4.8 Article

The COMA complex interacts with Cse4 and positions Sli15/Ipl1 at the budding yeast inner kinetochore

Journal

ELIFE
Volume 8, Issue -, Pages -

Publisher

ELIFE SCIENCES PUBLICATIONS LTD
DOI: 10.7554/eLife.42879

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Funding

  1. Deutsche Forschungsgemeinschaft Graduate School Quantitative Biosciences Munich
  2. Deutsche Forschungsgemeinschaft Graduate School [GRK 1721]
  3. Austrian Academy of Sciences DOC Fellowship
  4. European Research Council [281354, 638218]
  5. Human Frontier Science Program [RGP0008/2015]
  6. Bavarian Research Center for Molecular Biosystems
  7. Ludwig-Maximilians-Universitat Munchen
  8. European Research Council (ERC) [638218, 281354] Funding Source: European Research Council (ERC)

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Kinetochores are macromolecular protein complexes at centromeres that ensure accurate chromosome segregation by attaching chromosomes to spindle microtubules and integrating safeguard mechanisms. The inner kinetochore is assembled on CENP-A nucleosomes and has been implicated in establishing a kinetochore-associated pool of Aurora B kinase, a chromosomal passenger complex (CPC) subunit, which is essential for chromosome biorientation. By performing crosslink-guided in vitro reconstitution of budding yeast kinetochore complexes we showed that the Ame1/Okp1(CENP-U/Q) heterodimer, which forms the COMA complex with Ctf19/Mcm21(CENP-P/O), selectively bound Cse4(CENP-A) nucleosomes through the Cse4 N-terminus. The Sli15/Ipl1(INCENP/Aurora-B) core-CPC interacted with COMA in vitro through the Ctf19 C-terminus whose deletion affected chromosome segregation fidelity in Sli15 wild-type cells. Tethering Sli15 to Ame1/Okp1 rescued synthetic lethality upon Ctf19 depletion in a Sli15 centromere-targeting deficient mutant. This study shows molecular characteristics of the point-centromere kinetochore architecture and suggests a role for the Ctf19 C-terminus in mediating CPC-binding and accurate chromosome segregation.

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