A kinome siRNA screen identifies HGS as a potential target for liver cancers with oncogenic mutations in CTNNB1

Frédéric Canal; Elodie Anthony; Aurianne Lescure; Elaine Del Nery; Jacques Camonis; Franck Perez; Bruno Ragazzon; Christine Perret

doi:10.1186/s12885-015-2037-8

A kinome siRNA screen identifies HGS as a potential target for liver cancers with oncogenic mutations in CTNNB1

BMC Cancer. 2015 Dec 29:15:1020. doi: 10.1186/s12885-015-2037-8.

Authors

Frédéric Canal^{1

2

3

4

5}, Elodie Anthony⁶, Aurianne Lescure⁷, Elaine Del Nery⁸, Jacques Camonis⁹, Franck Perez¹⁰, Bruno Ragazzon^{11

12

13}, Christine Perret^{14

15

16

17}

Affiliations

¹ Department Development, Reproduction and Cancer, INSERM U1016, Institut Cochin, 24, rue du Faubourg Saint-Jacques, 75014, Paris, France. frederic.canal94@gmail.com.
² CNRS UMR8104, Paris, France. frederic.canal94@gmail.com.
³ Université Paris Descartes, Sorbonne, Paris Cité, France. frederic.canal94@gmail.com.
⁴ Equipe labellisée Ligue Nationale Contre le Cancer, Paris, France. frederic.canal94@gmail.com.
⁵ Laboratoire de Génétique et Biologie Cellulaire, Université de Versailles St-Quentin en Yvelines, Montigny le Bretonneux, France. frederic.canal94@gmail.com.
⁶ Department of Translational Research, the Biophenics High-Content Screening Laboratory, Institut Curie, PSL Research University, Paris, France. elodie.anth@gmail.com.
⁷ Department of Translational Research, the Biophenics High-Content Screening Laboratory, Institut Curie, PSL Research University, Paris, France. aurianne.lescure@curie.fr.
⁸ Department of Translational Research, the Biophenics High-Content Screening Laboratory, Institut Curie, PSL Research University, Paris, France. elaine.del.nery@curie.fr.
⁹ Department of Translational Research, the Biophenics High-Content Screening Laboratory, Institut Curie, PSL Research University, Paris, France. Jacques.camonis@gmail.com.
¹⁰ Department of Translational Research, the Biophenics High-Content Screening Laboratory, Institut Curie, PSL Research University, Paris, France. Franck.Perez@curie.fr.
¹¹ Department Development, Reproduction and Cancer, INSERM U1016, Institut Cochin, 24, rue du Faubourg Saint-Jacques, 75014, Paris, France. bruno.ragazzon@inserm.fr.
¹² CNRS UMR8104, Paris, France. bruno.ragazzon@inserm.fr.
¹³ Université Paris Descartes, Sorbonne, Paris Cité, France. bruno.ragazzon@inserm.fr.
¹⁴ Department Development, Reproduction and Cancer, INSERM U1016, Institut Cochin, 24, rue du Faubourg Saint-Jacques, 75014, Paris, France. christine.perret@inserm.fr.
¹⁵ CNRS UMR8104, Paris, France. christine.perret@inserm.fr.
¹⁶ Université Paris Descartes, Sorbonne, Paris Cité, France. christine.perret@inserm.fr.
¹⁷ Equipe labellisée Ligue Nationale Contre le Cancer, Paris, France. christine.perret@inserm.fr.

Abstract

Background: Aberrant activation of the Wnt/β-catenin pathway is a major and frequent event in liver cancer, but inhibition of oncogenic β-catenin signaling has proven challenging. The identification of genes that are synthetically lethal in β-catenin-activated cancer cells would provide new targets for therapeutic drug design.

Methods: We transfected the parental HuH6 hepatoblastoma cell line with a doxycycline-inducible shRNA against CTNNB1 (gene coding for β-catenin) to obtain an isogenic cell line pair with or without aberrant β-catenin signaling. Using this hepatoblastoma isogenic cell line pair, we performed a human kinome-wide siRNA screen to identify synthetic lethal interactions with oncogenic CTNNB1. The phenotypic readouts of the screen were cell proliferation, cell cycle arrest and apoptosis, which were assessed by image-based analysis. In addition, apoptosis was assessed by flow cytometric experiments and immunoblotting. The potential synthetic lethal relationship between candidates genes identified in the screen and oncogenic CTNNB1 was also investigated in a different cellular context, a colorectal HCT116 isogenic cell line pair.

Results: We first determined the experimental conditions that led to the efficient expression of shRNA against CTNNB1 and maximal reduction of β-catenin signaling activity in response to doxycycline treatment. Following high throughput screening in which 687 genes coding for kinases and proteins related to kinases (such as pseudokinases and phosphatases) were targeted, we identified 52 genes required for HuH6 survival. The silencing of five of these genes selectively impaired the viability of HuH6 cells with high β-catenin signaling: HGS, STRADA, FES, BRAF and PKMYT1. Among these candidates, HGS depletion had the strongest inhibitory effect on cell growth and led to apoptosis specifically in HuH6 with high β-catenin activity, while HuH6 with low β-catenin activity were spared. In addition, HGS was identified as a potential synthetic lethal partner of oncogenic CTNNB1 in the HCT116 colorectal isogenic cell line pair.

Conclusions: These results demonstrate the existence of crosstalk between β-catenin signaling and HGS. Importantly, HGS depletion specifically affected cells with uncontrolled β-catenin signaling activity in two different types of cancer (Hepatoblastoma HuH6 and colorectal HCT116), and thus may represent a new potential target for novel therapeutic strategies in liver and colorectal cancer.

Publication types

Research Support, Non-U.S. Gov't

MeSH terms

Apoptosis
Cell Cycle Checkpoints
Cell Line, Tumor
Cell Proliferation
Endosomal Sorting Complexes Required for Transport / genetics*
HCT116 Cells
Hepatoblastoma / genetics*
Humans
Liver Neoplasms / genetics*
Mutation*
Phosphoproteins / genetics*
Phosphotransferases / antagonists & inhibitors
RNA, Small Interfering / metabolism*
Wnt Signaling Pathway
beta Catenin / antagonists & inhibitors*
beta Catenin / genetics

Substances

CTNNB1 protein, human
Endosomal Sorting Complexes Required for Transport
Phosphoproteins
RNA, Small Interfering
beta Catenin
hepatocyte growth factor-regulated tyrosine kinase substrate
Phosphotransferases