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Genome analysis and gene expression profiling of neuroblastoma and ganglioneuroblastoma reveal differences between neuroblastic and Schwannian stromal cells

Cavazzana, Andrea; Di Cristofano, Claudio; Perri, Patrizia; Gambini, Claudio; Longo, Luca; Mazzocco, Katia; Moretti, Stefano; Bonassi, Stefano; Tonini, Gian Paolo; Coco, Simona; Defferrari, Raffaella; Scaruffi, Paola (2005), Genome analysis and gene expression profiling of neuroblastoma and ganglioneuroblastoma reveal differences between neuroblastic and Schwannian stromal cells, Journal of Pathology, 207, 3, p. 346-357. http://dx.doi.org/10.1002/path.1843

Type
Article accepté pour publication ou publié
Date
2005
Journal name
Journal of Pathology
Volume
207
Number
3
Publisher
Wiley
Pages
346-357
Publication identifier
http://dx.doi.org/10.1002/path.1843
Metadata
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Author(s)
Cavazzana, Andrea
Di Cristofano, Claudio
Perri, Patrizia
Gambini, Claudio
Longo, Luca
Mazzocco, Katia
Moretti, Stefano cc
Bonassi, Stefano
Tonini, Gian Paolo
Coco, Simona
Defferrari, Raffaella
Scaruffi, Paola
Abstract (EN)
Neuroblastic tumours are a group of paediatric cancers with marked morphological heterogeneity. Neuroblastoma (Schwannian stroma-poor) (NB-SP) is composed of undifferentiated neuroblasts. Ganglioneuroblastoma intermixed (Schwannian stroma-rich) (GNBi-SR) is predominantly composed of Schwannian stromal (SS) and neuroblastic (Nb) cells. There are contrasting reports suggesting that SS cells are non-neoplastic. In the present study, laser capture microdissection (LCM) was employed to isolate SS and Nb cells. Chromosome 1p36 deletion and MYCN gene amplification were found to be associated in two out of seven NB-SPs, whereas no abnormalities were observed in five GNBi-SRs. In some cases, loss of heterozygosity (LOH) at 1p36 loci was detected in Nb cells but not in the bulk tumour by LCM; furthermore, LOH was also identified in both SS and tumour tissue of a GNBi-SR. DNA gain and loss studied by comparative genomic hybridization were observed at several chromosome regions in NB-SP but in few regions of GNBi-SR. Finally, gene expression profiles studied using an oligo-microarray technique displayed two distinct signatures: in the first, 32 genes were expressed in NB-SP and in the second, 14 genes were expressed in GNBi-SR. The results show that NB-SP is composed of different morphologically indistinguishable malignant cell clones harbouring cryptic mutations that are detectable only after LCM. The degree of DNA imbalance is higher in NB-SP than in GNBi-SR. However, when the analysis of chromosome 1p36 is performed at the level of microdissection, LOH is also observed in SS cells. These data provide supportive evidence that SS cells have a less aggressive phenotype and play a role in tumour maturation. Copyright © 2005 Pathological Society of Great Britain and Ireland. Published by John Wiley & Sons, Ltd.
Subjects / Keywords
neuroblastic cell; Schwann cell; laser capture microdissection; gene expression profiling; comparative genomic hybridisation; loss of heterozygosity; neuroblastoma

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