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Centrosomal and ciliary targeting of CCDC66 requires cooperative action of centriolar satellites, microtubules and molecular motors

  • Deniz Conkar
  • , Halil Bayraktar
  • , Elif Nur Firat-Karalar*
  • *Bu çalışma için yazışmadan sorumlu yazar

Araştırma sonucu: Dergiye katkıMakalebilirkişi

31 Atıf (Scopus)

Özet

Mammalian centrosomes and cilia play key roles in many cellular processes and their deregulation is linked to cancer and ciliopathies. Spatiotemporal regulation of their biogenesis and function in response to physiological stimuli requires timely protein targeting. This can occur by different pathways, including microtubule-dependent active transport and via centriolar satellites, which are key regulators of cilia assembly and signaling. How satellites mediate their functions and their relationship with other targeting pathways is currently unclear. To address this, we studied retinal degeneration gene product CCDC66, which localizes to centrosomes, cilia, satellites and microtubules and functions in ciliogenesis. FRAP experiments showed that its centrosomal pool was dynamic and the ciliary pool associated with the ciliary axoneme and was stable. Centrosomal CCDC66 abundance and dynamics required microtubule-dependent active transport and tethering, and was inhibited by sequestration at satellites. Systematic quantitation of satellite dynamics identified only a small fraction to display microtubule-based bimodal motility, consistent with trafficking function. Majority displayed diffusive motility with unimodal persistence, supporting sequestration function. Together, our findings reveal new mechanisms of communication between membrane-less compartments.

Orijinal dilİngilizce
Makale numarası14250
DergiScientific Reports
Hacim9
Basın numarası1
DOI'lar
Yayın durumuYayınlandı - 1 Ara 2019

Bibliyografik not

Publisher Copyright:
© 2019, The Author(s).

Finansman

We acknowledge the Firat-Karalar lab members for insightful discussions regarding this work. HeLa::GFP-PCM1 BAC cells were a kind gift from Olivier Rosnet from CNRS. We thank Dr. Fadwa Joud at the CRUK CI Light Microscopy Facility (Cambridge) for the use of the Leica SP8 STED 3X scanning confocal microscope. This work was supported by ERC StG Grant 679140 and EMBO Installation Grant to ENF.

FinansörlerFinansör numarası
European Molecular Biology Organization
Horizon 2020 Framework Programme679140
H2020 European Research Council
European Research Council
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