低氧大鼠脑线粒体体外转录活性的研究

目的：探讨低氧对大鼠脑线粒体DNA表达的影响及其与能量生成的关系。方法：雄性Wistar大鼠随机分为3组：急性低氧组（AH）、慢性低氧组（CH）和对照组,其中急、慢性低氧组动物分别连续暴露于模拟海拔4000m高原3d(AH)和40d（CH）。分离脑线粒体,分别测定线粒体体外转录活性、F0F1－ATP酶活性以及ATP对线粒体体外转录的影响。结果：急性低氧大鼠脑线粒体体外转录活性及F0F1－ATP酶活性显著降低,慢性低氧时有所回升,两者呈线性相关。ATP对大鼠脑线粒体体外转录活性呈双相效应。结论：低氧时脑线粒体转录活性改变可能参与低氧抑制线粒体能量代谢的机制,ATP可能通过反馈作用对线粒体转录进行微调。     

低压缺氧对大鼠脑线粒体腺苷酸转运体特性的影响

本文探讨低压缺氧对大鼠脑线粒体内膜腺苷酸转运体（adenine nucleotide translocator,ANT）转运特性的影响。实验将雄性Wistar大鼠随机分为常氧对照组和缺氧组,后者分别连续暴露于模拟5000m高原1、5、15、30d（23h／d）。分别于平原和模拟4000m高原断头处死动物,分离脑线粒体,用抑制剂终止法测定线粒体对。H-ADP的转运效率,抑制剂滴定法测定ANT密度,HPLC测定线粒体内腺苷酸含量。结果显示：缺氧后ANT转运活性均明显低于常氧组,缺氧不同天数线粒体内膜ANT分布密度无显著改变,线粒体内（ATP＋ADP）含量下降与转运活性变化一致。以上观察结果表明,低压缺氧暴露可显著抑制ANT转运活性,降低能量产生和利用的周转率,但不改变ANT密度,提示ANT活性改变是低压缺氧时细胞能量代谢障碍的重要机制。     

棕榈酸对模拟高原低氧大鼠离体脑线粒体解耦联蛋白活性及质子漏的影响

本文旨在通过观察棕榈酸对模拟高原低氧大鼠离体脑线粒体解耦联蛋白(uncoupling proteins,UCPs)活性的影响及脑线粒体质子漏与膜电位的改变,探讨UCPs在介导游离脂肪酸对低氧时线粒体氧化磷酸化功能改变中的作用.将SpragueDawley大鼠随机分为对照组、急性低氧组和慢性低氧组.低氧大鼠于低压舱内模拟海拔5 000 m高原23 h/d作低氧暴露,分别连续低氧3 d和30 d.用差速密度梯度离心法提取脑线粒体,[3H-GTP法测定UCPs含量与活性,TPMP 电极与Clark氧电极结合法测量线粒体质子漏,罗丹明123荧光法测定线粒体膜电位.结果显示,低氧使脑线粒体内UCPs含量与活性升高、质子漏增加、线粒体膜电位降低;同时,低氧暴露降低脑线粒体对棕榈酸的反应性,UCPs活性的改变率低于对照组,且线粒体UCPs含量、质子漏、膜电位变化率亦出现相同趋势.线粒体质子漏与反映UCPs活性的Kd值呈线性负相关(P<0.01 r=-0.906),与反映UCPs含量的Bmax呈线性正相关(P<0.01,r=0.856),与膜电位呈线性负相关(P<0.01,r=-0.880).以上结果提示,低氧导致的脑线粒体质子漏增加及膜电位降低与线粒体内UCPs活性升高有关,同时低氧暴露能降低脑线粒体对棕榈酸的反应性,提示在高原低氧环境下,游离脂肪酸升高在维持线粒体能量代谢中起着自身保护和调节机制.     

