Don't Look: Growing Clonal Versus Nonclonal Neural Stem Cell Colonies

被引:123
作者
Coles-Takabe, Brenda L. K. [1 ]
Brain, Ian [2 ]
Purpura, Kelly A. [3 ,4 ]
Karpowicz, Phillip [1 ]
Zandstra, Peter W. [3 ,4 ]
Morshead, Cindi M. [2 ]
Van der Kooy, Derek [1 ]
机构
[1] Univ Toronto, Dept Mol Genet, Toronto, ON M5S 3E1, Canada
[2] Univ Toronto, Dept Surg, Div Anat, Toronto, ON M5S 3E1, Canada
[3] Univ Toronto, Dept Chem Engn & Appl Chem, Toronto, ON M5S 3E1, Canada
[4] Univ Toronto, Inst Biomat & Biomed Engn, Toronto, ON M5S 3E1, Canada
基金
加拿大健康研究院; 加拿大自然科学与工程研究理事会;
关键词
Stem cell; Clonality; Tissue culture; Fluorescent mice;
D O I
10.1634/stemcells.2008-0558
中图分类号
Q813 [细胞工程];
学科分类号
摘要
Recent reports have challenged the clonality of the neurosphere assay in assessing neural stem cell (NSC) numbers quantitatively. We tested the clonality of the neurosphere assay by culturing mixtures of differently labeled neural cells, watching single neural cells proliferate using video microscopy, and encapsulating single NSCs and their progeny. The neurosphere assay gave rise to clonal colonies when using primary cells plated at 10 cells/mu l or less; however, when using passaged NSCs, the spheres were clonal only if plated at 1 cell/mu l. Most important, moving the plates during the growth phase (to look at cultures microscopically) greatly increased the incidence of nonclonal colonies. To ensure clonal sphere formation and investigate nonautonomous effects on clonal sphere formation frequencies, single NSCs were encapsulated in agarose and proliferated as clonal free-floating spheres. We demonstrate that clonal neurospheres can be grown by avoiding movement-induced aggregation, by single-cell tracking, and by encapsulation of single cells. STEM CELLS 2008;26:2938-2944
引用
收藏
页码:2938 / 2944
页数:7
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