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通过平场光漂白印记显微镜实现高通量、低背景和宽视场显微镜观察

High-Throughput, Low Background, and Wide-Field Microscopy by Flat-Field Photobleaching Imprinting Microscopy.

作者信息

Qin Yizhi, Zhang Mengling, Hao Huiwen, Xue Boxin, Niu Jiahao, Sun Yujie

机构信息

State Key Laboratory of Membrane Biology, Biomedical Pioneer Innovation Center (BIOPIC), School of Life Sciences, Peking University, Beijing 100871, China.

College of Chemistry and Molecular Engineering, Peking University, Beijing 100871, China.

出版信息

Chem Biomed Imaging. 2023 Oct 28;1(9):843-851. doi: 10.1021/cbmi.3c00079. eCollection 2023 Dec 25.

Abstract

Wide-field photobleaching imprinting microscopy (PIM) can improve fluorescence image contrast by cleverly exploiting the fluorophores' photobleaching properties. However, as conventional wide-field PIM commonly adopts Gaussian illumination with a nonuniform lateral fluence distribution, the field-of-view (FOV) and sampling density are largely reduced. In addition, the slow axial fluence gradient of Gaussian illumination limits the signal-to-background ratio (SBR) improvement and optical sectioning capability of PIM. Here, we present flat-field photobleaching imprinting microscopy (ffPIM) with a uniform lateral excitation fluence and sharp axial intensity gradient at the focal plane. ffPIM demonstrates low background, large FOV, and thin optical section. More importantly, compared to either conventional wide-field PIM or light-sheet microscopy, ffPIM shows much better balance for FOV, sampling density, SBR, and optical sectioning capability. The performance of ffPIM is characterized by simulation and resolving multiple cellular structures. Finally, ffPIM can be easily implemented to a standard commercial wide-field microscope and, thereby, allow general laboratories to benefit from this technique.

摘要

宽场光漂白印记显微镜(PIM)通过巧妙利用荧光团的光漂白特性,可以提高荧光图像的对比度。然而,由于传统的宽场PIM通常采用高斯照明,其横向通量分布不均匀,视野(FOV)和采样密度会大幅降低。此外,高斯照明的轴向通量梯度缓慢,限制了PIM的信噪比(SBR)改善和光学切片能力。在此,我们提出了平场光漂白印记显微镜(ffPIM),其在焦平面具有均匀的横向激发通量和陡峭的轴向强度梯度。ffPIM具有低背景、大视野和薄光学切片的特点。更重要的是,与传统的宽场PIM或光片显微镜相比,ffPIM在视野、采样密度、SBR和光学切片能力方面表现出更好的平衡。通过模拟和解析多个细胞结构来表征ffPIM的性能。最后,ffPIM可以很容易地应用于标准的商用宽场显微镜,从而使普通实验室能够受益于这项技术。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/170f/11504465/64294a0386d0/im3c00079_0001.jpg

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