Cheong Jit Kong, Gunaratnam Lakshman, Zang Zhi Jiang, Yang Christopher M, Sun Xiaoming, Nasr Susan L, Sim Khe Guan, Peh Bee Keow, Rashid Suhaimi Bin Abdul, Bonventre Joseph V, Salto-Tellez Manuel, Hsu Stephen I
Renal Division, Department of Medicine, Brigham and Women's Hospital, Harvard Medical School, Boston, MA 02115, USA.
J Transl Med. 2009 Jan 20;7:8. doi: 10.1186/1479-5876-7-8.
Members of the TRIP-Br/SERTAD family of mammalian transcriptional coregulators have recently been implicated in E2F-mediated cell cycle progression and tumorigenesis. We, herein, focus on the detailed functional characterization of the least understood member of the TRIP-Br/SERTAD protein family, TRIP-Br2 (SERTAD2).
Oncogenic potential of TRIP-Br2 was demonstrated by (1) inoculation of NIH3T3 fibroblasts, which were engineered to stably overexpress ectopic TRIP-Br2, into athymic nude mice for tumor induction and (2) comprehensive immunohistochemical high-throughput screening of TRIP-Br2 protein expression in multiple human tumor cell lines and human tumor tissue microarrays (TMAs). Clinicopathologic analysis was conducted to assess the potential of TRIP-Br2 as a novel prognostic marker of human cancer. RNA interference of TRIP-Br2 expression in HCT-116 colorectal carcinoma cells was performed to determine the potential of TRIP-Br2 as a novel chemotherapeutic drug target.
Overexpression of TRIP-Br2 is sufficient to transform murine fibroblasts and promotes tumorigenesis in nude mice. The transformed phenotype is characterized by deregulation of the E2F/DP-transcriptional pathway through upregulation of the key E2F-responsive genes CYCLIN E, CYCLIN A2, CDC6 and DHFR. TRIP-Br2 is frequently overexpressed in both cancer cell lines and multiple human tumors. Clinicopathologic correlation indicates that overexpression of TRIP-Br2 in hepatocellular carcinoma is associated with a worse clinical outcome by Kaplan-Meier survival analysis. Small interfering RNA-mediated (siRNA) knockdown of TRIP-Br2 was sufficient to inhibit cell-autonomous growth of HCT-116 cells in vitro.
This study identifies TRIP-Br2 as a bona-fide protooncogene and supports the potential for TRIP-Br2 as a novel prognostic marker and a chemotherapeutic drug target in human cancer.
哺乳动物转录共调节因子TRIP-Br/SERTAD家族的成员最近被认为与E2F介导的细胞周期进程和肿瘤发生有关。在此,我们着重于TRIP-Br/SERTAD蛋白家族中了解最少的成员TRIP-Br2(SERTAD2)的详细功能特性研究。
通过以下方式证明TRIP-Br2的致癌潜力:(1)将经过基因工程改造以稳定过表达异位TRIP-Br2的NIH3T3成纤维细胞接种到无胸腺裸鼠体内以诱导肿瘤形成;(2)对多种人类肿瘤细胞系和人类肿瘤组织微阵列(TMA)进行全面的免疫组织化学高通量筛选,以检测TRIP-Br2蛋白的表达。进行临床病理分析以评估TRIP-Br2作为人类癌症新型预后标志物的潜力。在HCT-116结肠癌细胞中进行TRIP-Br2表达的RNA干扰,以确定TRIP-Br2作为新型化疗药物靶点的潜力。
TRIP-Br2的过表达足以转化鼠成纤维细胞并促进裸鼠体内肿瘤发生。转化后的表型特征是通过上调关键的E2F反应基因细胞周期蛋白E、细胞周期蛋白A2、细胞分裂周期蛋白6和二氢叶酸还原酶来解除对E2F/DP转录途径的调控。TRIP-Br2在癌细胞系和多种人类肿瘤中经常过表达。临床病理相关性分析表明,通过Kaplan-Meier生存分析,肝细胞癌中TRIP-Br2的过表达与较差的临床结局相关。小干扰RNA介导的(siRNA)TRIP-Br2敲低足以在体外抑制HCT-116细胞的自主生长。
本研究确定TRIP-Br2为真正的原癌基因,并支持TRIP-Br2作为人类癌症新型预后标志物和化疗药物靶点的潜力。
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