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From the Cover: Computerized microfluidic cell culture using elastomeric channels and Braille displays

机译:从封面开始:使用弹性通道和盲文显示器的计算机化微流体细胞培养

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摘要

Computer-controlled microfluidics would advance many types of cellular assays and microscale tissue engineering studies wherever spatiotemporal changes in fluidics need to be defined. However, this goal has been elusive because of the limited availability of integrated, programmable pumps and valves. This paper demonstrates how a refreshable Braille display, with its grid of 320 vertically moving pins, can power integrated pumps and valves through localized deformations of channel networks within elastic silicone rubber. The resulting computerized fluidic control is able to switch among: (i) rapid and efficient mixing between streams, (ii) multiple laminar flows with minimal mixing between streams, and (iii) segmented plug-flow of immiscible fluids within the same channel architecture. The same control method is used to precisely seed cells, compartmentalize them into distinct subpopulations through channel reconfiguration, and culture each cell subpopulation for up to 3 weeks under perfusion. These reliable microscale cell cultures showed gradients of cellular behavior from C2C12 myoblasts along channel lengths, as well as differences in cell density of undifferentiated myoblasts and differentiation patterns, both programmable through different flow rates of serum-containing media. This technology will allow future microscale tissue or cell studies to be more accessible, especially for high-throughput, complex, and long-term experiments. The microfluidic actuation method described is versatile and computer programmable, yet simple, well packaged, and portable enough for personal use.
机译:在需要定义流体时空变化的地方,计算机控制的微流体技术将推动许多类型的细胞测定和微观组织工程研究。但是,由于集成的可编程泵和阀的可用性有限,所以这个目标难以实现。本文展示了一个可刷新的盲文显示器,该显示器具有320个垂直移动的销钉网格,可以通过弹性硅橡胶中通道网络的局部变形来为集成的泵和阀提供动力。最终的计算机化流体控制能够在以下之间进行切换:(i)流之间的快速有效混合;(ii)流之间的最小混合的多个层流;以及(iii)同一通道架构内的不混溶流体的分段塞流。使用相同的控制方法来精确播种细胞,通过通道重构将它们划分为不同的亚群,并在灌注下将每个细胞亚群培养长达3周。这些可靠的微型细胞培养物显示了C2C12成肌细胞沿通道长度的细胞行为梯度,以及未分化成肌细胞的细胞密度和分化模式的差异,均可通过不同流速的含血清培养基进行编程。这项技术将使未来的微型组织或细胞研究变得更加容易,特别是对于高通量,复杂和长期的实验。所描述的微流体致动方法是通用的并且是计算机可编程的,但是简单,包装良好并且足够便携以供个人使用。

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