Cycloheximide Chase Analysis of Protein Degradation in &lt;em&gt;Saccharomyces cerevisiae&lt;/em&gt;

Buchanan, Bryce W.; Lloyd, Michael E.; Engle, Sarah M.; Rubenstein, Eric M.

doi:10.3791/53975

Cited by 59 publications

(50 citation statements)

References 62 publications

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“…We performed a cycloheximide (CX) chase analysis to observe the role of HUNK in EGFR degradation. CX inhibits translation by impairing ribosomal translocation, and over time an unstable protein will decrease in expression whereas a stable protein will not [27]. Consistent with Bao et al observations, HUNK down-regulation rescued EGFR degradation after CX treatment (Fig.…”

Section: Hunk Regulates Egfr Stability Leading To Downstream Signalinsupporting

confidence: 88%

HUNK phosphorylates EGFR to regulate breast cancer metastasis

et al. 2019

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Epidermal growth factor receptor (EGFR) is commonly over-expressed in metastatic breast cancer yet metastatic breast cancer is generally resistant to anti-EGFR therapies, and the mechanism for resistance to EGFR inhibitors in this setting is not fully understood. Hormonally up-regulated neu-associated kinase (HUNK) kinase is up-regulated in aggressive breast cancers and is thought to play a role in breast cancer metastasis. However, no studies have been conducted to examine a relationship between EGFR and HUNK in breast cancer metastasis. We performed a kinase substrate screen and identified that EGFR is phosphorylated by HUNK. Our studies show that HUNK phosphorylates EGFR at T654, enhancing receptor stability and downstream signaling. We found that increased phosphorylation of T654 EGFR correlates with increased epithelial to mesenchymal, migration and invasion, and metastasis. In addition, we found that HUNK expression correlates with overall survival and distant metastasis free survival. This study shows that HUNK directly phosphorylates EGFR at T654 to promote metastasis and is the first study to show that the phosphorylation of this site in EGFR regulates metastasis.

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Section: Hunk Regulates Egfr Stability Leading To Downstream Signalinsupporting

confidence: 88%

HUNK phosphorylates EGFR to regulate breast cancer metastasis

et al. 2019

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“…To obtain information about protein stability, synthesis has to be inhibited. Therefore, a cycloheximide-chase experiment was performed to determine FoxM1 protein stability in untreated SW480 cultures [23]. 40 µM cyc that effectively blocked protein synthesis were added to the culture medium, and protein lysates were obtained at different time points after addition of the inhibitor.…”

Section: C)mentioning

confidence: 99%

“…40 µM cyc that effectively blocked protein synthesis were added to the culture medium, and protein lysates were obtained at different time points after addition of the inhibitor. Protein abundance was assessed by western blot to determine the FoxM1 half-life [23]. ▶ Fig.…”

Section: C)mentioning

confidence: 99%

Destabilization of FoxM1 and Inhibition of Topoisomerase I Contribute to Cytotoxicity of Prenylated Xanthones Isolated from Metaxya rostrata

Mittermair

Schueffl²,

Heffeter³

et al. 2020

Planta Med

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We recently isolated the prenylated xanthones 2-deprenyl-rheediaxanthone B (XB) and 2-deprenyl-7-hydroxy-rheediaxanthone B (OH-XB) from the South American tree fern Metaxya rostrata. This study explores the mechanisms underlying the FoxM1 downregulation induced by both xanthones. Analysis of cell viability and cell-death induction in SW480, HCT116, Caco-2, DLD1 and HT29 exposed to xanthones found cell-loss and activation of caspase in all cell lines except HT29 that do not have high FoxM1 protein levels. To determine the cellular mechanism of xanthone-induced FoxM1 loss, protein stability was analyzed by cycloheximide-chase experiments and showed reduction of FoxM1 stability by XB but not OH-XB. Destabilization was prevented by inhibiting proteasome activity using MG-132 and moderately by the lysosomal inhibitor bafilomycin A1 (baf A1). OH-XB had a stronger impact than XB on FoxM1 mRNA expression by qRT-PCR, and MG-132 positively affected FoxM1 protein level in OH-XB exposed cells even though no decrease in protein abundance had been induced by the xanthone. Additionally, the compound inhibited topoisomerase I causing DNA DSB and early cell cycle arrest. This may reduce FoxM1 gene expression, which may in turn compromise DNA repair and enhance xanthone-induced cell death. With regard to xanthone-induced cell death, MG-132 protected cultures from cell loss induced by both compounds, and baf A1 was active against these XB-induced effects. In summary, both destabilization of FoxM1 protein and topoisomerase I inhibition contribute to both XB and OH-XB cytotoxic activity albeit at different ratios.

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“…These results suggested that HZ00 was possibly able to stabilize p53 through some other mechanism. We performed a cycloheximide chase study (195) to see whether HZ00 was able to stabilize p53 and prevent its degradation by the protein synthesis inhibitor. However, there was no indication that the main mechanism of action of the molecule was to stabilize p53.…”

Section: Characterization Of Hz00mentioning

confidence: 99%