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Published November 3, 2014 | Published + Supplemental Material
Journal Article Open

Plk4 Phosphorylates Ana2 to Trigger Sas6 Recruitment and Procentriole Formation

Dzhindzhev, Nikola S.
Tzolovsky, George
Lipinszki, Zoltan ORCID icon
Schneider, Sandra
Lattao, Ramona ORCID icon
Fu, Jingyan ORCID icon
Debski, Janusz ORCID icon
Dadlez, Michal ORCID icon
Glover, David M. ORCID icon

Abstract

Centrioles are 9-fold symmetrical structures at the core of centrosomes and base of cilia whose dysfunction has been linked to a wide range of inherited diseases and cancer [1]. Their duplication is regulated by a protein kinase of conserved structure, the C. elegans ZYG-1 or its Polo-like kinase 4 (Plk4) counterpart in other organisms [2, 3, 4]. Although Plk4's centriolar partners and mechanisms that regulate its stability are known, its crucial substrates for centriole duplication have never been identified. Here we show that Drosophila Plk4 phosphorylates four conserved serines in the STAN motif of the core centriole protein Ana2 to enable it to bind and recruit its Sas6 partner. Ana2 and Sas6 normally load onto both mother and daughter centrioles immediately after their disengagement toward the end of mitosis to seed procentriole formation. Nonphosphorylatable Ana2 still localizes to the centriole but can no longer recruit Sas6 and centriole duplication fails. Thus, following centriole disengagement, recruitment of Ana2 and its phosphorylation by Plk4 are the earliest known events in centriole duplication to recruit Sas6 and thereby establish the architecture of the new procentriole engaged with its parent.

Additional Information

© 2014 The Authors. This is an open access article under the CC BY license (http://creativecommons.org/licenses/by/3.0/). Received 18 July 2014, Revised 13 August 2014, Accepted 27 August 2014, Available online 25 September 2014. N.S.D., Z.L., R.L., J.F., and S.S. are supported from a Programme Grant to D.M.G. from Cancer Research UK. G.T. is supported from an MRC Programme Grant to D.M.G. M.D. is grateful for a Harmonia 5 Grant (2013/10/M/NZ2/00298) from the Polish National Science Center for collaboration with the D.M.G. lab. Z.L. is grateful for the Federation of European Biochemical Societies for the Long-term post-doctoral Fellowship and R.L. thanks the fellowship support received from Fondazione Italiana per la Ricerca sul Cancro. The authors are thankful for the Drosophila Genomics Resource Centre (supported by NIH grant 2P40OD010949-10A1) for the cDNA clones and Drosophila gateway destination vectors.

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Published - 1-s2.0-S0960982214010744-main.pdf

Supplemental Material - 1-s2.0-S0960982214010744-mmc1.pdf

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Additional details

Identifiers Funding Dates
Created:
August 20, 2023
Modified:
October 20, 2023