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Cross-species genomics matches driver mutations and cell compartments to model ependymoma

室管膜瘤 生物 转录组 CDKN2A 神经干细胞 基因 遗传学 病理 干细胞 基因表达 医学
作者
Robert A. Johnson,Karen Wright,Helen Poppleton,Kumarasamypet M. Mohankumar,David Finkelstein,Stanley Pounds,Vikki Rand,Sarah Leary,Elsie White,Christopher Eden,Twala L. Hogg,Paul A. Northcott,Stephen C. Mack,Geoffrey Neale,Yong‐Dong Wang,Beth Coyle,Jennifer M. Atkinson,Mariko DeWire,Tanya A. Kranenburg,G. Yancey Gillespie,Jeffrey C. Allen,Thomas E. Merchant,Fredrick A. Boop,Robert A. Sanford,Amar Gajjar,David W. Ellison,Michael D. Taylor,Richard G. Grundy,Richard J. Gilbertson
出处
期刊:Nature [Nature Portfolio]
卷期号:466 (7306): 632-636 被引量:346
标识
DOI:10.1038/nature09173
摘要

Ependymoma is a type of neural tumour that arises throughout the central nervous system. Using comparative transcriptomics in mouse and human tumours, Johnson et al. home in on mutations that are specific to individual tumour subgroups. In the course of their study, the authors generate the first mouse model of ependymoma and demonstrate the power of interspecific genomic comparisons to interrogate cancer subgroups. Ependymoma is a type of neural tumour that arises throughout the central nervous system. Using comparative transcriptomics in mouse and human tumours, these authors home in on mutations that are specific to individual tumour subgroups. In doing so, they generate the first mouse model of ependymoma and demonstrate the power of interspecific genomic comparisons to interrogate cancer subgroups. Understanding the biology that underlies histologically similar but molecularly distinct subgroups of cancer has proven difficult because their defining genetic alterations are often numerous, and the cellular origins of most cancers remain unknown1,2,3. We sought to decipher this heterogeneity by integrating matched genetic alterations and candidate cells of origin to generate accurate disease models. First, we identified subgroups of human ependymoma, a form of neural tumour that arises throughout the central nervous system (CNS). Subgroup-specific alterations included amplifications and homozygous deletions of genes not yet implicated in ependymoma. To select cellular compartments most likely to give rise to subgroups of ependymoma, we matched the transcriptomes of human tumours to those of mouse neural stem cells (NSCs), isolated from different regions of the CNS at different developmental stages, with an intact or deleted Ink4a/Arf locus (that encodes Cdkn2a and b). The transcriptome of human supratentorial ependymomas with amplified EPHB2 and deleted INK4A/ARF matched only that of embryonic cerebral Ink4a/Arf−/− NSCs. Notably, activation of Ephb2 signalling in these, but not other, NSCs generated the first mouse model of ependymoma, which is highly penetrant and accurately models the histology and transcriptome of one subgroup of human supratentorial tumour. Further, comparative analysis of matched mouse and human tumours revealed selective deregulation in the expression and copy number of genes that control synaptogenesis, pinpointing disruption of this pathway as a critical event in the production of this ependymoma subgroup. Our data demonstrate the power of cross-species genomics to meticulously match subgroup-specific driver mutations with cellular compartments to model and interrogate cancer subgroups.

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