Bright split red fluorescent proteins for the visualization of endogenous proteins and synapses

Author:

Feng SiyuORCID,Varshney Aruna,Coto Villa Doris,Modavi Cyrus,Kohler John,Farah Fatima,Zhou Shuqin,Ali Nebat,Müller Joachim D.,Van Hoven Miri K.,Huang BoORCID

Abstract

AbstractSelf-associating split fluorescent proteins (FPs) are split FPs whose two fragments spontaneously associate to form a functional FP. They have been widely used for labeling proteins, scaffolding protein assembly and detecting cell-cell contacts. Recently developments have expanded the palette of self-associating split FPs beyond the original split GFP1-10/11. However, these new ones have suffered from suboptimal fluorescence signal after complementation. Here, by investigating the complementation process, we have demonstrated two approaches to improve split FPs: assistance through SpyTag/SpyCatcher interaction and directed evolution. The latter has yielded two split sfCherry3 variants with substantially enhanced overall brightness, facilitating the tagging of endogenous proteins by gene editing. Based on sfCherry3, we have further developed a new red-colored trans-synaptic marker called Neuroligin-1 sfCherry3 Linker Across Synaptic Partners (NLG-1 CLASP) for multiplexed visualization of neuronal synapses in livingC.elegans, demonstrating its broad applications.

Funder

U.S. Department of Health & Human Services | National Institutes of Health

National Science Foundation

UCSF Program of Breakthrough Biomedical Reseearch Chan Zuckerberg Biohub

Publisher

Springer Science and Business Media LLC

Subject

General Agricultural and Biological Sciences,General Biochemistry, Genetics and Molecular Biology,Medicine (miscellaneous)

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