A Mouse Model of Cavernous Nerve Injury-Induced Erectile Dysfunction: Functional and Morphological Characterization of the Corpus Cavernosum |
| |
| Authors: | Hai-Rong Jin Yeun Goo Chung Woo Jean Kim Lu Wei Zhang Shuguang Piao Buyankhuu Tuvshintur Guo Nan Yin Sun Hwa Shin Munkhbayar Tumurbaatar Jee-Young Han Ji-Kan Ryu Jun-Kyu Suh |
| |
| Affiliation: | 2. Department of Pathology, Inha University School of Medicine, Incheon, Korea;1. Department of Sexual Medicine, Yijishan Hospital, Wannan Medical College, Wuhu, China;2. Department of Urology, Seoul National University Hospital, College of Medicine, University of Seoul, Seoul, South Korea;3. Department of Urology, College of Medicine, Dongguk University, Goyang, South Korea |
| |
| Abstract: | IntroductionWith the advent of genetically engineered mice, it seems important to develop a mouse model of cavernous nerve injury (CNI).AimTo establish a mouse model of CNI induced either by nerve crushing or by neurectomy and to evaluate time-dependent derangements in penile hemodynamics in vivo and subsequent histologic alterations in the cavernous tissue.MethodsTwelve-week-old C57BL/6J mice were divided into 4 groups (N = 36 per group): control, sham operation, bilateral cavernous nerve crush, and bilateral cavernous neurectomy group.Main Outcome MeasuresThree days and 1, 2, 4, 8, and 12 weeks after CNI, erectile function was measured by electrical stimulation of the cavernous nerve. The penis was then harvested and TUNEL was performed. Immunohistochemical analysis was performed assaying for caspase-3, transforming growth factor-β1 (TGF-β1), phospho-Smad2, PECAM-1, factor VIII, and smooth muscle α-actin. The numbers of apoptotic cells and phospho-Smad2-immunopositive cells in endothelial cells or smooth muscle cells were counted.ResultsErectile function was significantly less in the cavernous nerve crushing and neurectomy groups than in the control or sham group. This difference was observed at the earliest time point assayed (day 3) and persisted up to 4 weeks after nerve crushing and to 12 weeks after neurectomy. The apoptotic index peaked at 1 or 2 weeks after CNI and decreased thereafter. Cavernous TGF-β1 and phospho-Smad expression was also increased after CNI. The numbers of apoptotic cells and phospho-Smad2-immunopositive cells in cavernous endothelial cells and smooth muscle cells were significantly greater in the cavernous nerve crush and cavernous neurectomy groups than in the control or sham group.ConclusionThe mouse is a useful model for studying pathophysiologic mechanisms involved in erectile dysfunction after CNI. Early intervention to prevent apoptosis in smooth muscle cells and endothelial cells or to inhibit cavernous tissue fibrosis is required to restore erectile function. Jin H-R, Chung YG, Kim WJ, Zhang LW, Piao S, Tuvshintur B, Yin GN, Shin SH, Tumurbaatar M, Han J-Y, Ryu J-K, and Suh J-K. A mouse model of cavernous nerve injury-induced erectile dysfunction: Functional and morphological characterization of the corpus cavernosum. |
| |
| Keywords: | |
| 本文献已被 ScienceDirect 等数据库收录! |
|
