小鼠骨髓Thy-1和sca -1阳性细胞的神经元分化。

F Locatelli, S Corti, C Donadoni, M Guglieri, F Capra, S Strazzer, S Salani, R Del Bo, F Fortunato, A Bordoni, G P Comi
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引用次数: 49

摘要

最近的证据表明,骨髓细胞可以在细胞培养或动物模型和人脑移植后获得神经外胚层表型。然而,分离具有神经元分化潜力的骨髓细胞亚群仍然是一个挑战。为了从全鼠骨髓中分离和扩增神经祖细胞,我们从C57BL6小鼠后肢骨中获得骨髓,用含有碱性成纤维细胞生长因子和表皮生长因子的神经培养基进行培养。培养5-7天后,类似脑神经球的细胞球出现漂浮或附着在培养皿上。这些球体被收集、分离和膨胀。通过免疫细胞化学和逆转录聚合酶链反应,骨髓来源的球对巢蛋白呈阳性反应。磁性细胞分选的Thy-1和sca -1阳性骨髓细胞可获得较高的巢蛋白阳性球收率。在有或没有Sonic hedgehog基因的神经元分化培养基维甲酸中,检测到神经元标志物微管蛋白III (TuJ-1)和神经丝(NF)阳性的细胞。这些细胞的mRNA谱包括TuJ-1、神经元特异性烯醇化酶(NSE)和nf轻链的表达。为了评估这些细胞的体内行为,将转基因绿色荧光蛋白(GFP)小鼠骨髓来源的细胞制成的球移植到新生小鼠的大脑中。2个月后,小鼠神经皮层含有少量共表达神经元标记物(TuJ-1、NF、MAP-2、NeuN)的GFP(+)细胞。虽然不能排除与宿主细胞的细胞融合现象,但骨髓源性神经球移植可能是细胞介导基因治疗的一种策略。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
Neuronal differentiation of murine bone marrow Thy-1- and Sca-1-positive cells.

Recent evidence suggests that cells from bone marrow can acquire neuroectodermal phenotypes in cell culture or after transplantation in animal models and in the human brain. However, isolation of the bone marrow cell subpopulation with neuronal differentiation potential remains a challenge. To isolate and expand neural progenitors from whole murine bone marrow, bone marrow was obtained from hind limb bone of C57BL6 mice and plated in culture with neuronal medium with basic fibroblast growth factor and epidermal growth factor. After 5-7 days in culture, cellular spheres similar to brain neurospheres appeared either floating or attached to culture dishes. These spheres were collected, dissociated, and expanded. The bone marrow-derived spheres were positive for nestin as assessed by immunocytochemistry and by reverse transcriptase polymerase chain reaction. Thy-1- and Sca-1-positive bone marrow cells selected by magnetic cell sorting resulted in a higher yield of nestin-positive spheres. After exposure to neuronal differentiative medium retinoic acid with and without Sonic hedgehog, cells positive for neuronal markers tubulin III (TuJ-1) and neurofilament (NF) were detected. The mRNA profile of these cells included the expression of TuJ-1, neuronal-specific enolase (NSE), and NF-light chain. To evaluate the in vivo behavior of these cells, spheres derived from bone marrow-derived cells of transgenic green fluorescent protein (GFP) mice were transplanted into newborn mouse brain. Two months later, the mouse neural cortex contained a minor proportion of GFP(+) cells co-expressing neuronal markers (TuJ-1, NF, MAP-2, NeuN). Although cell fusion phenomena with the host cells could not be ruled out, bone marrow-derived neurosphere transplantation could be a strategy for cellular mediated gene therapy.

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