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首页> 外文期刊>Biochimica et biophysica acta. Biomembranes >Effects of mitochondrial respiratory stimulation on membrane lipids and proteins: an electron paramagnetic resonance investigation
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Effects of mitochondrial respiratory stimulation on membrane lipids and proteins: an electron paramagnetic resonance investigation

机译:线粒体呼吸刺激对膜脂质和蛋白质的影响:电子顺磁共振研究

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Previous studies have implicated mitochondria-derived reactive oxygen species (ROS) in both the aging process and age-related diseases such as Alzheimer's disease, amyotrophic lateral sclerosis, Parkinson's disease etc. The current study, utilizing electron paramagnetic resonance (EPR) spectroscopy, was designed to determine if mitochondrial respiratory stimulation, under state 4 conditions, caused extensive oxidative modifications to membrane cytoskeletal proteins and lipids in the brain. A mixed population of cortical synaptosomes and mitochondria, prepared by centrifugation techniques using rat brain cortex from adult (4-6 months) female Brown Norway rat brains, were labeled with the lipid-specific spin probe, 5-nitroxyl stearate (5-NS). Stimulation of the mitochondrial electron transport chain was accomplished using 20 mM succinate 25 ℃ for 3 h. Mitochondrially derived free radicals, when reacted with the paramagnetic center of the spin probe, result in a loss of paramagnetism resulting in loss of intensity. A significant lowering (23%, P < 0.0001) in the signal amplitude (B_0) of 5-NS, indicative of generation of oxyradicals, was found. The order parameter, an inverse EPR-measure of membrane fluidity of the 5-NS spin labeled mitochondrial and synaptosomal membranes, also decreased following mitochondrial respiratory stimulation (P < 0.005). Changes in the physical state of cytoskeletal and transmembrane proteins due to succinate oxidation were measured using MAL-6 (2,2,6,6-tetramethyl-4-maleimidopiperdin-1-oxyl), a thiol-specific nitroxide spin label. The ratio of the amplitudes of the weakly to strongly immobilized spin label reaction sites (W/S ratio) in the low-field region of the spectrum was used to determine any alteration in protein conformation. previous studies in our laboratory have established that increased protein oxidation is associated with a decreased W/S ratio. In the current study, our results indicated significant lowering of the W/S ratio in cortex (30%, P < 0.0001) upon stimulation of the mitochondria with 20 mM succinate. Thus, we conclude that respiratory stimulation of mitochondria, due to a hypermetabolic stress with succinate, caused significant oxidative modifications of cortical membrane lipids and proteins.
机译:先前的研究涉及线粒体来源的活性氧(ROS)与衰老过程以及与年龄相关的疾病,例如阿尔茨海默氏病,肌萎缩性侧索硬化症,帕金森氏病等。目前的研究是利用电子顺磁共振(EPR)光谱旨在确定在状态4的条件下线粒体呼吸刺激是否引起大脑膜细胞骨架蛋白和脂质的广泛氧化修饰。皮质突触小体和线粒体的混合群体,是通过离心技术使用成年(4-6个月)成年雌性褐挪威大鼠脑的大鼠大脑皮层制备的,并用脂质特异性自旋探针5-硝基硬脂酸5-硝基氧乙酯标记。用20 mM琥珀酸25℃刺激3 h来刺激线粒体电子传输链。线粒体衍生的自由基,当与自旋探针的顺磁性中心反应时,会导致顺磁性丧失,从而导致强度降低。发现5-NS的信号幅度(B_0)显着降低(23%,P <0.0001),这表明氧自由基的产生。线粒体呼吸刺激后,有序参数(5-NS自旋标记的线粒体和突触体膜的膜流动性的反向EPR量度)也降低了(P <0.005)。使用巯基特异性的一氧化氮自旋标记物MAL-6(2,2,6,6-四甲基-4-马来酰亚胺基哌啶-1-氧基)测量由于琥珀酸氧化引起的细胞骨架和跨膜蛋白的物理状态变化。光谱的低场区域中弱固定到强固定的自旋标记反应位点的振幅之比(W / S比)用于确定蛋白质构象的任何改变。我们实验室先前的研究已经确定,蛋白质氧化增加与W / S比率降低有关。在当前研究中,我们的结果表明,用20 mM琥珀酸酯刺激线粒体后,皮质中的W / S比显着降低(30%,P <0.0001)。因此,我们得出的结论是,由于琥珀酸盐的过度代谢应激,线粒体的呼吸刺激导致了皮质膜脂质和蛋白质的显着氧化修饰。

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