Abstract

2-component signaling is the principal form of signal transduction in prokaryotes with distinctive examples in eukaryotes. At the end of logarithmic growth, the """"""""transition state"""""""" Bacillus cell receives multiple signals from the environment that are simultaneously reporting conditions such as temperature, cell density, nutrition availability and oxygen tension. These signals are processed to determine the most appropriate gene expression and metabolic response for survival. The hypothesis we are testing is that """"""""The processing of the multiple signals is accomplished by regulatory networks involving multiple 2-component systems that function to establish dependencies or hierarchies between systems. Cross-system interaction between regulons provides a mechanism for signal integration and amplification, a mechanism which results in fine tuning of a given response that accommodates the entire signal input experienced by the organism at any 1 time."""""""" The Pho signal transduction network is comprised of at least 3 2-component systems: PhoP-PhoR, ResD-ResE and Spo0A, and global stress, catabolite, transition state and developmental regulators. We will examine the role of the Spo0A~P-AbrB pathway in the Pho signal transduction network by determining which of 6 phoPR promoter(s) respond to direct AbrB binding and if AbrB also has an indirect role via ScoC. We will determine what unknown regulatory circuits control phoPR P5 promoter regulation in the absence of a second Pi starvation global regulator, SigB. We will examine the positive feedback loop that is essential for resABCDE transcription (ResD and ResE production) during phosphate starvation by analyzing mutations that bypass the requirement for PhoP in resA transcription and via reconstruction of resA transcription in vitro to understand the essential but insufficient role of both PhoP and ResD. We will examine the cross-system interaction via the positive feedback loop that is essential for full induction of the Pho regulon by determining the role of upstream regulator, ResD, in controlling the Pi deficiency signal and/or modulation of that signal. We will determine how reduced menaquinones that inhibit the autophosphorylation of PhoR in vitro, modulate the phosphate deficiency signal in vivo and ask if redox-reactive cysteines play a role. These studies will contribute to the knowledge base of two-component signal transduction systems of gram-positive bacteria as targets for antimicrobial therapy. ? ?

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Institute of General Medical Sciences (NIGMS)
Type
Research Project (R01)
Project #
5R01GM033471-22
Application #
7475839
Study Section
Prokaryotic Cell and Molecular Biology Study Section (PCMB)
Program Officer
Anderson, James J
Project Start
1985-01-01
Project End
2010-06-30
Budget Start
2008-07-01
Budget End
2009-06-30
Support Year
22
Fiscal Year
2008
Total Cost
$291,910
Indirect Cost

  Institution

Name
University of Illinois at Chicago
Department
Biology
Type
Schools of Arts and Sciences
DUNS #
098987217
City
Chicago
State
IL
Country
United States
Zip Code
60612

  Publications

Kaushal, Bindiya; Paul, Salbi; Hulett, F Marion (2010) Direct regulation of Bacillus subtilis phoPR transcription by transition state regulator ScoC. J Bacteriol 192:3103-13
Puri-Taneja, Ankita; Schau, Matthew; Chen, Yinghua et al. (2007) Regulators of the Bacillus subtilis cydABCD operon: identification of a negative regulator, CcpA, and a positive regulator, ResD. J Bacteriol 189:3348-58
Eldakak, Amr; Hulett, F Marion (2007) Cys303 in the histidine kinase PhoR is crucial for the phosphotransfer reaction in the PhoPR two-component system in Bacillus subtilis. J Bacteriol 189:410-21
Puri-Taneja, Ankita; Paul, Salbi; Chen, Yinghua et al. (2006) CcpA causes repression of the phoPR promoter through a novel transcription start site, P(A6). J Bacteriol 188:1266-78
Abdel-Fattah, Wael R; Chen, Yinghua; Eldakak, Amr et al. (2005) Bacillus subtilis phosphorylated PhoP: direct activation of the E(sigma)A- and repression of the E(sigma)E-responsive phoB-PS+V promoters during pho response. J Bacteriol 187:5166-78
Schau, Matthew; Chen, Yinghua; Hulett, F Marion (2004) Bacillus subtilis YdiH is a direct negative regulator of the cydABCD operon. J Bacteriol 186:4585-95
Paul, Salbi; Birkey, Stephanie; Liu, Wei et al. (2004) Autoinduction of Bacillus subtilis phoPR operon transcription results from enhanced transcription from EsigmaA- and EsigmaE-responsive promoters by phosphorylated PhoP. J Bacteriol 186:4262-75
Chen, Yinghua; Abdel-Fattah, Wael R; Hulett, F Marion (2004) Residues required for Bacillus subtilis PhoP DNA binding or RNA polymerase interaction: alanine scanning of PhoP effector domain transactivation loop and alpha helix 3. J Bacteriol 186:1493-502
Schau, Matthew; Eldakak, Amr; Hulett, F Marion (2004) Terminal oxidases are essential to bypass the requirement for ResD for full Pho induction in Bacillus subtilis. J Bacteriol 186:8424-32
Birck, Catherine; Chen, Yinghua; Hulett, F Marion et al. (2003) The crystal structure of the phosphorylation domain in PhoP reveals a functional tandem association mediated by an asymmetric interface. J Bacteriol 185:254-61

Showing the most recent 10 out of 39 publications