Thyroid Hormone Metabolites Quantified in Pup and Adult Rat Cerebellum, Cortex and Whole-Brain Samples Using an Automated Online SPE-LC-MS/MS Method

Author:

Hindrichs Christiane12,Walk Tilmann1ORCID,Landsiedel Robert34,Kamp Hennicke1,Schneider Steffen3,Melching-Kollmuss Stephanie5,Funk-Weyer Dorothee3

Affiliation:

1. BASF Metabolome Solutions GmbH, Tegeler Weg 33, 10589 Berlin, Germany

2. Department of Chemistry, Rheinland-Pfälzischen Technischen Universität Kaiserslautern-Landau, Erwin-Schrödinger-Straße 52, 67663 Kaiserslautern, Germany

3. Experimental Toxicology and Ecology, BASF SE, Im Spitzenbusch 10, 67227 Frankenthal, Germany

4. Pharmacology and Toxicology, Institute of Pharmacy, Free University of Berlin, 14195 Berlin, Germany

5. Agricultural Solutions, BASF SE, Speyerer Str. 2, 67117 Limburgerhof, Germany

Abstract

Changes in thyroid hormone (TH) levels in rat brain at early developmental stages are correlated with adverse effects on offspring development. To characterize the ability of substances to interfere with the TH concentrations in, e.g., rat brain, it is essential to know the mean TH concentrations in this tissue under control conditions. In this publication, an online solid-phase extraction (SPE) liquid chromatography (LC) tandem mass spectrometry (MS/MS) method was validated and used to measure TH metabolites (T4, T3, rT3, T2 and T1) in the brains of untreated rats. Data on TH concentrations in the whole brain and separate data from the cerebellum and the cortex are shown. The corresponding samples were gathered from young rats at postnatal days (PND) 4 and 21/22 and from adult rats. The results show inter alia the high accuracy and precision of the method, and LOQs of 0.02 ng/mL were determined for T1, T2 and rT3 and of 0.15 ng/mL for T3 and T4. Technical variability is low, as shown by the relative standard deviations of 7.5–20%. For our rat model, we found that T4, T3 and T2 concentrations rise from PND4 to PND21, whereas the rT3 concentration decreases; as well as there is no statistical difference between TH concentrations in the male and female rat brain. This method is suitable to analyze TH metabolites in the brain and build up a database of historical TH concentrations in control rats. Together, this yields a robust diagnostic tool to detect potentially adverse disturbances of TH homeostasis in the most vulnerable anatomic structure.

Publisher

MDPI AG

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