Please use this identifier to cite or link to this item:
http://hdl.handle.net/1893/25191
Appears in Collections: | Faculty of Health Sciences and Sport Journal Articles |
Peer Review Status: | Refereed |
Title: | Multiple AMPK activators inhibit L-Carnitine uptake in C2C12 skeletal muscle myotubes |
Author(s): | Shaw, Andy Jeromson, Stewart Watterson, Kenneth R Pediani, John D Gallagher, Iain J Whalley, Tim Dreczkowski, Gillian Brooks, Naomi Galloway, S D Hamilton, David Lee |
Contact Email: | d.l.hamilton@stir.ac.uk |
Issue Date: | Jun-2017 |
Date Deposited: | 23-Mar-2017 |
Citation: | Shaw A, Jeromson S, Watterson KR, Pediani JD, Gallagher IJ, Whalley T, Dreczkowski G, Brooks N, Galloway SD & Hamilton DL (2017) Multiple AMPK activators inhibit L-Carnitine uptake in C2C12 skeletal muscle myotubes. American Journal of Physiology - Cell Physiology, 312 (6), pp. C689-C696. https://doi.org/10.1152/ajpcell.00026.2016 |
Abstract: | Mutations in the gene that encodes the principal L-Carnitine transporter, OCTN2, can lead to a reduced intracellular L-Carnitine pool and the disease Primary Carnitine Deficiency. L-Carnitine supplementation is used therapeutically to increase intracellular L-Carnitine. As AMPK and insulin regulate fat metabolism and substrate uptake we hypothesised that AMPK activating compounds and insulin would increase L-Carnitine uptake in C2C12myotubes. The cells express all three OCTN transporters at the mRNA level and immunohistochemistry confirmed expression at the protein level. Contrary to our hypothesis, despite significant activation of PKB and 2DG uptake, insulin did not increase L-Carnitine uptake at 100nM. However, L-Carnitine uptake was modestly increased at a dose of 150nM insulin. A range of AMPK activators that increase intracellular calcium content [caffeine (10mM, 5mM, 1mM, 0.5mM), A23187 (10μM)], inhibit mitochondrial function [Sodium Azide (75μM), Rotenone (1μM), Berberine (100μM), DNP (500μM)] or directly activate AMPK [AICAR (250μM)] were assessed for their ability to regulate L-Carnitine uptake. All compounds tested significantly inhibited L-Carnitine uptake. Inhibition by caffeine was not dantrolene (10μM) sensitive. Saturation curve analysis suggested that caffeine did not competitively inhibit L-Carnitine transport. However, the AMPK inhibitor Compound C (10μM) partially rescued the effect of caffeine suggesting that AMPK may play a role in the inhibitory effects of caffeine. However, caffeine likely inhibits L-Carnitine uptake by alternative mechanisms independently of calcium release. PKA activation or direct interference with transporter function may play a role. |
DOI Link: | 10.1152/ajpcell.00026.2016 |
Rights: | This item has been embargoed for a period. During the embargo please use the Request a Copy feature at the foot of the Repository record to request a copy directly from the author. You can only request a copy if you wish to use this work for your own research or private study. Publisher policy allows this work to be made available in this repository. Published in American Journal of Physiology - Cell Physiology, 2017, Vol. 312 no. 6, C689-C696 by American Physiological Society. The original publication is available at: https://doi.org/10.1152/ajpcell.00026.2016 |
Files in This Item:
File | Description | Size | Format | |
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93385_1_merged_1487700847.pdf | Fulltext - Accepted Version | 5.83 MB | Adobe PDF | View/Open |
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