中国男科学杂志
中國男科學雜誌
중국남과학잡지
CHINESE JOURNAL OF ANDROLOGY
2014年
6期
16-20
,共5页
沈寒坚%朱广友%沈彦%王飞翔%翁少峥
瀋寒堅%硃廣友%瀋彥%王飛翔%翁少崢
침한견%주엄우%침언%왕비상%옹소쟁
勃起功能障碍%氧化性应激%NADPH氧化酶
勃起功能障礙%氧化性應激%NADPH氧化酶
발기공능장애%양화성응격%NADPH양화매
neurogenic erectile dysfunction%oxidative stress%NADPH oxidase
目的:通过海绵体神经损伤建立神经性勃起功能障碍大鼠,研究其阴茎海绵体组织内氧化应激状态,及其对于大鼠阴茎勃起功能的影响。方法取成年雄性SD大鼠60只,随机分为3组:A组为假手术组(Sham组), B组为单侧海绵体神经切断组,C组为双侧海绵体神经切断组。各组大鼠造模手术后8周,进行勃起功能试验后处死,取大鼠阴茎海绵体组织,测定大鼠阴茎海绵体组织中超氧化物歧化酶(SOD)水平、谷胱甘肽过氧化物酶(GSH-PX)及内皮型一氧化氮合酶(eNOS)活力,丙二醛(MDA)、一氧化氮(NO)含量,以及NADPH氧化酶gp91phox和p22phox亚基的mRNA表达情况。结果单侧海绵体神经损伤组和双侧海绵体神经损伤组的阴茎海绵体组织SOD水平、GSH-PX活性低于假手术组。单侧海绵体神经损伤组和双侧海绵体神经损伤组的阴茎海绵体组织MDA含量高于于假手术组。单侧海绵体神经损伤组和双侧海绵体神经损伤组的阴茎海绵体组织NO浓度和eNOS活力均低于假手术组。单侧海绵体神经损伤组和双侧海绵体神经损伤组的阴茎海绵体组织内NADPH氧化酶的gp91phox亚基和p22phox亚基mRNA的相对表达倍数均高于假手术组。结论通过对大鼠阴茎海绵体组织氧化应激相关指标(SOD、GSH-PX、MDA)、血管内皮功能相关指标(NO、eNOS)以及NADPH氧化酶功能亚基mRNA的相对表达倍数的测定,单侧海绵体神经损伤组和双侧海绵体神经损伤组的上述指标与假手术组之间均存在统计学差异,说明大鼠海绵体神经损伤致阴茎勃起功能障碍的过程中,除了本身神经损伤以外,阴茎海绵体组织的氧化应激以及NADPH氧化酶相关的阴茎海绵体血管内皮损伤也是大鼠神经性ED的发生、发展的重要机制之一。
目的:通過海綿體神經損傷建立神經性勃起功能障礙大鼠,研究其陰莖海綿體組織內氧化應激狀態,及其對于大鼠陰莖勃起功能的影響。方法取成年雄性SD大鼠60隻,隨機分為3組:A組為假手術組(Sham組), B組為單側海綿體神經切斷組,C組為雙側海綿體神經切斷組。各組大鼠造模手術後8週,進行勃起功能試驗後處死,取大鼠陰莖海綿體組織,測定大鼠陰莖海綿體組織中超氧化物歧化酶(SOD)水平、穀胱甘肽過氧化物酶(GSH-PX)及內皮型一氧化氮閤酶(eNOS)活力,丙二醛(MDA)、一氧化氮(NO)含量,以及NADPH氧化酶gp91phox和p22phox亞基的mRNA錶達情況。結果單側海綿體神經損傷組和雙側海綿體神經損傷組的陰莖海綿體組織SOD水平、GSH-PX活性低于假手術組。單側海綿體神經損傷組和雙側海綿體神經損傷組的陰莖海綿體組織MDA含量高于于假手術組。單側海綿體神經損傷組和雙側海綿體神經損傷組的陰莖海綿體組織NO濃度和eNOS活力均低于假手術組。單側海綿體神經損傷組和雙側海綿體神經損傷組的陰莖海綿體組織內NADPH氧化酶的gp91phox亞基和p22phox亞基mRNA的相對錶達倍數均高于假手術組。結論通過對大鼠陰莖海綿體組織氧化應激相關指標(SOD、GSH-PX、MDA)、血管內皮功能相關指標(NO、eNOS)以及NADPH氧化酶功能亞基mRNA的相對錶達倍數的測定,單側海綿體神經損傷組和雙側海綿體神經損傷組的上述指標與假手術組之間均存在統計學差異,說明大鼠海綿體神經損傷緻陰莖勃起功能障礙的過程中,除瞭本身神經損傷以外,陰莖海綿體組織的氧化應激以及NADPH氧化酶相關的陰莖海綿體血管內皮損傷也是大鼠神經性ED的髮生、髮展的重要機製之一。
