A rapid, sensitive, scalable method for Precision Run-On sequencing (PRO-seq)

Author:

Judd JuliusORCID,Wojenski Luke A.,Wainman Lauren M.,Tippens Nathaniel D.ORCID,Rice Edward J.,Dziubek Alexis,Villafano Geno J.,Wissink Erin M.ORCID,Versluis Philip,Bagepalli Lina,Shah Sagar R.,Mahat Dig B.,Tome Jacob M.,Danko Charles G.,Lis John T.ORCID,Core Leighton J.

Abstract

AbstractTracking active transcription with the nuclear run-on (NRO) assays has been instrumental in uncovering mechanisms of gene regulation. The coupling of NROs with high-throughput sequencing has facilitated the discovery of previously unannotated or undetectable RNA classes genome-wide. Precision run-on sequencing (PRO-seq) is a run-on variant that maps polymerase active sites with nucleotide or near-nucleotide resolution. One main drawback to this and many other nascent RNA detection methods is the somewhat intimidating multi-day workflow associated with creating the libraries suitable for high-throughput sequencing. Here, we present an improved PRO-seq protocol where many of the enzymatic steps are carried out while the biotinylated NRO RNA remains bound to streptavidin-coated magnetic beads. These adaptations reduce time, sample loss and RNA degradation, and we demonstrate that the resulting libraries are of the same quality as libraries generated using the original published protocol. The assay is also more sensitive which permits reproducible, high-quality libraries from 104–105 cells instead of 106–107. Altogether, the improved protocol is more tractable allows for nascent RNA profiling from small samples, such as rare samples or FACS sorted cell populations.

Publisher

Cold Spring Harbor Laboratory

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