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Live-cell imaging

机译:活细胞成像

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摘要

It would be hard to argue that live-cell imaging has not changed our view of biology. The past 10 years have seen an explosion of interest in imaging cellular processes, down to the molecular level. There are now many advanced techniques being applied to live cell imaging. However, cellular health is often under appreciated. For many researchers, if the cell at the end of the experiment has not gone into apoptosis or is blebbed beyond recognition, than all is well. This is simply incorrect. There are many factors that need to be considered when performing live-cell imaging in order to maintain cellular health such as: imaging modality, media, temperature, humidity, PH, osmolality, and photon dose. The wavelength of illuminating light, and the total photon dose that the cells are exposed to, comprise two of the most important and controllable parameters of live-cell imaging. The lowest photon dose that achieves a measureable metric for the experimental question should be used, not the dose that produces cover photo quality images. This is paramount to ensure that the cellular processes being investigated are in their in vitro state and not shifted to an alternate pathway due to environmental stress. The timing of the mitosis is an ideal canary in the gold mine, in that any stress induced from the imaging will result in the increased length of mitosis, thus providing a control model for the current imagining conditions.
机译:很难说活细胞成像并没有改变我们对生物学的看法。在过去的10年中,人们对成像细胞过程的兴趣开始激增,直到分子水平。现在有许多先进的技术被应用于活细胞成像。然而,细胞健康常常受到重视。对于许多研究人员来说,如果实验结束时该细胞没有发生凋亡或无法识别地起泡,那一切都很好。这根本是不正确的。为了保持细胞健康,执行活细胞成像时需要考虑许多因素,例如:成像方式,介质,温度,湿度,PH,重量克分子渗透压浓度和光子剂量。照射光的波长以及细胞所暴露的总光子剂量包括活细胞成像的两个最重要且可控制的参数。应该使用达到实验问题可衡量指标的最低光子剂量,而不是产生掩盖照片质量图像的剂量。这对于确保所研究的细胞过程处于体外状态且不会因环境压力而转移至其他途径至关重要。有丝分裂的时机是金矿中的理想金丝雀,因为由成像引起的任何应力都会导致有丝分裂的长度增加,从而为当前成像条件提供了控制模型。

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