慢性间断低氧暴露对大鼠心肌线粒体ATP酶及吸链酶复合物的影响

目的:研究慢性间断低氧暴露对大鼠心肌线粒体Na 、K -ATPase和Ca2 、Mg2 -ATPase以及呼吸链酶复合物Ⅰ、Ⅱ、Ⅲ、Ⅳ活性的影响.方法:经慢性间断低氧暴露(模拟海拔3 000 m、5 000 m分别低氧,每天4 h,共2周,最后8 000 m低氧4 h)和急性低氧(模拟海拔8 000 m低氧4 h)的大鼠,断头处死,迅速取出心脏,分离心肌线粒体,用水解磷酸根法测定ATP酶活性,用Clark氧电极法测定呼吸链酶复合物的活性.结果:①慢性间断低氧暴露对大鼠心肌线粒体Na 、K -ATPase的活性无明显影响.②急性低氧大鼠心肌线粒体Ca2 、Mg2 -ATPase的活性较正常大鼠显著降低,而慢性间断低氧暴露大鼠心肌线粒体Ca2 、Mg2 -ATPase的活性则明显升高,接近正常水平.③急性低氧大鼠心肌线粒体呼吸链酶复合物I(NADH-CoQ还原酶)、复合物Ⅱ(琥珀酸-CoQ还原酶)、复合物IV(细胞色素氧化酶)活性较正常大鼠显著降低,而经慢性间断低氧暴露后,三者的活性均显著提高.相同实验条件下,低氧对复合物Ⅲ(CoQ-细胞色素C还原酶)活性无明显影响.结论:慢性间断低氧暴露可以显著提高心肌线粒体Ca2 、Mg2 -ATPase和呼吸链酶复合物Ⅰ、Ⅱ、Ⅳ的活性,从而改善低氧时心肌线粒体呼吸链的功能,维持心肌正常能量代谢,最终提高心肌收缩和舒张功能.     

CLA对急性缺氧大鼠肝脏线粒体呼吸链酶活性及氧化应激的影响

目的:观察共轭亚油酸(CLA)对急性缺氧大鼠肝脏线粒体呼吸链酶活性及肝脏内氧化应激(OS)的影响。方法:将60只SD大鼠随机分为正常对照组,模拟海拔5000米高原环境连续缺氧暴露3d的急性缺氧组,急性缺氧CLA干预组。生化法测定肝脏组织中丙二醛(MDA)、还原型谷胱甘肽(GSH)含量及超氧化物歧化酶(SOD)、过氧化氢酶(CAT)活性,Clark氧电极法观察大鼠肝脏线粒体呼吸链酶活性。结果:成功诱导大鼠急性缺氧模型。与对照组比,急性缺氧组大鼠肝脏MDA含量明显升高(P<0.05),同时肝脏线粒体呼吸链酶活性以及抗氧化酶活性(SOD,CAT)及GSH显著降低(P<0.05),与急性缺氧相比,CLA治疗组大鼠以上各项指标均有改善,并存在一定的剂量效应关系。结论:CLA通过抑制氧化应激增强大鼠肝脏线粒体呼吸链酶活性改善了急性缺氧大鼠肝脏的能量代谢障碍,对急性缺氧引起的氧化损伤有保护作用。     

一次性力竭运动对大鼠PHB1表达及线粒体功能的影响

目的:观察一次性力竭运动后大鼠脑、心、骨骼肌组织和线粒体中PHB1含量的变化及对大鼠线粒体功能的影响,探寻PHB1与线粒体功能和能量代谢的关系。方法:健康雄性SD大鼠40只,随机分为2组(n=20):对照组和一次性力竭运动组,大鼠进行一次性急性跑台运动建立力竭运动模型。收集各组大鼠的心、脑和骨骼肌组织样品并提取线粒体,检测其呼吸功能和ROS的变化。用Western blot方法检测组织和线粒体中PHB1蛋白表达水平;用分光光度计检测各器官中ATP含量以及线粒体中复合体V活性(ATP合酶活性)。结果:(1)一次性力竭运动后脑、心肌、骨骼肌中ATP含量显著性降低;(2)一次性力竭运动后脑、心肌、骨骼肌线粒体中复合体V活性、RCR、ROS显著性降低,ST4均显著性升高,ST3无显著性差异。(3)一次性力竭运动后心、脑、骨骼肌线粒体中PHB1的表达显著性减少。(4)通过相关性分析得出:一次性力竭运动后心、脑、骨骼肌中ATP含量与心、脑、骨骼肌中复合体V活性呈正相关;心、脑、骨骼肌中ATP含量和心、脑骨骼肌中PHB1的表达呈正相关。结论:一次性力竭运动后,降低线粒体氧化磷酸化功能,使大鼠脑、骨骼肌线粒体内ROS生成增加,PHB1的表达、ATP含量和复合体V活性均下降。一次性力竭运动使得大鼠线粒体内PHB1表达降低,线粒体功能减弱,机体能量代谢降低。     

