The WNK-regulated SPAK/OSR1 kinases directly phosphorylate and inhibit the K(+)–Cl(−) co-transporters

Precise homoeostasis of the intracellular concentration of Cl(−) is achieved via the co-ordinated activities of the Cl(−) influx and efflux. We demonstrate that the WNK (WNK lysine-deficient protein kinase)-activated SPAK (SPS1-related proline/alanine-rich kinase)/OSR1 (oxidative stress-responsive k...

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Autores principales: delos Heros, Paola, Alessi, Dario R., Gourlay, Robert, Campbell, David G., Deak, Maria, Macartney, Thomas J., Kahle, Kristopher T., Zhang, Jinwei
Formato: Online Artículo Texto
Lenguaje:English
Publicado: Portland Press Ltd. 2014
Materias:
Research Article
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC3940040/
https://www.ncbi.nlm.nih.gov/pubmed/24393035
http://dx.doi.org/10.1042/BJ20131478
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author delos Heros, Paola
Alessi, Dario R.
Gourlay, Robert
Campbell, David G.
Deak, Maria
Macartney, Thomas J.
Kahle, Kristopher T.
Zhang, Jinwei
author_facet delos Heros, Paola
Alessi, Dario R.
Gourlay, Robert
Campbell, David G.
Deak, Maria
Macartney, Thomas J.
Kahle, Kristopher T.
Zhang, Jinwei
author_sort delos Heros, Paola
collection PubMed
description Precise homoeostasis of the intracellular concentration of Cl(−) is achieved via the co-ordinated activities of the Cl(−) influx and efflux. We demonstrate that the WNK (WNK lysine-deficient protein kinase)-activated SPAK (SPS1-related proline/alanine-rich kinase)/OSR1 (oxidative stress-responsive kinase 1) known to directly phosphorylate and stimulate the N[K]CCs (Na(+)–K(+) ion co-transporters), also promote inhibition of the KCCs (K(+)–Cl(−) co-transporters) by directly phosphorylating a recently described C-terminal threonine residue conserved in all KCC isoforms [Site-2 (Thr(1048))]. First, we demonstrate that SPAK and OSR1, in the presence of the MO25 regulatory subunit, robustly phosphorylates all KCC isoforms at Site-2 in vitro. Secondly, STOCK1S-50699, a WNK pathway inhibitor, suppresses SPAK/OSR1 activation and KCC3A Site-2 phosphorylation with similar efficiency. Thirdly, in ES (embryonic stem) cells lacking SPAK/OSR1 activity, endogenous phosphorylation of KCC isoforms at Site-2 is abolished and these cells display elevated basal activity of (86)Rb(+) uptake that was not markedly stimulated further by hypotonic high K(+) conditions, consistent with KCC3A activation. Fourthly, a tight correlation exists between SPAK/OSR1 activity and the magnitude of KCC3A Site-2 phosphorylation. Lastly, a Site-2 alanine KCC3A mutant preventing SPAK/OSR1 phosphorylation exhibits increased activity. We also observe that KCCs are directly phosphorylated by SPAK/OSR1, at a novel Site-3 (Thr(5) in KCC1/KCC3 and Thr(6) in KCC2/KCC4), and a previously recognized KCC3-specific residue, Site-4 (Ser(96)). These data demonstrate that the WNK-regulated SPAK/OSR1 kinases directly phosphorylate the N[K]CCs and KCCs, promoting their stimulation and inhibition respectively. Given these reciprocal actions with anticipated net effects of increasing Cl(−) influx, we propose that the targeting of WNK–SPAK/OSR1 with kinase inhibitors might be a novel potent strategy to enhance cellular Cl(−) extrusion, with potential implications for the therapeutic modulation of epithelial and neuronal ion transport in human disease states.
