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首页> 外文期刊>Talanta: The International Journal of Pure and Applied Analytical Chemistry >Pragmatic and rapid analysis of carbonyl, oxidation and chlorination nucleoside-adducts in murine tissue by UPLC-ESI-MS/MS
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Pragmatic and rapid analysis of carbonyl, oxidation and chlorination nucleoside-adducts in murine tissue by UPLC-ESI-MS/MS

机译:UPLC-ESI-MS / MS的菌碳基,氧化和氯化核苷加合物的务实和快速分析

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摘要

Nucleoside-adduct analysis by liquid chromatography mass spectrometry is a powerful tool in genotoxicity studies. Efforts to date have quantified an impressive array of DNA damage products, although methodological diversity suggests quantification is still a challenging task. For example, inadequate co-examination of normal nucleosides, cumbersome sample preparation and large DNA requirements were identified to be recurring issues. A six-minute ultra-performance liquid chromatography method is presented which adequately separates seven candidate nucleoside-adducts from the four unmodified nucleosides. The method was sensitive to 1 adduct per 108 normal bases with 20 mu g DNA input for most targets. The method was shown to be accurate (81-119% across quintuplets of six tissue types) and precise (relative standard deviation 4-13%). The fast method time facilitated a second quantitation for normal nucleosides at an appropriate dilution, allowing DNA damage concentrations to be contextualised accurately sample-to-sample. From DNA samples, the analytical processing time was 8 h, and 96 samples can easily be prepared in a day. The method was used to quantify carbonyl, chloro- and oxo-adducts in murine tissue samples.
机译:通过液相色谱质谱法进行核苷 - 加合物分析是遗传毒性研究的强大工具。迄今为止的努力量化了令人印象深刻的DNA损伤产品阵列,尽管方法论多样性表明量化仍然是一个具有挑战性的任务。例如,对正常核苷的共同检查不足,鉴定了繁琐的样品制剂和大DNA要求是经常性问题。提出了六分钟的超高性能液相色谱法,其充分与四个未修饰的核苷分离出七个候选核苷加合物。该方法对每108个正常碱基的1加合加合物敏感,具有20μg的DNA输入,用于大多数靶标。该方法被证明是准确的(跨六种组织类型的Quintulet 81-119%),精确(相对标准偏差4-13%)。快速方法时间促进了适当稀释的正常核苷的第二种定量,使DNA损伤浓度待准确地样本至样本。从DNA样品中,分析处理时间是& 8小时,96个样品可以在一天内轻松制备。该方法用于量化小鼠组织样品中的羰基,氯和氧代加合物。

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