4.6 Article

Developmental and Cell Type-Specific Expression of Thyroid Hormone Transporters in the Mouse Brain and in Primary Brain Cells

Journal

GLIA
Volume 59, Issue 3, Pages 463-471

Publisher

WILEY
DOI: 10.1002/glia.21116

Keywords

astrocyte; neuron; blood brain-barrier; development

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Funding

  1. Deutsche Forschungsgemeinschaft Sonderforschungsbereich [SFB 665]

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Cellular thyroid hormone uptake and efflux are mediated by transmembrane transport proteins. One of these, monocarboxylate transporter 8 (MCT8) is mutated in Allan-Herndon-Dudley syndrome, a severe mental retardation associated with abnormal thyroid hormone constellations. Since mice deficient in Mct8 exhibit a milder neurological phenotype than patients, we hypothesized that alternative thyroid hormone transporters may compensate in murine brain cells for the lack of Mct8. Using qPCR, Western Blot, and immunocytochemistry, we investigated the expression of three different thyroid hormone transporters, i.e., Mct8 and L-type amino acid transporters Lat1 and Lat2, in mouse brain. All three thyroid hormone transporters are expressed from corticogenesis and peak around birth. Primary cultures of neurons and astrocytes express Mct8, Lat1, and Lat2. Microglia specifically expresses Met10 and Slco4a1 in addition to high levels of Lat2 mRNA and protein. As in vivo, a brain microvascular endothelial cell line expressed Mct8 and Lat1. 158N, an oligodendroglial cell line expressed Mct8 protein, consistent with delayed myelination in MCT8-deficient patients. Functional T-3- and T-4-transport assays into primary astrocytes showed K-M values of 4.2 and 3.7 mu M for T-3 and T-4. Pharmacological inhibition of L-type amino acid transporters by BCH and genetic inactivation of Lat2 reduced astrocytic T-3 uptake to the same extent. BSP, a broad spectrum inhibitor, including Mct8, reduced T-3 uptake further suggesting the cooperative activity of several T-3 transporters in astrocytes. (C)2010 Wiley-Liss, Inc.

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