中华实验外科杂志
中華實驗外科雜誌
중화실험외과잡지
CHINESE JOURNAL OF EXPERIMENTAL SURGERY
2009年
2期
202-204
,共3页
肠上皮细胞%缺血%肌动蛋白
腸上皮細胞%缺血%肌動蛋白
장상피세포%결혈%기동단백
Intestinal epithelial ceils%Ischemia%F-actin
目的 观察大鼠肠上皮细胞(IEC)缺血缺氧损伤后肌动蛋白及其结合蛋白的变化,探讨其与肠上皮细胞凋亡的关系及钙通道阻断剂对其的影响.方法 建立大鼠IEC分离与原代培养和体外模拟缺血缺氧环境,设立对照组(A组),缺血组(B组),缺氧组(C组),缺血缺氧组(D组)及加用维拉珀米2 mg/L的相应对照组.利用流式细胞仪(FCM)计算凋亡细胞率,激光共聚焦显微镜技术(LSCM)观察肌动蛋白(F-actin)、踝蛋白(talin)和α-辅肌动蛋白(α-actin)的形态及荧光强度的变化.结果 B、C、D组IEC凋亡较A组明显增加(P<0.05);加用钙通道阻断剂后的B1、C1、D1组较相应对照组减少(P<0.05);缺血缺氧损伤导致F-actin、talin和α-actin形态的改变,以D组最显著,同时B、C、D组的荧光强度较A组明显减弱(P<0.01),加用钙通道阻断剂后的B1、C1、D1组F-actin、talin和α-actin形态有所恢复,荧光强度增强,与损伤组比较,差异有统计学意义(P<0.05).结论 缺血缺氧损伤导致的肌动蛋白及其结合蛋白的改变与IEC脱落、凋亡相关;钙通道阻断剂可以减轻这种改变.
目的 觀察大鼠腸上皮細胞(IEC)缺血缺氧損傷後肌動蛋白及其結閤蛋白的變化,探討其與腸上皮細胞凋亡的關繫及鈣通道阻斷劑對其的影響.方法 建立大鼠IEC分離與原代培養和體外模擬缺血缺氧環境,設立對照組(A組),缺血組(B組),缺氧組(C組),缺血缺氧組(D組)及加用維拉珀米2 mg/L的相應對照組.利用流式細胞儀(FCM)計算凋亡細胞率,激光共聚焦顯微鏡技術(LSCM)觀察肌動蛋白(F-actin)、踝蛋白(talin)和α-輔肌動蛋白(α-actin)的形態及熒光彊度的變化.結果 B、C、D組IEC凋亡較A組明顯增加(P<0.05);加用鈣通道阻斷劑後的B1、C1、D1組較相應對照組減少(P<0.05);缺血缺氧損傷導緻F-actin、talin和α-actin形態的改變,以D組最顯著,同時B、C、D組的熒光彊度較A組明顯減弱(P<0.01),加用鈣通道阻斷劑後的B1、C1、D1組F-actin、talin和α-actin形態有所恢複,熒光彊度增彊,與損傷組比較,差異有統計學意義(P<0.05).結論 缺血缺氧損傷導緻的肌動蛋白及其結閤蛋白的改變與IEC脫落、凋亡相關;鈣通道阻斷劑可以減輕這種改變.
목적 관찰대서장상피세포(IEC)결혈결양손상후기동단백급기결합단백적변화,탐토기여장상피세포조망적관계급개통도조단제대기적영향.방법 건립대서IEC분리여원대배양화체외모의결혈결양배경,설립대조조(A조),결혈조(B조),결양조(C조),결혈결양조(D조)급가용유랍박미2 mg/L적상응대조조.이용류식세포의(FCM)계산조망세포솔,격광공취초현미경기술(LSCM)관찰기동단백(F-actin)、과단백(talin)화α-보기동단백(α-actin)적형태급형광강도적변화.결과 B、C、D조IEC조망교A조명현증가(P<0.05);가용개통도조단제후적B1、C1、D1조교상응대조조감소(P<0.05);결혈결양손상도치F-actin、talin화α-actin형태적개변,이D조최현저,동시B、C、D조적형광강도교A조명현감약(P<0.01),가용개통도조단제후적B1、C1、D1조F-actin、talin화α-actin형태유소회복,형광강도증강,여손상조비교,차이유통계학의의(P<0.05).결론 결혈결양손상도치적기동단백급기결합단백적개변여IEC탈락、조망상관;개통도조단제가이감경저충개변.
Objective To investigate the relationship between the apoptosis and the change of F-actin and actin binding protein in intstinal epithelial cells (IEC) under the ischemia and anoxia injury, and the effect of calcium channel antagonist. Methods Primary culture of rat IECs and ischemia and an-oxia injury model in vitro were established. IECs were divided into 8 groups : group A ( control group), group B (ischemia group) ,group C (anoxia group) ,group D (ischemia and anoxia group) ,group A1 ( A +2 mg/L Verapamil) ,group B1 (B +2 mg/L Verapamil) ,group C1 (C +2 mg/L Verapamil) ,group D1 ( D + 2 mg/L Verapamil). Apoptosis rate (AR) was determined by flow cytometry. F-actin, talin and α-ac-tin were observed by LSCM. Results The AR in groups B, C and D was significantly higher than in group A (P < 0.05). The AR in groups B1, C1 and D1 was lower than in groups B. C and D ( P < 0.05 ). The form and arragement of F-actin, talin and α-actin in groups B, C and D were changed with the decrease of fluorescence intensity compared with group A (P < 0.01 ), the most significant in group D. The change in groups B1, C1 and D1 was reduced and the fluorescence intensity was increased as compared with the cor-responding injury groups (P < 0.05). Conclusion The ischemia and anoxia injury results in the break-down of F-actin and actin binding protein, which is related to the apotosis of IEC. Calcium channel antago-nist can decrease AR and reduce the change of these cytoskeleton.
