7mkd Citations

Structural origins of Escherichia coli RNA polymerase open promoter complex stability.

Proc Natl Acad Sci U S A 118 (2021)
Related entries: 7mke, 7mki, 7mkj

Cited: 10 times
EuropePMC logo PMID: 34599106

Abstract

The first step in gene expression in all organisms requires opening the DNA duplex to expose one strand for templated RNA synthesis. In Escherichia coli, promoter DNA sequence fundamentally determines how fast the RNA polymerase (RNAP) forms "open" complexes (RPo), whether RPo persists for seconds or hours, and how quickly RNAP transitions from initiation to elongation. These rates control promoter strength in vivo, but their structural origins remain largely unknown. Here, we use cryoelectron microscopy to determine the structures of RPo formed de novo at three promoters with widely differing lifetimes at 37 °C: λPR (t1/2 ∼10 h), T7A1 (t1/2 ∼4 min), and a point mutant in λPR (λPR-5C) (t1/2 ∼2 h). Two distinct RPo conformers are populated at λPR, likely representing productive and unproductive forms of RPo observed in solution studies. We find that changes in the sequence and length of DNA in the transcription bubble just upstream of the start site (+1) globally alter the network of DNA-RNAP interactions, base stacking, and strand order in the single-stranded DNA of the transcription bubble; these differences propagate beyond the bubble to upstream and downstream DNA. After expanding the transcription bubble by one base (T7A1), the nontemplate strand "scrunches" inside the active site cleft; the template strand bulges outside the cleft at the upstream edge of the bubble. The structures illustrate how limited sequence changes trigger global alterations in the transcription bubble that modulate the RPo lifetime and affect the subsequent steps of the transcription cycle.

Reviews citing this publication (1)

  1. Diverse molecular mechanisms of transcription regulation by the bacterial alarmone ppGpp. Travis BA, Schumacher MA. Mol Microbiol 117 252-260 (2022)

Articles citing this publication (9)

  1. High-throughput, fluorescent-aptamer-based measurements of steady-state transcription rates for the Mycobacterium tuberculosis RNA polymerase. Jensen D, Ruiz Manzano A, Rector M, Tomko EJ, Record MT, Galburt EA. Nucleic Acids Res 51 e99 (2023)
  2. Quantitative parameters of bacterial RNA polymerase open-complex formation, stabilization and disruption on a consensus promoter. Bera SC, America PPB, Maatsola S, Seifert M, Ostrofet E, Cnossen J, Spermann M, Papini FS, Depken M, Malinen AM, Dulin D. Nucleic Acids Res 50 7511-7528 (2022)
  3. Real-Time Single-Molecule Studies of RNA Polymerase-Promoter Open Complex Formation Reveal Substantial Heterogeneity Along the Promoter-Opening Pathway. Malinen AM, Bakermans J, Aalto-Setälä E, Blessing M, Bauer DLV, Parilova O, Belogurov GA, Dulin D, Kapanidis AN. J Mol Biol 434 167383 (2022)
  4. Step-by-Step Regulation of Productive and Abortive Transcription Initiation by Pyrophosphorolysis. Plaskon D, Evensen C, Henderson K, Palatnik B, Ishikuri T, Wang HC, Doughty S, Thomas Record M. J Mol Biol 434 167621 (2022)
  5. Structural Insight into the Mechanism of σ32-Mediated Transcription Initiation of Bacterial RNA Polymerase. Lu Q, Chen T, Wang J, Wang F, Ye W, Ma L, Wu S. Biomolecules 13 738 (2023)
  6. Structural basis of transcriptional regulation by a nascent RNA element, HK022 putRNA. Hwang S, Olinares PDB, Lee J, Kim J, Chait BT, King RA, Kang JY. Nat Commun 13 4668 (2022)
  7. Structure of the transcription open complex of distinct σI factors. Li J, Zhang H, Li D, Liu YJ, Bayer EA, Cui Q, Feng Y, Zhu P. Nat Commun 14 6455 (2023)
  8. The structural mechanism for transcription activation by Caulobacter crescentus GcrA. Wu X, Yu C, Mu W, Gu Z, Feng Y, Zhang Y. Nucleic Acids Res 51 1960-1970 (2023)
  9. Transcription regulation by CarD in mycobacteria is guided by basal promoter kinetics. Zhu DX, Stallings CL. J Biol Chem 299 104724 (2023)