A Cell Biologist’s Field Guide to Aurora Kinase Inhibitors

Groot, Christian O. De; Hsia, Judy E.; Anzola, John V.; Motamedi, Amir; Yoon, Michelle; Wong, Yao Liang; Jenkins, David; Lee, Hyun Jae; Martinez, Mallory B.; Davis, Robert L.; Gahman, Timothy C.; Desai, Arshad; Shiau, Andrew K.

doi:10.3389/fonc.2015.00285

Cited by 89 publications

(121 citation statements)

References 117 publications

(145 reference statements)

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“…We then used the same antibody to look by immunofluorescence (IF) in fixed mitotic cells, marking centrosomes with γ-tubulin staining. All phospho-epitope signal on the centrosomes and spindle poles was abolished by treatment with AURKA inhibitor MLN8237, whereas the signal at the midbody (where the same antibody recognizes pT232 of AURKB) was insensitive to 100 nM MLN8237, indicating that the centrosomal pT288 signal is specific to AURKA as expected ( Figure 1B, Supplementary Figure S1) [34,35]. We quantified fluorescence intensity associated with pT288 at different stages of mitosis scored according to DNA morphology.…”

Section: Resultsmentioning

confidence: 62%

“…(Supplementary Figure S3). This finding was not unexpected for a diffusible biosensor, since some of the specificity in substrate phosphorylation by Aurora kinases is proposed to reside in the colocalization of kinase with substrates [3,35]. We transfected this biosensor into U2OS and FZR1 KO cells to measure Aurora kinase activity at mitosis and during mitotic exit.…”

Section: Resultsmentioning

confidence: 79%

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AURKA destruction is decoupled from its activity at mitotic exit but suppresses interphase activity

Abdelbaki

Akman

Poteau³

et al. 2019

Preprint

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Activity of AURKA is controlled through multiple mechanisms including phosphorylation, ubiquitinmediated degradation, and allosteric interaction with TPX2. Activity peaks at mitosis before AURKA is degraded during mitotic exit in a process strictly dependent on APC/C coactivator FZR1. We used FZR1 knockout cells (FZR1 KO ) and a novel FRET-based AURKA biosensor to investigate how activity is regulated in absence of destruction. We found that AURKA activity in FZR1 KO cells dropped at mitotic exit as rapidly as in parental cells, despite absence of destruction. Unexpectedly, TPX2 was degraded normally in FZR1 KO cells. Overexpression of an N-terminal TPX2 fragment sufficient for AURKA binding, but not degraded at mitotic exit, caused delay in AURKA inactivation. We conclude that AURKA inactivation in mitotic exit is determined not by its own degradation but by degradation of TPX2 and therefore dependent on CDC20 rather than FZR1. The biosensor revealed that FZR1 instead suppresses AURKA activity in interphase and is critically required for assembly of the interphase mitochondrial network after mitosis.

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Section: Resultsmentioning

confidence: 62%

Section: Resultsmentioning

confidence: 79%

AURKA destruction is decoupled from its activity at mitotic exit but suppresses interphase activity

Abdelbaki

Akman

Poteau³

et al. 2019

Preprint

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“…Hesperadin is an indolinone inhibitor of Aurora-B (half-maximal inhibitory concentration [IC 50 ] = 250 nM; de Groot et al., 2015), while LLY-507 is a potent inhibitor of KMT3C (IC 50 < 15 nM, >100-fold selectivity over other MTs; Nguyen et al., 2015). Short pretreatments with either compound inhibited TPA-induced PolII recruitment and histone modifications at Egr1 , Egr3 , and Fosl1 (Figure 7A).…”

Section: Resultsmentioning

confidence: 99%

ERK-Induced Activation of TCF Family of SRF Cofactors Initiates a Chromatin Modification Cascade Associated with Transcription

et al. 2017

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SummaryWe investigated the relationship among ERK signaling, histone modifications, and transcription factor activity, focusing on the ERK-regulated ternary complex factor family of SRF partner proteins. In MEFs, activation of ERK by TPA stimulation induced a common pattern of H3K9acS10ph, H4K16ac, H3K27ac, H3K9acK14ac, and H3K4me3 at hundreds of transcription start site (TSS) regions and remote regulatory sites. The magnitude of the increase in histone modification correlated well with changes in transcription. H3K9acS10ph preceded the other modifications. Most induced changes were TCF dependent, but TCF-independent TSSs exhibited the same hierarchy, indicating that it reflects gene activation per se. Studies with TCF Elk-1 mutants showed that TCF-dependent ERK-induced histone modifications required Elk-1 to be phosphorylated and competent to activate transcription. Analysis of direct TCF-SRF target genes and chromatin modifiers confirmed this and showed that H3S10ph required only Elk-1 phosphorylation. Induction of histone modifications following ERK stimulation is thus directed by transcription factor activation and transcription.

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“…MK-5108 (VX-689) inhibits proliferation of breast, colon, and non-small cell lung cancer, leukemia, nasopharyngeal carcinoma, uterine leiomyosarcoma, and ovarian cancer stem cells in vivo and in vitro . The duration of G2 is prolonged by MK-5108 treatment, as also observed in cells treated with siRNA targeting Aurora A [24]. MK-5108 treatment also prolongs mitosis [25, 26] and increases the proportion of H3-pS10–positive mitotic cells [25, 27–30].…”

Section: Discussionmentioning

confidence: 94%

The Aurora kinase A inhibitor TC-A2317 disrupts mitotic progression and inhibits cancer cell proliferation

Min

Kim

2016

Oncotarget

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Mitotic progression is crucial for the maintenance of chromosomal stability. A proper progression is ensured by the activities of multiple kinases. One of these enzymes, the serine/threonine kinase Aurora A, is required for proper mitosis through the regulation of centrosome and spindle assembly. In this study, we functionally characterized a newly developed Aurora kinase A inhibitor, TC-A2317. In human lung cancer cells, TC-A2317 slowed proliferation by causing aberrant formation of centrosome and microtubule spindles and prolonging the duration of mitosis. Abnormal mitotic progression led to accumulation of cells containing micronuclei or multinuclei. Furthermore, TC-A2317–treated cells underwent apoptosis, autophagy or senescence depending on cell type. In addition, TC-A2317 inactivated the spindle assembly checkpoint triggered by paclitaxel, thereby exacerbating mitotic catastrophe. Consistent with this, the expression level of Aurora A in tumors was inversely correlated with survival in lung cancer patients. Collectively, these data suggest that inhibition of Aurora kinase A using TC-A2317 is a promising target for anti-cancer therapeutics.

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A Cell Biologist’s Field Guide to Aurora Kinase Inhibitors

Cited by 89 publications

References 117 publications

AURKA destruction is decoupled from its activity at mitotic exit but suppresses interphase activity

AURKA destruction is decoupled from its activity at mitotic exit but suppresses interphase activity

ERK-Induced Activation of TCF Family of SRF Cofactors Initiates a Chromatin Modification Cascade Associated with Transcription

The Aurora kinase A inhibitor TC-A2317 disrupts mitotic progression and inhibits cancer cell proliferation

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