Puget Stéphanie, Grill Jacques, Valent Alexander, Bieche Ivan, Dantas-Barbosa Carmela, Kauffmann Audrey, Dessen Philippe, Lacroix Ludovic, Geoerger Birgit, Job Bastien, Dirven Clemens, Varlet Pascale, Peyre Mathieu, Dirks Peter B, Sainte-Rose Christian, Vassal Gilles
Department of Neurosurgery, Peter B Dirks, Christian Sainte-Rose, and Gilles Vassal Hôpital Necker Enfants Malades, Université Paris Descartes, France.
J Clin Oncol. 2009 Apr 10;27(11):1884-92. doi: 10.1200/JCO.2007.15.4195. Epub 2009 Mar 16.
The molecular pathogenesis of pediatric ependymoma remains unclear. Our study was designed to identify genetic changes implicated in ependymoma progression.
We characterized 59 ependymoma samples (33 at diagnosis and 26 at relapse) using array-comparative genomic hybridization (aCGH). Specific chromosomal imbalances were confirmed by fluorescent in situ hybridization, and candidate genes were assessed by real-time quantitative polymerase chain reaction (qPCR), immunohistochemistry, sequencing, and in vitro functional studies.
aCGH analysis revealed a significant increase in genomic imbalances on relapse compared with diagnosis, such as gain of 9qter and 1q (54% v 21% and 12% v 0%, respectively) and loss of 6q (27% v 6%). Supervised tumor classification showed that gain of 9qter was associated with tumor recurrence, age older than 3 years, and posterior fossa location. Using a candidate-gene strategy, we found an overexpression of two potential oncogenes at the locus 9qter: Tenascin-C and Notch1. Moreover, Notch pathway analysis (qPCR) revealed overexpression of Notch ligands, receptors, and target genes (Hes-1, Hey2, and c-Myc), and downregulation of Notch repressor Fbxw7. We confirmed by immunohistochemistry the overexpression of Tenascin-C and Hes-1. We detected Notch1 missense mutations in 8.3% of the tumors (only in the posterior fossa location and in case of 9q33-34 gain). Furthermore, inhibition of Notch pathway with a gamma-secretase inhibitor impaired the growth of ependymoma stem cell cultures.
The activation of the Notch pathway and Tenascin-C seem to be important events in ependymoma progression and may represent future targets for therapy. We report, to our knowledge for the first time, recurrent oncogenic mutations in pediatric posterior fossa ependymomas.
小儿室管膜瘤的分子发病机制尚不清楚。我们的研究旨在确定与室管膜瘤进展相关的基因变化。
我们使用阵列比较基因组杂交(aCGH)对59例室管膜瘤样本(33例诊断时样本和26例复发时样本)进行了特征分析。通过荧光原位杂交确认特定的染色体失衡,并通过实时定量聚合酶链反应(qPCR)、免疫组织化学、测序和体外功能研究评估候选基因。
aCGH分析显示,与诊断时相比,复发时基因组失衡显著增加,如9qter和1q增益(分别为54%对21%和12%对0%)以及6q缺失(27%对6%)。监督肿瘤分类显示,9qter增益与肿瘤复发、年龄大于3岁以及后颅窝位置相关。采用候选基因策略,我们发现9qter位点的两个潜在癌基因:腱生蛋白-C和Notch1过表达。此外,Notch通路分析(qPCR)显示Notch配体、受体和靶基因(Hes-1、Hey2和c-Myc)过表达,而Notch抑制因子Fbxw7下调。我们通过免疫组织化学证实了腱生蛋白-C和Hes-1的过表达。我们在8.3%的肿瘤中检测到Notch1错义突变(仅在后颅窝位置且存在9q33 - 34增益的情况下)。此外,用γ-分泌酶抑制剂抑制Notch通路会损害室管膜瘤干细胞培养物的生长。
Notch通路和腱生蛋白-C的激活似乎是室管膜瘤进展中的重要事件,可能代表未来的治疗靶点。据我们所知,我们首次报道了小儿后颅窝室管膜瘤中的复发性致癌突变。
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