Mechanisms of Inhibitory Effects of Breviscapine on Lipid Peroxidation in Rat Brain Mitochondria

The mechanisms by which breviscapine (Bre) inhibits the lipid preoxidation in rat brain mitochondria were investigated. The mitochondrial lipid peroxidation of rat brain induced by oxygen free radical was measured by thiobarbituric acid spectrophotometry. The chelating activities of Bre for Fe 2+ were tested by differential spectrum. Superoxide anion (O 2)from xanthine xanthine oxidase (Xan XO) system and hydroxyl radical (·OH) from FeSO 4 H 2O 2 system were determined with spectrophotometry. It was found that Bre could effectively inhibit the lipid peroxidation of brain mitochondria induced by free radicals driven from Xan XO and FeSO 4 H 2O 2 system. The IC 50 of Bre were 93 01 μmol·L -1 for Xan XO system and 62 18 μmol·L -1 for FeSO 4 H 2O 2 system. Bre also scavenged O 2 and ·OH produced by Xan XO and FeSO 4 H 2O 2 systems. The IC 50 of Bre were 32 63 μmol·L -1 for O - 2 and 20 22 μmol·L -1 for ·OH. Furthermore, the chelating Fe 2+ activity of Bre was shown. It may be concluded that Bre inhibited lipid peroxidation at different stages of the reaction of oxygen free redial with the mitochondria membrane: (1) the formation of ·OH; (2) the initiation of the lipid peroxidation, by chelating Fe 2+ and scavenging O 2 as well as ·OH. The scavenging oxygen free radicals and chelating iron are the mechanisms of inhibitory effect of Bre on lipid peroxidation.

Alterations in enterocyte mitochondrial respiratory function and enzyme activities in gastrointestinal dysfunction following brain injury

AIM: To determine the alterations in rat enterocyte mitochondrial respiratory function and enzyme activities following traumatic brain injury (TBI).

Telomerase and mTOR in the brain:the mitochondria connection

Telomerase is an enzyme that maintains telomeres in dividing cells using a template on its inherent RNA component.Additionally,the protein part TERT（Telomerase Reverse Transcriptase） has various non-canonical functions.For example,it can localize to mitochondria under increased stress and protect cells in vitro from oxidative stress,DNA damage and apoptosis.Recently it has been demonstrated that TERT protein persists in adult neurons in the brain and data emerge suggesting that it might have a protective function in these post-mitotic cells as well.We have recently published that TERT protein accumulated in mitochondria from brain tissue of mice that have undergone short-term dietary restriction（DR） and rapamycin treatment.This localization correlated to lower levels of oxidative stress in these brain mitochondria.Since rapamycin treatment decreases mTOR signaling which is also thought to play an important role for the beneficial effects of DR,we conclude that the mTOR pathway might be involved in the TERT localization and its effects in brain mitochondria in vivo.These data are in line with previous findings from our group about increased mitochondrial localization of TERT in Alzheimer＇s disease（AD） brains and a protective function of TERT protein in neurons in vitro against pathological tau.

Stimulating mitochondria to protect the brain following traumatic brain injury

Traumatic brain injury （TBI） is an acquired injury to the brain that occurs with sudden trauma that can range from mild （concussive） to severe. TBI is considered a leading cause of death in children and young adults, with the Centers for Disease Control and Prevention estimating that approximately 1.7 million cases of TBI occur in the United States annually （Faul et al., 2010）. Further, since the begin- ning of the global war on terrorism, the Department of Defense has reported over 344,000 U.S. Service Members have been diagnosed with traumatic brain injury from penetrating injuries to mild forms of TBI. TBI, caused by a sudden impact, penetration, or rapid move- ment of the brain, interrupts the normal functioning of the brain. While the intracranial location and severity of injury contribute to the extent of functional deficits.

