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Cryopreservation of Cortical Tissue Blocks for the Generation of Highly Enriched Neuronal Cultures

机译:冻存的皮质组织块的高度丰富的神经元文化的产生。

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摘要

In this study, we outline a standardized protocol for the successful cryopreservation and thawing of cortical brain tissue blocks to generate highly enriched neuronal cultures. For this protocol the freezing medium used is 10% dimethyl sulfoxide (DMSO) diluted in Hank's Buffered Salt Solution (HBSS). Blocks of cortical tissue are transferred to cryovials containing the freezing medium and slowly frozen at -1°C/min in a rate-controlled freezing container. Post-thaw processing and dissociation of frozen tissue blocks consistently produced neuronal-enriched cultures which exhibited rapid neuritic growth during the first 5 days in culture and significant expansion of the neuronal network within 10 days. Immunocytochemical staining with the astrocytic marker glial fibrillary acidic protein (GFAP) and the neuronal marker beta-tubulin class III, revealed high numbers of neurons and astrocytes in the cultures. Generation of neural precursor cell cultures after tissue block dissociation resulted in rapidly expanding neurospheres, which produced large numbers of neurons and astrocytes under differentiating conditions. This simple cryopreservation protocol allows for the rapid, efficient, and inexpensive preservation of cortical brain tissue blocks, which grants increased flexibility for later generation of neuronal, astrocyte, and neuronal precursor cell cultures.
机译:在这项研究中,我们概述了成功冷冻保存和解冻皮质脑组织块以生成高度丰富的神经元文化的标准化协议。对于此协议,使用的冷冻介质是在Hank缓冲盐溶液(HBSS)中稀释的10%二甲基亚砜(DMSO)。将皮质组织块转移到装有冷冻介质的冷冻管中,并在速率控制的冷冻容器中以-1°C / min的速度缓慢冷冻。解冻后的处理和冷冻组织块的解离始终产生富含神经元的培养物,其在培养的前5天内表现出快速的神经生长,在10天内神经元网络显着扩展。用星形细胞标记神经胶质原纤维酸性蛋白(GFAP)和神经元标记β-微管蛋白III类进行的免疫细胞化学染色显示培养物中神经元和星形胶质细胞的数量很高。组织块解离后神经前体细胞培养物的产生导致神经球迅速膨胀,在分化条件下产生大量神经元和星形胶质细胞。这种简单的冷冻保存方案可以快速,有效和廉价地保存皮质脑组织块,从而为以后的神经元,星形胶质细胞和神经元前体细胞培养物提供了更大的灵活性。

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