线粒体ATP合酶抑制因子(ATPIF1)在能量代谢中的作用

线粒体是真核细胞中动态双层膜结构的细胞器,由外至内可以划分为四个功能区,分别是线粒体外膜(OMM),线粒体膜间隙,线粒体内膜(IMM)和线粒体基质。在线粒体内膜上的复合体V(complex V)即为ATP合酶,其主要功能是合成ATP。实际上,ATP合酶既合成也水解ATP,对细胞ATP水平有双向调节作用。ATP合酶的活性受抑制因子(ATPIF1)的调节。ATPIF1与ATP合酶结合后,对其ATP合成和水解功能进行抑制,从而影响线粒体和细胞内ATP水平。ATPIF1活性受到组氨酸质子化状态和丝氨酸磷酸化修饰的调节。在缺氧,交感神经兴奋和肿瘤等条件下,ATPIF1发挥重要代谢调节作用,但其在代谢紊乱疾病中的作用尚不明确。本文在综述ATPIF1文献的基础上,对其在糖脂代谢紊乱疾病中的作用进行分析及展望。     

人参皂甙对缺氧大鼠海马DG区神经细胞DNA损伤保护作用的研究

目的:用单细胞凝胶电泳技术(SCGE)研究急慢性缺氧大鼠海马DG区神经细胞细胞DNA损伤和人参皂甙对缺氧大鼠海马细胞DNA的保护作用.方法:健康成年SD大鼠随机分为急、慢性缺氧正常对照组、急性缺氧组和慢性缺氧组(分别在模拟海拔5000米高原环境连续缺氧暴露0d、3d和30d)、急性缺氧人参皂甙干预组、慢性缺氧人参皂甙干预组.应用SCGE检测海马DG区神经细胞DNA损伤.结果:随着缺氧时间的增加,海马DG区神经细胞DNA的损伤程度加重,尾长、尾部DNA百分含量和尾距显著增加(P＜0.05).人参皂甙能使缺氧损伤的海马DG区神经细胞的尾长、尾部DNA百分含量和尾距均较缺氧组减少(P＜0.05).结论:人参皂甙能有效地减轻缺氧引起的海马组织细胞DNA的断裂损伤.     

HIF-1α修饰的骨髓间充质干细胞增强其抗PC12细胞缺氧损伤作用

该文探讨了HIF-1α修饰的大鼠骨髓间充质干细胞(mesenchymal stem cells,MSCs)对缺氧损伤所致神经元样PC12细胞凋亡的作用及其可能机制。PC12细胞分别与MSCs、HIF-1α-MSCs细胞在缺氧环境下体外共培养,分为正常组、缺氧组、MSCs组及HIF-1α-MSCs组。MTT检测不同缺氧时间PC12细胞活性。HE染色观察PC12细胞形态。Hoechst 33258染色与Annexin V-FITC双染色法检测PC12细胞凋亡。RT-PCR及细胞免疫荧光检测caspase-3的m RNA及蛋白质水平。MTT结果显示,PC12细胞活性随着缺氧时间而下降,缺氧12 h细胞活性下降至45.1%。与正常组相比,缺氧组PC12细胞凋亡率明显增高,caspase-3的m RNA和蛋白质水平明显上调,两者有显著差异(P0.05)。与缺氧组相比,MSCs组及HIF-1α-MSCs组的凋亡率降低(P0.05),caspase-3的m RNA和蛋白质水平下调(P0.05),且HIF-1α-MSCs组更为明显(P0.05)。结果证明,HIF-1α修饰的MSCs能增强MSCs的抗PC12缺氧损伤作用,其机制可能与HIF-1α-MSCs降低PC12细胞caspase-3基因表达有关。     

慢性缺氧对肺动脉内皮依赖性和非内皮依赖性舒张反应的影响

本实验用生物测定法观察了模拟海拔5000m高度连续缺氧20d对大鼠肺动脉内皮依赖性和非内皮依赖性舒张反应的影响。结果显示慢性缺氧明显抑制了肺内和肺外动脉对乙酰胆碱、ATP、硝普钠和异丙肾上腺素舒张反应的敏感性和反应性。在浓度为10~(-6)mol/L时,缺氧组大鼠肺内动脉对乙酰胆碱、硝普钠和异丙肾上腺素的舒张反应分别只有对照组大鼠的61.3％、75.9％和61.7％,对浓度为1.8×10~(-5)mol/L的ATP的舒张反应只有对照组大鼠的64.9％。研究表明,ATP和乙酰胆碱主要是通过内皮舒张因子使肺动脉产生内皮依赖性舒张反应,硝普钠和异丙肾上腺素分别通过直接激活血管平滑肌细胞鸟苷酸环化酶和β受体使血管产生非内皮依赖性舒张反应。缺氧同时抑制了肺动脉内皮依赖性和非内皮依赖性舒张反应,提示慢性缺氧可能抑制了正常肺内舒血管活性物质的生理作用。     

