RNA polymerase mutations that impair conversion to a termination-resistant complex by Q antiterminator proteins

  1. Thomas J. Santangelo1,
  2. Rachel Anne Mooney2,
  3. Robert Landick2, and
  4. Jeffrey W. Roberts1,3
  1. 1Department of Molecular Biology and Genetics, Cornell University, Ithaca, New York 14853, USA; 2Department of Bacteriology, University of Wisconsin-Madison, Madison, Wisconsin 53706, USA

Abstract

Bacteriophage λ Q-protein stably binds and modifies RNA polymerase (RNAP) to a termination-resistant form. We describe amino acid substitutions in RNAP that disrupt Q-mediated antitermination in vivo and in vitro. The positions of these substitutions in the modeled RNAP/DNA/RNA ternary elongation complex, and their biochemical properties, suggest that they do not define a binding site for Q in RNAP, but instead act by impairing interactions among core RNAP subunits and nucleic acids that are essential for Q modification. A specific conjecture is that Q modification stabilizes interactions of RNAP with the DNA/RNA hybrid and optimizes alignment of the nucleic acids in the catalytic site. Such changes would inhibit the activity of the RNA hairpin of an intrinsic terminator to disrupt the 5′-terminal bases of the hybrid and remove the RNA 3′ terminus from the active site.

Keywords

Footnotes

  • 3 Corresponding author.

  • E-MAIL jwr7{at}cornell.edu; FAX (607) 255-2428.

  • Article and publication are at http://www.genesdev.org/cgi/doi/10.1101/gad.1082103.

    • Received February 7, 2003.
    • Accepted March 24, 2003.
| Table of Contents

This Article

  1. doi: 10.1101/gad.1082103 Genes & Dev. 17: 1281-1292 Cold Spring Harbor Laboratory Press

Article Category

Share

Current Issue

  1. March 1, 2024, 38 (5-6)
  1. Current Issue
  1. Alert me to new issues of G&D

Life Science Alliance