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Marker-independent Method for Isolating Slow-Dividing Cancer Stem Cells in Human Glioblastoma

Abstract Glioblastoma (GBM) is a devastating brain tumor with a poor survival outcome. It is generated and propagated by a small subpopulation of rare and hierarchically organized cells that share stem-like features with normal stem cells but, however, appear dysregulated in terms of self-renewal an...

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Published in:	Neoplasia (New York, N.Y.) N.Y.), 2013-07, Vol.15 (7), p.840-IN39
Main Authors:	Richichi, Cristina, Brescia, Paola, Alberizzi,, Valeria, Fornasari, Lorenzo, Pelicci, Giuliana
Format:	Article
Language:	English
Subjects:	Animals Antigens, Surface - metabolism Brain Neoplasms - genetics Brain Neoplasms - metabolism Cell Cycle Cell Separation - methods Cell Transformation, Neoplastic - genetics Cell Transformation, Neoplastic - metabolism Flow Cytometry Glioblastoma - genetics Glioblastoma - metabolism Heterografts Humans Immunophenotyping Mice Neoplastic Stem Cells - cytology Neoplastic Stem Cells - metabolism Neoplastic Stem Cells - transplantation Oncology Organic Chemicals - metabolism Spheroids, Cellular Transcriptome Tumor Cells, Cultured Tumor Stem Cell Assay
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creator	Richichi, Cristina Brescia, Paola Alberizzi,, Valeria Fornasari, Lorenzo Pelicci, Giuliana
description	Abstract Glioblastoma (GBM) is a devastating brain tumor with a poor survival outcome. It is generated and propagated by a small subpopulation of rare and hierarchically organized cells that share stem-like features with normal stem cells but, however, appear dysregulated in terms of self-renewal and proliferation and aberrantly differentiate into cells forming the bulk of the disorganized cancer tissues. The complexity and heterogeneity of human GBMs underlie the lack of standardized and effective treatments. This study is based on the assumption that available markers defining cancer stem cells (CSCs) in all GBMs are not conclusive and further work is required to identify the CSC. We implemented a method to isolate CSCs independently from cell surface markers: four patient-derived GBM neurospheres containing stem, progenitors, and differentiated cells were labeled with PKH-26 fluorescent dye that reliably selects for cells that divide at low rate. Through in vitro and in vivo assays, we investigated the growth and self-renewal properties of the two different compartments of high- and slow-dividing cells. Our data demonstrate that only slow-dividing cells retain the ability of a long-lasting self-renewal capacity after serial in vitro passaging, while high-dividing cells eventually exhaust. Moreover, orthotopic transplantation assay revealed that the incidence of tumors generated by the slow-dividing compartment is significantly higher in the four patient-derived GBM neurospheres analyzed. Importantly, slow-dividing cells feature a population made up of homogeneous stem cells that sustain tumor growth and therefore represent a viable target for GBM therapy development.
doi_str_mv	10.1593/neo.13662
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Through in vitro and in vivo assays, we investigated the growth and self-renewal properties of the two different compartments of high- and slow-dividing cells. Our data demonstrate that only slow-dividing cells retain the ability of a long-lasting self-renewal capacity after serial in vitro passaging, while high-dividing cells eventually exhaust. Moreover, orthotopic transplantation assay revealed that the incidence of tumors generated by the slow-dividing compartment is significantly higher in the four patient-derived GBM neurospheres analyzed. 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Through in vitro and in vivo assays, we investigated the growth and self-renewal properties of the two different compartments of high- and slow-dividing cells. Our data demonstrate that only slow-dividing cells retain the ability of a long-lasting self-renewal capacity after serial in vitro passaging, while high-dividing cells eventually exhaust. Moreover, orthotopic transplantation assay revealed that the incidence of tumors generated by the slow-dividing compartment is significantly higher in the four patient-derived GBM neurospheres analyzed. 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subjects	Animals Antigens, Surface - metabolism Brain Neoplasms - genetics Brain Neoplasms - metabolism Cell Cycle Cell Separation - methods Cell Transformation, Neoplastic - genetics Cell Transformation, Neoplastic - metabolism Flow Cytometry Glioblastoma - genetics Glioblastoma - metabolism Heterografts Humans Immunophenotyping Mice Neoplastic Stem Cells - cytology Neoplastic Stem Cells - metabolism Neoplastic Stem Cells - transplantation Oncology Organic Chemicals - metabolism Spheroids, Cellular Transcriptome Tumor Cells, Cultured Tumor Stem Cell Assay
title	Marker-independent Method for Isolating Slow-Dividing Cancer Stem Cells in Human Glioblastoma
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