A minimal number of MELT repeats supports all functions of KNL1 in chromosome segregation

Zhang, Gang; Lischetti, Tiziana; Nilsson, Jakob

doi:10.1242/jcs.139725

Cited by 102 publications

(165 citation statements)

References 43 publications

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“…In C. elegans, PP1 binding to Knl1 plays a role in SAC silencing, which might ensure the timely removal of Bub1 and BubR1 from the kinetochore (Espeut et al, 2012). In agreement with this, the Nilsson laboratory recently reported that deletion of the first 150 or 300 amino acids of Knl1, or the mutation of the Nterminal Knl1 PP1-binding site, results in increased levels of Bub1 and BubR1 at the kinetochore compared with that in cells expressing wild-type Knl1, suggesting that PP1 negatively regulates the recruitment of Bub1 and BubR1 (Zhang et al, 2014;London et al, 2012;Meadows et al, 2011;Rosenberg et al, 2011). In addition to PP1, Knl1 indirectly mediates the recruitment of PP2A through the recruitment of BubR1, which binds directly to the B56 family of PP2A regulatory subunits (Suijkerbuijk et al, 2012;Kruse et al, 2013;Xu et al, 2013).…”

Section: Knl1 Protein-interacting Regions Silk and Rvsf Motifsmentioning

confidence: 63%

“…Structural and biochemical evidence has demonstrated that phosphorylated MELT motifs bind directly and with high affinity to Bub3 (Primorac et al, 2013;Zhang et al, 2014). The crystal structure of Bub3 from budding yeast in complex with a synthetic MELT phosphopeptide and the Bub3-binding region of Bub1 (a protein motif commonly referred to as the GLEBS motif) identified a well-conserved region on the side of the b-propeller structure that is formed by the Bub3 WD40 repeats (Box 2) as the site that binds to the phosphorylated MELT motif (Primorac et al, 2013; Fig.…”

Section: Knl1 Protein-interacting Regions Silk and Rvsf Motifsmentioning

confidence: 99%

“…The stoichiometric relationship between phosphorylated MELT and Bub3 has led to the suggestion that each MELT repeat constitutes a functional binding site that is 'read' by a Bub3 molecule (Primorac et al, 2013;Zhang et al, 2014;Vleugel et al, 2013). This is supported by the observation that a drop in the amount of BUBs that are recruited is proportional to the number of MELT repeats that have been removed, and that increasing the number of MELT arrays proportionally augments the amount of Bub1 recruited (Zhang et al, 2014;Vleugel et al, 2013).…”

Section: Knl1 Protein-interacting Regions Silk and Rvsf Motifsmentioning

confidence: 99%

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The dynamic protein Knl1 – a kinetochore rendezvous

Ghongane

Kapanidou

Asghar³

et al. 2014

Journal of Cell Science

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Knl1 (also known as CASC5, UniProt Q8NG31) is an evolutionarily conserved scaffolding protein that is required for proper kinetochore assembly, spindle assembly checkpoint (SAC) function and chromosome congression. A number of recent reports have confirmed the prominence of Knl1 in these processes and provided molecular details and structural features that dictate Knl1 functions in higher organisms. Knl1 recruits SAC components to the kinetochore and is the substrate of certain protein kinases and phosphatases, the interplay of which ensures the exquisite regulation of the aforementioned processes. In this Commentary, we discuss the overall domain organization of Knl1 and the roles of this protein as a versatile docking platform. We present emerging roles of the protein interaction motifs present in Knl1, including the RVSF, SILK, MELT and KI motifs, and their role in the recruitment and regulation of the SAC proteins Bub1, BubR1, Bub3 and Aurora B. Finally, we explore how the regions of low structural complexity that characterize Knl1 are implicated in the cooperative interactions that mediate binding partner recognition and scaffolding activity by Knl1.

