A Time-Resolved Fluorescence Resonance Energy Transfer Assay for High-Throughput Screening of 14-3-3 Protein–Protein Interaction Inhibitors

Du, Yuhong; Fu, Robert W.; Liu, Bin; Zhao, Jingquan; Qui, Min; Khuri, Fadlo R.; Fu, Haian

doi:10.1089/adt.2013.507

Cited by 29 publications

(24 citation statements)

References 42 publications

(57 reference statements)

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“…Procedures for TR-FRET assay were the same as previously described (Du et al, 2013; Du and Havel, 2012). Briefly, overexpressed proteins (Drosha-FLAG, FLAG-MKK3, GST-p38 and GST-MKK3) from various cell lysates after transfection were collected and diluted in FRET buffer.…”

Section: Methodsmentioning

confidence: 99%

Stress Induces p38 MAPK-Mediated Phosphorylation and Inhibition of Drosha-Dependent Cell Survival

Yang

She

et al. 2015

Molecular Cell

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SUMMARY MicroRNAs (miRNAs) regulate the translational potential of their mRNA targets and control many cellular processes. The key step in canonical miRNA biogenesis is the cleavage of the primary transcripts by the nuclear RNase III enzyme Drosha. Emerging evidence suggests that the miRNA biogenic cascade is tightly controlled. However, little is known whether Drosha is regulated. Here we show that Drosha is targeted by stress. Under stress, p38 MAPK directly phosphorylates Drosha at its N-terminus. This reduces its interaction with DiGeorge syndrome critical region 8, and promotes its nuclear export and degradation by calpain. This regulatory mechanism mediates stress-induced inhibition of Drosha function. Reduction of Drosha sensitizes cells to stress and increases death. In contrast, increase in Drosha attenuates stress-induced death. These findings reveal a critical regulatory mechanism by which stress engages p38 MAPK pathway to destabilize Drosha and inhibit Drosha-mediated cellular survival.

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Section: Methodsmentioning

confidence: 99%

Stress Induces p38 MAPK-Mediated Phosphorylation and Inhibition of Drosha-Dependent Cell Survival

Yang

She

et al. 2015

Molecular Cell

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“…The positive control Bad pS136 peptide and R18, which specifically bind to the amphipathic groove of 14-3-3 with high affinity, completely blocked the binding of GST-Cables1 with His-14-3-3γ at 10 μM. Next, we tested whether these Cables1 peptides can directly interact with 14-3-3 protein in a defined in vitro system using a homogenous TR-FRET assay (26). The TR-FRET assay provides a sensitive measurement for proximity based molecular interactions to evaluate the binding of the donor-fluorophore (Tb)-coupled 14-3-3 proteins with FITC-labeled Cables1 peptides.…”

Section: Resultsmentioning

confidence: 99%

“…Our published protocols for the TR-FRET assay were followed (26, 27). FITC-conjugated Cables1 T44 (FITC-Ahx-ENAPLRRCRTLSGSPR), T150 (FITC-Ahx-TNAFGARRNTIDSTSS), pT44 (FITC-Ahx-ENAPLRRCR (pT) LSGSPR) and pT150 (FITC-Ahx-TNAFGARRN (pT) IDSTSS) peptides were synthesized by Peptide 2.0 Inc (>80% purity).…”

Section: Methodsmentioning

confidence: 99%

Cables1 Complex Couples Survival Signaling to the Cell Death Machinery

Shi

Park

et al. 2015

Cancer Research

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Cables1 is a candidate tumor suppressor that negatively regulates cell growth by inhibiting cyclin-dependent kinases. Cables1 expression is lost frequently in human cancer but little is known about its regulation. Here we report that Cables1 levels are controlled by a phosphorylation and 14-3-3 dependent mechanism. Mutagenic analyses identified two residues, T44 and T150, that are specifically critical for 14-3-3 binding and that serve as substrates for phosphorylation by the cell survival kinase Akt, which by binding directly to Cables1 recruits 14-3-3 to the complex. In cells Cables1 overexpression induced apoptosis and inhibited cell growth in part by stabilizing p21 and decreasing Cdk2 kinase activity. Ectopic expression of activated Akt prevented Cables1-induced apoptosis. Clinically, levels of phosphorylated Cables1 and phosphorylated Akt correlated with each other in human lung cancer specimens, consistent with pathophysiologic significance. Together, our results illuminated a dynamic regulatory system through which activated Akt and 14-3-3 work directly together to neutralize a potent tumor suppressor function of Cables1.

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“…21), these efforts have proven challenging at least in part due to difficulty in developing high-throughput screens for 14-3-3 activity (although recent progress has been made in this area (31)). This challenge motivated us to look for other ways to manipulate 14-3-3 binding, potentially via 14-3-3 regulatory mechanisms.…”

Section: Acetylated Lysines Within the 14-3-3 Binding Pocket Andmentioning

confidence: 99%

Histone Deacetylase 6 (HDAC6) Promotes the Pro-survival Activity of 14-3-3ζ via Deacetylation of Lysines within the 14-3-3ζ Binding Pocket

Mortenson¹,

Heppler²,

Banks³

et al. 2015

Journal of Biological Chemistry

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A Time-Resolved Fluorescence Resonance Energy Transfer Assay for High-Throughput Screening of 14-3-3 Protein–Protein Interaction Inhibitors

Cited by 29 publications

References 42 publications

Stress Induces p38 MAPK-Mediated Phosphorylation and Inhibition of Drosha-Dependent Cell Survival

Stress Induces p38 MAPK-Mediated Phosphorylation and Inhibition of Drosha-Dependent Cell Survival

Cables1 Complex Couples Survival Signaling to the Cell Death Machinery

Histone Deacetylase 6 (HDAC6) Promotes the Pro-survival Activity of 14-3-3ζ via Deacetylation of Lysines within the 14-3-3ζ Binding Pocket

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