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Flat-top TIRF illumination boosts DNA-PAINT imaging and quantification

机译:平顶TIRF照明可增强DNA-PAINT成像和定量

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摘要

Super-resolution (SR) techniques have extended the optical resolution down to a few nanometers. However, quantitative treatment of SR data remains challenging due to its complex dependence on a manifold of experimental parameters. Among the different SR variants, DNA-PAINT is relatively straightforward to implement, since it achieves the necessary ‘blinking’ without the use of rather complex optical or chemical activation schemes. However, it still suffers from image and quantification artifacts caused by inhomogeneous optical excitation. Here we demonstrate that several experimental challenges can be alleviated by introducing a segment-wise analysis approach and ultimately overcome by implementing a flat-top illumination profile for TIRF microscopy using a commercially-available beam-shaping device. The improvements with regards to homogeneous spatial resolution and precise kinetic information over the whole field-of-view were quantitatively assayed using DNA origami and cell samples. Our findings open the door to high-throughput DNA-PAINT studies with thus far unprecedented accuracy for quantitative data interpretation.
机译:超分辨率(SR)技术将光学分辨率扩展到了几纳米。但是,由于SR数据对多种实验参数的复杂依赖性,因此对其进行定量处理仍然具有挑战性。在不同的SR变体中,DNA-PAINT相对容易实现,因为它无需使用相当复杂的光学或化学激活方案即可实现必要的“闪烁”。然而,它仍然遭受由不均匀的光激发引起的图像和量化伪像。在这里,我们证明了通过引入逐段分析方法可以减轻几个实验挑战,并最终通过使用商用光束整形设备实现TIRF显微镜的平顶照明配置文件来最终克服。使用DNA折纸和细胞样品定量分析了在整个视野内均质空间分辨率和精确动力学信息方面的改进。我们的发现为高通量DNA-PAINT研究打开了大门,迄今为止,该研究为定量数据解释提供了前所未有的准确性。

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