Pindone is a highly effective anticoagulant rodenticide. In this paper, an improved assay for the analysis and confirmation of pindone in human plasma has been proposed. After the samples protein precipitation with 10% (v/v) methanol in acetonitrile and cleaning with solid-phase extraction, the separation was carried out on an IonPac AS11-HC analytical column (250 mm x 2 mm) using 20 mmol L(-1) KOH containing 10% (v/v) methanol as organic modifier by eluent generator reagent free ion chromatography. Quantification was performed by a negative electrospray ionization ion trap mass spectrometry using diphacinone as an internal standard. The transition for quantitative analysis was m/z 229 -> 172, and for qualitative analysis were m/z 229 -> 145 and m/z 229 -> 214 for pindone. The transition for quantitative analysis was m/z 339 -> 167 for IS. The limit of detection, the limit of quantification, recovery, linearity, precision, and stability were well validated. The cracking approach of characteristic fragments for pindone and IS were proposed. It was confirmed that this method could be used in clinical diagnosis and forensic toxicology analysis.

• 出版日期2009-10
• 单位浙江工商大学