OsO2 as the Contrast‐Generating Chemical Species of Osmium‐Stained Biological Tissues in Electron Microscopy

Author:

Li Ruiyu12ORCID,Wildenberg Gregg34,Boergens Kevin5ORCID,Yang Yingjie5,Weber Kassandra5,Rieger Janek2ORCID,Arcidiacono Ashley2ORCID,Klie Robert5ORCID,Kasthuri Narayanan34ORCID,King Sarah B.12ORCID

Affiliation:

1. Department of Chemistry University of Chicago Chicago, IL USA

2. James Franck Institute University of Chicago Chicago, IL USA

3. Department of Neurobiology The University of Chicago Chicago, IL USA

4. Argonne National Laboratory, Biosciences Division Lemont, IL USA

5. Department of Physics University of Illinois Chicago Chicago, IL USA

Abstract

AbstractElectron imaging of biological samples stained with heavy metals has enabled visualization of subcellular structures critical in chemical‐, structural‐, and neuro‐biology. In particular, osmium tetroxide (OsO4) has been widely adopted for selective lipid imaging. Despite the ubiquity of its use, the osmium speciation in lipid membranes and the process for contrast generation in electron microscopy (EM) have continued to be open questions, limiting efforts to improve staining protocols and therefore high‐resolution nanoscale imaging of biological samples. Following our recent success using photoemission electron microscopy (PEEM) to image mouse brain tissues with synaptic resolution, we have used PEEM to determine the nanoscale electronic structure of Os‐stained biological samples. Os(IV), in the form of OsO2, generates nanoaggregates in lipid membranes, leading to a strong spatial variation in the electronic structure and electron density of states. OsO2 has a metallic electronic structure that drastically increases the electron density of states near the Fermi level. Depositing metallic OsO2 in lipid membranes allows for strongly enhanced EM signals and conductivity of biological materials. The identification of the chemical species and understanding of the membrane contrast mechanism of Os‐stained biological specimens provides a new opportunity for the development of staining protocols for high‐resolution, high‐contrast EM imaging.

Funder

National Science Foundation

University of Chicago

Army Research Office

Publisher

Wiley

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