Polydatin prevents the induction of secondary brain injury after traumatic brain injury by protecting neuronal mitochondria

Polydatin is thought to protect mitochondria in different cell types in various diseases.Mitochondrial dysfunction is a major contributing factor in secondary brain injury resulting from traumatic brain injury.To investigate the protective effect of polydatin after traumatic brain injury,a rat brain injury model of lateral fluid percussion was established to mimic traumatic brain injury insults.Rat models were intraperitoneally injected with polydatin(30 mg/kg)or the SIRT1 activator SRT1720(20 mg/kg,as a positive control to polydatin).At 6 hours post-traumatic brain injury insults,western blot assay was used to detect the expression of SIRT1,endoplasmic reticulum stress related proteins and p38 phosphorylation in cerebral cortex on the injured side.Flow cytometry was used to analyze neuronal mitochondrial superoxide,mitochondrial membrane potential and mitochondrial permeability transition pore opened.Ultrastructural damage in neuronal mitochondria was measured by transmission electron microscopy.Our results showed that after treatment with polydatin,release of reactive oxygen species in neuronal mitochondria was markedly reduced;swelling of mitochondria was alleviated;mitochondrial membrane potential was maintained;mitochondrial permeability transition pore opened.Also endoplasmic reticulum stress related proteins were inhibited,including the activation of p-PERK,spliced XBP-1 and cleaved ATF6.SIRT1 expression and activity were increased;p38 phosphorylation and cleaved caspase-9/3 activation were inhibited.Neurological scores of treated rats were increased and the mortality was reduced compared with the rats only subjected to traumatic brain injury.These results indicated that polydatin protectrd rats from the consequences of traumatic brain injury and exerted a protective effect on neuronal mitochondria.The mechanisms may be linked to increased SIRT1 expression and activity,which inhibits the p38 phosphorylation-mediated mitochondrial apoptotic pathway.This study was approved by the Animal Care and Use Committee of the Southern Medical University,China(approval number:L2016113)on January 1,2016.

Bmi-1基因杂合子缺失对小鼠脑老化的影响

目的:Bmi-1(B-cell specific moloney leukemia virus insertion site 1)基因在干细胞增殖和分化中的作用已有大量文献报道,但其在老年小鼠脑中发挥的作用尚不清楚。本研究旨在探讨Bmi-1在脑衰老中的病理生理作用。方法:选取17月龄的Bmi-1杂合子(Bmi-1^(+/-))小鼠和野生型(wild-type,WT)小鼠,采用行为学检测、免疫组化及Masson染色等技术,比较Bmi-1^(+/-)小鼠和WT小鼠的整体健康状况及长期记忆能力;通过HE染色、电子显微镜及Western blot等方法,研究Bmi-1基因半剂量敲除对小鼠脑衰老进程的潜在影响。结果:Bmi-1^(+/-)小鼠较同窝WT小鼠出现了长期空间记忆功能的减弱(P<0.05),伴随着海马齿状回(dentate gyrus,DG)区域特异性的神经细胞发生减少(P<0.05),神经元数目降低(P<0.05)和灰质区体积缩小(P<0.05)。进一步研究发现,与WT小鼠相比,Bmi-1^(+/-)小鼠DG区神经元线粒体膨大、肿胀,线粒体嵴减少的比例增加(P<0.05),且DG区神经元细胞质中脂褐素的数量明显增加(P<0.05);此外,Bmi-1^(+/-)小鼠DG区神经元线粒体能量代谢相关蛋白泛醌氧化还原酶核心亚基V2[NADH dehydrogenase(ubiquinone)flavoprotein 2,NDUFV2]和泛醌氧化还原酶核心亚基S3[NADH dehydrogenase(ubiqui-none)ferrithionein 3,NDUFS3]的表达量均下调(P<0.05),三羧酸循环的重要催化酶二氢硫辛酰琥珀酰转移酶蛋白(dihydroli-poyl S-succinyltransferase,DLST)也显著下调(P<0.01);同时Bmi-1调控的细胞周期因子中,细胞周期蛋白依赖性激酶抑制剂p27和肿瘤蛋白p53显著上调(P<0.05)。结论:Bmi-1基因的半剂量缺失抑制了老龄鼠脑内海马区新生神经元的产生,导致海马DG区体积的特异性缩小,长期记忆功能障碍,其机制可能与老化相关蛋白p27、p53表达异常和神经元线粒体变性有关。

