Human plasma ricinine quantification by LC–HRMS after micro‐solid‐phase elution

Author:

Thiebot Pauline12ORCID,Maaziz Nada1,Oppon Chrystelle1,Bertolo Laetitia1,Magny Romain12,Chevillard Lucie2,Mégarbane Bruno23,Houzé Pascal124,Labat Laurence12ORCID

Affiliation:

1. Laboratoire de Toxicologie Biologique, Fédération de Toxicologie Hôpital Lariboisière, APHP Paris France

2. INSERM UMRS‐1144 Université Paris Cité Paris France

3. Réanimation Médicale et Toxicologique, Fédération de Toxicologie Hôpital Lariboisière, APHP Paris France

4. Unité de Technologies Chimiques et Biologiques pour la Santé, CNRS UMR8258‐U1022 Université Paris Cité Paris France

Abstract

AbstractA rapid, sensitive and specific method for ricinine identification and quantification in plasma has been developed by LC–HRMS. Deuterated ricinine was used as the internal standard. From 100 μL of plasma, ricinine was extracted using micro‐solid‐phase elution, which allows a reduced extraction time, by eliminating the evaporation step. Eluate is directly injected into the LC–HRMS system. Chromatographic separation was performed using a reverse‐phase C18 column with a 4.5 min gradient elution. The method was validated according to European Medicines Agency guidelines. Linearity was verified between 0.25 and 500.0 ng/mL; the maximum precision calculated was 19.9% for the lower limit of quantitation and 9.6% for quality control, and accuracy was within ± 5.6% of the nominal concentrations. Selectivity, carryover, matrix effect and stability were also verified according to European Medicines Agency guidelines. The method allows the rapid and reliable identification of ricin‐exposed victims in case of terrorist attacks or poisonings: three intoxication cases are reported.

Publisher

Wiley

Subject

Clinical Biochemistry,Drug Discovery,Pharmacology,Molecular Biology,General Medicine,Biochemistry,Analytical Chemistry

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