Tran Thi-Hang, Lukmanto Donny, Chen Mei, Strauß Olaf, Yamashita Toshiharu, Ohneda Osamu, Fukuda Shinichi
Laboratory of Advanced Vision Science, Institute of Medicine, University of Tsukuba, Tsukuba, Japan.
Laboratory of Regenerative Medicine and Stem Cell Biology, Institute of Medicine, University of Tsukuba, Tsukuba, Japan.
Front Cell Dev Biol. 2025 May 9;13:1513163. doi: 10.3389/fcell.2025.1513163. eCollection 2025.
Primary Müller glia (MG) have been reported to exhibit a neurogenic capacity induced by small molecules. However, whether immortalized mouse MG cell lines exhibit neurogenic capacities similar to those of primary mouse MG remains unclear. In this study, we examined the morphology, proliferation rate, and marker profile of primary MG cells isolated from postnatal mouse pups with two immortalized mouse MG cell lines, QMMuC-1 and ImM10, in a standard growth medium. After chemical induction, we compared the morphology, markers, direct neuronal reprogramming efficiency, and axon length of these cell types in two culture media: Neurobasal and DMEM/F12. Our results showed that in standard growth medium, QMMuC-1 and ImM10 cells displayed similar morphology and marker profiles as primary MG cells, with the only differences observed in nestin expression. However, QMMuC-1 and ImM10 cells exhibited much higher proliferation rates than the primary MG cells. Following chemical treatment in both Neurobasal and DMEM/F12 media, a subset of primary MG, QMMuC-1, and ImM10 cells was induced to differentiate into immature neuron-like cells by day 7. While primary MG cells showed similar neuronal reprogramming efficiency and axon length extension in both media, QMMuC-1 and ImM10 cells displayed variations between the two culture media. Moreover, some of the induced neuronal cells derived from primary MG cells expressed HuC/D and Calbindin markers, whereas none of the cells derived from QMMuC-1 and ImM10 cells expressed these markers. Subsequent observations revealed that induced immature neuron-like cells derived from primary MG cells in both types of media and those derived from ImM10 cells cultured in DMEM/F12 survived until day 14. Taken together, our findings suggest that the two immortalized cell lines, QMMuC-1 and ImM10, exhibited neurogenic capacities similar to those of primary MG cells to some extent but did not fully recapitulate all their characteristics. Therefore, careful consideration should be given to culture conditions and the validation of key results when using immortalized cells as a substitute for primary MG cells.
据报道,原代穆勒胶质细胞(MG)可表现出由小分子诱导的神经发生能力。然而,永生化小鼠MG细胞系是否表现出与原代小鼠MG相似的神经发生能力仍不清楚。在本研究中,我们在标准生长培养基中,用两种永生化小鼠MG细胞系QMMuC-1和ImM10,检测了从出生后小鼠幼崽中分离的原代MG细胞的形态、增殖率和标志物谱。化学诱导后,我们在两种培养基Neurobasal和DMEM/F12中比较了这些细胞类型的形态、标志物、直接神经元重编程效率和轴突长度。我们的结果表明,在标准生长培养基中,QMMuC-1和ImM10细胞与原代MG细胞表现出相似的形态和标志物谱,仅在巢蛋白表达上存在差异。然而,QMMuC-1和ImM10细胞的增殖率比原代MG细胞高得多。在Neurobasal和DMEM/F12培养基中进行化学处理后,到第7天,一部分原代MG、QMMuC-1和ImM10细胞被诱导分化为未成熟的神经元样细胞。虽然原代MG细胞在两种培养基中表现出相似的神经元重编程效率和轴突长度延长,但QMMuC-1和ImM10细胞在两种培养基之间存在差异。此外,一些源自原代MG细胞的诱导神经元细胞表达HuC/D和钙结合蛋白标志物,而源自QMMuC-1和ImM10细胞的细胞均不表达这些标志物。随后的观察发现,两种培养基中源自原代MG细胞的诱导未成熟神经元样细胞以及在DMEM/F12中培养的源自ImM10细胞的诱导未成熟神经元样细胞存活至第14天。综上所述,我们的研究结果表明,两种永生化细胞系QMMuC-1和ImM10在一定程度上表现出与原代MG细胞相似的神经发生能力,但并未完全重现其所有特征。因此,在使用永生化细胞替代原代MG细胞时,应仔细考虑培养条件和关键结果的验证。
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