天津医药
天津醫藥
천진의약
TIANJIN MEDICAL JOURNAL
2013年
12期
1191-1194
,共4页
靳春杰%周伟%江荣才%张士俊%杨大伟%张建宁
靳春傑%週偉%江榮纔%張士俊%楊大偉%張建寧
근춘걸%주위%강영재%장사준%양대위%장건저
脑损伤%神经元特异性烯醇化酶%辛伐他汀%大鼠,Sprague-Dawley
腦損傷%神經元特異性烯醇化酶%辛伐他汀%大鼠,Sprague-Dawley
뇌손상%신경원특이성희순화매%신벌타정%대서,Sprague-Dawley
brain injuries%neurone-specific enolase%simvastatin%rats,Sprague-Dawley
目的:通过观察辛伐他汀对创伤性脑损伤(TBI)大鼠神经元特异性烯醇化酶(NSE)在脑组织和血清中表达的影响,探讨辛伐他汀对大鼠TBI的治疗作用。方法8周龄的SD大鼠90只,随机分为假致伤组、对照组、治疗组,每组30只。对照组、治疗组参照改良的Feeney氏自由落体法制造TBI模型。治疗组大鼠于造模前晚及伤后每晚给予辛伐他汀10 mg/kg灌胃;对照组及假致伤组同时给予等量淀粉灌胃。3组大鼠分别于伤后3 h、12 h、24 h、3 d、7 d、14 d取5只大鼠的颈总动脉血3 mL,ELISA法测定NSE浓度;断头取脑,免疫组化法检测伤侧海马CA3区NSE表达。结果(1)ELISA法测定:对照组,伤后3 h血清NSE即开始升高,24 h至3 d达高峰,14 d仍高于假致伤和治疗组;治疗组,伤后3 h血清NSE水平升高,24 h达高峰,3 d至7 d下降,明显低于对照组,伤后14 d接近假致伤组。(2)免疫组化检测:对照组伤后3 h伤侧海马CA3区NSE光密度值下降,3 d至7 d达低谷,14 d时仍显著低于假致伤组;治疗组的大鼠伤后3 h伤侧海马CA3区NSE光密度值下降,12 h至24 h达低谷,但明显高于对照组,7 d开始回升,14 d时接近假致伤组水平。结论辛伐他汀可促进TBI后血清NSE水平的下降,提高损伤侧海马神经元的NSE表达,对TBI后大鼠损伤的神经元有保护作用。
目的:通過觀察辛伐他汀對創傷性腦損傷(TBI)大鼠神經元特異性烯醇化酶(NSE)在腦組織和血清中錶達的影響,探討辛伐他汀對大鼠TBI的治療作用。方法8週齡的SD大鼠90隻,隨機分為假緻傷組、對照組、治療組,每組30隻。對照組、治療組參照改良的Feeney氏自由落體法製造TBI模型。治療組大鼠于造模前晚及傷後每晚給予辛伐他汀10 mg/kg灌胃;對照組及假緻傷組同時給予等量澱粉灌胃。3組大鼠分彆于傷後3 h、12 h、24 h、3 d、7 d、14 d取5隻大鼠的頸總動脈血3 mL,ELISA法測定NSE濃度;斷頭取腦,免疫組化法檢測傷側海馬CA3區NSE錶達。結果(1)ELISA法測定:對照組,傷後3 h血清NSE即開始升高,24 h至3 d達高峰,14 d仍高于假緻傷和治療組;治療組,傷後3 h血清NSE水平升高,24 h達高峰,3 d至7 d下降,明顯低于對照組,傷後14 d接近假緻傷組。(2)免疫組化檢測:對照組傷後3 h傷側海馬CA3區NSE光密度值下降,3 d至7 d達低穀,14 d時仍顯著低于假緻傷組;治療組的大鼠傷後3 h傷側海馬CA3區NSE光密度值下降,12 h至24 h達低穀,但明顯高于對照組,7 d開始迴升,14 d時接近假緻傷組水平。結論辛伐他汀可促進TBI後血清NSE水平的下降,提高損傷側海馬神經元的NSE錶達,對TBI後大鼠損傷的神經元有保護作用。
목적:통과관찰신벌타정대창상성뇌손상(TBI)대서신경원특이성희순화매(NSE)재뇌조직화혈청중표체적영향,탐토신벌타정대대서TBI적치료작용。방법8주령적SD대서90지,수궤분위가치상조、대조조、치료조,매조30지。대조조、치료조삼조개량적Feeney씨자유락체법제조TBI모형。치료조대서우조모전만급상후매만급여신벌타정10 mg/kg관위;대조조급가치상조동시급여등량정분관위。3조대서분별우상후3 h、12 h、24 h、3 d、7 d、14 d취5지대서적경총동맥혈3 mL,ELISA법측정NSE농도;단두취뇌,면역조화법검측상측해마CA3구NSE표체。결과(1)ELISA법측정:대조조,상후3 h혈청NSE즉개시승고,24 h지3 d체고봉,14 d잉고우가치상화치료조;치료조,상후3 h혈청NSE수평승고,24 h체고봉,3 d지7 d하강,명현저우대조조,상후14 d접근가치상조。(2)면역조화검측:대조조상후3 h상측해마CA3구NSE광밀도치하강,3 d지7 d체저곡,14 d시잉현저저우가치상조;치료조적대서상후3 h상측해마CA3구NSE광밀도치하강,12 h지24 h체저곡,단명현고우대조조,7 d개시회승,14 d시접근가치상조수평。결론신벌타정가촉진TBI후혈청NSE수평적하강,제고손상측해마신경원적NSE표체,대TBI후대서손상적신경원유보호작용。
Objective To study the effect of simvastatin (SIM) on the expression of neuron specific enoalse (NSE) in rat brain and serum after traumatic brain injury (TBI), and therapeutic effects of SIM on TBI thereof. Methods A total of 90 Sprague-Dwalye (SD) rats aged 8 weeks were randomly divided into sham TBI group, control group and treatment group (n=30). The TBI model was established in control group and treatment group by using Feeney method. Rats in treatment group were fed SIM 10 mg/kg in the evening pre-injury and in every evening post-injury while those in control group were fed the same dose of starch at the same time. Blood samples (3 mL) were collected from carotid atrery in three groups, then rats were sacrificed and brains were collected at different time points (3 h, 12 h, 24 h, 3 d, 7 d and 14 d post-injury). The serum ex-pressions of NSE were detected by ELISA method. The NSE expressions in hippocampal area CA3 were detected with immu-nohistochemistry. Results (1) In control group, the serum NSE level was significantly increased at 3 h after injury, reached the peak at 3 d, and was still higher than that of sham injury group at 14 d. In treatment group, the serum NSE level was in-creased 3 h after injury, reached the peak at 24 h, decreased after 3 d, and was near the sham injury group at 14 d after inju-ry, but was significantly lower than that of control group. (2) Immunohistochemical detection showed that the NSE optical density values in hippocampal area CA3 area were decreased at 3 h after injury in control group. The optical density values reached the lowest level between 3 d to 7 d and were still significantly lower than those of sham injury group at 14 d. In treat-ment group the optical density value was decreased at 3 h after injury, reached the lowest level between 12 h to 24 h and re-bounded significantly at 7 d, then at 14 d up to the level of sham injury group. Conclusion SIM can promote the decrease of serum NSE level in TBI rats and increase the NSE expression of hippocampal neurons of injured side, showing protective effects on neuronal damage after traumatic brain injury.