| Literature DB >> 33904409 |
James Rae1, Charles Ferguson1, Nicholas Ariotti2, Richard I Webb3, Han-Hao Cheng4, James L Mead4, James D Riches5, Dominic Jb Hunter6, Nick Martel7, Joanne Baltos8, Arthur Christopoulos8, Nicole Sarah Bryce9, Maria Lastra Cagigas10, Sachini Fonseka1, Marcel Ethan Sayre11, Edna C Hardeman12, Peter W Gunning12, Yann Gambin13, Thomas E Hall7, Robert G Parton11.
Abstract
Genetic tags allow rapid localization of tagged proteins in cells and tissues. APEX, an ascorbate peroxidase, has proven to be one of the most versatile and robust genetic tags for ultrastructural localization by electron microscopy. Here we describe a simple method, APEX-Gold, which converts the diffuse oxidized diaminobenzidine reaction product of APEX into a silver/gold particle akin to that used for immunogold labelling. The method increases the signal to noise ratio for EM detection, providing unambiguous detection of the tagged protein, and creates a readily quantifiable particulate signal. We demonstrate the wide applicability of this method for detection of membrane proteins, cytoplasmic proteins and cytoskeletal proteins. The method can be combined with different electron microscopic techniques including fast freezing and freeze substitution, focussed ion beam scanning electron microscopy, and electron tomography. Quantitation of expressed APEX-fusion proteins is achievable using membrane vesicles generated by a cell-free expression system. These membrane vesicles possess a defined quantum of signal, which can act as an internal standard for determination of the absolute density of expressed APEX-fusion proteins. Detection of fusion proteins expressed at low levels in cells from CRISPR-edited mice demonstrates the high sensitivity of the APEX-Gold method.Entities:
Keywords: cell biology; mouse
Year: 2021 PMID: 33904409 DOI: 10.7554/eLife.64630
Source DB: PubMed Journal: Elife ISSN: 2050-084X Impact factor: 8.140