中华麻醉学杂志
中華痳醉學雜誌
중화마취학잡지
CHINESE JOURNAL OF ANESTHESIOLOGY
2012年
7期
870-873
,共4页
孙美艳%赵晓勇%吕海港%任鹏程%高昌俊%柴伟%孙绪德
孫美豔%趙曉勇%呂海港%任鵬程%高昌俊%柴偉%孫緒德
손미염%조효용%려해항%임붕정%고창준%시위%손서덕
异氟醚%再灌注损伤%脑损伤%TLR4-MyD88信号通路
異氟醚%再灌註損傷%腦損傷%TLR4-MyD88信號通路
이불미%재관주손상%뇌손상%TLR4-MyD88신호통로
Isoflurane%Reperfusion injury%Brain injuries%TLR4-MyD88 signaling pathway
目的 探讨异氟醚预处理对局灶性脑缺血再灌注损伤大鼠缺血半暗带TLR4-MyD88信号通路的影响.方法 成年雄性SD大鼠54只,体重250 ~ 280 g,采用随机数字表法,将其随机分为3组(n=18):假手术组(S组)、脑缺血再灌注组(I/R组)和异氟醚预处理组(IP组).S组仅分离血管不留置线栓;I/R组采用线栓法制备右侧局灶性脑缺血再灌注损伤模型,缺血2h,再灌注24 h;IP组吸入2.0%异氟醚2h,预处理结束后24h时制备右侧局灶性脑缺血再灌注损伤模型.于再灌注24 h时行神经功能缺陷评分,随后处死大鼠,每组随机抽取5只大鼠,取脑组织,测定脑梗死体积,采用Westernblot法和RT-PCR法检测大鼠右侧脑缺血半暗带区HSP60、TLR4、MyD88蛋白及mRNA的表达情况;每组剩余的3只大鼠,采用TUNEL法检测大鼠右侧脑缺血半暗带区细胞凋亡情况.结果 与S组比较,I/R组和IP组神经功能缺陷评分升高,脑梗死体积增大,右侧脑缺血半暗带区凋亡指数升高,HSP60、TLR4、MyD88蛋白及mRNA表达均上调(P<0.05);与I/R组比较,IP组神经功能缺陷评分降低,脑梗死体积减小,右侧脑缺血半暗带区凋亡指数降低,HSP60、TLR4、MyD88蛋白及mRNA表达均下调(P<0.05).结论 异氟醚预处理可保护脑缺血再灌注大鼠缺血半暗带,其机制可能与抑制大鼠脑缺血半暗带TLR4-MyD88信号通路有关.
目的 探討異氟醚預處理對跼竈性腦缺血再灌註損傷大鼠缺血半暗帶TLR4-MyD88信號通路的影響.方法 成年雄性SD大鼠54隻,體重250 ~ 280 g,採用隨機數字錶法,將其隨機分為3組(n=18):假手術組(S組)、腦缺血再灌註組(I/R組)和異氟醚預處理組(IP組).S組僅分離血管不留置線栓;I/R組採用線栓法製備右側跼竈性腦缺血再灌註損傷模型,缺血2h,再灌註24 h;IP組吸入2.0%異氟醚2h,預處理結束後24h時製備右側跼竈性腦缺血再灌註損傷模型.于再灌註24 h時行神經功能缺陷評分,隨後處死大鼠,每組隨機抽取5隻大鼠,取腦組織,測定腦梗死體積,採用Westernblot法和RT-PCR法檢測大鼠右側腦缺血半暗帶區HSP60、TLR4、MyD88蛋白及mRNA的錶達情況;每組剩餘的3隻大鼠,採用TUNEL法檢測大鼠右側腦缺血半暗帶區細胞凋亡情況.結果 與S組比較,I/R組和IP組神經功能缺陷評分升高,腦梗死體積增大,右側腦缺血半暗帶區凋亡指數升高,HSP60、TLR4、MyD88蛋白及mRNA錶達均上調(P<0.05);與I/R組比較,IP組神經功能缺陷評分降低,腦梗死體積減小,右側腦缺血半暗帶區凋亡指數降低,HSP60、TLR4、MyD88蛋白及mRNA錶達均下調(P<0.05).結論 異氟醚預處理可保護腦缺血再灌註大鼠缺血半暗帶,其機製可能與抑製大鼠腦缺血半暗帶TLR4-MyD88信號通路有關.