Effects of microwave radiation on brain energy metabolism and related mechanisms

With the rapid development of electronic technologies, anxiety regarding the potential health hazards induced by microwave radiation(MW) has been growing in recent years. The brain is one of the most sensitive target organs for microwave radiation, where mitochondrial injury occurs earlier and more severely than in other organs. Energy metabolism disorders do play an important role during the process of microwave radiation-induced brain damage. In this paper, we will review the biological effects of microwave radiation, the features of brain energy supply and consumption and the effects of microwave radiation on mitochondrial energy metabolism and potential related mechanisms.

Effects of Chinese herbal monomers on oxidative phosphorylation and membrane potential in cerebral mitochondria isolated from hypoxia-exposed rats in vitro

Mitochondrial dysfunction is the key pathogenic mechanism of cerebral injury induced by high-altitude hypoxia. Some Chinese herbal monomers may exert anti-hypoxic effects through enhancing the efficiency of oxidative phosphorylation, in this study, effects of 10 kinds of Chinese herbal monomers on mitochondrial respiration and membrane potential of cerebral mitochondria isolated from hypoxia-exposed rats in vitro were investigated to screen anti-hypoxic drugs. Rats were exposed to a low-pressure environment of 405.35 mm Hg （54.04 kPa） for 3 days to establish high-altitude hypoxic models. Cerebral mitochondria were isolated and treated with different concentrations of Chinese herbal monomers （sinomenine, silymarin, glycyrrhizic acid, baicalin, quercetin, ginkgolide B, saffron, pipedne, ginsenoside Rgl and oxymatrine） for 5 minutes in vitro. Mitochondrial oxygen consumption and membrane potential were measured using a Clark oxygen electrode and the rhodamine 123 fluorescence analysis method, respectively. Hypoxic exposure significantly decreased the state 3 respiratory rate, respiratory control rate and mitochondrial membrane potential, and significantly increased the state 4 respiratory rate. Treatment with saffron ginsenoside Rgl and oxymatrine increased the respiratory control rate in cerebral mitochondria isolated from hypoxia-exposed rats in dose-dependent manners in vitro, while ginsenoside Rgl, piperine and oxymatrine significantly increased the mitochondrial membrane potential in cerebral mitochondria from hypoxia-exposed rats. The Chinese herbal monomers saffron, ginsenoside Rgl piperine and oxymatrine could thus improve cerebral mitochondrial disorders in oxidative phosphorylation induced by hypobaric hypoxia exposure in vitro.

Inhibition of endoplasmic reticulum stress alleviates secondary injury after traumatic brain injury

Apoptosis after traumatic brain injury has been shown to be a major factor influencing prognosis and outcome. Endoplasmic reticulum stress may be involved in mitochondrial mediated neuronal apoptosis. Therefore, endoplasmic reticulum stress has become an important mechanism of secondary injury after traumatic brain injury. In this study, a rat model of traumatic brain injury was established by lateral fluid percussion injury. Fluorescence assays were used to measure reactive oxygen species content in the cerebral cortex. Western blot assays were used to determine expression of endoplasmic reticulum stress-related proteins. Hematoxylin-eosin staining was used to detect pathological changes in the cerebral cortex. Transmission electron microscopy was used to measure ultrastructural changes in the endoplasmic reticulum and mitochondria. Our results showed activation of the endoplasmic reticulum stress-related unfolded protein response. Meanwhile, both the endoplasmic reticulum stress response and mitochondrial apoptotic pathway were activated at different stages post-traumatic brain injury. Furthermore, pretreatment with the endoplasmic reticulum stress inhibitor, salubrinal（1 mg/kg）, by intraperitoneal injection 30 minutes before injury significantly inhibited the endoplasmic reticulum stress response and reduced apoptosis. Moreover, salubrinal promoted recovery of mitochondrial function and inhibited activation of the mitochondrial apoptotic pathway post-traumatic brain injury. These results suggest that endoplasmic reticulum stress might be a key factor for secondary brain injury post-traumatic brain injury.

