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Super-resolution scanning microscopy with virtually structured illumination

机译:超分辨率扫描显微镜,具有几乎结构的照明

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The resolution of optical microscopy fundamentally limited by diffraction is at best 200 nm. Super-resolution structured illumination microscopy (SR-SIM) provides an elegant way of overcoming the diffraction limit in conventional widefield microscope by superimposing a grid pattern generated through interference of diffraction orders on the specimen while capturing images. The use of non-uniform illumination field "shift" high specimen frequencies which are out-ofband into the pass-band of the microscope through spatial frequency mixing with the illumination field. Therefore the effective bandwidth of SR-SIM is approximately twice as conventional microscopy, corresponding to a 2-fold resolution enhancement, if the difference between excitation and emission wavelength is ignored. However, such a wide-field scheme typically can only image optically thin samples and is incompatible with multiphoton processes. In this paper, we propose a Super-resolution scanning scheme with virtually structured illumination, utilizes detection sensitivity modulation on line by programming or off line by numerical processing together with temporally cumulative imaging, the excitation intensity is constant while capturing images. In this case a nondescanned array detector such as CCD camera is needed. When combined with multiphoton excitation, this scheme can image thick samples with threedimensional optical sectioning and much improved resolution.
机译:通过衍射基本限制的光学显微镜的分辨率最高为200nm。超分辨率结构照明显微镜(SR-SIM)通过叠加通过样品上的衍射订单的干扰产生的网格图案来提供克服常规宽场显微镜中衍射极限的优雅方式。使用非均匀照明场“换档”高标本频率,其通过与照明场的空间频率混合在显微镜的通带中的频段。因此,如果忽略激励和发射波长之间的差异,则SR-SIM的有效带宽约为常规显微镜的常规显微镜的两倍。然而,这种宽场方案通常只能图像是光学薄的样本,并且与多光子过程不相容。在本文中,我们提出了一种具有几乎结构的照明的超分辨率扫描方案,通过数值处理在时间累积成像一起通过编程或离线进行检测灵敏度调制,激励强度在捕获图像时恒定。在这种情况下,需要一个非金刚的阵列检测器,例如CCD相机。当与多光电激励结合时,该方案可以通过三维光学切片和大大改进的分辨率来图像厚的样本。

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