Electron cryotomography analysis of Dam1C/DASH at the kinetochore–spindle interface in situ

Author:

Ng Cai Tong1ORCID,Deng Li1,Chen Chen1,Lim Hong Hwa23ORCID,Shi Jian1ORCID,Surana Uttam234ORCID,Gan Lu1ORCID

Affiliation:

1. Department of Biological Sciences and Centre for BioImaging Sciences, National University of Singapore, Singapore

2. Institute of Molecular and Cell Biology Agency for Science Technology and Research, Singapore

3. Bioprocessing Technology Institute, Agency for Science Technology and Research, Singapore

4. Department of Pharmacology, National University of Singapore, Singapore

Abstract

In dividing cells, depolymerizing spindle microtubules move chromosomes by pulling at their kinetochores. While kinetochore subcomplexes have been studied extensively in vitro, little is known about their in vivo structure and interactions with microtubules or their response to spindle damage. Here we combine electron cryotomography of serial cryosections with genetic and pharmacological perturbation to study the yeast chromosome segregation machinery in vivo. Each kinetochore microtubule has one (rarely, two) Dam1C/DASH outer kinetochore assemblies. Dam1C/DASH contacts the microtubule walls and does so with its flexible “bridges”; there are no contacts with the protofilaments’ curved tips. In metaphase, ∼40% of the Dam1C/DASH assemblies are complete rings; the rest are partial rings. Ring completeness and binding position along the microtubule are sensitive to kinetochore attachment and tension, respectively. Our study and those of others support a model in which each kinetochore must undergo cycles of conformational change to couple microtubule depolymerization to chromosome movement.

Funder

NUS

Ministry of Education

Biomedical Research Council of A*STAR

Publisher

Rockefeller University Press

Subject

Cell Biology

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