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An Engineered Approach to Stem Cell Culture: Automating the Decision Process for Real-Time Adaptive Subculture of Stem Cells

机译:一种工程化的干细胞培养方法:自动进行干细胞实时自适应继代培养的决策过程

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摘要

Current cell culture practices are dependent upon human operators and remain laborious and highly subjective, resulting in large variations and inconsistent outcomes, especially when using visual assessments of cell confluency to determine the appropriate time to subculture cells. Although efforts to automate cell culture with robotic systems are underway, the majority of such systems still require human intervention to determine when to subculture. Thus, it is necessary to accurately and objectively determine the appropriate time for cell passaging. Optimal stem cell culturing that maintains cell pluripotency while maximizing cell yields will be especially important for efficient, cost-effective stem cell-based therapies. Toward this goal we developed a real-time computer vision-based system that monitors the degree of cell confluency with a precision of 0.791±0.031 and recall of 0.559±0.043. The system consists of an automated phase-contrast time-lapse microscope and a server. Multiple dishes are sequentially imaged and the data is uploaded to the server that performs computer vision processing, predicts when cells will exceed a pre-defined threshold for optimal cell confluency, and provides a Web-based interface for remote cell culture monitoring. Human operators are also notified via text messaging and e-mail 4 hours prior to reaching this threshold and immediately upon reaching this threshold. This system was successfully used to direct the expansion of a paradigm stem cell population, C2C12 cells. Computer-directed and human-directed control subcultures required 3 serial cultures to achieve the theoretical target cell yield of 50 million C2C12 cells and showed no difference for myogenic and osteogenic differentiation. This automated vision-based system has potential as a tool toward adaptive real-time control of subculturing, cell culture optimization and quality assurance/quality control, and it could be integrated with current and developing robotic cell cultures systems to achieve complete automation.
机译:当前的细胞培养方法依赖于人类操作者,并且仍然费力且主观性高,导致较大的差异和不一致的结果,尤其是在使用目视评估细胞融合度来确定传代细胞的适当时间时。尽管正在努力通过机器人系统实现细胞培养自动化,但大多数此类系统仍需要人工干预才能确定何时进行亚培养。因此,有必要准确客观地确定细胞传代的适当时间。最佳的干细胞培养在保持细胞多能性的同时最大程度地提高细胞产量,对于基于干细胞的高效,低成本治疗尤其重要。为了实现这一目标,我们开发了一种基于实时计算机视觉的系统,该系统以0.791±0.031的精度和0.559±0.043的召回率监控细胞的融合程度。该系统由一个自动相衬延时显微镜和一台服务器组成。依次对多个培养皿进行成像,并将数据上传到执行计算机视觉处理的服务器,预测何时细胞将超过最佳阈值以实现最佳细胞融合,并为远程细胞培养监控提供基于Web的界面。在达到此阈值之前4小时,一旦达到此阈值,也会通过文本消息和电子邮件通知操作人员。该系统已成功用于指导范式干细胞群体C2C12细胞的扩增。计算机控制和人类控制的亚培养需要3个连续培养,以实现5000万个C2C12细胞的理论目标细胞产量,并且在成肌和成骨分化方面没有差异。这种基于视觉的自动化系统具有潜力,可用于自适应实时控制亚培养,细胞培养优化和质量保证/质量控制,并且可以与当前和正在开发的机器人细胞培养系统集成以实现完全自动化。

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