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采用紫外光化学蒸气发生-同位素稀释电感耦合等离子体质谱法测定生物组织中的总汞。

Determination of total mercury in biological tissue by isotope dilution ICPMS after UV photochemical vapor generation.

机构信息

Mineral Resources Chemistry Key Laboratory of Sichuan Higher Education Institutions, College of Materials and Chemistry & Chemical Engineering, Chengdu University of Technology, Chengdu 610059, China.

出版信息

Talanta. 2013 Dec 15;117:371-5. doi: 10.1016/j.talanta.2013.09.024. Epub 2013 Sep 25.

Abstract

A method is developed for the determination of trace mercury in biological samples using photo chemical vapor generation (PVG) and isotope dilution inductively coupled plasma mass spectrometry (ID ICPMS) detection. Biological tissues were solubilized in formic acid. Subsequently, the sample solutions were exposed to an ultraviolet (UV) source for the reduction of mercury into vapor species prior to ICPMS measurements. The formic acid served not only as a tissue solubilizer in the sample preparation procedure, but also as a photochemical reductant for mercury in the PVG process. The problem arising from the opaque formic acid digested solution was efficiently solved by using ID method. The optimum conditions for sample treatment and PVG were investigated. A limit of detection (LOD) of 0.5 pg g(-1), based on an external calibration, provided 350-fold improvement over that obtained by utilizing conventional pneumatic nebulization sample introduction. Method validation was demonstrated by the determination of total mercury in several biological tissue certified reference materials (CRMs). The results were in good agreement with the certified values.

摘要

建立了一种利用光化学蒸气发生(PVG)和同位素稀释电感耦合等离子体质谱(ID ICPMS)检测测定生物样品中痕量汞的方法。生物组织在甲酸中溶解。随后,将样品溶液暴露于紫外(UV)光源下,将汞还原成蒸气物种,然后进行 ICPMS 测量。甲酸不仅在样品制备过程中用作组织溶剂,而且在 PVG 过程中用作汞的光化学还原剂。通过使用 ID 方法,有效地解决了由不透明的甲酸消解溶液引起的问题。考察了样品处理和 PVG 的最佳条件。基于外部校准,检测限(LOD)为 0.5 pg g(-1),与利用常规气动雾化样品引入相比,灵敏度提高了 350 倍。通过对几种生物组织标准物质(CRM)中总汞的测定验证了方法的准确性。结果与证书值吻合良好。

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