Super-resolution multicolor fluorescence microscopy enabled by an apochromatic super-oscillatory lens with extended depth-of-focus

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作者
Wenli Li
Pei He
Dangyuan Lei
Yulong Fan
Yangtao Du
Bo Gao
Zhiqin Chu
Longqiu Li
Kaipeng Liu
Chengxu An
Weizheng Yuan
Yiting Yu
机构
[1] Northwestern Polytechnical University,Ningbo Institute of Northwestern Polytechnical University, College of Mechanical Engineering
[2] Northwestern Polytechnical University,Key Laboratory of Micro/Nano Systems for Aerospace (Ministry of Education)
[3] Northwestern Polytechnical University,Shaanxi Province Key Laboratory of Micro and Nano Electro
[4] City University of Hong Kong,Mechanical Systems
[5] Fudan University,Department of Materials Science and Engineering
[6] Xi’an Institute of Optics and Precision Mechanics,The Institute of AI and Robotics
[7] Chinese Academy of Sciences,Key Laboratory of Spectral Imaging Technology of Chinese Academy of Sciences
[8] The University of Hong Kong,Department of Electrical and Electronic Engineering, Joint Appointment with School of Biomedical Sciences
[9] Harbin Institute of Technology,State Key Laboratory of Robotics and System
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摘要
Planar super-oscillatory lens (SOL), a far-field subwavelength-focusing diffractive device, holds great potential for achieving sub-diffraction-limit imaging at multiple wavelengths. However, conventional SOL devices suffer from a numerical-aperture-related intrinsic tradeoff among the depth of focus (DoF), chromatic dispersion and focusing spot size. Here, we apply a multi-objective genetic algorithm (GA) optimization approach to design an apochromatic binary-phase SOL having a prolonged DoF, customized working distance (WD), minimized main-lobe size, and suppressed side-lobe intensity. Experimental implementation demonstrates simultaneous focusing of blue, green and red light beams into an optical needle of ~0.5λ in diameter and DOF > 10λ at WD = 428 μm. By integrating this SOL device with a commercial fluorescence microscope, we perform, for the first time, three-dimensional super-resolution multicolor fluorescence imaging of the “unseen” fine structures of neurons. The present study provides not only a practical route to far-field multicolor super-resolution imaging but also a viable approach for constructing imaging systems avoiding complex sample positioning and unfavorable photobleaching.
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