Fas-L在大鼠脑液压冲击伤后的表达

目的为探讨轻型闭合性颅脑损伤的病理诊断及损伤时间推断依据。方法通过建立大鼠脑液压冲击伤模型,用免疫组化染色方法与图像分析技术分别检测大鼠轻型闭合性颅脑损伤后15,30min,1,3,6,12h,1,4,7,14d以及正常对照组与手术对照组大鼠大脑皮质、丘脑、海马等部位Fas-L的表达。结果发现伤后1hFas-L开始在大脑皮质及海马出现表达,随时间增加表达逐渐增强,伤后3hFas-L表达显著增加,伤后12h达高峰,损伤4d后Fas-L表达逐渐减弱,14d基本恢复正常。本研究证明,Fas-L介导的细胞凋亡不仅出现于脑损伤邻近,在远离损伤部位的脑组织亦有Fas-L介导的细胞凋亡发生。结论Fas-L表达可望为轻型闭合性颅脑损伤早期诊断提供依据;根据Fas-L阳性表达的变化规律可作为脑损伤时间推测的指标之一。

人胚神经干细胞移植对大鼠脑液压冲击伤的影响

目的 通过人胚神经干细胞 (HNSCs)移植大鼠脑液压冲击伤 (FPI)探讨HNSCs对脑损伤修复的影响。方法 体外培养HNSCs并用 5 溴脱氧尿嘧啶 (BrdU)标记 ,液压冲击大鼠右侧大脑皮质运动感觉区制作脑外伤模型 ,脑外伤后 2 4h移植HNSCs ,分别于脑外伤前、脑外伤后 2 4h、4周行神经运动行为学评分 (NMFE)和检测左下肢的短潜伏期体感诱发电位 (SLSEP)及免疫组织化学染色检测BrdU、巢蛋白 (nestin)、微管相关蛋白 2 (MAP2 )、胶质纤维酸性蛋白 (GFAP)和半乳糖脑苷 (GalC)蛋白表达。结果 大鼠液压冲击伤后 2 4h ,左下肢功能障碍明显 ,运动评分14 .3 75 0± 2 .13 3 9,SLSEP潜伏期 3 0 .463± 4.64 0与损伤前相比均差异有显著性 (P <0 .0 1) ,但移植HNSCs组与对照组差异无显著性 ;HNSCs移植后 1周 ,BrdU阳性细胞从移植区域向周围扩散 ,邻片nestin、MAP2和GFAP均为阳性 ,但MAP2阳性细胞较多 ;HNSCs移植后 4周 ,未见nestin阳性细胞 ,液压冲击区域聚集GFAP/BrdU双阳性细胞和MAP2 /BrdU双阳性细胞 ,且GFAP/BrdU阳性细胞较多。结论 HNSCs移植对大鼠脑液压冲击伤的功能恢复无影响 ,但早期HNSCs多数分化为神经细胞 ,晚期多数分化为神经胶质细胞。

大鼠脑液压冲击伤后细胞色素C表达的实验研究

目的 为法医学上闭合性颅脑损伤的早期诊断和损伤时间推断提供依据。 方法 建立大鼠脑液压冲击模型。用免疫组化与图像分析技术分别检测伤后不同时间大鼠脑皮质、海马等部位细胞色素C(CytochromeC ,CytC)的表达。 结果 对照组大鼠脑内CytC有微量表达 ,伤后 15分钟表达开始增强 ,伤后 3小时达高峰 ,1天后开始减弱 ,7天后基本恢复正常。 结论 CytC表达的规律性可望为闭合性颅脑损伤的早期诊断及损伤时间推断提供依据。

