Tomlins Scott A, Laxman Bharathi, Dhanasekaran Saravana M, Helgeson Beth E, Cao Xuhong, Morris David S, Menon Anjana, Jing Xiaojun, Cao Qi, Han Bo, Yu Jindan, Wang Lei, Montie James E, Rubin Mark A, Pienta Kenneth J, Roulston Diane, Shah Rajal B, Varambally Sooryanarayana, Mehra Rohit, Chinnaiyan Arul M
Michigan Center for Translational Pathology, Department of Pathology, University of Michigan Medical School, Ann Arbor, Michigan 48109, USA.
Nature. 2007 Aug 2;448(7153):595-9. doi: 10.1038/nature06024.
Recently, we identified recurrent gene fusions involving the 5' untranslated region of the androgen-regulated gene TMPRSS2 and the ETS (E26 transformation-specific) family genes ERG, ETV1 or ETV4 in most prostate cancers. Whereas TMPRSS2-ERG fusions are predominant, fewer TMPRSS2-ETV1 cases have been identified than expected on the basis of the frequency of high (outlier) expression of ETV1 (refs 3-13). Here we explore the mechanism of ETV1 outlier expression in human prostate tumours and prostate cancer cell lines. We identified previously unknown 5' fusion partners in prostate tumours with ETV1 outlier expression, including untranslated regions from a prostate-specific androgen-induced gene (SLC45A3) and an endogenous retroviral element (HERV-K_22q11.23), a prostate-specific androgen-repressed gene (C15orf21), and a strongly expressed housekeeping gene (HNRPA2B1). To study aberrant activation of ETV1, we identified two prostate cancer cell lines, LNCaP and MDA-PCa 2B, that had ETV1 outlier expression. Through distinct mechanisms, the entire ETV1 locus (7p21) is rearranged to a 1.5-megabase prostate-specific region at 14q13.3-14q21.1 in both LNCaP cells (cryptic insertion) and MDA-PCa 2B cells (balanced translocation). Because the common factor of these rearrangements is aberrant ETV1 overexpression, we recapitulated this event in vitro and in vivo, demonstrating that ETV1 overexpression in benign prostate cells and in the mouse prostate confers neoplastic phenotypes. Identification of distinct classes of ETS gene rearrangements demonstrates that dormant oncogenes can be activated in prostate cancer by juxtaposition to tissue-specific or ubiquitously active genomic loci. Subversion of active genomic regulatory elements may serve as a more generalized mechanism for carcinoma development. Furthermore, the identification of androgen-repressed and insensitive 5' fusion partners may have implications for the anti-androgen treatment of advanced prostate cancer.
最近,我们在大多数前列腺癌中发现了涉及雄激素调节基因TMPRSS2的5'非翻译区与ETS(E26转化特异性)家族基因ERG、ETV1或ETV4的复发性基因融合。虽然TMPRSS2-ERG融合最为常见,但根据ETV1高(异常)表达频率,已鉴定出的TMPRSS2-ETV1病例比预期的要少(参考文献3-13)。在此,我们探讨人类前列腺肿瘤和前列腺癌细胞系中ETV1异常表达的机制。我们在具有ETV1异常表达的前列腺肿瘤中鉴定出了以前未知的5'融合伴侣,包括来自前列腺特异性雄激素诱导基因(SLC45A3)和内源性逆转录病毒元件(HERV-K_22q11.23)的非翻译区、一个前列腺特异性雄激素抑制基因(C15orf21)以及一个高表达的管家基因(HNRPA2B1)。为了研究ETV1的异常激活,我们鉴定了两个具有ETV1异常表达的前列腺癌细胞系,LNCaP和MDA-PCa 2B。通过不同的机制,在LNCaP细胞(隐匿性插入)和MDA-PCa 2B细胞(平衡易位)中,整个ETV1基因座(7p21)重排至14q13.3-14q21.1处一个1.5兆碱基的前列腺特异性区域。由于这些重排的共同因素是ETV1的异常过表达,我们在体外和体内重现了这一事件,证明良性前列腺细胞和小鼠前列腺中ETV1的过表达赋予了肿瘤表型。ETS基因重排不同类型的鉴定表明,在前列腺癌中,休眠癌基因可通过与组织特异性或普遍活跃的基因组位点并列而被激活。活跃基因组调控元件的颠覆可能是癌症发展的一种更普遍机制。此外,雄激素抑制和不敏感的5'融合伴侣的鉴定可能对晚期前列腺癌的抗雄激素治疗具有重要意义。
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