Acute high-altitude hypoxic brain injury Identification of ten differential proteins

Hypobaric hypoxia can cause severe brain damage and mitochondrial dysfunction, and is involved in hypoxic brain injury. However, little is currently known about the mechanisms responsible for mi- tochondrial dysfunction in hypobaric hypoxic brain damage. In this study, a rat model of hypobaric hypoxic brain injury was established to investigate the molecular mechanisms associated with mi- tochondrial dysfunction. As revealed by two-dimensional electrophoresis analysis, 16, 21, and 36 differential protein spots in cerebral mitochondria were observed at 6, 12, and 24 hours post-hypobaric hypoxia, respectively. Furthermore, ten protein spots selected from each hypobaric hypoxia subgroup were similarly regulated and were identified by mass spectrometry. These de- tected proteins included dihydropyrimidinase-related protein 2, creatine kinase B-type, is- ovaleryI-CoA dehydrogenase, elongation factor Ts, ATP synthase beta-subunit, 3-mercaptopyruvate sulfurtransferase, electron transfer flavoprotein alpha-subunit, Chain A of 2-enoyI-CoA hydratase, NADH dehydrogenase iron-sulfur protein 8 and tropomyosin beta chain. These ten proteins are all involved in the electron transport chain and the function of ATP synthase. Our findings indicate that hypobaric hypoxia can induce the differential expression of several cerebral mitochondrial proteins, which are involved in the regulation of mitochondrial energy production.

Selective brain hypothermia-induced neuroprotection against focal cerebral ischemia/reperfusion injury is associated with Fis1 inhibition

Selective brain hypothermia is considered an effective treatment for neuronal injury after stroke,and avoids the complications of general hypothermia.However,the mechanisms by which selective brain hypothermia affects mitochondrial fission remain unknown.In this study,we investigated the effect of selective brain hypothermia on the expression of fission 1 (Fis1) protein,a key factor in the mitochondrial fission system,during focal cerebral ischemia/reperfusion injury.Sprague-Dawley rats were divided into four groups.In the sham group,the carotid arteries were exposed only.In the other three groups,middle cerebral artery occlusion was performed using the intraluminal filament technique.After 2 hours of occlusion,the filament was slowly removed to allow blood reperfusion in the ischemia/reperfusion group.Saline,at 4℃ and 37℃,were perfused through the carotid artery in the hypothermia and normothermia groups,respectively,followed by restoration of blood flow.Neurological function was assessed with the Zea Longa 5-point scoring method.Cerebral infarct volume was assessed by 2,3,5-triphenyltetrazolium chloride staining,and apoptosis was assessed by terminal deoxynucleotidyl transferase-mediated dUTP nick-end labeling staining.Fis1 and cytosolic cytochrome c levels were assessed by western blot assay.Fis1 mRNA expression was assessed by quantitative reverse transcription-polymerase chain reaction.Mitochondrial ultrastructure was evaluated by transmission electron microscopy.Compared with the sham group,apoptosis,Fis1 protein and mRNA expression and cytosolic cytochrome c levels in the cortical ischemic penumbra and cerebral infarct volume were increased after reperfusion in the other three groups.These changes caused by cerebral ischemia/reperfusion were inhibited in the hypothermia group compared with the normothermia group.These findings show that selective brain hypothermia inhibits Fis1 expression and reduces apoptosis,thereby ameliorating focal cerebral ischemia/reperfusion injury in rats.Experiments were authorized by the Ethics Committee of Qingdao Municipal Hospital of China (approval No.2019008).

