| Article ID | Journal | Published Year | Pages | File Type |
|---|---|---|---|---|
| 2176642 | Developmental Cell | 2014 | 14 Pages |
•High-resolution microscopy reveals CCAN protein architecture in human kinetochores•Proper intrakinetochore stretch depends on the CCAN linkers to the Ndc80 complex•Ndc80/Hec1 phosphorylation is inhibited by hyper-intrakinetochore stretch•CCAN DNA binding proteins play a minor role in the compaction of CENP-A chromatin
SummaryConstitutive centromere-associated network (CCAN) proteins, particularly CENP-C, CENP-T, and the CENP-H/-I complex, mechanically link CENP-A-containing centromeric chromatin within the inner kinetochore to outer kinetochore proteins, such as the Ndc80 complex, that bind kinetochore microtubules. Accuracy of chromosome segregation depends critically upon Aurora B phosphorylation of Ndc80/Hec1. To determine how CCAN protein architecture mechanically constrains intrakinetochore stretch between CENP-A and Ndc80/Hec1 for proper Ndc80/Hec1 phosphorylation, we used super-resolution fluorescence microscopy and selective protein depletion. We found that at bi-oriented chromosomes in late prometaphase cells, CENP-T is stretched ∼16 nm to the inner end of Ndc80/Hec1, much less than expected for full-length CENP-T. Depletion of various CCAN linker proteins induced hyper-intrakinetochore stretch (an additional 20–60 nm) with corresponding significant decreases in Aurora B phosphorylation of Ndc80/Hec1. Thus, proper intrakinetochore stretch is required for normal kinetochore function and depends critically on all the CCAN mechanical linkers to the Ndc80 complex.
