Distinct Roles of the Chromosomal Passenger Complex in the Detection of and Response to Errors in Kinetochore-Microtubule Attachment

Haase, Julian; Bonner, Mary Kate; Halas, Hyunmi; Kelly, Alexander E.

doi:10.1016/j.devcel.2017.08.022

Cited by 40 publications

(71 citation statements)

References 91 publications

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“…Because activation of Aurora B depends on clustering of the CPC (Kelly et al, 2007, 2010; Wang et al, 2011), clustering and activation of Aurora B most likely takes place at an alternative location, in the absence of Haspin and Bub1 activity. This could simply be chromatin, as we observed low levels of Aurora B dispersed over the chromatin in Bub1-inhibited Haspin CM cells, and in Xenopus laevis egg extracts this was shown to be sufficient for the activation of Aurora B kinase activity (Haase et al, 2017; Kelly et al, 2007). Alternatively, recent work proposed a role for microtubules that traverse the centromere in depositing active Aurora B from the centromere at the kinetochore (Trivedi et al, 2019).…”

Section: Discussionmentioning

confidence: 86%

“…We deem it unlikely that a microtubule-associated pool of the CPC is responsible for the KT substrate phosphorylation in Bub1-inhibited Haspin CM cells because we observed no difference in Hec1 phosphorylation in either low (0.33 µM) or high (3.3 µM) concentrations of nocodazole. However, we cannot exclude that the CPC core complex, consisting of Borealin, Survivin, and the N terminus of INCENP, might play a role in Aurora B–dependent KT substrate phosphorylation independently of microtubule binding and inner centromere clustering of Aurora B (Haase et al, 2017). Finally, a potential third, transient kinetochore-associated pool of Aurora B, one that does not depend on Haspin and Bub1 kinase activity, may phosphorylate the KMN network (Caldas et al, 2013; DeLuca et al, 2011; Fischböck-Halwachs et al, 2019; García-Rodríguez et al, 2019; Broad et al, 2020).…”

Section: Discussionmentioning

confidence: 99%

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Untangling the contribution of Haspin and Bub1 to Aurora B function during mitosis

Hadders

Hindriksen

Truong

et al. 2020

Journal of Cell Biology

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Aurora B kinase is essential for faithful chromosome segregation during mitosis. During (pro)metaphase, Aurora B is concentrated at the inner centromere by the kinases Haspin and Bub1. However, how Haspin and Bub1 collaborate to control Aurora B activity at centromeres remains unclear. Here, we show that either Haspin or Bub1 activity is sufficient to recruit Aurora B to a distinct chromosomal locus. Moreover, we identified a small, Bub1 kinase–dependent Aurora B pool that supported faithful chromosome segregation in otherwise unchallenged cells. Joined inhibition of Haspin and Bub1 activities fully abolished Aurora B accumulation at centromeres. While this impaired the correction of erroneous KT–MT attachments, it did not compromise the mitotic checkpoint, nor the phosphorylation of the Aurora B kinetochore substrates Hec1, Dsn1, and Knl1. This suggests that Aurora B substrates at the kinetochore are not phosphorylated by centromere-localized pools of Aurora B, and calls for a reevaluation of the current spatial models for how tension affects Aurora B–dependent kinetochore phosphorylation.

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Section: Discussionmentioning

confidence: 86%

Section: Discussionmentioning

confidence: 99%

Untangling the contribution of Haspin and Bub1 to Aurora B function during mitosis

Hadders

Hindriksen

Truong

et al. 2020

Journal of Cell Biology

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“…Outer kinetochore assembly is entirely dependent on the phosphorylation of Dsn1 by Aurora B kinase in Xenopus egg extracts In Xenopus egg extracts, the assembly and maintenance of kinetochores is completely dependent on the mitotic kinase Aurora B, but the underlying phosphosubstrates are unclear (Emanuele et al, 2005(Emanuele et al, , 2008Haase et al, 2017). In human, chicken, and yeast cells, Aurora B phosphorylation of multiple residues within the Dsn1 subunit of the Mis12C plays a partial role in kinetochore assembly ( Fig.…”

