| Literature DB >> 33707009 |
Xavier Heiligenstein1, Marit de Beer2, Jérôme Heiligenstein3, Frédérique Eyraud4, Laurent Manet3, Fabrice Schmitt5, Edwin Lamers6, Joerg Lindenau7, Mariska Kea-Te Lindert8, Jean Salamero9, Graça Raposo10, Nico Sommerdijk11, Martin Belle3, Anat Akiva12.
Abstract
With the development of advanced imaging methods that took place in the last decade, the spatial correlation of microscopic and spectroscopic information-known as multimodal imaging or correlative microscopy (CM)-has become a broadly applied technique to explore biological and biomedical materials at different length scales. Among the many different combinations of techniques, Correlative Light and Electron Microscopy (CLEM) has become the flagship of this revolution. Where light (mainly fluorescence) microscopy can be used directly for the live imaging of cells and tissues, for almost all applications, electron microscopy (EM) requires fixation of the biological materials. Although sample preparation for EM is traditionally done by chemical fixation and embedding in a resin, rapid cryogenic fixation (vitrification) has become a popular way to avoid the formation of artifacts related to the chemical fixation/embedding procedures. During vitrification, the water in the sample transforms into an amorphous ice, keeping the ultrastructure of the biological sample as close as possible to the native state. One immediate benefit of this cryo-arrest is the preservation of protein fluorescence, allowing multi-step multi-modal imaging techniques for CLEM. To minimize the delay separating live imaging from cryo-arrest, we developed a high-pressure freezing (HPF) system directly coupled to a light microscope. We address the optimization of sample preservation and the time needed to capture a biological event, going from live imaging to cryo-arrest using HPF. To further explore the potential of cryo-fixation related to the forthcoming transition from imaging 2D (cell monolayers) to imaging 3D samples (tissue) and the associated importance of homogeneous deep vitrification, the HPF core technology has been revisited to allow easy modification of the environmental parameters during vitrification. Lastly, we will discuss the potential of our HPM within CLEM protocols especially for correlating live imaging using the Zeiss LSM900 with electron microscopy.Entities:
Keywords: Bio-imaging; Correlative Light and Electron Microscopy; Cryo-electron microscopy; Cryo-light microscopy; Electron microscopy; High-pressure freezing; Live cell imaging; Vitrification; Volume electron microscopy
Year: 2021 PMID: 33707009 DOI: 10.1016/bs.mcb.2020.10.022
Source DB: PubMed Journal: Methods Cell Biol ISSN: 0091-679X Impact factor: 1.441