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  5. Pseudophosphatase STYX modulates cell-fate decisions and cell migration by spatiotemporal regulation of ERK1/2
 
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Pseudophosphatase STYX modulates cell-fate decisions and cell migration by spatiotemporal regulation of ERK1/2

Author(s)
Reiterer, V.  
Fey, Dirk  
Kolch, Walter  
et al.  
Uri
http://hdl.handle.net/10197/5567
Date Issued
2013-07-11
Date Available
2014-05-02T08:32:11Z
Abstract
Serine/threonine/tyrosine-interacting protein (STYX) is a catalytically inactive member of the dual-specificity phosphatases (DUSPs) family. Whereas the role of DUSPs in cellular signaling is well explored, the function of STYX is still unknown. Here, we identify STYX as a spatial regulator of ERK signaling. We used predictive-model simulation to test several hypotheses for possible modes of STYX action. We show that STYX localizes to the nucleus, competes with nuclear DUSP4 for binding to ERK, and acts as a nuclear anchor that regulates ERK nuclear export. Depletion of STYX increases ERK activity in both cytosol and nucleus. Importantly, depletion of STYX causes an ERK-dependent fragmentation of the Golgi apparatus and inhibits Golgi polarization and directional cell migration. Finally, we show that overexpression of STYX reduces ERK1/2 activation, thereby blocking PC12 cell differentiation. Overall, our results identify STYX as an important regulator of ERK1/2 signaling critical for cell migration and PC12 cell differentiation.
Type of Material
Journal Article
Publisher
National Academy of Sciences
Journal
Proceedings of the National Academy of Sciences
Volume
110
Issue
31
Start Page
E2934
End Page
E2943
Copyright (Published Version)
2013 National Academy of Sciences
Subjects

Computational modelin...

MAPK

DOI
10.1073/pnas.1301985110
Language
English
Status of Item
Peer reviewed
This item is made available under a Creative Commons License
https://creativecommons.org/licenses/by-nc-nd/3.0/ie/
File(s)
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Name

Paper215.pdf

Size

8.8 MB

Format

Adobe PDF

Checksum (MD5)

8eb03de1bec4c55eabcf68558306bbd5

Owning collection
SBI Research Collection
Mapped collections
Conway Institute Research Collection

Item descriptive metadata is released under a CC-0 (public domain) license: https://creativecommons.org/public-domain/cc0/.
All other content is subject to copyright.

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