Please use this identifier to cite or link to this item: http://hdl.handle.net/11452/25400
Title: Mechanism of S100b release from rat cortical slices determined under basal and stimulated conditions
Authors: Uludağ Üniversitesi/Tıp Fakültesi/Tıbbi Farmakoloji Anabilim Dalı.
Gürsoy, Murat
Büyükuysal, Rıfat Levent
AAH-1657-2021
57197640824
6602686612
Keywords: S100B release
Oxygen-glucose deprivation (OGD)
Re-oxygenation
Protein-kinase-C
Delayed neuronal injury
In-vitro trauma
Cerebral-ischemia
Brain-slices
Hippocampal-neurons
Damage
Secretion
Glutamate
Toxicity
Biochemistry & molecular biology
Neurosciences & neurology
Rattus
Issue Date: Mar-2010
Publisher: Springer/Plenum Publishers
Citation: Gürsoy, M. ve Büyükuysal, R. L. (2010). "Mechanism of S100b release from rat cortical slices determined under basal and stimulated conditions". Neurochemical Research, 35(3), 429-436.
Abstract: Incubation of rat cortical slices in a medium that was not containing oxygen and glucose (oxygen-glucose deprivation, OGD) caused a 200% increase in the release of S100B. However, when slices were transferred to a medium containing oxygen and glucose (reoxygenation conditions, or REO), S100B release reached 500% of its control value. Neither inhibition of nitric oxide (NO) synthase by L-NAME nor addition of the NO donors sodium nitroprussid (SNP) or hydroxylamine (HA) to the medium altered basal S100B release. Similarly, the presence of SNP, HA or NO precursor l-arginine in the medium, or inhibition of NO synthase by L-NAME also failed to alter OGD- and REO-induced S100B outputs. Moreover, individual inhibition of PKC, PLA(2) or PLC all failed to attenuate the S100B release determined under control condition or enhanced by either OGD or REO. Blockade of calcium channels with verapamil, chelating the Ca+2 ions with BAPTA or blockade of sodium channels with tetrodotoxin (TTX) did not alter OGD- and REO-induced S100B release. In contrast to the pharmacologic manipulations mentioned above, glutamate and alpha-ketoglutarate added at high concentrations to the medium prevented both OGD- and REO-induced S100B outputs. These results indicate that neither NO nor the activation of PKC, PLA(2) or PLC seem to be involved in basal or OGD- and REO-induced S100B outputs. Additionally, calcium and sodium currents that are sensitive to verapamil and TTX, respectively, are unlikely to contribute to the enhanced S100B release observed under these conditions.
URI: https://doi.org/10.1007/s11064-009-0075-9
https://link.springer.com/article/10.1007/s11064-009-0075-9
http://hdl.handle.net/11452/25400
ISSN: 0364-3190
1573-6903
Appears in Collections:PubMed
Scopus
Web of Science

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