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J Neurophysiol (November 2, 2005). doi:10.1152/jn.00499.2005
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Submitted on May 12, 2005
Accepted on October 26, 2005

Macrophage migration inhibitory factor (MIF) increases neuronal delayed rectifier K+ current

Tomokazu Matsuura1, Chengwen Sun1, Lin Leng2, Aphrodite Kapurniotu3, Jurgen Bernhagen3, Richard Bucala2, Anatoly E. Martynyuk4, and Colin Sumners1*

1 Physiology and Functional Genomics, University of Florida, Gainesville, Florida, USA
2 Medicine, Yale University School of Medicine, New Haven, Connecticut, USA
3 Biochemistry and Molecular Cell Biology, University Hospital RWTH Aachen, Aachen, Germany
4 Anesthesiology, University of Florida, Gainesville, Florida, USA

* To whom correspondence should be addressed. E-mail: csumners{at}phys.med.ufl.edu.

Macrophage migration inhibitory factor (MIF) has widespread actions in the immune, endocrine and nervous systems. Previously, we reported that increases in the intracellular levels of MIF depress the firing of hypothalamus/brainstem neurons in culture, including the chronotropic actions of angiotensin II (Ang II). The objective of this study was to investigate the effects of MIF on delayed rectifier K+ current (IKv), one of the component currents whose activity contributes to neuronal firing. Intracellular perfusion of MIF (80 nM) into Sprague Dawley rat neuronal cultures caused a significant increase in IKv, as measured by patch-clamp recordings. This effect was apparent by 3 minutes, and was maximal after 20-30 minutes. IKv current density (pA/pF) increased from 31.58 ± 2.36 in controls to 41.88 ± 3.76 in MIF-treated neurons (mean ± SE; n=9; p<0.01). MIF that had been inactivated by boiling did not alter IKv, and MIF-neutralizing antibodies abolished the action of rMIF. The stimulatory effect of MIF on IKv current density was mimicked by intracellular application of either P1S-MIF (80 nM) or the peptide MIF-(50-65) [0.8-8 µM], both of which harbor the thiol-protein oxidoreductase (TPOR) activity of the MIF molecule. Conversely, neither C60S-MIF (80 nM) nor the MIF homologue D-dopachrome tautomerase (DCT, 80 nM), both of which lack TPOR activity, altered IKv. Lastly, the increase in IKv produced by rMIF was abolished by the superoxide scavenger Tiron (1 mM). These studies indicate that the neuronal action of MIF includes a stimulatory action on IKv that may be mediated via a TPOR/superoxide-scavenging mechanism.




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