ORANGE: A CRISPR/Cas9-based genome editing toolbox for epitope tagging of endogenous proteins in neurons

Willems, Jelmer and de Jong, Arthur P. H. and Scheefhals, Nicky and Mertens, Eline and Catsburg, Lisa A. E. and Poorthuis, Rogier B. and de Winter, Fred and Verhaagen, Joost and Meye, Frank J. and MacGillavry, Harold D. and Hsueh, Yi-Ping (2020) ORANGE: A CRISPR/Cas9-based genome editing toolbox for epitope tagging of endogenous proteins in neurons. PLOS Biology, 18 (4). e3000665. ISSN 1545-7885

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Abstract

The correct subcellular distribution of proteins establishes the complex morphology and function of neurons. Fluorescence microscopy techniques are invaluable to investigate subcellular protein distribution, but they suffer from the limited ability to efficiently and reliably label endogenous proteins with fluorescent probes. We developed ORANGE: Open Resource for the Application of Neuronal Genome Editing, which mediates targeted genomic integration of epitope tags in rodent dissociated neuronal culture, in organotypic slices, and in vivo. ORANGE includes a knock-in library for in-depth investigation of endogenous protein distribution, viral vectors, and a detailed two-step cloning protocol to develop knock-ins for novel targets. Using ORANGE with (live-cell) superresolution microscopy, we revealed the dynamic nanoscale organization of endogenous neurotransmitter receptors and synaptic scaffolding proteins, as well as previously uncharacterized proteins. Finally, we developed a mechanism to create multiple knock-ins in neurons, mediating multiplex imaging of endogenous proteins. Thus, ORANGE enables quantification of expression, distribution, and dynamics for virtually any protein in neurons at nanoscale resolution.

Item Type: Article
Subjects: Apsci Archives > Biological Science
Depositing User: Unnamed user with email support@apsciarchives.com
Date Deposited: 09 Jan 2023 07:15
Last Modified: 02 Oct 2023 12:38
URI: http://eprints.go2submission.com/id/eprint/16

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