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Query: UMLS:C0033036 (
APC
)
10,214
document(s) hit in 31,850,051 MEDLINE articles (0.00 seconds)
The spindle assembly checkpoint (SAC) is required to block sister chromatid separation until all chromosomes are properly attached to the mitotic apparatus. The SAC prevents cells from entering anaphase by inhibiting the ubiquitylation of cyclin B1 and securin by the anaphase promoting complex/cyclosome (
APC
/C) ubiquitin ligase. The target of the SAC is the essential
APC
/C activator Cdc20. It is unclear how the SAC inactivates Cdc20 but most current models suggest that Cdc20 forms a stable complex with the
Mad2
checkpoint protein. Here we show that most Cdc20 is not in a complex with
Mad2
; instead
Mad2
is required for Cdc20 to form a complex with another checkpoint protein, BubR1. We further show that during the SAC, the
APC
/C ubiquitylates Cdc20 to target it for degradation. Thus, ubiquitylation of human Cdc20 is not required to release it from the checkpoint complex, but to degrade it to maintain mitotic arrest.
...
PMID:The APC/C maintains the spindle assembly checkpoint by targeting Cdc20 for destruction. 1904 31
A given protein generally has only one native tertiary fold, which is the conformation with the lowest Gibbs free energy.
Mad2
, a protein involved in the spindle checkpoint, however, has two natively folded states with similar Gibbs free energies. Through binding to its target Cdc20,
Mad2
inhibits the multisubunit ubiquitin ligase, the anaphase-promoting complex or cyclosome (
APC
/C), and delays the onset of anaphase until all sister chromatids achieve bipolar attachment to the mitotic spindle. Without ligand binding or covalent modifications,
Mad2
adopts two topologically and functionally distinct native folds in equilibrium under physiological conditions. The transition between the two
Mad2
states is regulated by multiple mechanisms and is central to the activation and inactivation of the spindle checkpoint. This review summarizes recent structural and biochemical studies on the two-state behavior of
Mad2
and discusses the generality and implications of structural malleability of proteins.
...
PMID:Protein metamorphosis: the two-state behavior of Mad2. 1900 Aug 14
The spindle assembly checkpoint (SAC) is an important mechanism that prevents the separation of sister chromatids until the microtubules radiating from the spindle poles are correctly attached to the kinetochores. Cdc20, an activator of the Anaphase Promoting Complex/Cyclosome (
APC
/C), is known as a major downstream target for inhibition by the SAC through the binding of mitotic checkpoint proteins, such as
Mad2
and BubR1. Here, we report that the SAC negatively regulates the stability of Cdc20 by targeting it for proteasome-dependent degradation. Once the checkpoint is activated by spindle poisons, a major population of Cdc20 is degraded via
APC
/C, an event that requires the binding of Cdc20 to
Mad2
. We propose that the degradation of Cdc20 represents a critical control mechanism to ensure inactivation of
APC
/C(Cdc20) in response to the SAC.
...
PMID:APC/C- and Mad2-mediated degradation of Cdc20 during spindle checkpoint activation. 1916 54
Mad2
is a key component of the spindle assembly checkpoint, a safety device ensuring faithful sister chromatid separation in mitosis. The target of
Mad2
is Cdc20, an activator of the anaphase-promoting complex/cyclosome (
APC
/C).
Mad2
binding to Cdc20 is a complex reaction that entails the conformational conversion of
Mad2
from an open (O-Mad2) to a closed (C-Mad2) conformer. Previously, it has been hypothesized that the conversion of O-
Mad2
is accelerated by its conformational dimerization with C-
Mad2
. This hypothesis, known as the
Mad2
-template hypothesis, is based on the unproven assumption that the natural conversion of O-
Mad2
required to bind Cdc20 is slow. Here, we provide evidence for this fundamental assumption and demonstrate that conformational dimerization of
Mad2
accelerates the rate of
Mad2
binding to Cdc20. On the basis of our measurements, we developed a set of rate equations that deliver excellent predictions of experimental binding curves under a variety of different conditions. Our results strongly suggest that the interaction of
Mad2
with Cdc20 is rate limiting for activation of the spindle checkpoint. Conformational dimerization of
Mad2
is essential to accelerate Cdc20 binding, but it does not modify the equilibrium of the
Mad2
:Cdc20 interaction, i.e., it is purely catalytic. These results surpass previously formulated objections to the
Mad2
-template model and predict that the release of
Mad2
from Cdc20 is an energy-driven process.
