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Label free, quantitative single-cell fate tracking of time-lapse movies

机译:无标签,定量的延时电影单细胞命运跟踪

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Historically, the ability to perform multi-day time-lapse imaging of adherent cells required expensive and specialized microscopy equipment. As byproduct of this cost, many labs would synchronize cells using inhibitors such as hydroxyurea and thymidine, and or use fluorescent biosensors to minimize time required on the microscope. These methods introduce significant artefacts including phototoxicity, increased DNA replication stress and mitotic defects, thereby limiting the ability to characterize various cell cycle phenotypes. However, increased access to low cost live cell microscopes has removed many of the economic barriers thereby allowing multi-day imaging on asynchronous cells on a regular basis. Here we describe our protocol for manually tracking individual cell fates across multiple generations of random daughter cells using only low toxicity brightfield based imaging. Importantly, our pipeline relies on the free open-source software ImageJ/Fiji and an easy to use Microsoft Excel spreadsheet. Furthermore, annotated files can be saved to allow later recall of any individual cell. In summary, our method provides quantitative data on interphase and mitotic transit time, points of cell cycle arrest and critically, the ability to link these events with cell fate.
机译:从历史上看,对贴壁细胞进行多天延时成像的能力需要昂贵且专用的显微镜​​设备。作为此费用的副产品,许多实验室将使用抑制剂(例如羟基脲和胸苷)来同步细胞,或者使用荧光生物传感器来最大限度地减少显微镜所需的时间。这些方法引入了明显的伪像,包括光毒性,增加的DNA复制压​​力和有丝分裂缺陷,从而限制了表征各种细胞周期表型的能力。但是,越来越多地使用低成本活细胞显微镜消除了许多经济障碍,从而允许定期在异步细胞上进行多日成像。在这里,我们描述了仅使用基于低毒性明场的成像技术来手动跟踪多代随机子细胞中各个细胞命运的方案。重要的是,我们的管道依赖于免费的开源软件ImageJ / Fiji和易于使用的Microsoft Excel电子表格。此外,可以保存带注释的文件,以便以后调用任何单个单元格。总之,我们的方法提供了有关相间和有丝分裂渡越时间,细胞周期停滞点以及至关重要的将这些事件与细胞命运联系起来的能力的定量数据。

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