A novel regulatory locus of phosphorylation in the C terminus of the potassium chloride cotransporter KCC2 that interferes with N-ethylmaleimide or staurosporine-mediated activation

Maren Weber; Anna-Maria Hartmann; Timo Beyer; Anne Ripperger; Hans Gerd Nothwang

doi:10.1074/jbc.M114.567834

A novel regulatory locus of phosphorylation in the C terminus of the potassium chloride cotransporter KCC2 that interferes with N-ethylmaleimide or staurosporine-mediated activation

J Biol Chem. 2014 Jul 4;289(27):18668-79. doi: 10.1074/jbc.M114.567834. Epub 2014 May 21.

Authors

Maren Weber¹, Anna-Maria Hartmann², Timo Beyer¹, Anne Ripperger¹, Hans Gerd Nothwang³

Affiliations

¹ From the Neurogenetics Group, Center of Excellence Hearing4All, School of Medicine and Health Sciences.
² From the Neurogenetics Group, Center of Excellence Hearing4All, School of Medicine and Health Sciences, Systematics and Evolutionary Biology Group, Institute for Biology and Environmental Sciences, and.
³ From the Neurogenetics Group, Center of Excellence Hearing4All, School of Medicine and Health Sciences, the Research Center for Neurosensory Sciences, Carl von Ossietzky University Oldenburg, 26111 Oldenburg, Germany hans.g.nothwang@uni-oldenburg.de.

Abstract

The neuron-specific cation chloride cotransporter KCC2 plays a crucial role in hyperpolarizing synaptic inhibition. Transporter dysfunction is associated with various neurological disorders, raising interest in regulatory mechanisms. Phosphorylation has been identified as a key regulatory process. Here, we retrieved experimentally observed phosphorylation sites of KCC2 from public databases and report on the systematic analysis of six phosphorylated serines, Ser(25), Ser(26), Ser(937), Ser(1022), Ser(1025), and Ser(1026). Alanine or aspartate substitutions of these residues were analyzed in HEK-293 cells. All mutants were expressed in a pattern similar to wild-type KCC2 (KCC2(WT)). Tl(+) flux measurements demonstrated unchanged transport activity for Ser(25), Ser(26), Ser(1022), Ser(1025), and Ser(1026) mutants. In contrast, KCC2(S937D), mimicking phosphorylation, resulted in a significant up-regulation of transport activity. Aspartate substitution of Thr(934), a neighboring putative phosphorylation site, resulted in a comparable increase in KCC2 transport activity. Both KCC2(T934D) and KCC2(S937D) mutants were inhibited by the kinase inhibitor staurosporine and by N-ethylmaleimide, whereas KCC2(WT), KCC2(T934A), and KCC2(S937A) were activated. The inverse staurosporine effect on aspartate versus alanine substitutions reveals a cross-talk between different phosphorylation sites of KCC2. Immunoblot and cell surface labeling experiments detected no alterations in total abundance or surface expression of KCC2(T934D) and KCC2(S937D) compared with KCC2(WT). These data reveal kinetic regulation of transport activity by these residues. In summary, our data identify a novel key regulatory phosphorylation site of KCC2 and a functional interaction between different conformation-changing post-translational modifications. The action of pharmacological agents aimed to modulate KCC2 activity for therapeutic benefit might therefore be highly context-specific.

Keywords: Cation Chloride Cotransporter; Cell Culture; Chloride Transport; Evolution; Mutation; Neurophysiology; Phosphorylation; Post-translational Modification; Protein Conformation.

Publication types

Research Support, Non-U.S. Gov't

MeSH terms

Amino Acid Sequence
Amino Acid Substitution
Animals
Binding Sites
Data Mining
Databases, Protein
Ethylmaleimide / pharmacology*
Gene Expression Regulation / drug effects
HEK293 Cells
Humans
K Cl- Cotransporters
Mice
Molecular Sequence Data
Mutation
Phosphoproteins / chemistry
Phosphoproteins / genetics
Phosphoproteins / metabolism
Phosphorylation / drug effects
Phylogeny
Protein Transport / drug effects
Rats
Staurosporine / pharmacology*
Symporters / chemistry
Symporters / genetics
Symporters / metabolism*

Substances

Phosphoproteins
Symporters
Staurosporine
Ethylmaleimide