大鼠脑线粒体体外蛋白翻译体系的建立及蛋白产物的鉴定

目的 :建立大鼠脑组织线粒体的体外蛋白合成体系并对其合成产物进行电泳分离和分子量鉴定。方法 :分离大鼠脑组织线粒体 ,用3 H 亮氨酸掺入法探索线粒体体外翻译的最佳条件 ,3 5S 蛋氨酸掺入并对翻译后产物经SDS 聚丙烯酰胺凝胶电泳和放射自显影进行分子量鉴定。结果 :分离的线粒体氧化磷酸化偶联程度高 ,呼吸控制率(RCR)在 3.5～ 5 .5之间 ;体外3 H 亮氨酸的掺入活性在 6 0min内近似线性增长 ,而后维持在一相对稳定水平 ;3 H 亮氨酸的掺入活性随线粒体蛋白浓度而增加 ,而单位线粒体蛋白的掺入活性在 1mg/ml时最高 ;3 5S 蛋氨酸掺入SDS 聚丙烯酰胺凝胶电泳后可观察到清晰的 8条自显影带 ,分子量分别为 (单位Kda) 86、6 6、5 6、43、33、2 9、2 5、18。结论 :用此方法建立的脑线粒体离体翻译反应体系具有高活性和翻译忠实性等特点 ,是研究脑mtDNA在翻译水平的表达及调控的有效方法     

Protein synthesis by hepatic mitochondria isolated from carbon tetrachloride-exposed rats

Hepatic mitochondria isolated from rats 40 h after dosage with 1.1 ml/kg CCl4 are uncoupled and display structural damage. Mitochondrial function returns during hepatic recovery. Because the products of mitochondrial protein synthesis are essential to mitochondrial structure and function, the effects of CCl4 on the rate of mitochondrial protein synthesis, and on the products, was studied using mitochondria from CCl4-exposed rats during the early, maximum development and resolution stages of CCl4-induced mitochondrial damage. Rates of mitochondrial protein synthesis (incorporation of [35S]methionine) were elevated 300% over that of mitochondria from non-exposed rats 17 h after exposure; depressed by 50% at 40 h and above control at 113 h. When the radiolabeled products of incorporation were separated and examined by autoradiography, a novel, low-molecular-weight band, of approx. 9700, was apparent 40 h after CCl4 exposure. A band of similar molecular weight appeared when control mitochondria were incubated without an exogenous supply of ATP. Mitochondria from exposed rats which displayed rates of protein synthesis greater than control consistently had a relative increase in a band that corresponded in size to that of cytochrome oxidase subunit I. It was concluded that the loss of mitochondrial function induced by CCl4 could not be attributed to inhibition of mitochondrial protein synthesis, and that the mitochondria may not always synthesize protein in constant proportions.     

