PO.ET06.01 · 实验与分子治疗

USP7 and ITCH/UBE4B ubiquitin ligase regulate the switch between apoptosis and necroptosis via Ku70 and c-FLIPL polyubiquitination in neuroblastoma

海报缩略图:USP7 and ITCH/UBE4B ubiquitin ligase regulate the switch between apoptosis and necroptosis via Ku70 and c-FLIPL polyubiquitination in neuroblastoma
编号 5668 展板 6 时间 4/21 02:00–05:00 区域 Section 11 主讲 Christophe Le Clorennec, PhD
分会场 Cell Death Pathways and Treatment
查看完整资料 下载 PDF 登录后可访问当前开放资料 AACR 官方页面 ↗

作者与单位

Christophe Le Clorennec1, Carla Sampaio2, Peter E. Zage2

1UCSD Moores Cancer Center, La Jolla, CA,2Pediatrics, UCSD Moores Cancer Center, La Jolla, CA

摘要 Abstract

Dysregulation of the Ubiquitin Proteasome System has been linked to many human diseases, including cancer. Expression of UBE4B ubiquitin ligase is associated with neuroblastoma patient outcomes and its functional roles in neuroblastoma pathogenesis are not known. We have recently identified an ubiquitin ligase complex ITCH/UBE4B which mediates ubiquitination of Ku70 and c-FLIPL proteins for proteasomal degradation allowing HDAC inhibitor-mediated caspase-8 dependent apoptosis. We also confirmed that the deubiquitinase USP7, critical player in tumor suppression and DNA repair, can be a potential therapeutic target for neuroblastoma. Highly selective USP7 inhibitors have demonstrated significant antitumor activity in preclinical models of adult cancer, and we reported that these inhibitors alone can be more effective against neuroblastoma tumor growth. Our hypothesis is that USP7 inhibition will be more effective against neuroblastoma tumors through destabilization of ITCH/UBE4B complex protein targets allowing a stronger induction of cell death in response to treatment for the children. To evaluate efficacy of USP7 inhibitors in combination with HDAC inhibitors or chemotherapy against neuroblastoma tumor growth, neuroblastoma cell lines depleted for UBE4B or USP7 were treated with increasing concentrations of USP7 inhibitors alone or in combination with chemotherapy or with HDAC inhibitors. Cell proliferation was measured using continuous live cell imaging and apoptosis by caspase cleavage and PARP cleavage detection by western blot. We have evaluated also, whether ubiquitination/deubiquitination and degradation rates of p53, Ku70 and c-FLIPL proteins could modulate induction of apoptosis and necroptosis. USP7 inhibition resulted in decreases in cell viability in p53 wild-type neuroblastoma cell lines via the induction of apoptosis and necroptosis by increasing phosphorylation of MLKL, RIPK3 and RIPK1. In UBE4B or USP7 depleted cells, a huge induction of necroptosis and a small rate of apoptosis were observed. We also identified USP7 as a deubiquitinase of Ku70 and c-FLIPL, stabilizing the Ku70/c-FLIPL/Bax “FLIPosome” complex. USP7 inhibition destabilizes ku70 and c-FLIPL for protein degradation leading to induction of apoptosis as well as necroptosis. UBE4B depletion in neuroblastoma inhibits HDAC inhibitors mediated caspase-8 mediated apoptosis but enhances necroptosis, notably because the stabilization of the FLIPosome can allow the blockade of caspase-8 activation and can trigger the activation of the necroptosome. Our data suggests that USP7 and ITCH/UBE4B can control the switch between apoptosis and necroptosis in response to USP7 and HDAC inhibitors. USP7 inhibition and ITCH/UBE4B activation by HDAC inhibitors could be a promising therapeutic strategy for children with high-risk and relapsed neuroblastoma.
利益披露 Disclosure
C. Le Clorennec, None.. C. Sampaio, None.. P. E. Zage, None.

在会议检索中打开