Loss-of-function of the ciliopathy protein Cc2d2a disorganizes the vesicle fusion machinery at the periciliary membrane and indirectly affects Rab8-trafficking in zebrafish photoreceptors

PLoS Genet. 2017 Dec 27;13(12):e1007150. doi: 10.1371/journal.pgen.1007150. eCollection 2017 Dec.

Abstract

Ciliopathies are human disorders caused by dysfunction of primary cilia, ubiquitous organelles involved in transduction of environmental signals such as light sensation in photoreceptors. Concentration of signal detection proteins such as opsins in the ciliary membrane is achieved by RabGTPase-regulated polarized vesicle trafficking and by a selective barrier at the ciliary base, the transition zone (TZ). Dysfunction of the TZ protein CC2D2A causes Joubert/Meckel syndromes in humans and loss of ciliary protein localization in animal models, including opsins in retinal photoreceptors. The link between the TZ and upstream vesicle trafficking has been little explored to date. Moreover, the role of the small GTPase Rab8 in opsin-carrier vesicle (OCV) trafficking has been recently questioned in a mouse model. Using correlative light and electron microscopy and live imaging in zebrafish photoreceptors, we provide the first live characterization of Rab8-mediated trafficking in photoreceptors in vivo. Our results support a possibly redundant role for both Rab8a/b paralogs in OCV trafficking, based on co-localization of Rab8 and opsins in vesicular structures, and joint movement of Rab8-tagged particles with opsin. We further investigate the role of the TZ protein Cc2d2a in Rab8-mediated trafficking using cc2d2a zebrafish mutants and identify a requirement for Cc2d2a in the latest step of OCV trafficking, namely vesicle fusion. Progressive accumulation of opsin-containing vesicles in the apical portion of photoreceptors lacking Cc2d2a is caused by disorganization of the vesicle fusion machinery at the periciliary membrane with mislocalization and loss of the t-SNAREs SNAP25 and Syntaxin3 and of the exocyst component Exoc4. We further observe secondary defects on upstream Rab8-trafficking with cytoplasmic accumulation of Rab8. Taken together, our results support participation of Rab8 in OCV trafficking and identify a novel role for the TZ protein Cc2d2a in fusion of incoming ciliary-directed vesicles, through organization of the vesicle fusion machinery at the periciliary membrane.

Publication types

  • Research Support, Non-U.S. Gov't

MeSH terms

  • Animals
  • Animals, Genetically Modified
  • Biological Transport
  • Cell Movement
  • Cilia / genetics
  • Cilia / metabolism
  • Humans
  • Membranes / metabolism
  • Opsins / genetics
  • Opsins / metabolism
  • Photoreceptor Cells, Vertebrate / metabolism
  • Protein Transport
  • Vesicular Transport Proteins / genetics*
  • Vesicular Transport Proteins / metabolism*
  • Zebrafish
  • Zebrafish Proteins / genetics*
  • Zebrafish Proteins / metabolism*
  • rab GTP-Binding Proteins / genetics
  • rab GTP-Binding Proteins / metabolism*

Substances

  • CC2D2A protein, zebrafish
  • Opsins
  • Vesicular Transport Proteins
  • Zebrafish Proteins
  • Rab8a protein, zebrafish
  • RAB8A protein, human
  • rab GTP-Binding Proteins

Grants and funding

Funding was provided by the Swiss National Science Foundation http://www.snf.ch/en/Pages/default.aspx, grant numbers PZP00P3_163979/1, PZP00P3_142404 and PP00P3_170681/1 to RBG and 31003A_153289/1 to SCFN. The funders had no role in study design, data collection and analysis, decision to publish, or preparation of the manuscript.