缺氧肺动脉平滑肌细胞中线粒体ATP敏感钾通道开放对细胞色素C的分布及细胞增殖的作用

为了探讨线粒体ATP敏感钾通道（mitochondrial ATP-sensitive K^＋channel,mito KATP）和线粒体膜电位（△ψm）在细胞缺氧信号转导中的作用以及对缺氧肺动脉平滑肌细胞中细胞色素C在细胞内的分布及细胞增殖的影响,本实验将人肺动脉平滑肌细胞进行常氧或24h缺氧培养,并将标本分为六组：（1）对照组;（2）mito KATP,开放剂diazoxide组;（3）mito KATP阻断剂5-HD组;（4）24h缺氧组;（5）24h缺氧＋diazoxide组;（6）24h缺氧＋5-HD组。利用激光共聚焦显微镜成像法检测△、ψm;线粒体／胞浆成分分离试剂盒（Bio Vision）分离线粒体和胞浆成分后,Western blot检测两者细胞色素C;Western blot检测细胞中caspase-9的蛋白表达量;MTT法及PI染色后流式细胞仪检测细胞增殖情况。结果显示：（1）diazoxide作用24h后,R-123荧光明显增强,胞浆细胞色素C与线粒体细胞色素C的比值明显降低,caspase-9的蛋白表达显著减少,细胞增殖明显增多、凋亡减少,与正常对照组相比较,均P〈0．05;而5-HD作用24h与正常对照组比较,上述指标无明显变化（P〉0．05）。（2）缺氧24h组,结果与diazoxide组相似,R-123荧光明显增强,胞浆细胞色素C与线粒体细胞色素C的比值明显降低,caspase-9的蛋白表达显著减少,细胞增殖明显增多、凋亡减少,与正常对照组相比较,均P〈0．05;24h缺氧＋diazoxide组与缺氧组相比较,R-123荧光明显增强,胞浆细胞色素C与线粒体细胞色素C的比值明显降低,caspase-9的蛋白表达显著减少,细胞增殖明显增多、凋亡减少（P〈0．05）;而24h缺氧＋5-HD组与缺氧组比较,R-123荧光明显降低,胞浆细胞色素C与线粒体细胞色素C的比值明显升高,caspase-9的蛋白表达显著增加,细胞增殖明显减少、凋亡增多（P〈0．05）。上述实验结果提示,缺氧可以引起mito KATP,的开放以及△ψm的去极化,并进而抑制细胞色素C从线粒体释放到胞浆,抑制线粒体凋亡途径,从而参与并影响肺动脉高压的发生、发展。     

Hypoxia affects mitochondrial protein expression in rat skeletal muscle

Hypoxia affects mammalian mitochondrial function, as well as mitochondria-based energy metabolism. The detail mechanism has not been fully understood. In this study, we detected protein expression levels in mitochondrial fractions of Wistar rats exposed to hypobaric hypoxia by use of proteomic methods. Adult male Wistar rats were randomized into an hypoxic (4,500?m, 30 days) group and a normoxic control group (sea level). Gastrocnemius muscles mitochondria were extracted and purified. Mitochondrial oxygen consumption was measured with a Clark oxygen electrode; mitochondrial transmembrane potential was detected with Rhodamine 123 as a fluoresce probe. Using 2-DE and MALDI-TOF MS analysis, we identified eight mitochondrial protein spots that were differentially expressed in the hypoxic group compared with the normoxic control. These proteins included Chain A of F1-ATPase, voltage dependent anion channel 1 (VDAC), hydroxyacyl Coenzyme A dehydrogenase α-subunit, mitochondrial F1 complex γ-subunit, androgen-regulated protein and tripartite motif protein 50. Two of the spots, VDAC and ATP synthase α-subunit, were confirmed by Western blotting analysis. Oxygen consumption during State 3 respiration, as well as the respiratory control ratio (RCR) was significantly higher in the control than that in the hypoxic group; mitochondrial transmembrane potential was significantly higher in hypoxic group than that in the control. With successful use of multiple proteomic analysis techniques, we demonstrates that 30 days hypoxia exposure has effects on the expression of mitochondrial proteins involved in ATP production and lipid metabolism, decrease the stability of mitochondrial membrane, and affect the mitochondrial electron transport chain.     

Adaptation of brain monoamine synthesis to hypoxia in the rat.

Oxygen is a substrate in the synthesis of the neurotransmitters, norepinephrine, dopamine, and serotonin. Changes in environmental oxygen appear to cause corresponding alterations in brain monoamine synthesis in vivo. The effect of chronic hypoxia was studied by exposing rats to 10% oxygen for up to 36 h. Brain monoamine synthesis, estimated in vivo, decreased initially and then returned to control levels, despite continued exposure to 10% oxygen. During this apparent adaptation to hypoxia, there were no changes in the concentration of brain serotonin, norepinephrine, dopamine, or tryptophan, while brain tryosine increased after 24 h of exposure. Tyrosine hydroxylase activity in vitro was not altered by the exposure to 10% oxygen. Evidence of hypoxic adaptation in these rats, a rightward shift of their hemoglobin dissociation curves, was found after 24 h of exposure. The adaptation of brain monoamine synthesis to hypoxia appeared to correlate with adaptive changes in brain tissue oxygen rather than any change in the intraneuronal regulation of amine synthesis.