.2, and 48.98 ± 27.8 ml, respectively. Post-operatively, the capacities were 26.11 ± 4.8, 60.4 ± 24.7, and 57.80 ± 27.7 ml, respectively. There was a significant decrease in the bladder volume of group A, and no significant difference in group B; however, the bladder volume was significantly increased in group C (24 weeks post-operation; P = 0.001). The bladder compliance of groups A, B, and C pre-operatively was not significantly different post-operation (Table 1).

Regenerated detrusor strips in group A had visible slight vibration waves, the frequency and amplitude of which could not be measured; the group A strips were significantly different from normal detrusor strips. In group B, the frequency (min-1) of regenerated detrusor strips was 2.88 ± 0.49 (min-1) and the amplitude was 0.13 ± 0.014 (g), which was significantly different from normal detrusor strips. The frequency (3.64 ± 0.98) and amplitude (4.35 ± 1.25) of regenerated detrusor strips in group C were not significantly different compared with normal detrusor strips (Table 2).