Abstract

The long-term goal of our research is to understand fundamental aspects of ribosome synthesis and function. We propose experiments to study factors and conditions influencing rrn gene expression and specific aspects of ribosome function. Expression will be studied from two different perspectives, the rrn transcription antitermination system, and how the transcription apparatus responds to several conditions that lead to down-regulation of rRNA synthesis. Functional studies will highlight our new rrn deletion strains and are aimed at addressing questions uniquely suited to the use of these strains. In fast growing bacteria how transcription of rRNA genes occurs at increased elongation rates and bypasses terminators is very poorly understood. We will examine antitermination and map out the RNA/protein and protein/protein interactions involved. We propose to examine, using electron microscopy, how rRNA operon transcription responds to conditions requiring drastically reduced levels of operon expression. We will also ask what features of the ribosome guide its response to two specific problems in translation - sticky peptides in the exit channel and switching to tmRNA when stalled. Our ability to produce strains encoding homogenous populations of mutated ribosomes allows us to use these strains to ask where sticky peptides and their effecters interact with the ribosome and what specific features of the ribosome enable it to switch to a tmRNA molecule when a block in further translation is encountered. We have developed an rrn D strain in which we can shut off all synthesis of rRNA. Using this special strain we propose to questions such as: What rules govern the efficiency of mRNA translation when ribosomes are limiting? Are newly synthesized ribosomes required for cells to respond to a cold shock? How stable are ribosomes? The current renaissance of information and studies of the ribosome and translation process put our work into the context of contributing to fundamental information about the cellular translation machinery that apply to all living systems. ? ?

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Institute of General Medical Sciences (NIGMS)
Type
Research Project (R01)
Project #
5R01GM024751-29
Application #
7109375
Study Section
Microbial Physiology and Genetics Subcommittee 2 (MBC)
Program Officer
Rhoades, Marcus M
Project Start
1979-04-01
Project End
2007-01-31
Budget Start
2006-09-01
Budget End
2007-01-31
Support Year
29
Fiscal Year
2006
Total Cost
$28,232
Indirect Cost

  Institution

Name
Tufts University
Department
Biochemistry
Type
Schools of Medicine
DUNS #
039318308
City
Boston
State
MA
Country
United States
Zip Code
02111

  Publications

Quan, Selwyn; Skovgaard, Ole; McLaughlin, Robert E et al. (2015) Markerless Escherichia coli rrn Deletion Strains for Genetic Determination of Ribosomal Binding Sites. G3 (Bethesda) 5:2555-7
Cabrera, Julio E; Cagliero, Cedric; Quan, Selwyn et al. (2009) Active transcription of rRNA operons condenses the nucleoid in Escherichia coli: examining the effect of transcription on nucleoid structure in the absence of transertion. J Bacteriol 191:4180-5
Arnvig, Kristine B; Zeng, Shirley; Quan, Selwyn et al. (2008) Evolutionary comparison of ribosomal operon antitermination function. J Bacteriol 190:7251-7
Cruz-Vera, Luis R; New, Aaron; Squires, Catherine et al. (2007) Ribosomal features essential for tna operon induction: tryptophan binding at the peptidyl transferase center. J Bacteriol 189:3140-6
Quan, Selwyn; Zhang, Ning; French, Sarah et al. (2005) Transcriptional polarity in rRNA operons of Escherichia coli nusA and nusB mutant strains. J Bacteriol 187:1632-8
Cruz-Vera, Luis Rogelio; Rajagopal, Soumitra; Squires, Catherine et al. (2005) Features of ribosome-peptidyl-tRNA interactions essential for tryptophan induction of tna operon expression. Mol Cell 19:333-43
Torres, Martha; Balada, Joan-Miquel; Zellars, Malcolm et al. (2004) In vivo effect of NusB and NusG on rRNA transcription antitermination. J Bacteriol 186:1304-10
Zaporojets, Dmitry; French, Sarah; Squires, Catherine L (2003) Products transcribed from rearranged rrn genes of Escherichia coli can assemble to form functional ribosomes. J Bacteriol 185:6921-7
Seoh, Hyuk Kyu; Weech, Michelle; Zhang, Ning et al. (2003) rRNA antitermination functions with heat shock promoters. J Bacteriol 185:6486-9
Torres, M; Condon, C; Balada, J M et al. (2001) Ribosomal protein S4 is a transcription factor with properties remarkably similar to NusA, a protein involved in both non-ribosomal and ribosomal RNA antitermination. EMBO J 20:3811-20

Showing the most recent 10 out of 27 publications