목적:통과해면체신경손상건립신경성발기공능장애대서,연구기음경해면체조직내양화응격상태,급기대우대서음경발기공능적영향。방법취성년웅성SD대서60지,수궤분위3조:A조위가수술조(Sham조), B조위단측해면체신경절단조,C조위쌍측해면체신경절단조。각조대서조모수술후8주,진행발기공능시험후처사,취대서음경해면체조직,측정대서음경해면체조직중초양화물기화매(SOD)수평、곡광감태과양화물매(GSH-PX)급내피형일양화담합매(eNOS)활력,병이철(MDA)、일양화담(NO)함량,이급NADPH양화매gp91phox화p22phox아기적mRNA표체정황。결과단측해면체신경손상조화쌍측해면체신경손상조적음경해면체조직SOD수평、GSH-PX활성저우가수술조。단측해면체신경손상조화쌍측해면체신경손상조적음경해면체조직MDA함량고우우가수술조。단측해면체신경손상조화쌍측해면체신경손상조적음경해면체조직NO농도화eNOS활력균저우가수술조。단측해면체신경손상조화쌍측해면체신경손상조적음경해면체조직내NADPH양화매적gp91phox아기화p22phox아기mRNA적상대표체배수균고우가수술조。결론통과대대서음경해면체조직양화응격상관지표(SOD、GSH-PX、MDA)、혈관내피공능상관지표(NO、eNOS)이급NADPH양화매공능아기mRNA적상대표체배수적측정,단측해면체신경손상조화쌍측해면체신경손상조적상술지표여가수술조지간균존재통계학차이,설명대서해면체신경손상치음경발기공능장애적과정중,제료본신신경손상이외,음경해면체조직적양화응격이급NADPH양화매상관적음경해면체혈관내피손상야시대서신경성ED적발생、발전적중요궤제지일。
Objective To investigate oxidative stress status in corpus cavernosum tissue of neurogenic erectile dysfunction rats. Methods Total of 60 male SD rats were divided them into three groupsincluding Group A (sham operated group); Group B(ratswith one side of Cavernous nerve transection; Group C( rats both sides of Cavernous nerve transection). At the 8th weeks after surgery, rats received erectile function test and then were executed. Corpus cavernosum tissues of rats were collected. The levels of Superoxide Dismutase (SOD), Malondialdehyde (MDA), Nitric Oxide (NO), vitality of Glutathione Peroxidase (GSH-PX) and Endothelial Nitric Oxide Synthase (eNOS), and expression of NADPH oxidase subunits gp91phox and p22phox in corpus cavernosum tisues were measured. Results SOD level and vitality of GSH-PX in Group B and C were lower, than those in Group Awhereas level of MDA was higher. Also, the level of NO and vitality of eNOS in Group B and C were lower than those in Group A, but expressions of NADPH oxidase subunits gp91phox and p22phox were increased as compared with those of shamed operated group. Conclusion Theses results suggest that apart from nerve injury, oxidative stress of corpus cavernosum tissue and NADPH oxidase related Corpus cavernosum endothelial damage may also be major triggers for neurogenic erectile dysfunction of rats.