| Literature DB >> 35762204 |
Tsuyoshi Imasaki1,2,3, Satoshi Kikkawa1, Shinsuke Niwa4, Yumiko Saijo-Hamano1, Hideki Shigematsu5,6, Kazuhiro Aoyama7,8, Kaoru Mitsuoka8, Takahiro Shimizu1, Mari Aoki3, Ayako Sakamoto3, Yuri Tomabechi3, Naoki Sakai5,6, Mikako Shirouzu3, Shinya Taguchi1, Yosuke Yamagishi1, Tomiyoshi Setsu1, Yoshiaki Sakihama1, Eriko Nitta1, Masatoshi Takeichi9, Ryo Nitta1,3.
Abstract
Microtubules are dynamic polymers consisting of αβ-tubulin heterodimers. The initial polymerization process, called microtubule nucleation, occurs spontaneously via αβ-tubulin. Since a large energy barrier prevents microtubule nucleation in cells, the γ-tubulin ring complex is recruited to the centrosome to overcome the nucleation barrier. However, a considerable number of microtubules can polymerize independently of the centrosome in various cell types. Here, we present evidence that the minus-end-binding calmodulin-regulated spectrin-associated protein 2 (CAMSAP2) serves as a strong nucleator for microtubule formation by significantly reducing the nucleation barrier. CAMSAP2 co-condensates with αβ-tubulin via a phase separation process, producing plenty of nucleation intermediates. Microtubules then radiate from the co-condensates, resulting in aster-like structure formation. CAMSAP2 localizes at the co-condensates and decorates the radiating microtubule lattices to some extent. Taken together, these in vitro findings suggest that CAMSAP2 supports microtubule nucleation and growth by organizing a nucleation centre as well as by stabilizing microtubule intermediates and growing microtubules.Entities:
Keywords: CAMSAP; E. coli; LLPS; TIRF; cell biology; cryo-EM; microtubule; molecular biophysics; mouse; nucleation; structural biology
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Year: 2022 PMID: 35762204 PMCID: PMC9239687 DOI: 10.7554/eLife.77365
Source DB: PubMed Journal: Elife ISSN: 2050-084X Impact factor: 8.713