首页> 外文期刊>Talanta: The International Journal of Pure and Applied Analytical Chemistry >Microwave-assisted derivatization combined with coacervative extraction for determining glutathione in biomatrix samples, followed by capillary liquid chromatography
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Microwave-assisted derivatization combined with coacervative extraction for determining glutathione in biomatrix samples, followed by capillary liquid chromatography

机译:微波辅助衍生化结合凝聚萃取来确定生物裂纹样品中的谷胱甘肽,其次是毛细管液相色谱法

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摘要

In this study, an ecofriendly analytical method was developed for determining glutathione (GSH) levels in biomatrix samples. 9-(bromomethyl)acridine was used for the first time as a derivatization reagent in GSH analysis. Microwave-assisted derivatization reduced the reaction time to 1 min. After derivatization, coacervative extraction was employed to extract GSH derivative from the complex biomatrix and to increase sensitivity. Because the negatively charged group of the GSH derivative was neutralized by the extracting agent Aliquat 336, aggregates formed without any coacervating agents. Furthermore, capillary liquid chromatography coupled with ultraviolet detection was applied to decrease waste generation and increase selectivity. This method successfully quantified GSH levels in various biomatrices, including erythrocytes, HaCaT cells, BALB/3T3 cells, and 313-L1 fibroblasts. This method only required a low sample volume (< 10 A standard addition method was utilized to spike the biomatrix samples with 0-4.8 nmol GSH to construct calibration curves. The proposed method performed well, with a determination coefficient of 0.999 and relative standard deviations of less than 6.59% for the slope and the intercept, as determined by linear regression analysis. The limit of detection of GSH in the standard solution was 800 nM or 0.4 pmol. Compared to non-derivatized GSH, the proposed method for detecting derivatized GSH provides 750-fold greater sensitivity.
机译:在该研究中,开发了一种Ecofriendly分析方法,用于测定生物斑纹样品中的谷胱甘肽(GSH)水平。作为GSH分析中的衍生化试剂首次使用9-(溴甲基)吖啶。微波辅助衍生化将反应时间降至1分钟。在衍生化之后,使用凝结性萃取来从复合生物斑纹中提取GSH衍生物并增加敏感性。因为通过萃取剂Aliquat 336中和GSH衍生物的带负电荷的组,所以在没有任何凝聚剂的情况下形成的聚集体。此外,施用含有紫外检测的毛细管液相色谱法以降低废物产生并增加选择性。该方法在各种生物滴答中成功地量化了GSH水平,包括红细胞,HACAT细胞,BALB / 3T3细胞和313-L1成纤维细胞。该方法仅需要低样品体积(<10,使用标准添加方法用0-4.8 nmol GSH刺破Biomatrix样品以构建校准曲线。所提出的方法良好,确定系数为0.999和相对标准偏差斜坡和截距小于6.59%,如线性回归分析所确定的。标准溶液中GSH的检测极限为800nm或0.4pmol。与非衍生GSH相比,所提出的检测衍生GSH的方法提供敏感度为750倍。

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