Section: Resultsmentioning

confidence: 99%

Enrichment of Aurora B kinase at the inner kinetochore controls outer kinetochore assembly

Bonner

Haase

Swinderman

et al. 2019

Journal of Cell Biology

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Outer kinetochore assembly enables chromosome attachment to microtubules and spindle assembly checkpoint (SAC) signaling in mitosis. Aurora B kinase controls kinetochore assembly by phosphorylating the Mis12 complex (Mis12C) subunit Dsn1. Current models propose Dsn1 phosphorylation relieves autoinhibition, allowing Mis12C binding to inner kinetochore component CENP-C. Using Xenopus laevis egg extracts and biochemical reconstitution, we found that autoinhibition of the Mis12C by Dsn1 impedes its phosphorylation by Aurora B. Our data indicate that the INCENP central region increases Dsn1 phosphorylation by enriching Aurora B at inner kinetochores, close to CENP-C. Furthermore, centromere-bound CENP-C does not exchange in mitosis, and CENP-C binding to the Mis12C dramatically increases Dsn1 phosphorylation by Aurora B. We propose that the coincidence of Aurora B and CENP-C at inner kinetochores ensures the fidelity of kinetochore assembly. We also found that the central region is required for the SAC beyond its role in kinetochore assembly, suggesting that kinetochore enrichment of Aurora B promotes the phosphorylation of other kinetochore substrates.

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“…Intriguingly, in the Xenopus egg extract system, the inner kinetochore was not fully assembled when INCENP lacked its N-terminus (in contrast to human cells); in this circumstance, this INCENP mutant could no longer support error correction even if the outer kinetochore assembly seemed normal [40]. Therefore, inner kinetochore components may indeed support Aurora B-INCENP localization and error correction, independently of Survivin, in vertebrate cells.…”

Section: Discussionmentioning

confidence: 99%

Aurora B-INCENP localization at centromeres/inner kinetochores is essential for chromosome bi-orientation in budding yeast

García-Rodríguez

Kasciukovic

Denninger

et al. 2019

Preprint

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To promote chromosome bi-orientation, Aurora B kinase weakens and disrupts aberrant kinetochore-MT interaction. It has long been debated how Aurora B halts this action when biorientation is established and tension is applied across sister kinetochores. Pertinent to this debate, it was shown that Bir1 (yeast Survivin), which recruits Ipl1-Sli15 (yeast Aurora B-INCENP) to centromeres, is dispensable for bi-orientation, raising the possibility that Aurora B localization at centromeres is not required for bi-orientation. Here, we show that the COMA inner kinetochore sub-complex physically interacts with Sli15, recruits Ipl1-Sli15 to the inner kinetochore and promotes chromosome bi-orientation, independently of Bir1, in budding yeast. Moreover, using an engineered recruitment of Ipl1-Sli15 to the inner kinetochore when both Bir1 and COMA are defective, we show that localization of Ipl1-Sli15 at centromeres/ inner kinetochores is essential for bi-orientation, refuting the above possibility. Our results give important insight into how Aurora B disrupts kinetochore-MT interaction in a tensiondependent manner, to promote chromosome bi-orientation. (164 words)

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Distinct Roles of the Chromosomal Passenger Complex in the Detection of and Response to Errors in Kinetochore-Microtubule Attachment

Cited by 40 publications

References 91 publications

Untangling the contribution of Haspin and Bub1 to Aurora B function during mitosis

Untangling the contribution of Haspin and Bub1 to Aurora B function during mitosis

Enrichment of Aurora B kinase at the inner kinetochore controls outer kinetochore assembly

Aurora B-INCENP localization at centromeres/inner kinetochores is essential for chromosome bi-orientation in budding yeast

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