干涉测量
光学
干扰(通信)
物理
干涉显微镜
分辨率(逻辑)
显微镜
职位(财务)
显微镜
涡流
相(物质)
分束器
超分辨显微术
方向(向量空间)
计算机科学
人工智能
数学
几何学
激光器
扫描共焦电子显微镜
计算机网络
经济
财务
量子力学
频道(广播)
热力学
作者
Wei Wang,Zengxin Huang,Yilin Wang,Hangfeng Li,Pakorn Kanchanawong
标识
DOI:10.1103/physrevlett.134.073802
摘要
Super-resolution imaging methods that combine interferometric axial (z) analysis with single-molecule localization microscopy (iSMLM) have achieved ultrahigh 3D precision and contributed to the elucidation of important biological ultrastructures. However, their dependence on imaging multiple phase-shifted output channels necessitates complex instrumentation and operation. To solve this problem, we develop an interferometric superresolution microscope capable of optimal direct axial nanoscopy, termed VILM (Vortex Interference Localization Microscopy). Using a pair of vortex phase plates with opposite orientation for each dual-opposed objective lens, the detection point-spread functions (PSFs) adopt a bilobed profile whose rotation encodes the axial position. Thus, direct 3D single-molecule coordinate determination can be achieved with a single output image. By reducing the number of output channels to as few as one and utilizing a simple 50∶50 beam splitter, the imaging system is significantly streamlined, while the optimal iSMLM imaging performance is retained, with axial precision 2 times better than the lateral. The capability of VILM is demonstrated by resolving the architecture of microtubules and probing the organization of tyrosine-phosphorylated signaling proteins in integrin-based cell adhesions.
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