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Microtubule stabilization drives 3D centrosome migration to initiate primary ciliogenesis

Amandine Pitaval, Fabrice Senger, Gaëlle Letort, Xavier Gidrol, Laurent Guyon, James Sillibourne, Manuel Théry
doi: https://doi.org/10.1101/080556
Amandine Pitaval
1Univ. Grenoble-Alpes, CEA, INSERM, Biosciences & Biotechnology Institute of Grenoble, UMR_S 1038, Biomics Lab, 38054, Grenoble, France.
2Univ. Grenoble-Alpes CEA, INRA, CNRS, Biosciences & Biotechnology Institute of Grenoble, UMR5168, CytoMorpho Lab, 38054, Grenoble, France.
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Fabrice Senger
2Univ. Grenoble-Alpes CEA, INRA, CNRS, Biosciences & Biotechnology Institute of Grenoble, UMR5168, CytoMorpho Lab, 38054, Grenoble, France.
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Gaëlle Letort
2Univ. Grenoble-Alpes CEA, INRA, CNRS, Biosciences & Biotechnology Institute of Grenoble, UMR5168, CytoMorpho Lab, 38054, Grenoble, France.
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Xavier Gidrol
1Univ. Grenoble-Alpes, CEA, INSERM, Biosciences & Biotechnology Institute of Grenoble, UMR_S 1038, Biomics Lab, 38054, Grenoble, France.
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Laurent Guyon
3Univ. Grenoble-Alpes, CEA, INSERM, Biosciences & Biotechnology Institute of Grenoble, Biology of Cancer and Infection UMR_S 1036, 38054, Grenoble, France.
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James Sillibourne
2Univ. Grenoble-Alpes CEA, INRA, CNRS, Biosciences & Biotechnology Institute of Grenoble, UMR5168, CytoMorpho Lab, 38054, Grenoble, France.
3Univ. Grenoble-Alpes, CEA, INSERM, Biosciences & Biotechnology Institute of Grenoble, Biology of Cancer and Infection UMR_S 1036, 38054, Grenoble, France.
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  • For correspondence: sillibou@gmail.com manuel.thery@cea.fr
Manuel Théry
2Univ. Grenoble-Alpes CEA, INRA, CNRS, Biosciences & Biotechnology Institute of Grenoble, UMR5168, CytoMorpho Lab, 38054, Grenoble, France.
4Univ. Paris Diderot, INSERM, Hopital Saint Louis, Institut Universitaire d’Hematologie, UMRS1160, CytoMorpho Lab, 75010, Paris, France.
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  • For correspondence: sillibou@gmail.com manuel.thery@cea.fr
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Abstract

Primary cilia are sensory organelles located at the cell surface. Their assembly is primed by centrosome migration to the apical surface. Yet surprisingly little is known about this initiating step. To gain insight into the mechanisms driving centrosome migration, we exploited the reproducibility of cell architecture on adhesive micropatterns to investigate the cytoskeletal remodeling supporting it. Microtubule network densification and bundling, with the transient formation of an array of cold-stable microtubules, and actin cytoskeleton asymmetric contraction participated in concert to destabilize basal centrosome position and drive apical centrosome migration. The distal appendage protein Cep164 appeared to be a key actor involved in the cytoskeleton remodeling and centrosome migration, whereas IFT88's role seemed to be restricted to axoneme elongation. Together our data elucidate the hitherto unexplored mechanism of centrosome migration and show that it is driven by the increase and clustering of mechanical forces to push the centrosome toward the cell apical pole.

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The copyright holder for this preprint is the author/funder, who has granted bioRxiv a license to display the preprint in perpetuity. It is made available under a CC-BY-NC-ND 4.0 International license.
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Posted May 18, 2017.
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Microtubule stabilization drives 3D centrosome migration to initiate primary ciliogenesis
Amandine Pitaval, Fabrice Senger, Gaëlle Letort, Xavier Gidrol, Laurent Guyon, James Sillibourne, Manuel Théry
bioRxiv 080556; doi: https://doi.org/10.1101/080556
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Microtubule stabilization drives 3D centrosome migration to initiate primary ciliogenesis
Amandine Pitaval, Fabrice Senger, Gaëlle Letort, Xavier Gidrol, Laurent Guyon, James Sillibourne, Manuel Théry
bioRxiv 080556; doi: https://doi.org/10.1101/080556

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