Repurposing an endogenous degradation system for rapid and targeted depletion of C. elegans proteins

Author:

Armenti Stephen T.1,Lohmer Lauren L.2,Sherwood David R.2,Nance Jeremy13

Affiliation:

1. Helen L. and Martin S. Kimmel Center for Biology and Medicine at the Skirball Institute of Biomolecular Medicine, NYU School of Medicine, New York, NY 10016, USA

2. Department of Biology, Duke University, Box 90338, Durham, NC 27708, USA

3. Department of Cell Biology, NYU School of Medicine, New York, NY 10016, USA

Abstract

The capability to conditionally inactivate gene function is essential for understanding the molecular basis of development. In gene and mRNA targeting approaches, protein products can perdure, complicating genetic analysis. Current methods for selective protein degradation require drug treatment or take hours for protein removal, limiting their utility in studying rapid developmental processes in vivo. Here, we repurpose an endogenous protein degradation system to rapidly remove targeted C. elegans proteins. We show that upon expression of the E3 ubiquitin ligase substrate-recognition subunit ZIF-1, proteins tagged with the ZF1 zinc-finger domain can be quickly degraded in all somatic cell types examined with temporal and spatial control. We demonstrate that genes can be engineered to become conditional loss-of-function alleles by introducing sequences encoding the ZF1 tag into endogenous loci. Finally, we use ZF1 tagging to establish the site of cdc-42 gene function during a cell invasion event. ZF1 tagging provides a powerful new tool for the analysis of dynamic developmental events.

Publisher

The Company of Biologists

Subject

Developmental Biology,Molecular Biology

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