Apolipoprotein E mimetic peptide protects against diffuse brain injury

Apolipoprotein E plays a crucial role in inhibiting chronic neurodegenerative processes. Howev-er, its impact on neurological function following diffuse brain injury is still unclear. This study was designed to evaluate the therapeutic effects and mechanisms of action of apolipoprotein E mimetic peptide on diffuse brain injury. Apolipoprotein E mimetic peptide was administered into the caudal vein of rats with diffuse brain injury before and after injury. We found that apo-lipoprotein E mimetic peptide signiifcantly decreased the number of apoptotic neurons, reduced extracellular signal-regulated kinase1/2 phosphorylation, down-regulated Bax and cytochrome c expression, decreased malondialdehyde content, and increased superoxide dismutase activity in a dose-dependent manner. These experimental ifndings demonstrate that apolipoprotein E mimetic peptide improves learning and memory function and protects against diffuse brain injury-induced apoptosis by inhibiting the extracellular signal-regulated kinase1/2-Bax mito-chondrial apoptotic pathway.

线粒体质量控制系统在中枢神经系统疾病中的研究进展

线粒体质量控制(mitoQC)是指线粒体通过不间断的生物发生、动力学(分裂/融合)、自噬、有丝分裂和转运之间的动态协调循环过程。mitoQC正在成为中枢神经系统(CNS)稳态的核心调控者。线粒体作为神经元的“能源工厂”,是神经元新陈代谢和保持稳态最重要的细胞器之一,维持线粒体活性和功能完整性对神经元健康至关重要。神经元死亡和功能缺陷是造成CNS疾病患者神经功能障碍的重要原因。现重点探讨mitoQC紊乱与CNS疾病之间的内在联系,旨在对维持和/或恢复神经元线粒体稳态及其相关细胞生命过程的研究机制进行综述。

菌粒阴阳学说:基于“人微共生体”探讨中医阴阳学说的学术思考

中医阴阳学说是中医经典理论体系中的关键与核心内容之一,对于理解人体的生理机能和病机过程以及中医药治疗疾病具有重要意义,然而如何使用现代科学语言对其进行解读和表征,长期以来是困扰中医发展和中西医结合的难题之一。鉴于近年来学术界逐渐发现人是由人体和共生微生物尤其是肠道菌群组成的“超级共生体”,且大量慢病与肠道菌群密切相关,提示数量众多、种类繁杂的人体共生微生物可能在病因病机传变过程中具有未曾预料到的重要作用。结合此前的新发现“饥饿源于菌群”以及“呼吸源于线粒体”的新理解,在对生命起源与进化、生物学、微生物学、医学(含中医、西医和中西医结合)等领域相关知识进行深度交叉融合和综合关联分析的基础上,以学术思考的方式提出“菌粒阴阳学说”,从肠道菌群在人体相对主“阴”(简称为“菌脑主阴”)、线粒体相对主“阳”(简称为“粒脑主阳”)以及“人体主和”(即人体调控阴阳平衡)的角度进行探讨,为理解中医阴阳学说提供新思路,有助于推动传统中医理论与现代生命科学的对接与融合,促进中西医结合学科的建设与发展。