목적 탐토이불미예처리대국조성뇌결혈재관주손상대서결혈반암대TLR4-MyD88신호통로적영향.방법 성년웅성SD대서54지,체중250 ~ 280 g,채용수궤수자표법,장기수궤분위3조(n=18):가수술조(S조)、뇌결혈재관주조(I/R조)화이불미예처리조(IP조).S조부분리혈관불류치선전;I/R조채용선전법제비우측국조성뇌결혈재관주손상모형,결혈2h,재관주24 h;IP조흡입2.0%이불미2h,예처리결속후24h시제비우측국조성뇌결혈재관주손상모형.우재관주24 h시행신경공능결함평분,수후처사대서,매조수궤추취5지대서,취뇌조직,측정뇌경사체적,채용Westernblot법화RT-PCR법검측대서우측뇌결혈반암대구HSP60、TLR4、MyD88단백급mRNA적표체정황;매조잉여적3지대서,채용TUNEL법검측대서우측뇌결혈반암대구세포조망정황.결과 여S조비교,I/R조화IP조신경공능결함평분승고,뇌경사체적증대,우측뇌결혈반암대구조망지수승고,HSP60、TLR4、MyD88단백급mRNA표체균상조(P<0.05);여I/R조비교,IP조신경공능결함평분강저,뇌경사체적감소,우측뇌결혈반암대구조망지수강저,HSP60、TLR4、MyD88단백급mRNA표체균하조(P<0.05).결론 이불미예처리가보호뇌결혈재관주대서결혈반암대,기궤제가능여억제대서뇌결혈반암대TLR4-MyD88신호통로유관.
Objective To investigate the effect of isoflurane preconditioning on Toll-like receptor 4 (TLR4)-myeloid differentiation factor 88 (MyD88) signaling pathway in ischemic penumbra following focal cerebral ischemia-reperfusion (I/R) in rats.Methods Fifty-four healthy male SD rats,aged 3 months,weighing 250-280 g,were randomly divided into 3 groups (n =18 each):sham operation group (group S),I/R group and isoflurane preconditioning group (group IP).Focal cerebral I/R was induced by middle cerebral artery occlusion.In groups I/R and IP,a nylon thread with rounded tip was inserted into the right internal jugular vein and threaded cranially until resistance was met.The middle cerebral artery was occluded for 2 h,followed by 24 h reperfusion.In group IP,the animals inhaled 2.0% isoflurane for 2 h,and middle cerebral artery occlusion was performed at 24 h after the end of preconditioning.Neurological deficit was scored at 24 h of reperfusion and then the rats were sacrificed.Five rats in each group were chosen and the brains removed for measurement of the cerebral infarct volume.The right cerebral ischemic penumbra was removed for detection of the expression of HSP60,TLR4,MyD88 protein and mRNA by Western blot analysis and real time-PCR.Apoptosis was detected in the ischemic penumbra in the left 3 rats in each group using TUNEL.Apoptosis index (AI) was calculated.Results Neurological deficit scores and AI were significantly increased,the cerebral infarct volume was significantly enlarged,and the expression of HSP60,TLR4,MyD88 protein and mRNA was up-regulated in groups I/R and IP as compared with group S ( P < 0.05).Isoflurane preconditioning significantly reduced the cerebral infarct volume and decreased neurological deficit scores and AI,and down-regulated the expression of HSP60,TLR4,MyD88 protein and mRNA (P < 0.05).Conclusion The mechanisn by which isoflurane preconditioning protects ischenic penumbra following focal cerebral I/R may be related to inhibition of TLR4-MyD88 signaling pathway.