WDR92 is required for axonemal dynein heavy chain stability in cytoplasm

Author:

Patel-King Ramila S.1,Sakato-Antoku Miho1,Yankova Maya12,King Stephen M.12ORCID

Affiliation:

1. Department of Molecular Biology and Biophysics, University of Connecticut Health Center, Farmington, CT 06030-3305

2. Electron Microscopy Facility, University of Connecticut Health Center, Farmington, CT 06030-3305

Abstract

WDR92 associates with a prefoldin-like cochaperone complex and known dynein assembly factors. WDR92 has been very highly conserved and has a phylogenetic signature consistent with it playing a role in motile ciliary assembly or activity. Knockdown of WDR92 expression in planaria resulted in ciliary loss, reduced beat frequency and dyskinetic motion of the remaining ventral cilia. We have now identified a Chlamydomonas wdr92 mutant that encodes a protein missing the last four WD repeats. The wdr92-1 mutant builds only ∼0.7-μm cilia lacking both inner and outer dynein arms, but with intact doublet microtubules and central pair. When cytoplasmic extracts prepared by freeze/thaw from a control strain were fractionated by gel filtration, outer arm dynein components were present in several distinct high molecular weight complexes. In contrast, wdr92-1 extracts almost completely lacked all three outer arm heavy chains, while the IFT dynein heavy chain was present in normal amounts. A wdr92-1 tpg1-2 double mutant builds ∼7-μm immotile flaccid cilia that completely lack dynein arms. These data indicate that WDR92 is a key assembly factor specifically required for the stability of axonemal dynein heavy chains in cytoplasm and suggest that cytoplasmic/IFT dynein heavy chains use a distinct folding pathway.

Publisher

American Society for Cell Biology (ASCB)

Subject

Cell Biology,Molecular Biology

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