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ESR and HPLC analysis of the interaction of hydroxyl radical with DMSO: Rapid reduction and quantification of POBN and PBN nitroxides

机译:ESR和HPLC分析羟基自由基与DMSO的相互作用:POBN和PBN一氧化氮的快速还原和定量

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The low stability of hydroxyl radical (OH.)-derived nitroxides is a limiting factor for direct spin-trapping of OH. in biological systems. The latter experimental difficulty is partly solved with the introduction of dimethyl sulfoxide (DMSO) into the studied systems. Hydroxyl radical oxidizes DMSO to methyl radical, which forms relatively stable nitroxides. The results of the present work provide evidence that in alpha-(4-pyridyl-1-oxide)-N-tert-butylnitrone (POBN) and alpha-phenyl-N-tert-butylnitrone (PBN) spin-trapping experiments aimed to detect methyl radical in biological systems, the nitroxides formed can be reduced to their ESR-"silent" hydroxylamine derivatives. The nitroxides and their hydroxylamine derivatives were successfully analyzed by HPLC with electrochemical (EC) and UV detection. The lowest limits of UV and EC detection of POBN/CH3 hydroxylamine was evaluated to be in the micro- and nanomolar range, respectively. In parallel ESR and HPLC-EC analysis of the metabolism of menadione by either HepG2 cells or isolated rat hepatocytes in the presence of DMSO, the HPLC-EC method has proven to be more sensitive in detecting the production of methyl radical. The use of the HPLC-EC detection of POBN/CH3 and PBN/CH3 is expected to be advantageous in detection of hydroxyl radical in biological systems in the presence of DMSO. [References: 31]
机译:羟基自由基(OH。)衍生的一氧化氮的低稳定性是直接旋转捕集OH的限制因素。在生物系统中。通过将二甲基亚砜(DMSO)引入到研究的系统中,可以部分解决后一个实验难题。羟基将DMSO氧化为甲基,形成相对稳定的氮氧化物。本工作的结果提供了证据,证明在α-(4-吡啶基-1-氧化物)-N-叔丁基硝酮(POBN)和α-苯基-N-叔丁基硝酮(PBN)的自旋捕集实验旨在检测如果在生物系统中具有甲基自由基,则形成的氮氧化物可以还原成其ESR-“沉默”羟胺衍生物。使用电化学(EC)和UV检测的HPLC成功分析了氮氧化物及其羟胺衍生物。估计POBN / CH3羟胺的UV和EC检测最低限分别在微摩尔和纳摩尔范围内。在存在DMSO的情况下,HepG2细胞或分离的大鼠肝细胞对甲萘醌代谢的ESR和HPLC-EC并行分析表明,HPLC-EC方法对检测甲基自由基的产生更为敏感。在DMSO存在下,使用HPLC-EC检测POBN / CH3和PBN / CH3有望在生物系统中检测羟基自由基方面具有优势。 [参考:31]

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