...
PMID:The influence of catalysis on mad2 activation dynamics. 1914 72
The mitotic checkpoint delays chromosome segregation until the last chromosome has correctly attached to the spindle. Exactly how this unattached chromosome can generate a checkpoint signal and inhibit the anaphase promoting complex/cyclosome (
APC
/C) is unknown. Two Developmental Cell papers in this issue by Kulukian et al. and Malureanu et al. now provide insight into how checkpoint components
Mad2
and BubR1 relay the checkpoint signal from kinetochores to
APC
/C.
...
PMID:Relaying the checkpoint signal from kinetochore to APC/C. 1915 23
Premature anaphase onset is prevented by the mitotic checkpoint through production of a "wait anaphase" inhibitor(s) that blocks recognition of cyclin B and securin by Cdc20-activated
APC
/C, an E3 ubiquitin ligase that targets them for destruction. Using physiologically relevant levels of
Mad2
, Bub3, BubR1, and Cdc20, we demonstrate that unattached kinetochores on purified chromosomes catalytically generate a diffusible Cdc20 inhibitor or inhibit Cdc20 already bound to
APC
/C. Furthermore, the chromosome-produced inhibitor requires both recruitment of
Mad2
by Mad1 that is stably bound at unattached kinetochores and dimerization-competent
Mad2
. We show that purified chromosomes promote BubR1 binding to
APC
/C-Cdc20 by acting directly on
Mad2
, but not BubR1. Our results support a model in which immobilized Mad1/
Mad2
at kinetochores provides a template for initial assembly of
Mad2
bound to Cdc20 that is then converted to a final mitotic checkpoint inhibitor with Cdc20 bound to BubR1.
...
PMID:Unattached kinetochores catalyze production of an anaphase inhibitor that requires a Mad2 template to prime Cdc20 for BubR1 binding. 1915 13
Cdc20, an activator of the anaphase promoting complex/cyclosome (
APC
/C) ubiquitin ligase, initiates the destruction of key mitotic regulators to facilitate mitosis, while it is negatively regulated by the spindle assembly checkpoint (SAC) to prevent premature anaphase entry. Activation of the p38 mitogen-activated protein kinase could contribute to mitotic arrest, but the underlying mechanism is unknown. Here we report a novel pathway in which the p38 signaling triggers Cdc20 destruction under SAC elicited by cadmium, a human carcinogen. We found that the cadmium-induced prometaphase arrest was linked to decreased Cdc20 and accumulated cyclin A protein levels in human cells, whereas the activity of cyclin B1-Cdk1 was unaffected. The Cdc20 half-life was markedly shortened along with its ubiquitination and degradation via 26S proteasome in cadmium-treated asynchronous or G(2)-enriched cells. Depletion of APC3 markedly suppressed the cadmium-induced Cdc20 ubiquitination and proteolysis, while depletion of Cdh1, another activator of
APC
/C, did not. Intriguingly, blockage of p38 activity restored the Cdc20 levels for continuing mitosis under cadmium, while inhibition of JNK activity had no effect. The cadmium-induced Cdc20 proteolysis was also suppressed during transient depletion of p38alpha or stable expression a dominant negative form of p38. Inhibition of p38 abolished the induction of
Mad2
-Cdc20-APC3 complex by cadmium. Moreover, forced expression of MKK6-p38 signaling could promote Cdc20 degradation in a Cdh1-independent
APC
/C pathway. In summary, accelerated ubiquitination and proteolysis of Cdc20 is essential for prometaphase arrest that is mediated via the p38 signaling during SAC activation.
...
PMID:Cdc20 proteolysis requires p38 MAPK signaling and Cdh1-independent APC/C ubiquitination during spindle assembly checkpoint activation by cadmium. 2005 26
The mitotic (or spindle assembly) checkpoint system ensures accurate segregation of chromosomes by delaying anaphase until all chromosomes are correctly attached to the mitotic spindle. This system acts by inhibiting the activity of the anaphase-promoting complex/cyclosome (
APC
/C) ubiquitin ligase to target securin for degradation.
