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XB-ART-57338
Dev Biol 2020 Nov 01;4671-2:108-117. doi: 10.1016/j.ydbio.2020.08.008.
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A systematic, label-free method for identifying RNA-associated proteins in vivo provides insights into vertebrate ciliary beating machinery.

Drew K , Cox RM , Dang V , Devitt CC , McWhite CD , Papoulas O , Huizar RL , Marcotte EM , Wallingford JB .


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Cell-type specific RNA-associated proteins are essential for development and homeostasis in animals. Despite a massive recent effort to systematically identify RNA-associated proteins, we currently have few comprehensive rosters of cell-type specific RNA-associated proteins in vertebrate tissues. Here, we demonstrate the feasibility of determining the RNA-associated proteome of a defined vertebrate embryonic tissue using DIF-FRAC, a systematic and universal (i.e., label-free) method. Application of DIF-FRAC to cultured tissue explants of Xenopus mucociliary epithelium identified dozens of known RNA-associated proteins as expected, but also several novel RNA-associated proteins, including proteins related to assembly of the mitotic spindle and regulation of ciliary beating. In particular, we show that the inner dynein arm tether Cfap44 is an RNA-associated protein that localizes not only to axonemes, but also to liquid-like organelles in the cytoplasm called DynAPs. This result led us to discover that DynAPs are generally enriched for RNA. Together, these data provide a useful resource for a deeper understanding of mucociliary epithelia and demonstrate that DIF-FRAC will be broadly applicable for systematic identification of RNA-associated proteins from embryonic tissues.

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Species referenced: Xenopus
Genes referenced: cfap44 tnf
GO keywords: maintenance of ciliary planar beating movement pattern


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References [+] :
Aizer, The dynamics of mammalian P body transport, assembly, and disassembly in vivo. 2008, Pubmed