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Evidence for disulfide bonds in SR Protein Kinase 1 (SRPK1) that are required for activity and nuclear localization

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Συγγραφέας
Koutroumani M., Papadopoulos G.E., Vlassi M., Nikolakaki E., Giannakouros T.
Ημερομηνία
2017
Γλώσσα
en
DOI
10.1371/journal.pone.0171328
Λέξη-κλειδί
cysteine
protein serine kinase
recombinant protein
serine arginine protein kinase 1
unclassified drug
disulfide
protein serine threonine kinase
SRPK1 protein, human
Article
catalysis
controlled study
disulfide bond
enzyme activity
enzyme conformation
enzyme localization
enzyme structure
HeLa cell line
human
human cell
immunofluorescence microscopy
mutant
plasmid
polyacrylamide gel electrophoresis
protein domain
protein interaction
protein processing
reporter gene
RNA splicing
stress
Western blotting
amino acid sequence
cell line
cell nucleus
chemistry
enzyme activation
gene expression
genetics
metabolism
molecular model
mutation
protein conformation
protein transport
Amino Acid Sequence
Cell Line
Cell Nucleus
Disulfides
Enzyme Activation
Gene Expression
Genes, Reporter
Humans
Models, Molecular
Mutation
Protein Conformation
Protein Processing, Post-Translational
Protein Transport
Protein-Serine-Threonine Kinases
RNA Splicing
Public Library of Science
Εμφάνιση Μεταδεδομένων
Επιτομή
Serine/arginine protein kinases (SRPKs) phosphorylate Arg/Ser dipeptide-containing proteins that play crucial roles in a broad spectrum of basic cellular processes. The existence of a large internal spacer sequence that separates the bipartite kinase catalytic core is a unique structural feature of SRPKs. Previous structural studies on a catalytically active fragment of SRPK1, which lacks the main part of the spacer domain, revealed that SRPK1 remains in an active state without any post-translational modifications or specific intra-protein interactions, while the spacer domain is depicted as a loop structure, outside the kinase core. Using systematic mutagenesis we now provide evidence that replacement of any individual cysteine residue in the spacer, apart from Cys414, or in its proximal flaking ends of the two kinase catalytic domains has an impact on kinase activity. Furthermore, the cysteine residues are critical for nuclear translocation of SRPK1 in response to genotoxic stress and SRPK1-dependent splicing of a reporter gene. While replacement of Cys207, Cys502 and Cys539 of the catalytic domains is predicted to distort the kinase active structure, our findings suggest that Cys356, Cys386, Cys427 and Cys455 of the spacer domain and Cys188 of the first catalytic domain are engaged in disulfide bridging. We propose that such a network of intramolecular disulfide bonds mediates the bending of the spacer region thus allowing the proximal positioning of the two catalytic subunits which is a prerequisite for SRPK1 activity. © 2017 Koutroumani et al. 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 author and source are credited.
URI
http://hdl.handle.net/11615/75400
Collections
  • Δημοσιεύσεις σε περιοδικά, συνέδρια, κεφάλαια βιβλίων κλπ. [19735]

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