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首页> 外文期刊>Stem cells translational medicine. >Lineage-Specific Purification of Neural Stem/Progenitor Cells From Differentiated Mouse Induced Pluripotent Stem Cells
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Lineage-Specific Purification of Neural Stem/Progenitor Cells From Differentiated Mouse Induced Pluripotent Stem Cells

机译:从分化的小鼠诱导多能干细胞的神经干/祖细胞的谱系特异性纯化。

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Since induced pluripotent stem (iPS) cells have differentiation potential into all three germ layer-derived tissues, efficient purification of target cells is required in many fields of iPS research. One useful strategy is isolation of desired cells from differentiated iPS cells by lineage-specific expression of a drug-resistance gene, followed by drug selection. With this strategy, we purified neural stem/progenitor cells (NSCs), a good candidate source for regenerative therapy, from differentiated mouse iPS cells. We constructed a bicistronic expression vector simultaneously expressing blasticidin S resistance gene and DsRed under the control of tandem enhancer of a 257-base pair region of nestin second intron, an NSC-specific enhancer. This construct was efficiently inserted into the iPS genome by piggyBac transposon-mediated gene transfer, and the established subclone was differentiated into NSCs in the presence or absence of blasticidin S. Consequently, incubation with blasticidin S led to purification of NSCs from differentiated iPS cells. Our results suggest that a lineage-specific drug selection strategy is useful for purification of NSCs from differentiated iPS cells and that this strategy can be applied for the purification of other cell types.
机译:由于诱导多能干(iPS)细胞具有分化为所有三个胚层来源的组织的潜力,因此在iPS研究的许多领域中都需要有效纯化靶细胞。一种有用的策略是通过抗药性基因的谱系特异性表达,然后进行药物选择,从分化的iPS细胞中分离所需的细胞。通过这种策略,我们从分化的小鼠iPS细胞中纯化了神经干/祖细胞(NSC),它是再生疗法的良好候选来源。我们构建了一个双顺反子表达载体,同时在Nestin第二内含子(一个NSC特异性增强子)的257个碱基对区域的串联增强子的控制下同时表达稻瘟菌素S抗性基因和DsRed。该构建体通过piggyBac转座子介导的基因转移有效地插入到iPS基因组中,并且在存在或不存在杀稻瘟菌素S的情况下,将已建立的亚克隆分化为NSC。我们的结果表明,谱系特异性药物选择策略可用于从分化的iPS细胞纯化NSC,并且该策略可用于纯化其他细胞类型。

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