3D super-resolution live-cell imaging with radial symmetry and Fourier light-field microscopy

Author:

Han Keyi1ORCID,Hua Xuanwen1,Vasani Vishwa2,Kim Ge-Ah R.2,Liu Wenhao1,Takayama Shuichi1,Jia Shu1ORCID

Affiliation:

1. Georgia Institute of Technology and Emory University

2. Georgia Institute of Technology

Abstract

Live-cell imaging reveals the phenotypes and mechanisms of cellular function and their dysfunction that underscore cell physiology, development, and pathology. Here, we report a 3D super-resolution live-cell microscopy method by integrating radiality analysis and Fourier light-field microscopy (rad-FLFM). We demonstrated the method using various live-cell specimens, including actins in Hela cells, microtubules in mammary organoid cells, and peroxisomes in COS-7 cells. Compared with conventional wide-field microscopy, rad-FLFM realizes scanning-free, volumetric 3D live-cell imaging with sub-diffraction-limited resolution of ∼150 nm (x-y) and 300 nm (z), milliseconds volume acquisition time, six-fold extended depth of focus of ∼6 µm, and low photodamage. The method provides a promising avenue to explore spatiotemporal-challenging subcellular processes in a wide range of cell biological research.

Funder

National Science Foundation

National Institutes of Health

Publisher

Optica Publishing Group

Subject

Atomic and Molecular Physics, and Optics,Biotechnology

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