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Correlation of organelle dynamics between light microscopic live imaging and electron microscopic 3D architecture using FIB-SEM
Author(s) -
Keisuke Ohta,
Shingo Hirashima,
Yoshihiro Miyazono,
Akinobu Togo,
Keiichiro Nakamura
Publication year - 2020
Publication title -
microscopy
Language(s) - English
Resource type - Journals
SCImago Journal Rank - 0.545
H-Index - 52
eISSN - 2050-5701
pISSN - 2050-5698
DOI - 10.1093/jmicro/dfaa071
Subject(s) - organelle , live cell imaging , electron microscope , microscopy , electron tomography , ultrastructure , focused ion beam , face (sociological concept) , nanotechnology , biology , biophysics , microbiology and biotechnology , optics , materials science , physics , cell , anatomy , ion , scanning transmission electron microscopy , quantum mechanics , genetics , social science , sociology
Correlative light and electron microscopy (CLEM) methods combined with live imaging can be applied to understand the dynamics of organelles. Although recent advances in cell biology and light microscopy have helped in visualizing the details of organelle activities, observing their ultrastructure or organization of surrounding microenvironments is a challenging task. Therefore, CLEM, which allows us to observe the same area as an optical microscope with an electron microscope, has become a key technique in cell biology. Unfortunately, most CLEM methods have technical drawbacks, and many researchers face difficulties in applying CLEM methods. Here, we propose a live three-dimensional CLEM method, combined with a three-dimensional reconstruction technique using focused ion beam scanning electron microscopy tomography, as a solution to such technical barriers. We review our method, the associated technical limitations and the options considered to perform live CLEM.

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