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首页> 外文期刊>Biophysical Journal >Extended-Depth 3D Super-Resolution Imaging Using Probe-Refresh STORM
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Extended-Depth 3D Super-Resolution Imaging Using Probe-Refresh STORM

机译:使用探针刷新风暴的扩展深度3D超分辨率成像

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摘要

Single-molecule localization microscopy methods for super-resolution fluorescence microscopy such as STORM (stochastic optical reconstruction microscopy) are generally limited to thin three-dimensional (3D) sections (= 600 nm) because of photobleaching of molecules outside the focal plane. Although multiple focal planes may be imaged before photobleaching by focusing progressively deeper within the sample, image quality is compromised in this approach because the total number of measurable localizations is divided between detection planes. Here, we solve this problem on fixed samples by developing an imaging method that we call probe-refresh STORM (prSTORM), which allows bleached fluorophores to be straightforwardly replaced with nonbleached fluorophores. We accomplish this by immunostaining the sample with DNA-conjugated antibodies and then reading out their distribution using fluorescently-labeled DNA-reporter oligonucleotides that can be fully replaced in successive rounds of imaging. We demonstrate that prSTORM can acquire 3D images over extended depths without sacrificing the density of localizations at any given plane. We also show that prSTORM can be adapted to obtain high-quality, 3D multichannel images with extended depth that would be challenging or impossible to achieve using established probe methods.
机译:用于超分辨率荧光显微镜的单分子定位显微镜方法如风暴(随机光学重建显微镜)通常限于薄的三维(3D)部分(& = 600nm),因为焦裂在焦平面外的分子照射。尽管在通过在样本内聚焦逐渐深入地聚焦,但是在该方法中逐渐呼吸的图像质量在光截面之前,因此由于可测量的本地化的总数在检测平面之间划分图像质量。在这里,我们通过开发我们呼叫探针 - 刷新暴风雨(Prstorm)的成像方法来解决固定样本上的该问题,这允许漂白荧光团直截了当地用非苄荧光团替换。我们通过用DNA缀合的抗体免疫样品来实现这一点,然后使用可荧光标记的DNA-Reporter寡核苷酸读出它们的分布,该寡核苷酸可以在连续回合的成像中完全取代。我们证明Prstrorm可以在扩展深度上获取3D图像,而不会在任何给定平面处牺牲本地化的密度。我们还表明,PSTROM可以调整以获得高质量的3D多通道图像,其延长深度,这将是具有挑战性的,或者不可能使用已建立的探针方法来实现。

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