大鼠液压冲击脑损伤核因子E2相关因子2-抗氧化反应元件通路的时程表达变化

目的 观察大鼠液压冲击脑损伤核因子E2相关因子2（Nrf2）-抗氧化反应元件（ARE）信号通路及其下游因子血红素氧化酶-1（HO-1） 和磷酸酰胺腺嘌呤二核苷酸醌氧化还原酶-1（NQO-1）时程表达变化.方法 成年雄性SD大鼠56只,制作液压冲击颅脑损伤模型,术后1、6、12、24h、3、7d对大鼠进行神经功能评分,用干湿重法测定脑含水量;Western blot测定胞质、胞核Nrf2蛋白以及HO-1、NQO-1蛋白表达;实时荧光定量聚合酶链反应（FQ-PCR）测定Nrf2-mRNA表达.结果 创伤性脑损伤（TBI）组脑含水量于冲击伤后6h开始增加[（78.98±0.12）%],24h达高峰（82.98±0.62）%],3d开始下降[（82.26±0.72）%],神经功能评分趋势与之相反,24h下降至最低值（2.78±0.66）,差异均有统计学意义（F=98.712、78.806,P=0.000）.Western blot证实TBI组胞核Nrf2于1h开始升高（0.82±0.18）,24h达到高峰（1.87±0.82）,3d时降低（1.42±0.55）,而胞质Nrf2自12h开始持续走低（1.14±0.22）,呈相反趋势,差异均有统计学意义（F=11.566、17.928,P=0.001）.HO-1和NQO-1蛋白表达与胞核Nrf2蛋白趋势一致（F=16.175、12.694,P=0.001）.FQ-PCR结果显示TBI组冲击伤后各时间点Nrf2-mRNA表达水平无明显变化（F=0.802,P=0.968）.结论 大鼠脑液压冲击伤Nrf2-ARE通路激活,可能在创伤性颅脑损伤中发挥抗氧化应激损伤作用.

Changes in and effective factors of microtubule associated protein 2 in traumatic neurons

Objective To investigate alterations in the microtubule-associated protein 2 (MAP-2) of neurons in Wistar rats and the effect of nimodipine (Nim), D-2-amino-5-phosphonovaleric acid (D-AP-5) and mild hypothermia on neuronal MAP-2 following fluid percussion injury (FPI).Methods Alterations of MAP-2 in Wistar rat neurons following FPI were measured by a confocal laserscanning microscope using MAP-2 immunofluorescence staining as a MAP-2 indicator.Results MAP-2 immunofluorescence staining was limited to the cell bodies and dendritic compartments of neurons and more intense in dendrites than in cell bodies. The loss of MAP-2 was marked at 3 h posttrauma ( P ＜ 0.01 ), and reached a maximum at 48 h post-trauma. Afterwards, fluorescence recovered partly at 72 h post-trauma. The application of Nim markedly reduced the loss of MAP-2 immunoreectivity within 1 h post-trauma ( P ＜ 0.01 ), and the application of D-AP-5 markedly reduced the loss of MAP-2immunoreactivity within 10 h post-injury ( P ＜ 0.01 ). The application of mild hypothermia decreased the loss of MAP-2 immunoreactivity within 1 h post-injury (P＜ 0.05).Conclusions The partial recovery of fluorescence at 72 h post-trauma indicate that the partial structure of the neuronal microtubules can be repaired by itself. Nim, D-AP-5 and mild hypothermia reduce the degradation of MAP-2 by different mechanisms. The treatment of neuronal cytoskeleton degradation following FPI must employ multiple therapeutic approaches.

Spatial and temporal profile of apoptosis following lateral fluid percussion brain injury

Objective: To investigate the spatial and temporal profile of neural cell apoptosis following traumatic brain injury (TBI). Methods: In addition to morphological evidence of apoptosis, TUNEL histochemistry assay was used to identify DNA fragmentation in situ at both light and electron microscopic levels, whereas characteristic internucleosomal DNA fragmentation of apoptosis was demonstrated by DNA gel electrophoresis. Results: Using TUNEL method, we detected massive cells with extensive DNA fragmentation in different regions of the brains of rats subjected to experimental traumatic brain injury. Compared with the sham controls, in the injured cortex, the apoptotic cells were detectable for up to 24 h and reached a peak at 1 week after injury. The number of apoptotic cells in the white matter had a significant increase as early as 12 h after injury and peaked at 1 week. The number of apoptotic cells increased in the hippocampus at 72 h, whereas in the thalamus, the peak of apoptotic cells was at 2 weeks after injury. The number of apoptotic cells in most regions returned to sham values 2 months after injury. Gel electrophoresis of DNA extracted from affected areas of the injured brain revealed only internucleosomal fragmentation at 185-bp intervals, a feature originally described in apoptotic cell death. And no DNA ladder was detectable in the cortex and hippocampus contralateral to the injured hemisphere.Conclusions: These data suggest that in addition to the well described necrotic cell death, a temporal course of apoptotic cell death is initiated after brain trauma in selected brain regions.