Autoinhibition and relief mechanism for Polo-like kinase 4

Klebba, Joseph E.; Buster, Daniel W.; McLamarrah, Tiffany A.; Rusan, Nasser M.; Rogers, Gerald S.

doi:10.1073/pnas.1417967112

Cited by 71 publications

(104 citation statements)

References 55 publications

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“…Our biochemical assays reveal that Cep78 interacts predominantly with the N-terminal domain of Plk4 and only weakly with the C-terminus. Given that the C-terminal Plk4 fragment heterodimerizes with full-length Plk4 (Klebba et al, 2015), it is conceivable that Cep78 was pulled out bound to the N-terminal part of full-length Plk4. We further established the interaction by immunoprecipitation of endogenous Cep78 and Plk4 (Fig.…”

Section: Results and Discussion Cep78 Is A Plk4-interacting Proteinmentioning

confidence: 99%

Cep78 is a new centriolar protein involved in Plk4-induced centriole overduplication

Brunk

Zhu

Bärenz

et al. 2016

Journal of Cell Science

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Centrioles are core components of centrosomes, the major microtubule-organizing centers of animal cells, and act as basal bodies for cilia formation. Control of centriole number is therefore crucial for genome stability and embryogenesis. Centriole duplication requires the serine/threonine protein kinase Plk4. Here, we identify Cep78 as a human centrosomal protein and a new interaction partner of Plk4. Cep78 is mainly a centriolar protein that localizes to the centriolar wall. Furthermore, we find that Plk4 binds to Cep78 through its N-terminal domain but that Cep78 is not an in vitro Plk4 substrate. Cep78 colocalizes with Plk4 at centrioles and is required for Plk4-induced centriole overduplication. Interestingly, upon depletion of Cep78, newly synthesized Plk4 is not localized to centrosomes. Our results suggest that the interaction between Cep78 and the N-terminal catalytic domain of Plk4 is a new and important element in the centrosome overduplication process.

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Section: Results and Discussion Cep78 Is A Plk4-interacting Proteinmentioning

confidence: 99%

Cep78 is a new centriolar protein involved in Plk4-induced centriole overduplication

Brunk

Zhu

Bärenz

et al. 2016

Journal of Cell Science

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“…Therefore, PLK4 protein levels and kinase activity must be tightly regulated. This is achieved in part by PLK4 protein stability being regulated by auto-phosphorylation, which triggers ubiquitin-mediated proteasomal degradation (reviewed in refs 28, 29, 30). Whereas the mechanisms regulating PLK4 activation, protein ubiquitination and degradation have been clarified, those modulating PLK4 kinase activity remain elusive.…”

mentioning

confidence: 99%

KAT2A/KAT2B-targeted acetylome reveals a role for PLK4 acetylation in preventing centrosome amplification

et al. 2016

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Lysine acetylation is a widespread post-translational modification regulating various biological processes. To characterize cellular functions of the human lysine acetyltransferases KAT2A (GCN5) and KAT2B (PCAF), we determined their acetylome by shotgun proteomics. One of the newly identified KAT2A/2B substrate is polo-like kinase 4 (PLK4), a key regulator of centrosome duplication. We demonstrate that KAT2A/2B acetylate the PLK4 kinase domain on residues K45 and K46. Molecular dynamics modelling suggests that K45/K46 acetylation impairs kinase activity by shifting the kinase to an inactive conformation. Accordingly, PLK4 activity is reduced upon in vitro acetylation of its kinase domain. Moreover, the overexpression of the PLK4 K45R/K46R mutant in cells does not lead to centrosome overamplification, as observed with wild-type PLK4. We also find that impairing KAT2A/2B-acetyltransferase activity results in diminished phosphorylation of PLK4 and in excess centrosome numbers in cells. Overall, our study identifies the global human KAT2A/2B acetylome and uncovers that KAT2A/2B acetylation of PLK4 prevents centrosome amplification.

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“…13 PLK4 has a kinase domain at its amino terminal and three PB domains mediating centriole localization and homodimerization at its carboxyl terminal. 14 PLK4 autophosphorylation regulates its activity, 15,16 which is strictly controlled in terms of timing and location during the cell cycle. 17 We have shown from our current analyses that the p.(C779Y) PLK4 variant lacks the normal function in centriole duplication.…”

Section: Discussionmentioning

confidence: 99%

“…It is thus probable that the p.(C779Y) variant in the PB2 domain impedes the homodimerization of PLK4 and consequently the loss of normal protein function due to the prevalence of the monomeric form. 16 On the other hand, the p.(M148V) variant in the kinase domain of PLK4 could amplify the number of centrioles at WT levels when overexpressed in HeLa cells. It is therefore possible that the overexpressed p.(M148V) variant does not reduce the overall kinase activity levels of PLK4 in the presence of the WT protein even if it lacks kinase activity itself.…”

Section: Discussionmentioning

confidence: 99%

Novel compound heterozygous variants in PLK4 identified in a patient with autosomal recessive microcephaly and chorioretinopathy

et al. 2016

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Autoinhibition and relief mechanism for Polo-like kinase 4

Cited by 71 publications

References 55 publications

Cep78 is a new centriolar protein involved in Plk4-induced centriole overduplication

Cep78 is a new centriolar protein involved in Plk4-induced centriole overduplication

KAT2A/KAT2B-targeted acetylome reveals a role for PLK4 acetylation in preventing centrosome amplification

Novel compound heterozygous variants in PLK4 identified in a patient with autosomal recessive microcephaly and chorioretinopathy

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