3D high-density localization microscopy using hybrid astigmatic/biplane imaging and sparse image reconstruction

被引:33
|
作者
Min, Junhong [1 ]
Holden, Seamus J. [2 ]
Carlini, Lina [2 ]
Unser, Michael [3 ]
Manley, Suliana [2 ]
Ye, Jong Chul [1 ]
机构
[1] Korea Adv Inst Sci & Technol, Dept Bio & Brain Engn, Taejon 305701, South Korea
[2] Ecole Polytech Fed Lausanne, Inst Phys Biol Syst, CH-1015 Lausanne, Switzerland
[3] Ecole Polytech Fed Lausanne, Biomed Imaging Grp, CH-1015 Lausanne, Switzerland
来源
BIOMEDICAL OPTICS EXPRESS | 2014年 / 5卷 / 11期
基金
欧洲研究理事会;
关键词
D O I
10.1364/BOE.5.003935
中图分类号
Q5 [生物化学];
学科分类号
071010 ; 081704 ;
摘要
Localization microscopy achieves nanoscale spatial resolution by iterative localization of sparsely activated molecules, which generally leads to a long acquisition time. By implementing advanced algorithms to treat overlapping point spread functions (PSFs), imaging of densely activated molecules can improve the limited temporal resolution, as has been well demonstrated in two-dimensional imaging. However, three-dimensional (3D) localization of high-density data remains challenging since PSFs are far more similar along the axial dimension than the lateral dimensions. Here, we present a new, high-density 3D imaging system and algorithm. The hybrid system is implemented by combining astigmatic and biplane imaging. The proposed 3D reconstruction algorithm is extended from our state-of-the art 2D high-density localization algorithm. Using mutual coherence analysis of model PSFs, we validated that the hybrid system is more suitable than astigmatic or biplane imaging alone for 3D localization of high-density data. The efficacy of the proposed method was confirmed via simulation and real data of microtubules. Furthermore, we also successfully demonstrated fluorescent-protein-based live cell 3D localization microscopy with a temporal resolution of just 3 seconds, capturing fast dynamics of the endoplasmic recticulum. (C) 2014 Optical Society of America
引用
收藏
页码:3935 / 3948
页数:14
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