APC
/C is inhibited by a mitotic checkpoint complex (MCC) composed of BubR1, Bub3,
Mad2
, and Cdc20. The molecular mechanisms of the inactivation of the mitotic checkpoint, including the release of
APC
/C from inhibition, remain obscure. It has been reported that polyubiquitylation by the
APC
/C is required for the inactivation of the mitotic checkpoint [Reddy SK, Rape M, Margansky WA, Kirschner MW (2007) Nature, 446:921-924]. We confirmed the involvement of polyubiquitylation, but found that another process, which requires ATP cleavage at the beta-gamma position (as opposed to alpha-beta bond scission involved in ubiquitylation), is essential for the release of
APC
/C from checkpoint inhibition. ATP (beta-gamma) cleavage is required both for the dissociation of MCC components from
APC
/C and for the disassembly of free MCC, whereas polyubiquitylation is involved only in the former process. We find that the requirement for ATP (beta-gamma) cleavage is not due to the involvement of the 26S proteasome and that the phenomena observed are not due to sustained activity of protein kinase Cdk1/cyclin B, caused by inhibition of the degradation of cyclin B. Thus, some other energy-consuming process is needed for the inactivation of the mitotic checkpoint.
...
PMID:ATP is required for the release of the anaphase-promoting complex/cyclosome from inhibition by the mitotic checkpoint. 2021 61
Spo13 is a key meiosis-specific regulator required for centromere cohesion and coorientation, and for progression through two nuclear divisions. We previously reported that it causes a G2/M arrest and may delay the transition from late anaphase to G1, when overexpressed in mitosis. Yet its mechanism of action has remained elusive. Here we show that Spo13, which is phosphorylated and stabilized at G2/M in a Cdk/Clb-dependent manner, acts at two stages during mitotic cell division. Spo13 provokes a G2/M arrest that is reversible and largely independent of the
Mad2
spindle checkpoint. Since mRNAs whose induction requires Cdc14 activation are reduced, we propose that its anaphase delay results from inhibition of Cdc14 function. Indeed, the Spo13-induced anaphase delay correlates with Cdc14 phosphatase retention in the nucleolus and with cyclin B accumulation, which both impede anaphase exit. At the onset of arrest, Spo13 is primarily associated with the nucleolus, where Cdc14 accumulates. Significantly, overexpression of separase (Esp1), which promotes G2/M and anaphase progression, suppresses Spo13 effects in mitosis, arguing that Spo13 acts upstream or parallel to Esp1. Given that Spo13 overexpression reduces Pds1 and cyclin B degradation, our findings are consistent with a role for Spo13 in regulating
APC
, which controls both G2/M and anaphase. Similar effects of Spo13 during meiotic MI may prevent cell cycle exit and initiation of DNA replication prior to MII, thereby ensuring two successive chromosome segregation events without an intervening S phase.
...
PMID:Mitotic expression of Spo13 alters M-phase progression and nucleolar localization of Cdc14 in budding yeast. 2040 33
To prevent aneuploidy, cells require a mitotic surveillance mechanism, the spindle assembly checkpoint (SAC). The SAC prevents metaphase/anaphase transition by blocking the ubiquitylation and destruction of cyclin B and securin via the Cdc20-activated anaphase-promoting complex or cyclosome (
APC
/C)-mediated proteolysis pathway. This checkpoint involves the kinetochore proteins
Mad2
, BubR1, and Cdc20.
Mad2
and BubR1 are inhibitors of the
APC
/C, but Cdc20 is an activator. Exactly how the SAC regulates Cdc20 via unattached kinetochores remains unclear; in vertebrates, most current models suggest that kinetochore-bound
Mad2
is required for initial binding to Cdc20 to form a stable complex that includes BubR1. Here, we show that the
Mad2
kinetochore dimerization recruitment mechanism is conserved and that the recruitment of Cdc20 to kinetochores in Drosophila requires BubR1 but not
Mad2
. BubR1 and
Mad2
can bind to Cdc20 independently, and the interactions are enhanced after cells are arrested at mitosis by the depletion of Cdc27 using RNA interference (RNAi) in S2 cells or by MG132 treatment in syncytial embryos. These findings offer an explanation of why BubR1 is more important than
Mad2
for SAC function in flies. These findings could lead to a better understanding of vertebrate SAC mechanisms.
...
PMID:Recruitment of Cdc20 to the kinetochore requires BubR1 but not Mad2 in Drosophila melanogaster. 2042 17
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