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5DN7

Crescerin uses a TOG domain array to regulate microtubules in the primary cilium

Summary for 5DN7
Entry DOI10.2210/pdb5dn7/pdb
DescriptorProtein FAM179B (2 entities in total)
Functional Keywordstog domain, structural protein
Biological sourceMus musculus (Mouse)
Total number of polymer chains1
Total formula weight32495.52
Authors
Das, A.,Dickinson, D.J.,Wood, C.C.,Goldstein, B.,Slep, K.C. (deposition date: 2015-09-09, release date: 2015-09-23, Last modification date: 2024-03-06)
Primary citationDas, A.,Dickinson, D.J.,Wood, C.C.,Goldstein, B.,Slep, K.C.
Crescerin uses a TOG domain array to regulate microtubules in the primary cilium.
Mol.Biol.Cell, 26:4248-4264, 2015
Cited by
PubMed Abstract: Eukaryotic cilia are cell-surface projections critical for sensing the extracellular environment. Defects in cilia structure and function result in a broad range of developmental and sensory disorders. However, mechanisms that regulate the microtubule (MT)-based scaffold forming the cilia core are poorly understood. TOG domain array-containing proteins ch-TOG and CLASP are key regulators of cytoplasmic MTs. Whether TOG array proteins also regulate ciliary MTs is unknown. Here we identify the conserved Crescerin protein family as a cilia-specific, TOG array-containing MT regulator. We present the crystal structure of mammalian Crescerin1 TOG2, revealing a canonical TOG fold with conserved tubulin-binding determinants. Crescerin1's TOG domains possess inherent MT-binding activity and promote MT polymerization in vitro. Using Cas9-triggered homologous recombination in Caenorhabditis elegans, we demonstrate that the worm Crescerin family member CHE-12 requires TOG domain-dependent tubulin-binding activity for sensory cilia development. Thus, Crescerin expands the TOG domain array-based MT regulatory paradigm beyond ch-TOG and CLASP, representing a distinct regulator of cilia structure.
PubMed: 26378256
DOI: 10.1091/mbc.E15-08-0603
PDB entries with the same primary citation
Experimental method
X-RAY DIFFRACTION (2.2 Å)
Structure validation

226707

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