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Using an adherent cell culture of the mouse subependymal zone to study the behavior of adult neural stem cells on a single-cell level
Author(s) -
Felipe Ortega,
Marcos R. Costa,
Tatiana SimonEbert,
Timm Schroeder,
Magdalena Götz,
Benedikt Berninger
Publication year - 2011
Publication title -
nature protocols
Language(s) - English
Resource type - Journals
SCImago Journal Rank - 7.471
H-Index - 245
eISSN - 1754-2189
pISSN - 1750-2799
DOI - 10.1038/nprot.2011.404
Subject(s) - subependymal zone , neural stem cell , neuroblast , microbiology and biotechnology , biology , cell division , stem cell , lineage (genetic) , immunocytochemistry , live cell imaging , cell , neurogenesis , neuroscience , genetics , gene , endocrinology
A comprehensive understanding of the cell biology of adult neural stem cells (aNSCs) requires direct observation of aNSC division and lineage progression in the absence of niche-dependent signals. Here we describe a culture preparation of the adult mouse subependymal zone (SEZ), which allows for continuous single-cell tracking of aNSC behavior. The protocol involves the isolation (approximately 3 h) and culture of cells from the adult SEZ at low density in the absence of mitogenic growth factors in chemically defined medium and subsequent live imaging using time-lapse video microscopy (5-7 d); these steps are followed by postimaging immunocytochemistry to identify progeny (approximately 7 h). This protocol enables the observation of the progression from slow-dividing aNSCs of radial/astroglial identity up to the neuroblast stage, involving asymmetric and symmetric cell divisions of distinct fast-dividing precursors. This culture provides an experimental system for studying instructive or permissive effects of signal molecules on aNSC modes of cell division and lineage progression.

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