补充辅酶Q10及递增负荷跑台运动训练对大鼠心肌和脑线粒体电子传递链酶复合体活性的影响

目的:观察递增负荷跑台运动训练及补充CoQ_(10)对力竭运动大鼠心肌和脑线粒体呼吸链复合体Ⅰ、Ⅱ和Ⅲ活性的影响。方法:36只健康雄性、Wister大鼠随机分为安静对照组、补充CoQ_(10)组、训练组和训练结合补充CoQ_(10)组。差速离心提取心肌和脑线粒体;分光光度法测定线粒体呼吸链酶复合体(Ⅰ～Ⅲ)活性。结果:1)安静状态下补充CoQ_(10) 7周,与安静对照组相比较,力竭运动后即刻心肌线粒体呼吸链CⅡ活性增强(P<0.01),CⅠ和CⅢ活性减弱(P<0.01);脑线粒体呼吸链CⅡ活性显著性降低(P<0.01)。2)递增负荷运动训练7周,与安静对照组相比较,力竭运动后即刻心肌线粒体呼吸链CⅠ和CⅡ活性减弱(P<0.01)、CⅢ活性增强(P<0.05)。3)递增负荷训练结合补充CoQ_(10) 7周,与安静对照组相比较,力竭运动后即刻心肌线粒体呼吸链CⅠ和CⅡ活性减弱(P<0.01),脑线粒体呼吸链CⅡ活性显著性下降(P<0.01)。4)递增负荷训练结合补充CoQ_(10)与单纯补充CoQ_(10)组相比,力竭运动后即刻心肌线粒体呼吸链CⅡ活性减弱(P<0.01)、CⅢ活性增强(P<0.01);脑线粒体呼吸链CⅡ活性显著性下降(P<0.01)。5)递增负荷训练结合补充CoQ_(10)与单纯运动训练组相比,力蝎运动后即刻心肌线粒体呼吸链CⅡ和CⅢ活性减弱(P<0.01);脑线粒体呼吸链CⅡ活性显著性下降(P<0.01)。结论:外源性补充CoQ_(10)对大鼠体重增长无负面影响,运动训练可以降低大鼠体重增长幅度。单纯补充CoQ_(10)可增强力竭运动后即刻大鼠心肌线粒体呼吸链CⅡ活性;降低脑线粒体呼吸链CⅡ活性;对力竭运动时间无影响。递增负荷训练可增强力竭运动后即刻大鼠心肌线粒体呼吸链CⅢ活性;对脑线粒体呼吸链CⅠ、CⅡ和CⅢ活性无明显影响;运动能力得到提高。递增负荷训练结合补充CoQ_(10)可维持力竭运动后即刻大鼠心肌线粒体呼吸链CⅢ活性不降低;脑线粒体呼吸链CⅡ活性显著性下降、CⅠ和CⅢ活性无显著性变化;运动能力得到提高;运动训练与补充CoQ_(10)对改善心肌和脑线粒体呼吸链CⅠ、CⅡ和CⅢ活性及运动能力方面无协同作用。训练组及训练结合补充CoQ_(10)组大鼠力竭运动时间的延长可能还与体重增长较慢及其他机制有关。

人参皂苷Rg_1对脑缺血再灌注损伤大鼠脑线粒体功能的影响

目的:观察人参皂苷Rg1对缺血再灌注大鼠脑损伤的保护作用及其对线粒体功能、抗氧化酶系的影响。方法:采用大鼠右侧大脑中动脉阻断(MCAO)局灶性脑缺血再灌注模型。缺血前灌胃人参皂苷Rg125,50, 100 mg·kg-1,给药7d。末次给药1 h后制备MCAO模型,缺血2 h,再灌注24 h后,用Longa’s法、TTC染色法、干燥失重法评价大鼠神经功能状态、脑梗死面积及脑水肿程度;电镜下观察线粒体超微结构,检测海马线粒体呼吸酶、ATPase、抗氧化酶活性及MDA含量的变化。结果:人参皂苷Rg1(50,100 mg·kg-1)明显减少MCAO再灌后脑梗死面积、脑水肿程度及改善神经功能症状,减轻线粒体损伤．升高线粒体呼吸酶、超氧化物歧化酶(SOD)、谷胱甘肽过氧化物酶(GSH-Px)和Na+／K+-ATPase,Ca2+-ATPase活性,降低MDA含量。结论:人参皂苷Rg1对脑缺血再灌注损伤有明显的保护作用,其可能的作用机制之一是保护线粒体功能及抗氧自由基。

