Randall Division, King's College London, New Hunts House, Guy's Campus, London SE1 1UL, UK.
Nat Commun. 2017 Jan 12;8:13558. doi: 10.1038/ncomms13558.
Localization microscopy allows biological samples to be imaged at a length scale of tens of nanometres. Live-cell super-resolution imaging is rare, as it is generally assumed to be too slow for dynamic samples. The speed of data acquisition can be optimized by tuning the density of activated fluorophores in each time frame. Here, we show that the maximum achievable imaging speed for a particular structure varies by orders of magnitude, depending on the sample dimensionality (that is, whether the sample is more like a point, a strand or an extended structure such as a focal adhesion). If too high an excitation density is used, we demonstrate that the analysis undergoes silent failure, resulting in reconstruction artefacts. We are releasing a tool to allow users to identify areas of the image in which the activation density was too high and correct for them, in both live- and fixed-cell experiments.
定位显微镜可以在数十纳米的长度尺度上对生物样本进行成像。活细胞超分辨率成像很少见,因为通常认为它对于动态样本来说太慢了。通过调整每个时间帧中激活荧光团的密度,可以优化数据采集速度。在这里,我们表明,对于特定结构,最大可实现的成像速度相差几个数量级,具体取决于样品的维度(即样品更像一个点、一条线还是像焦点粘连这样的扩展结构)。如果使用太高的激发密度,我们证明分析会出现无声故障,导致重建伪影。我们正在发布一个工具,允许用户识别图像中激活密度过高的区域,并在活细胞和固定细胞实验中对其进行校正。