What is it about?

Bacillus stearothermophilus ArgR binds efficiently to the Escherichia coli carAB operator, whereas the E. coli repressor binds very poorly to the argCo operator of B. stearothermophilus. In order to elucidate this contradictory behavior between ArgRs, we constructed chimeric proteins by swapping N-terminal DNA-binding and C-terminal oligomerization domains or by exchanging the linker peptide. Chimeras carrying the E. coli DNA-binding domain and the B. stearothermophilus oligomerization domain showed sequence-nonspecific rather than sequence-specific interactions with arg operators. Chimeras carrying the B. stearothermophilus DNA-binding domain and E. coli oligomerization domain exhibited a high DNA-binding affinity for the B. stearothermophilus argCo and E. coli carAB operators and repressed the reporter-gene transcription from the B. stearothermophilus PargCo control region in vitro; arginine had no effect on, and indeed even decreased, their DNA-binding affinity. With the protein array method, we showed that the wild-type B. stearothermophilus ArgR and derivatives of it containing only the exchanged linker from E. coli ArgR or carrying the B. stearothermophilus DNA-binding domain along with the linker and the 4 regions were able to bind argCo containing the single Arg box. This binding was weaker than binding to the two-box operator but was no longer arginine dependent. Several lines of observations indicate that the 4 helix in the oligomerization domain and the linker peptide can contribute to the recognition of single or double Arg boxes and therefore to the operator DNA-binding specificity in similar but not identical ArgR repressors from two distant bacteria.

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Why is it important?

Protein-DNA interactions govern the expression of genes in procaryotes and eucaryotes. However, different exogenous and endogenous factors modulate gene expression through affecting properties of regulatory proteins. This study describes differences and similarities in the functional capacity of chimeric regulatory proteins (mesophilic and thermophilic bacteria) to bind specific DNA sites. It suggests the evolutionary way from simplicity to more complex protein-DNA interactions.

Perspectives

The paradigm of arginine genes regulation provides the possibility to understand better protein-DNA and small molecule-protein interactions in distanced bacteria, and thereby, contribute to elucidation of evolution of molecular interactions. Protein arrays used for the first time to study ArgR interactions with DNA is a promising method for large-scale investigation of regulatory networks in micro-organisms.

Professor Vehary Sakanyan
University of Nantes

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This page is a summary of: Arginine Operator Binding by Heterologous and Chimeric ArgR Repressors from Escherichia coli and Bacillus stearothermophilus, Journal of Bacteriology, December 2002, ASM Journals,
DOI: 10.1128/jb.184.23.6602-6614.2002.
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