Correlative in-resin super-resolution and electron microscopy using standard fluorescent proteins

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作者
Errin Johnson
Elena Seiradake
E. Yvonne Jones
Ilan Davis
Kay Grünewald
Rainer Kaufmann
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[1] Sir William Dunn School of Pathology,Division of Structural Biology
[2] University of Oxford,Department of Biochemistry
[3] Wellcome Trust Centre for Human Genetics,undefined
[4] University of Oxford,undefined
[5] University of Oxford,undefined
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We introduce a method for correlative in-resin super-resolution fluorescence and electron microscopy (EM) of biological structures in mammalian culture cells. Cryo-fixed resin embedded samples offer superior structural preservation, performing in-resin super-resolution, however, remains a challenge. We identified key aspects of the sample preparation procedure of high pressure freezing, freeze substitution and resin embedding that are critical for preserving fluorescence and photo-switching of standard fluorescent proteins, such as mGFP, mVenus and mRuby2. This enabled us to combine single molecule localization microscopy with transmission electron microscopy imaging of standard fluorescent proteins in cryo-fixed resin embedded cells. We achieved a structural resolution of 40–50 nm (~17 nm average single molecule localization accuracy) in the fluorescence images without the use of chemical fixation or special fluorophores. Using this approach enabled the correlation of fluorescently labeled structures to the ultrastructure in the same cell at the nanometer level and superior structural preservation.
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