High-throughput, fluorescent-aptamer-based measurements of steady-state transcription rates for the Mycobacterium tuberculosis RNA polymerase

Author:

Jensen Drake1ORCID,Ruiz Manzano Ana1,Rector Maxwell2,Tomko Eric J1,Record M Thomas2,Galburt Eric A1ORCID

Affiliation:

1. Department of Biochemistry and Molecular Biophysics, Washington University School of Medicine , Saint Louis , MO 63108 , USA

2. Department of Biochemistry, University of Wisconsin , Madison , WI 53706 , USA

Abstract

Abstract The first step in gene expression is the transcription of DNA sequences into RNA. Regulation at the level of transcription leads to changes in steady-state concentrations of RNA transcripts, affecting the flux of downstream functions and ultimately cellular phenotypes. Changes in transcript levels are routinely followed in cellular contexts via genome-wide sequencing techniques. However, in vitro mechanistic studies of transcription have lagged with respect to throughput. Here, we describe the use of a real-time, fluorescent-aptamer-based method to quantitate steady-state transcription rates of the Mycobacterium tuberculosis RNA polymerase. We present clear controls to show that the assay specifically reports on promoter-dependent, full-length RNA transcription rates that are in good agreement with the kinetics determined by gel-resolved, α-32P NTP incorporation experiments. We illustrate how the time-dependent changes in fluorescence can be used to measure regulatory effects of nucleotide concentrations and identity, RNAP and DNA concentrations, transcription factors, and antibiotics. Our data showcase the ability to easily perform hundreds of parallel steady-state measurements across varying conditions with high precision and reproducibility to facilitate the study of the molecular mechanisms of bacterial transcription.

Funder

National Institutes of Health

Publisher

Oxford University Press (OUP)

Subject

Genetics

Reference91 articles.

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