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首页> 外文期刊>Neuroscience: An International Journal under the Editorial Direction of IBRO >The differentiation potential of precursor cells from the mouse lateral ganglionic eminence is restricted by in vitro expansion.
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The differentiation potential of precursor cells from the mouse lateral ganglionic eminence is restricted by in vitro expansion.

机译:从小鼠外侧神经节隆起的前体细胞的分化潜力受到体外扩增的限制。

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We have investigated whether the differentiation potential of attached cultures derived from the mouse lateral ganglionic eminence (LGE) is influenced by in vitro expansion. Primary neuronal cultures derived from the LGE give rise to neurons expressing the striatal projection neuron markers Islet1 (ISL1) and dopamine and cAMP-regulated phosphoprotein of 32 kilodaltons (DARPP-32) as well as the olfactory bulb interneuron marker Er81. Our previous results showed that after expansion in vitro, LGE precursor cells can be induced to differentiate into neurons which exhibit molecular characteristics of the LGE, such as the homeobox transcription factors DLX and MEIS2. We show here that while attached LGE cultures maintain Er81 expression through five passages, they lose the ability to generate ISL1- or dopamine and cAMP-regulated phosphoprotein of 32 kilodaltons-expressing neurons already after the first passage. This indicates that the expansion of LGE precursor cells restricts their differentiation potential in vitro. Interestingly, the undifferentiated LGE cultures retain the expression of both the Isl1 and Er81 genes, suggesting that precursor cells for both striatal projection neurons and olfactory bulb interneurons are present in these cultures. Thus the restriction in differentiation potential of the expanded LGE cultures likely reflects deficiencies in the differentiation conditions used.
机译:我们已经调查了源自小鼠侧神经节隆起(LGE)的附着培养物的分化潜能是否受到体外扩增的影响。源自LGE的初级神经元培养物产生表达纹状体投射神经元标记Islet1(ISL1)和多巴胺和cAMP调节的32千道尔顿的磷酸化蛋白(DARPP-32)以及嗅球中神经元标记Er81的神经元。我们以前的结果表明,体外扩增后,LGE前体细胞可以被诱导分化为具有LGE分子特征的神经元,例如同源盒转录因子DLX和MEIS2。我们在这里显示,虽然附着的LGE培养物通过五次传代维持Er81表达,但它们在第一次传代后已经失去了生成ISL1或多巴胺和cAMP调节的表达32道尔顿神经元的磷蛋白的能力。这表明LGE前体细胞的扩增限制了它们在体外的分化潜力。有趣的是,未分化的LGE培养物保留了Isl1和Er81基因的表达,表明这些培养物中同时存在着纹状体投射神经元和嗅球间神经元的前体细胞。因此,扩大的LGE培养物分化潜能的限制可能反映了所用分化条件的不足。

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