hGRAD: A versatile “one-fits-all” system to acutely deplete RNA binding proteins from condensates

Author:

Arnold Benjamin1ORCID,Riegger Ricarda J.1ORCID,Okuda Ellen Kazumi12ORCID,Slišković Irena1ORCID,Keller Mario13ORCID,Bakisoglu Cem13ORCID,McNicoll François1ORCID,Zarnack Kathi13ORCID,Müller-McNicoll Michaela1ORCID

Affiliation:

1. Institute of Molecular Biosciences, Goethe University Frankfurt 1 , Frankfurt am Main, Germany

2. International Max Planck Research School for Cellular Biophysics 2 , Frankfurt am Main, Germany

3. Buchmann Institute for Molecular Life Sciences, Goethe University Frankfurt 3 , Frankfurt am Main, Germany

Abstract

Nuclear RNA binding proteins (RBPs) are difficult to study because they often belong to large protein families and form extensive networks of auto- and crossregulation. They are highly abundant and many localize to condensates with a slow turnover, requiring long depletion times or knockouts that cannot distinguish between direct and indirect or compensatory effects. Here, we developed a system that is optimized for the rapid degradation of nuclear RBPs, called hGRAD. It comes as a “one-fits-all” plasmid, and integration into any cell line with endogenously GFP-tagged proteins allows for an inducible, rapid, and complete knockdown. We show that the nuclear RBPs SRSF3, SRSF5, SRRM2, and NONO are completely cleared from nuclear speckles and paraspeckles within 2 h. hGRAD works in various cell types, is more efficient than previous methods, and does not require the expression of exogenous ubiquitin ligases. Combining SRSF5 hGRAD degradation with Nascent-seq uncovered transient transcript changes, compensatory mechanisms, and an effect of SRSF5 on transcript stability.

Funder

Deutsche Forschungsgemeinschaft

Deutscher Akademischer Austauschdienst

Publisher

Rockefeller University Press

Subject

Cell Biology

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