Kinesin-12 KLP-18 contributes to the kinetochore-microtubule poleward flux during the metaphase of C. elegans one-cell embryo
Nina Soler, Mathis Da Silva, Christophe Tascon, Laurent Chesneau, Pauline Foliard, H\'el\`ene Bouvrais, Sylvain Pastezeur, Lo\"ic Le Marrec, Jacques Pecreaux

TL;DR
This study reveals that in C. elegans embryos, kinetochore microtubules exhibit poleward flux driven by KLP-18 kinesin, a process that is spatially restricted and differs from global flux observed in other organisms.
Contribution
It demonstrates that kinetochore microtubules undergo localized flux in C. elegans, mediated by KLP-18, contrasting with the global flux seen in other species.
Findings
Kinetochore microtubules show localized poleward flux near chromosomes.
Flux depends on kinetochore regulators NDC-80, CLS-2, and ZYG-9.
Depleting KLP-18 reduces microtubule flux.
Abstract
The mitotic spindle partitions chromosomes during cell division by connecting the poles to kinetochores through microtubules (MTs). Their plus-ends, facing the chromosomes, exhibit dynamic instability, which is critical for proper attachment. The poleward flux implicates the displacement of Mts towards the spindle poles, while plus-ends polymerise. It may result from minus-end depolymerisation (treadmilling), sliding by kinesins (e.g., Kinesin-5), or pushing by chromokinesins. Intriguingly, such flux had not been reported in the C. elegans zygote, despite homologs of flux-associated proteins being present. To investigate this, we fluorescently labelled Mts and used photobleaching. We observed no global flux; instead, the bleached zone's edges moved inward. The centrosome-facing front reflected MT dynamic instability, but the chromosome-facing front showed faster recovery, suggesting…
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