Posttranslational modification of voltage-dependent potassium channel Kv1.5: COOH-terminal palmitoylation modulates its biological properties

doi:10.1152/ajpheart.01374.2007

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Am J Physiol Heart Circ Physiol 294: H2012-H2021, 2008. First published March 14, 2008; doi:10.1152/ajpheart.01374.2007
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TRANSLATIONAL PHYSIOLOGY

Posttranslational modification of voltage-dependent potassium channel Kv1.5: COOH-terminal palmitoylation modulates its biological properties

Hitesh K. Jindal,¹^,* Eduardo J. Folco,²^,* Gong Xin Liu,¹ and Gideon Koren¹

¹Division of Cardiology, Cardiovascular Research Center, Rhode Island Hospital, Warren Alpert Medical School of Brown University, Providence, Rhode Island; and ²Cardiovascular Division, Brigham and Women's Hospital, Boston, Massachusetts

Submitted 27 November 2007 ; accepted in final form 14 March 2008

The physiological function of ion channels is affected by protein-proteinand protein-membrane interactions that modulate their activityand/or localization. Palmitoylation modulates protein functionby facilitating targeted membrane association, interaction withother proteins, and determining subcellular localization. Inthis study, we demonstrate that the voltage-dependent potassium(Kv) channel Kv1.5 is palmitoylated and that the mutation ofCOOH-terminal cysteines is sufficient to abolish the palmitoylationof the Kv1.5 polypeptide in Chinese hamster ovary (CHO) cells.The labeling represented the thioester linkage of the labeledpalmitic acid to cysteine rather than amide and oxygen esterlinkages as judged by the release of the palmitic acid uponthe treatment of the gel with hydroxylamine at a neutral pH.Site-directed mutagenesis and radiolabeling studies revealedthat C593 was the sole site of palmitoylation. The elucidationof the biological function of palmitoylation revealed that theexpression of the FLAG-Kv1.5 palmitoylation-deficient mutant(FL-Kv1.5^Palm–) in stable CHO cells increased membraneexpression as determined by the biotinylation of surface proteinsand quantitative immunofluorescence analyses of these cells,in turn enhancing the outward potassium current. This enhancedsurface expression and the currents were consequential to theslower rate of internalization, causing an increased localizationof FL-Kv1.5^Palm– in the plasma membrane compared withthe wild-type FL-Kv1.5 channels. We conclude that the Kv1.5channel is palmitoylated and that its palmitoylation modulatesits biological functions and, therefore, might provide a physiologicallink between the metabolic state and the expression of Kv1.5on the plasma membrane.

internalization; trafficking

Address for reprint requests and other correspondence: G. Koren, Cardiovascular Research Center, Rhode Island Hospital, Brown Univ. School of Medicine, 1 Hoppin St., West Coro-5, Providence, RI 02903 (e-mail: Gideon_Koren{at}Brown.edu)