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Section: Knl1 Protein-interacting Regions Silk and Rvsf Motifsmentioning

confidence: 63%

Section: Knl1 Protein-interacting Regions Silk and Rvsf Motifsmentioning

confidence: 99%

Section: Knl1 Protein-interacting Regions Silk and Rvsf Motifsmentioning

confidence: 99%

See 1 more Smart Citation

The dynamic protein Knl1 – a kinetochore rendezvous

Ghongane

Kapanidou

Asghar³

et al. 2014

Journal of Cell Science

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“…It has been speculated that since binding affinity of BUB1:BUB3 to an individual MELT P is very high, each MELT repeat can potentially recruit a BUB1:BUB3 complex and therefore multiple BUB1:BUB3 complexes can concurrently bind to multiple MELT P repeats at a given time. 23,24,30 Variations in the level of phosphorylation of different active repeats is likely to function as a governing factor or may provide a subtle layer of regulation in controlling the strength of SAC response but this hypothesis needs to be substantiated experimentally. In addition, the MELT repeats function cooperatively with the 2 N-terminally located, 10-12 amino acids long, and closely related yet distinct KI (LysIle) motifs, KI1 (KIDTTSFLANLK) and KI2 (KIDFNDFIKRLK) to directly recruit BUB1 and BUBR1, respectively, by binding to their tetratricopeptide repeat (TPR) domains to ensure robust SAC activity (Fig.…”

Section: The Ndc80 Complexmentioning

confidence: 99%

How the SAC gets the axe: Integrating kinetochore microtubule attachments with spindle assembly checkpoint signaling

Agarwal

Varma

2015

BioArchitecture

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ABSTRACT. Mitosis entails the bona fide segregation of duplicated chromosomes. This process is accomplished by the attachment of kinetochores on chromosomes to microtubules (MTs) of the mitotic spindle. Once the appropriate attachment is achieved, the spindle assembly checkpoint (SAC) that delays the premature onset of anaphase needs to be silenced for the cell to proceed to anaphase and cytokinesis. Therefore, while it is imperative to preserve the SAC when kinetochores are unattached, it is of paramount importance that SAC components are removed post kinetochore microtubule (kMT) attachment. Precise knowledge of how kMT attachments trigger the removal of SAC components from kinetochores or how the checkpoint proteins feedback in to the attachment machinery remains elusive. This review aims to describe the recent advances that provide an insight into the interplay of molecular events that coordinate and regulate the SAC activity in response to kMT attachment during cell division.

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“…When phosphorylated, these motifs recruit BUB1-BUB3 dimers that are essential for SAC signaling and chromosome bi-orientation (Krenn et al, 2014;Primorac et al, 2013;Vleugel et al, 2013Vleugel et al, , 2015Zhang et al, 2014). Since the discovery of BUB1, the molecular mechanism by which it participates in SAC activation has been a matter of controversy.…”

Section: Introductionmentioning

confidence: 99%

Dissecting the roles of human BUB1 in the spindle assembly checkpoint

Vleugel

Hoek

Tromer

et al. 2015

Journal of Cell Science

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Mitotic chromosome segregation is initiated by the anaphase promoting complex/cyclosome (APC/C) and its co-activator CDC20 (forming APC/C CDC20 ). APC/C CDC20 is inhibited by the spindle assembly checkpoint (SAC) when chromosomes have not attached to spindle microtubules. Unattached kinetochores catalyze the formation of a diffusible APC/C CDC20 inhibitor that comprises BUBR1 (also known as BUB1B), BUB3, MAD2 (also known as MAD2L1) and a second molecule of CDC20. Recruitment of these proteins to the kinetochore, as well as SAC activation, rely on the mitotic kinase BUB1, but the molecular mechanism by which BUB1 accomplishes this in human cells is unknown. We show that kinetochore recruitment of BUBR1 and BUB3 by BUB1 is dispensable for SAC activation. Unlike its yeast and nematode orthologs, human BUB1 does not associate stably with the MAD2 activator MAD1 (also known as MAD1L1) and, although required for accelerating the loading of MAD1 onto kinetochores, BUB1 is dispensable for the maintenance of steady-state levels of MAD1 there. Instead, we identify a 50-amino-acid segment that harbors the recently reported ABBA motif close to a KEN box as being crucial for the role of BUB1 in SAC signaling. The presence of this segment correlates with SAC activity and efficient binding of CDC20 but not of MAD1 to kinetochores.

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A minimal number of MELT repeats supports all functions of KNL1 in chromosome segregation

Cited by 102 publications

References 43 publications

The dynamic protein Knl1 – a kinetochore rendezvous

The dynamic protein Knl1 – a kinetochore rendezvous

How the SAC gets the axe: Integrating kinetochore microtubule attachments with spindle assembly checkpoint signaling

Dissecting the roles of human BUB1 in the spindle assembly checkpoint

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