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Novel Coiled-Coil Proteins Regulate Exocyst Association with Cortical Microtubules in Xylem Cells via the Conserved Oligomeric Golgi-Complex 2 Protein
Author(s) -
Yoshihisa Oda,
Yuki Iida,
Yoshinobu Nagashima,
Yuki Sugiyama,
Hiroo Fukuda
Publication year - 2014
Publication title -
plant and cell physiology
Language(s) - English
Resource type - Journals
SCImago Journal Rank - 1.975
H-Index - 152
eISSN - 1471-9053
pISSN - 0032-0781
DOI - 10.1093/pcp/pcu197
Subject(s) - exocyst , microtubule , microbiology and biotechnology , golgi apparatus , vesicle , live cell imaging , protein subunit , chemistry , biology , coiled coil , cell , biochemistry , endoplasmic reticulum , gene , membrane
Xylem vessel cells develop secondary cell walls in distinct patterns. Cortical microtubules are rearranged into distinct patterns and regulate secondary cell wall deposition; however, it is unclear how exocytotic membrane trafficking is linked to cortical microtubules. Here, we show that the novel coiled-coil proteins vesicle tethering 1 (VETH1) and VETH2 recruit EXO70A1, an exocyst subunit essential for correct patterning of secondary cell wall deposition, to cortical microtubules via the conserved oligomeric Golgi complex (COG) 2 protein. VETH1 and VETH2 encode an uncharacterized domain of an unknown function designated DUF869, and were preferentially up-regulated in xylem cells. VETH1-green fluorescent protein (GFP) and VETH2-GFP co-localized at novel vesicle-like small compartments, which exhibited microtubule plus-end-directed and end-tracking dynamics. VETH1 and VETH2 interacted with COG2, and this interaction promoted the association between cortical microtubules and EXO70A1 These results suggest that the VETH-COG2 complex ensures the correct secondary cell wall deposition pattern by recruiting exocyst components to cortical microtubules.

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