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抗坏血酸盐保护神经元免受氧化应激:一项拉曼显微光谱研究。

Ascorbate protects neurons against oxidative stress: a Raman microspectroscopic study.

作者信息

Dutta Abhaya, Gautam Rekha, Chatterjee Sreejata, Ariese Freek, Sikdar Sujit Kumar, Umapathy Siva

机构信息

LaserLaB, Faculty of Sciences, VU University Amsterdam , 1081 HV Amsterdam, The Netherlands.

出版信息

ACS Chem Neurosci. 2015 Nov 18;6(11):1794-801. doi: 10.1021/acschemneuro.5b00106. Epub 2015 Aug 19.

Abstract

Oxidative stress due to excessive accumulation of reactive oxygen or nitrogen species in the brain as seen in certain neurodegenerative diseases can have deleterious effects on neurons. Hydrogen peroxide, endogenously generated in neurons under normal physiological conditions, can produce an excess of hydroxyl radical via a Fenton mediated mechanism. This may induce acute oxidative injury if not scavenged or removed effectively by antioxidants. There are several biochemical assay methods to estimate oxidative injury in cells; however, they do not provide information on the biochemical changes as the cells get damaged progressively under oxidative stress. Raman microspectroscopy offers the possibility of real time monitoring of the chemical composition of live cells undergoing oxidative stress under physiological conditions. In the present study, a hippocampal neuron coculture was used to observe the acute impact of hydroxyl radicals generated by hydrogen peroxide in the presence of Fe(2+) (Fenton reaction). Raman peaks related to nucleic acids (725, 782, 1092, 1320, 1340, 1420, and 1576 cm(-1)) showed time-dependent changes over the experimental period (60 min), indicating the breakdown of the phosphodiester backbone as well as nuclear bases. Interestingly, ascorbic acid (a potent antioxidant) when cotreated with Fenton reactants showed protection of cells as inferred from the Raman spectra, presumably by scavenging hydroxyl radicals. Little or no change in the Raman spectra was observed for untreated control cells and for cells exposed to Fe(2+) only, H2O2 only, and ascorbate only. A live-dead assay study also supported the current observations. Hence, Raman microspectroscopy has the potential to be an excellent noninvasive tool for early detection of oxidative stress that is seen in neurodegenerative diseases.

摘要

在某些神经退行性疾病中,大脑中活性氧或氮物种的过度积累所导致的氧化应激会对神经元产生有害影响。在正常生理条件下,神经元内源性产生的过氧化氢可通过芬顿介导的机制产生过量的羟基自由基。如果抗氧化剂不能有效清除或去除这种自由基,可能会引发急性氧化损伤。有几种生化检测方法可用于评估细胞中的氧化损伤;然而,当细胞在氧化应激下逐渐受损时,这些方法无法提供有关生化变化的信息。拉曼光谱显微镜提供了在生理条件下实时监测遭受氧化应激的活细胞化学成分的可能性。在本研究中,使用海马神经元共培养物来观察在Fe(2+)存在下过氧化氢产生的羟基自由基的急性影响(芬顿反应)。与核酸相关的拉曼峰(725、782、1092、1320、1340、1420和1576 cm(-1))在实验期间(60分钟)呈现出随时间的变化,表明磷酸二酯主链以及核碱基的分解。有趣的是,从拉曼光谱推断,抗坏血酸(一种有效的抗氧化剂)与芬顿反应物共同处理时显示出对细胞的保护作用,可能是通过清除羟基自由基实现的。对于未处理的对照细胞以及仅暴露于Fe(2+)、仅暴露于H2O2和仅暴露于抗坏血酸盐的细胞,拉曼光谱几乎没有变化。活死检测研究也支持了当前的观察结果。因此,拉曼光谱显微镜有潜力成为一种出色的非侵入性工具,用于早期检测神经退行性疾病中出现的氧化应激。

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