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A high-throughput assay for directly monitoring nucleolar rRNA biogenesis.

Authors :
Bryant CJ
McCool MA
Abriola L
Surovtseva YV
Baserga SJ
Source :
Open biology [Open Biol] 2022 Jan; Vol. 12 (1), pp. 210305. Date of Electronic Publication: 2022 Jan 26.
Publication Year :
2022

Abstract

Studies of the regulation of nucleolar function are critical for ascertaining clearer insights into the basic biological underpinnings of ribosome biogenesis (RB), and for future development of therapeutics to treat cancer and ribosomopathies. A number of high-throughput primary assays based on morphological alterations of the nucleolus can indirectly identify hits affecting RB. However, there is a need for a more direct high-throughput assay for a nucleolar function to further evaluate hits. Previous reports have monitored nucleolar rRNA biogenesis using 5-ethynyl uridine (5-EU) in low-throughput. We report a miniaturized, high-throughput 5-EU assay that enables specific calculation of nucleolar rRNA biogenesis inhibition, based on co-staining of the nucleolar protein fibrillarin (FBL). The assay uses two siRNA controls: a negative non-targeting siRNA control and a positive siRNA control targeting RNA Polymerase 1 (RNAP1; POLR1A ), and specifically quantifies median 5-EU signal within nucleoli. Maximum nuclear 5-EU signal can also be used to monitor the effects of putative small-molecule inhibitors of RNAP1, like BMH-21, or other treatment conditions that cause FBL dispersion. We validate the 5-EU assay on 68 predominately nucleolar hits from a high-throughput primary screen, showing that 58/68 hits significantly inhibit nucleolar rRNA biogenesis. Our new method establishes direct quantification of nucleolar function in high-throughput, facilitating closer study of RB in health and disease.

Details

Language :
English
ISSN :
2046-2441
Volume :
12
Issue :
1
Database :
MEDLINE
Journal :
Open biology
Publication Type :
Academic Journal
Accession number :
35078352
Full Text :
https://doi.org/10.1098/rsob.210305