Negative regulation of EB1 turnover at microtubule plus ends by interaction with microtubule-associated protein ATIP3

Lauriane Velot; Angie Molina; Sylvie Rodrigues-Ferreira; Anne Nehlig; Benjamin Pierre Bouchet; Marina Morel; Ludovic Leconte; Laurence Serre; Isabelle Arnal; Diane Braguer; Ariel Savina; Stéphane Honore; Clara Nahmias

doi:10.18632/oncotarget.6196

Oncotarget

Oncotarget (a primarily oncology-focused, peer-reviewed, open access journal) aims to maximize research impact through insightful peer-review; eliminate borders between specialties by linking different fields of oncology, cancer research and biomedical sciences; and foster application of basic and clinical science.

Its scope is unique. The term "oncotarget" encompasses all molecules, pathways, cellular functions, cell types, and even tissues that can be viewed as targets relevant to cancer as well as other diseases. The term was introduced in the inaugural Editorial, Introducing Oncotarget.

As of January 1, 2022, Oncotarget has shifted to a continuous publishing model. Papers will now be published continuously within yearly volumes in their final and complete form and then quickly released to Pubmed.

Subscribe to receive alerts once a paper has been published by Oncotarget.

Impact Journals, LLC is the publisher of Oncotarget: www.impactjournals.com.

Impact Journals is a member of the Wellcome Trust List of Compliant Publishers.

Impact Journals is a member of the Society for Scholarly Publishing.

On December 23, 2022, Oncotarget server experienced a DDoS attack. As a result, Oncotarget site was inaccessible for a few hours. Oncotarget team swiftly dealt with the situation and took it under control. This malicious action will be reported to the FBI.

Research Papers:

Negative regulation of EB1 turnover at microtubule plus ends by interaction with microtubule-associated protein ATIP3

Lauriane Velot, Angie Molina, Sylvie Rodrigues-Ferreira, Anne Nehlig, Benjamin Pierre Bouchet, Marina Morel, Ludovic Leconte, Laurence Serre, Isabelle Arnal, Diane Braguer, Ariel Savina, Stéphane Honore and Clara Nahmias _

PDF | HTML | Supplementary Files | How to cite

Oncotarget. 2015; 6:43557-43570. https://doi.org/10.18632/oncotarget.6196

Metrics: PDF 2156 views | HTML 3828 views | ?

Abstract

Lauriane Velot1,2,3,*, Angie Molina1,2,3,*, Sylvie Rodrigues-Ferreira1,2,3, Anne Nehlig1,2, Benjamin Pierre Bouchet4, Marina Morel3, Ludovic Leconte5, Laurence Serre6, Isabelle Arnal6, Diane Braguer7,8, Ariel Savina9, Stéphane Honore7,8 and Clara Nahmias1,2,3

1 Inserm U981, Institut Gustave Roussy Department of Molecular Medicine, Villejuif, France

2 Université Paris-Saclay, Villejuif, France

3 CNRS UMR8104, Institut Cochin, Paris, France

4 Cell Biology, Faculty of Science, Utrecht University, Padualaan, CH Utrecht, The Netherlands

5 Cell and Tissue Imaging Core Facilty, PICT-IBiSA, CNRS UMR144 Institut Curie, Centre de Recherche, Paris, France

6 Inserm U836, Grenoble Institut des Neurosciences, Grenoble, France

7 Aix Marseille Université, Inserm, CRO2 UMR_S 911, Marseille, France

8 APHM, Hôpital Timone, Marseille, France

9 Scientific Partnerships Roche SAS, Boulogne Billancourt, France

* These authors have contributed equally to this work

Correspondence to:

Clara Nahmias, email:

Keywords: EB1, MTUS1, protein interaction, +TIP, microtubule dynamics

Received: May 07, 2015 Accepted: October 14, 2015 Published: October 20, 2015

Abstract

The regulation of microtubule dynamics is critical to ensure essential cell functions. End binding protein 1 (EB1) is a master regulator of microtubule dynamics that autonomously binds an extended GTP/GDP-Pi structure at growing microtubule ends and recruits regulatory proteins at this location. However, negative regulation of EB1 association with growing microtubule ends remains poorly understood. We show here that microtubule-associated tumor suppressor ATIP3 interacts with EB1 through direct binding of a non-canonical proline-rich motif. Results indicate that ATIP3 does not localize at growing microtubule ends and that in situ ATIP3-EB1 molecular complexes are mostly detected in the cytosol. We present evidence that a minimal EB1-interacting sequence of ATIP3 is both necessary and sufficient to prevent EB1 accumulation at growing microtubule ends in living cells and that EB1-interaction is involved in reducing cell polarity. By fluorescence recovery of EB1-GFP after photobleaching, we show that ATIP3 silencing accelerates EB1 turnover at microtubule ends with no modification of EB1 diffusion in the cytosol. We propose a novel mechanism by which ATIP3-EB1 interaction indirectly reduces the kinetics of EB1 exchange on its recognition site, thereby accounting for negative regulation of microtubule dynamic instability. Our findings provide a unique example of decreased EB1 turnover at growing microtubule ends by cytosolic interaction with a tumor suppressor.

All site content, except where otherwise noted, is licensed under a Creative Commons Attribution 4.0 License.
PII: 6196

Publication Alerts

Research Papers:

Negative regulation of EB1 turnover at microtubule plus ends by interaction with microtubule-associated protein ATIP3

Abstract