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Controlling fluid flow to improve cell seeding uniformity

机译:控制流体流动以提高细胞接种均匀性

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摘要

Standard methods for seeding monolayer cell cultures in a multiwell plate or dish do not uniformly distribute cells on the surface. With traditional methods, users find aggregation around the circumference, in the centre, or a combination of the two. This variation is introduced due to the macro scale flow of the cell seeding suspension, and movement of the dish before cells can settle and attach to the surface. Reproducibility between labs, users, and experiments is hampered by this variability in cell seeding. We present a simple method for uniform and user-independent the cell seeding using an easily produced uniform cell seeder (UCS) device. This allows precise control of cell density in a reproducible manner. By containing the cell seeding suspension in a defined volume above the culture surface with the UCS, fluctuations in cell density are minimised. Seeding accuracy, as defined by the actual cell density versus the target seeding density is improved dramatically across users with various levels of expertise. We go on to demonstrate the impact of local variation in cell density on the lineage commitment of human embryonic stem cells (hESCs) towards pancreatic endoderm (PE). Variations in the differentiation profile of cells across a culture well closely mirror variations in cell density introduced by seeding method–with the UCS correcting variations in differentiation efficiency. The UCS device provides a simple and reproducible method for uniform seeding across multiple culture systems.
机译:在多孔板或培养皿中接种单层细胞培养物的标准方法不能将细胞均匀分布在表面上。使用传统方法,用户可以在周围,中心或两者的组合中找到聚集点。由于细胞接种悬浮液的宏观流动以及在细胞沉降并附着到表面之前培养皿的移动,引入了这种变化。细胞接种中的这种可变性阻碍了实验室,用户和实验之间的可重复性。我们提出了一种使用容易产生的均匀细胞播种机(UCS)设备进行均匀且用户独立的细胞播种的简单方法。这允许以可再现的方式精确控制细胞密度。通过在UCS的培养表面上方以规定的体积容纳细胞接种悬浮液,可将细胞密度的波动降至最低。由具有不同专业知识水平的用户,由实际细胞密度与目标播种密度定义的播种精度得到了显着提高。我们继续证明细胞密度的局部变化对人类胚胎干细胞(hESCs)向胰腺内胚层(PE)谱系承诺的影响。整个培养孔中细胞分化概况的变化与接种方法引入的细胞密度变化密切相关,而UCS可以校正分化效率的变化。 UCS设备为跨多个培养系统的均匀播种提供了一种简单且可重现的方法。

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