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Pumpless microfluidic system driven by hydrostatic pressure induces and maintains mouse spermatogenesis in vitro

机译:静水压驱动的无泵微流系统在体外诱导和维持小鼠精子发生

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摘要

Three-dimensional aggregation and organ culture methods are critical for recreating in vivo cellular phenomena outside the body. Previously, we used the conventional gas liquid interphase organ culture method to induce complete mouse spermatogenesis. After incorporating microfluidic systems, we achieved a significant increase in efficiency and duration of spermatogenesis. One of the major drawbacks preventing the popularization of microfluidics, however, is the use of a power-pump to generate medium flow. In this study, we produced a pumpless microfluidic device using hydrostatic pressure and a resistance circuit to facilitate slow, longer lasting medium flow. During three months of culture, results in induction and maintenance of spermatogenesis showed no difference between pumpless and pump-driven devices. Correspondingly, the spermatogonial population was favorably maintained in the pumpless device compared to the conventional method. These results show the advantage of using microfluidic systems for organ culture experiments. Our pumpless device could be applied to a variety of other tissues and organs, and may revolutionize organ culture methods as a whole.
机译:三维聚集和器官培养方法对于在体外重建体内细胞现象至关重要。以前,我们使用常规的气液间期器官培养方法来诱导小鼠完全生精。纳入微流控系统后,我们显着提高了生精效率和持续时间。然而,阻止微流体普及的主要缺点之一是使用功率泵来产生介质流。在这项研究中,我们使用静水压力和阻力回路制造了无泵微流体装置,以促进缓慢,持久的介质流动。在培养的三个月中,诱导和维持精子发生的结果显示无泵和泵驱动设备之间没有差异。相应地,与常规方法相比,在无泵装置中有利地维持了精原细胞群。这些结果显示了使用微流体系统进行器官培养实验的优势。我们的无泵设备可以应用于多种其他组织和器官,并且可以彻底改变整个器官的培养方法。

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