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Identification of an imidazoline binding protein: Creatine kinase and an imidazoline-2 binding site

Drugs that bind to imidazoline binding proteins have major physiological actions. To date, three subtypes of such proteins, I(1), I(2) and I(3), have been proposed, although characterisations of these binding proteins are lacking. I(2) binding sites are found throughout the brain, particularly dense...

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Detalles Bibliográficos
Autores principales: Kimura, Atsuko, Tyacke, Robin J., Robinson, James J., Husbands, Stephen M., Minchin, Michael C.W., Nutt, David J., Hudson, Alan L.
Formato: Texto
Lenguaje:English
Publicado: Elsevier/North-Holland Biomedical Press 2009
Materias:
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC2722693/
https://www.ncbi.nlm.nih.gov/pubmed/19410564
http://dx.doi.org/10.1016/j.brainres.2009.04.044
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author Kimura, Atsuko
Tyacke, Robin J.
Robinson, James J.
Husbands, Stephen M.
Minchin, Michael C.W.
Nutt, David J.
Hudson, Alan L.
author_facet Kimura, Atsuko
Tyacke, Robin J.
Robinson, James J.
Husbands, Stephen M.
Minchin, Michael C.W.
Nutt, David J.
Hudson, Alan L.
author_sort Kimura, Atsuko
collection PubMed
description Drugs that bind to imidazoline binding proteins have major physiological actions. To date, three subtypes of such proteins, I(1), I(2) and I(3), have been proposed, although characterisations of these binding proteins are lacking. I(2) binding sites are found throughout the brain, particularly dense in the arcuate nucleus of the hypothalamus. Selective I(2) ligands demonstrate antidepressant-like activity and the identity of the proteins that respond to such ligands remained unknown until now. Here we report the isolation of a ∼ 45 kDa imidazoline binding protein from rabbit and rat brain using a high affinity ligand for the I(2) subtype, 2-BFI, to generate an affinity column. Following protein sequencing of the isolated ∼ 45 kDa imidazoline binding protein, we identified it to be brain creatine kinase (B-CK). B-CK shows high binding capacity to selective I(2) ligands; [(3)H]-2-BFI (5 nM) specifically bound to B-CK (2330 ± 815 fmol mg protein(− 1)). We predicted an I(2) binding pocket near the active site of B-CK using molecular modelling. Furthermore, B-CK activity was inhibited by a selective I(2) irreversible ligand, where 20 μM BU99006 reduced the enzyme activity by 16%, confirming the interaction between B-CK and the I(2) ligand. In summary, we have identified B-CK to be the ∼ 45 kDa imidazoline binding protein and we have demonstrated the existence of an I(2) binding site within this enzyme. The importance of B-CK in regulating neuronal activity and neurotransmitter release may well explain the various actions of I(2) ligands in brain and the alterations in densities of I(2) binding sites in psychiatric disorders.
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spelling pubmed-27226932009-08-18 Identification of an imidazoline binding protein: Creatine kinase and an imidazoline-2 binding site Kimura, Atsuko Tyacke, Robin J. Robinson, James J. Husbands, Stephen M. Minchin, Michael C.W. Nutt, David J. Hudson, Alan L. Brain Res Research Report Drugs that bind to imidazoline binding proteins have major physiological actions. To date, three subtypes of such proteins, I(1), I(2) and I(3), have been proposed, although characterisations of these binding proteins are lacking. I(2) binding sites are found throughout the brain, particularly dense in the arcuate nucleus of the hypothalamus. Selective I(2) ligands demonstrate antidepressant-like activity and the identity of the proteins that respond to such ligands remained unknown until now. Here we report the isolation of a ∼ 45 kDa imidazoline binding protein from rabbit and rat brain using a high affinity ligand for the I(2) subtype, 2-BFI, to generate an affinity column. Following protein sequencing of the isolated ∼ 45 kDa imidazoline binding protein, we identified it to be brain creatine kinase (B-CK). B-CK shows high binding capacity to selective I(2) ligands; [(3)H]-2-BFI (5 nM) specifically bound to B-CK (2330 ± 815 fmol mg protein(− 1)). We predicted an I(2) binding pocket near the active site of B-CK using molecular modelling. Furthermore, B-CK activity was inhibited by a selective I(2) irreversible ligand, where 20 μM BU99006 reduced the enzyme activity by 16%, confirming the interaction between B-CK and the I(2) ligand. In summary, we have identified B-CK to be the ∼ 45 kDa imidazoline binding protein and we have demonstrated the existence of an I(2) binding site within this enzyme. The importance of B-CK in regulating neuronal activity and neurotransmitter release may well explain the various actions of I(2) ligands in brain and the alterations in densities of I(2) binding sites in psychiatric disorders. Elsevier/North-Holland Biomedical Press 2009-07-07 /pmc/articles/PMC2722693/ /pubmed/19410564 http://dx.doi.org/10.1016/j.brainres.2009.04.044 Text en © 2009 Elsevier B.V. https://creativecommons.org/licenses/by/3.0/ Open Access under CC BY 3.0 (https://creativecommons.org/licenses/by/3.0/) license
spellingShingle Research Report
Kimura, Atsuko
Tyacke, Robin J.
Robinson, James J.
Husbands, Stephen M.
Minchin, Michael C.W.
Nutt, David J.
Hudson, Alan L.
Identification of an imidazoline binding protein: Creatine kinase and an imidazoline-2 binding site
title Identification of an imidazoline binding protein: Creatine kinase and an imidazoline-2 binding site
title_full Identification of an imidazoline binding protein: Creatine kinase and an imidazoline-2 binding site
title_fullStr Identification of an imidazoline binding protein: Creatine kinase and an imidazoline-2 binding site
title_full_unstemmed Identification of an imidazoline binding protein: Creatine kinase and an imidazoline-2 binding site
title_short Identification of an imidazoline binding protein: Creatine kinase and an imidazoline-2 binding site
title_sort identification of an imidazoline binding protein: creatine kinase and an imidazoline-2 binding site
topic Research Report
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC2722693/
https://www.ncbi.nlm.nih.gov/pubmed/19410564
http://dx.doi.org/10.1016/j.brainres.2009.04.044
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