Fast high-resolution 3D total internal reflection fluorescence microscopy by incidence angle scanning and azimuthal averaging

被引:69
|
作者
Boulanger, Jerome [1 ]
Gueudry, Charles [2 ,3 ]
Muench, Daniel [2 ,3 ]
Cinquin, Bertrand [1 ]
Paul-Gilloteaux, Perrine [1 ,2 ]
Bardin, Sabine [1 ]
Guerin, Christophe [4 ]
Senger, Fabrice [4 ]
Blanchoin, Laurent [4 ]
Salamero, Jean [1 ,2 ]
机构
[1] Inst Curie, CNRS UMR144, F-75005 Paris, France
[2] Inst Curie, Plateforme Imagerie Cellulaire & Tissulaire Infra, F-75005 Paris, France
[3] Roper Sci, F-91017 Evry, France
[4] Univ Grenoble 1, INRA,CEA, CNRS,Inst Rech Technol & Sci Vivant, Lab Physiol Cellulaire & Vegetale, F-38054 Grenoble, France
关键词
TIRFM; high resolution; living cells; 3D image reconstruction; membrane recycling; LIMIT; ILLUMINATION; GRANULES; LANGERIN; RECEPTOR; TIRF;
D O I
10.1073/pnas.1414106111
中图分类号
O [数理科学和化学]; P [天文学、地球科学]; Q [生物科学]; N [自然科学总论];
学科分类号
07 ; 0710 ; 09 ;
摘要
Total internal reflection fluorescence microscopy (TIRFM) is the method of choice to visualize a variety of cellular processes in particular events localized near the plasma membrane of live adherent cells. This imaging technique not relying on particular fluorescent probes provides a high sectioning capability. It is, however, restricted to a single plane. We present here a method based on a versatile design enabling fast multiwavelength azimuthal averaging and incidence angles scanning to computationally reconstruct 3D images sequences. We achieve unprecedented 50-nm axial resolution over a range of 800 nm above the coverslip. We apply this imaging modality to obtain structural and dynamical information about 3D actin architectures. We also temporally decipher distinct Rab11a-dependent exocytosis events in 3D at a rate of seven stacks per second.
引用
收藏
页码:17164 / 17169
页数:6
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