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spelling pubmed-39400402014-03-12 The WNK-regulated SPAK/OSR1 kinases directly phosphorylate and inhibit the K(+)–Cl(−) co-transporters delos Heros, Paola Alessi, Dario R. Gourlay, Robert Campbell, David G. Deak, Maria Macartney, Thomas J. Kahle, Kristopher T. Zhang, Jinwei Biochem J Research Article Precise homoeostasis of the intracellular concentration of Cl(−) is achieved via the co-ordinated activities of the Cl(−) influx and efflux. We demonstrate that the WNK (WNK lysine-deficient protein kinase)-activated SPAK (SPS1-related proline/alanine-rich kinase)/OSR1 (oxidative stress-responsive kinase 1) known to directly phosphorylate and stimulate the N[K]CCs (Na(+)–K(+) ion co-transporters), also promote inhibition of the KCCs (K(+)–Cl(−) co-transporters) by directly phosphorylating a recently described C-terminal threonine residue conserved in all KCC isoforms [Site-2 (Thr(1048))]. First, we demonstrate that SPAK and OSR1, in the presence of the MO25 regulatory subunit, robustly phosphorylates all KCC isoforms at Site-2 in vitro. Secondly, STOCK1S-50699, a WNK pathway inhibitor, suppresses SPAK/OSR1 activation and KCC3A Site-2 phosphorylation with similar efficiency. Thirdly, in ES (embryonic stem) cells lacking SPAK/OSR1 activity, endogenous phosphorylation of KCC isoforms at Site-2 is abolished and these cells display elevated basal activity of (86)Rb(+) uptake that was not markedly stimulated further by hypotonic high K(+) conditions, consistent with KCC3A activation. Fourthly, a tight correlation exists between SPAK/OSR1 activity and the magnitude of KCC3A Site-2 phosphorylation. Lastly, a Site-2 alanine KCC3A mutant preventing SPAK/OSR1 phosphorylation exhibits increased activity. We also observe that KCCs are directly phosphorylated by SPAK/OSR1, at a novel Site-3 (Thr(5) in KCC1/KCC3 and Thr(6) in KCC2/KCC4), and a previously recognized KCC3-specific residue, Site-4 (Ser(96)). These data demonstrate that the WNK-regulated SPAK/OSR1 kinases directly phosphorylate the N[K]CCs and KCCs, promoting their stimulation and inhibition respectively. Given these reciprocal actions with anticipated net effects of increasing Cl(−) influx, we propose that the targeting of WNK–SPAK/OSR1 with kinase inhibitors might be a novel potent strategy to enhance cellular Cl(−) extrusion, with potential implications for the therapeutic modulation of epithelial and neuronal ion transport in human disease states. Portland Press Ltd. 2014-02-28 2014-03-15 /pmc/articles/PMC3940040/ /pubmed/24393035 http://dx.doi.org/10.1042/BJ20131478 Text en © 2014 The author(s) has paid for this article to be freely available under the terms of the Creative Commons Attribution Licence (CC-BY)(http://creativecommons.org/licenses/by/3.0/) which permits unrestricted use, distribution and reproduction in any medium, provided the original work is properly cited. http://creativecommons.org/licenses/by/3.0/ This is an open-access article distributed under the terms of the Creative Commons Attribution License, which permits unrestricted use, distribution and reproduction in any medium, provided the original work is properly cited.
spellingShingle Research Article
delos Heros, Paola
Alessi, Dario R.
Gourlay, Robert
Campbell, David G.
Deak, Maria
Macartney, Thomas J.
Kahle, Kristopher T.
Zhang, Jinwei
The WNK-regulated SPAK/OSR1 kinases directly phosphorylate and inhibit the K(+)–Cl(−) co-transporters
title The WNK-regulated SPAK/OSR1 kinases directly phosphorylate and inhibit the K(+)–Cl(−) co-transporters
title_full The WNK-regulated SPAK/OSR1 kinases directly phosphorylate and inhibit the K(+)–Cl(−) co-transporters
title_fullStr The WNK-regulated SPAK/OSR1 kinases directly phosphorylate and inhibit the K(+)–Cl(−) co-transporters
title_full_unstemmed The WNK-regulated SPAK/OSR1 kinases directly phosphorylate and inhibit the K(+)–Cl(−) co-transporters
title_short The WNK-regulated SPAK/OSR1 kinases directly phosphorylate and inhibit the K(+)–Cl(−) co-transporters
title_sort wnk-regulated spak/osr1 kinases directly phosphorylate and inhibit the k(+)–cl(−) co-transporters
topic Research Article
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC3940040/
https://www.ncbi.nlm.nih.gov/pubmed/24393035
http://dx.doi.org/10.1042/BJ20131478
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