急性重复低氧对小鼠脑组织血氧饱和度、线粒体功能以及ATP水平的影响

目的:探讨急性重复低氧对脑组织血氧饱和度与线粒体功能的影响。方法:将BALB/c小鼠置于低氧密闭罐中,通过小鼠呼吸消耗罐内氧造成罐内低氧,以小鼠出现喘呼吸为低氧耐受极限,然后将小鼠转到另一低氧密闭罐中,依此类推,连续进行5次低氧。记录小鼠每次的缺氧耐受时间、局部脑组织血氧饱和度,测定每次低氧暴露结束时的脑组织的线粒体复合体I活性和ATP含量。结果:小鼠的缺氧耐受时间随缺氧暴露次数增加而显著延长。脑组织血氧饱和度在第1、2次缺氧暴露时急剧下降,但在第3、4、5低氧暴露时先小幅度下降再逐渐恢复至正常水平,然后再缓慢降低。脑组织线粒体复合体I的活性随着缺氧次数的增加逐渐被抑制,ATP含量在第1次低氧暴露结束时低于正常水平,在第3、5次低氧暴露结束时高于正常水平。结论:急性重复低氧导致脑组织血氧饱和度降低的速度减慢、线粒体功能抑制以及脑组织ATP水平增高,后者很可能是动物脑组织耐缺氧能力增强的重要机制。

滋补脾阴方药对老龄大鼠脑线粒体膜ATP酶活性的影响

目的 :探讨滋补脾阴方药对老龄大鼠脑线粒体膜ATP酶活性的影响。方法 :以 2 3月龄SD大鼠为自然衰老鼠 ,以脑线粒体膜共轭双烯 (CD)、丙二醛 (MDA)、谷胱甘肽过氧化物酶 (GSH Px)、超氧化物歧化酶 (SOD)、Na+ K+ ATP酶、Ca2 + Mg2 + ATP酶为主要指标 ,观察滋补脾阴方药的作用。结果 :老龄大鼠脑线粒体膜存在脂质过氧化损伤和能量代谢障碍。滋补脾阴方药可增强其抗氧化酶和ATP酶活性 ,降低脂质过氧化物含量。结论 :滋补脾阴方药延缓脑老化的机理可能在于通过对老龄大鼠脑线粒体膜脂质过氧化损伤有明显的保护作用 ,对脑细胞能量代谢障碍有显著改善。

亚低温对颅脑创伤大鼠脑线粒体活性氧和ATP酶合成能力的影响

目的:研究亚低温治疗对颅脑创伤(TBI)大鼠线粒体活性氧(ROS)生成和ATP酶合成能力的影响。方法:72只动物随机分为假手术组、常温TBI组(肛温36℃～37℃)、亚低温TBI组(肛温31℃～33℃,亚低温持续2h),后2组利用液压打击(FPI)制作中度TBI模型。各组于脑外伤后2h,24h,3d和7d断头取伤侧大脑组织,差速离心法提取伤侧脑线粒体,酶荧光法检测线粒体ATP合成能力,荧光法测定线粒体ROS的生成。结果:常温TBI组脑创伤后线粒体ATP合成能力显著下降,24h降至最低,至7d时仍显著低于假手术组,ROS在各时间点均显著升高,3d时为最高。亚低温TBI组线粒体ATP合成能力在各时间点均高于常温TBI组,除2h外,其他时间点ROS低于常温TBI组。结论:颅脑创伤后线粒体ATP合成能力显著下降,ROS显著升高,亚低温可以改善线粒体ATP酶合成能力,抑制活性氧大量生成,从而保护脑组织。

黄芪对大鼠脑外伤后脑组织线粒体酶活性影响的研究

目的 探讨黄芪对大鼠创伤性脑损伤后脑组织线粒体酶活性水平的影响。方法 建立大鼠自由落体脑挫裂伤模型 ,伤后立即腹腔注射黄芪注射液 ,采用生化检测的方法分别测定治疗后 4小时、2 4小时和 4 8小时及各自的对照组大鼠脑组织线粒体ATP酶和超氧化物歧化酶 (SOD)活性以及丙二醛 (MDA)水平。结果 黄芪治疗后 2 4小时和 4 8小时大鼠脑组织线粒体ATP酶和SOD活性均高于各自时间点对照组 (P <0 .0 5 ,P <0 .0 1) ,而MDA水平则明显低于各自对照组 (P <0 .0 1)。结论 黄芪可以通过影响线粒体功能而减轻大鼠创伤性脑损伤后的继发性脑损害 。