Rough Deal and Zw10 are required for the metaphase checkpoint in Drosophila

Basto, Renata; Gomes, Rui; Karess, Roger E.

doi:10.1038/35046592

Cited by 126 publications

(108 citation statements)

References 29 publications

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“…It remains unclear whether the SAC component, Mps1p, also plays a role in centrosome duplication in higher eukaryotes [Fischer et al, 2004;Fisk et al, 2003;Liu et al, 2003;Stucke et al, 2004;Stucke et al, 2002] as it does in budding [Winey et al, 1991] but not in fission yeast [He et al, 1998]. The mammalian Ndc80p complex [McCleland et al, 2003], the ROD and ZW10 kinetochore proteins [Basto et al, 2000;Chan et al, 2000], the outer kinetochore protein Zwint-1 [Obuse et al, 2004;Wang et al, 2004a], and the kinetochore-associated NEK2A protein [Lou et al, 2004] are also required for the spindle checkpoint, indicating that the kinetochore's role in SAC signaling is evolutionarily conserved, although no ROD, ZW10, or Zwint-1 homologues have been identified in yeast. The mammalian survivin/Aurora B complex regulates BubR1p and Mad2p localization to kinetochores [Lens et al, 2003] and, like the budding yeast Ipl1p/Aurora, is required for SAC function when insufficient tension is applied across sister kinetochores [Carvalho et al, 2003;Hauf et al, 2003;Lens et al, 2003].…”

Section: Higher Eukaryotesmentioning

confidence: 99%

SAC‐ing mitotic errors: How the spindle assembly checkpoint (SAC) plays defense against chromosome mis‐segregation

Kadura

Sazer

2005

Cell Motil. Cytoskeleton

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Section: Higher Eukaryotesmentioning

confidence: 99%

SAC‐ing mitotic errors: How the spindle assembly checkpoint (SAC) plays defense against chromosome mis‐segregation

Kadura

Sazer

2005

Cell Motil. Cytoskeleton

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“…Cytoplasmic dynein at kinetochores also does not appear essential for Mad2 binding to unattached kinetochores because we found Mad2 highly concentrated on kinetochores in prophase nuclei that show no staining for cytoplasmic dynein. In addition, depletion of zw10, rod, or dynein/dynactin also does not prevent Mad1, Mad2, or BubR1 from binding unattached prometaphase kinetochores (Chan et al, 2000), but zw10 and rod, proteins that target cytoplasmic dynein to kinetochores, do appear required for maintenance of checkpoint activity (Chan et al, 2000;Basto et al, 2000). Howell et al (2000) has shown that Mad2 binding sites are transported poleward from unattached kinetochores to the poles.…”

Section: Future Considerationsmentioning

confidence: 99%

Microtubule-dependent Changes in Assembly of Microtubule Motor Proteins and Mitotic Spindle Checkpoint Proteins at PtK1 Kinetochores

Hoffman

Pearson

Yen

et al. 2001

MBoC

328

351

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The ability of kinetochores to recruit microtubules, generate force, and activate the mitotic spindle checkpoint may all depend on microtubule-and/or tension-dependent changes in kinetochore assembly. With the use of quantitative digital imaging and immunofluorescence microscopy of PtK1 tissue cells, we find that the outer domain of the kinetochore, but not the CREST-stained inner core, exhibits three microtubule-dependent assembly states, not directly dependent on tension. First, prometaphase kinetochores with few or no kinetochore microtubules have abundant punctate or oblate fluorescence morphology when stained for outer domain motor proteins CENP-E and cytoplasmic dynein and checkpoint proteins BubR1 and Mad2. Second, microtubule depolymerization induces expansion of the kinetochore outer domain into crescent and ring morphologies around the centromere. This expansion may enhance recruitment of kinetochore microtubules, and occurs with more than a 20-to 100-fold increase in dynein and relatively little change in CENP-E, BubR1, and Mad2 in comparison to prometaphase kinetochores. Crescents disappear and dynein decreases substantially upon microtubule reassembly. Third, when kinetochores acquire their full metaphase complement of kinetochore microtubules, levels of CENP-E, dynein, and BubR1 decrease by three-to sixfold in comparison to unattached prometaphase kinetochores, but remain detectable. In contrast, Mad2 decreases by 100-fold and becomes undetectable, consistent with Mad2 being a key factor for the "wait-anaphase" signal produced by unattached kinetochores. Like previously found for Mad2, the average amounts of CENP-E, dynein, or BubR1 at metaphase kinetochores did not change with the loss of tension induced by taxol stabilization of microtubules.

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“…In another study, Savoian and colleagues used zw10 and rod Drosophila mutant spermatocytes to specifically perturb dynein localization at kinetochores [99,100] and showed that anaphase chromosome motion to the poles was severely affected in those mutants. However, some potential caveats with this experimental approach are related with the fact that zw10/rod are also required to recruit the SAC protein Mad2 to unattached kinetochores, thereby compromising SAC function [101][102][103]. Kinetochore dynein is also involved in the initial MT capture at the entry of mitosis, which could indirectly compromise chromosome motility if anaphase is triggered with normal kinetics [100].…”

Section: Kinetochore Dyneinmentioning

confidence: 99%

The perpetual movements of anaphase

Maiato

Lince-Faria

2010

Cell. Mol. Life Sci.

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One of the most extraordinary events in the lifetime of a cell is the coordinated separation of sister chromatids during cell division. This is truly the essence of the entire mitotic process and the reason for the most profound morphological changes in cytoskeleton and nuclear organization that a cell may ever experience. It all occurs within a very short time window known as "anaphase", as if the cell had spent the rest of its existence getting ready for this moment in an ultimate act of survival. And there is a good reason for this: no space for mistakes. Problems in the distribution of chromosomes during cell division have been correlated with aneuploidy, a common feature observed in cancers and several birth defects, and the main cause of spontaneous abortion in humans. In this paper we critically review the mechanisms of anaphase chromosome motion that resisted the scrutiny of more than one hundred years of research as part of a tribute to the pioneering work of Miguel Mota.

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Rough Deal and Zw10 are required for the metaphase checkpoint in Drosophila

Cited by 126 publications

References 29 publications

SAC‐ing mitotic errors: How the spindle assembly checkpoint (SAC) plays defense against chromosome mis‐segregation

SAC‐ing mitotic errors: How the spindle assembly checkpoint (SAC) plays defense against chromosome mis‐segregation

Microtubule-dependent Changes in Assembly of Microtubule Motor Proteins and Mitotic Spindle Checkpoint Proteins at PtK1 Kinetochores

The perpetual movements of anaphase

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