Curation Information

Publication: Functional analysis of the Pseudomonas putida regulatory protein CatR: transcriptional studies and determination of the CatR DNA-binding site by hydroxyl-radical footprinting.;Rothmel RK, Shinabarger DL, Parsek MR, Aldrich TL, Chakrabarty AM;Journal of bacteriology 1991 Aug; 173(15):4717-24 [1649820]
TF: CatR [Q88GK5, view regulon]
Reported TF sp.: Pseudomonas putida PRS2000
Reported site sp.: Pseudomonas putida PRS2000
Created by: Matthew Coveyou
Curation notes: -

Experimental Process

The promoter region of Pseudomonas putida PRS2000 gene catR was determined by reverse transcriptase mapping. Beta-gal assay of both the catR gene promoter and catBCA operon promoter indicated constitutive autoregulation of catR and inducer-dependent activation of catBCA. CatR was purified via DNA affinity column, and functionality was confirmed by EMSA. Hydroxyl-radical footprinting identified three points of direct contact between the promoter and catR across 24 bp. Footprints were not influence by the presence of the inducer.

Transcription Factor Binding Sites

Sites reported in the paper
Sites matched in the genome

TCCATCAGACCTCCAGGGTATGGT

Gene Regulation

Regulated genes for each binding site are displayed below. Gene regulation diagrams show binding sites, positively-regulated genes, negatively-regulated genes, both positively and negatively regulated genes, genes with unspecified type of regulation. For each indvidual site, experimental techniques used to determine the site are also given.

Site sequence	Regulated genes	Gene diagram	Experimental techniques	TF function	TF type
TCCATCAGACCTCCAGGGTATGGT	catB, catC, catA,		Experimental technique details Beta-gal reporter assay Beta-gal reporter assay Reporter assay using the beta-galactosidase (lacZ) gene. The lacZ gene is typically fused to the promoter of interest. Differential regulation of the promoter mediated by the TF is assessed by induction of the system and evaluation of lacZ expression. Bacteria expressing lacZ appear blue when grown on a X-gal medium. The assay is often performed using a plasmid borne construction on a lacZ(def) strain. - Experimental technique details DNA affinity purification (ECO:0005629) DNA affinity purification - ECO:0005629 In DNA affinity purification, DNA from promoter regions thought to be bound by the protein is labelled (e.g. biotinylated) and bound to beads (or some type of matrix). The protein is then left to interact with DNA and eventually eluted. Bound protein will remain attached to beads. This can be detected through gel electophoresis. The protein can then be sequenced by mass-spectrometry. The techinque can be used to demonstrate binding of a purified protein, or to purify the binding protein from crude extract or a mix of proteins. - Experimental technique details EMSA (ECO:0001807) EMSA - ECO:0001807 Electro-mobility shift-assays (or gel retardation assays) are a standard way of assessing TF-binding. A fragment of DNA of interest is amplified and labeled with a fluorophore. The fragment is left to incubate in a solution containing abundant TF and non-specific DNA (e.g. randomly cleaved DNA from salmon sperm, of all things) and then a gel is run with the incubated sample and a control (sample that has not been in contact with the TF). If the TF has bound the sample, the complex will migrate more slowly than unbound DNA through the gel, and this retarded band can be used as evidence of binding. The unspecific DNA ensures that the binding is specific to the fragment of interest and that any non-specific DNA-binding proteins left-over in the TF purification will bind there, instead of on the fragment of interest. EMSAs are typically carried out in a bunch of fragments, shown as multiple double (control+experiment) lanes in a wide picture. Certain additional controls are run in at least one of the fragments to ascertain specificity. In the most basic of these, specific competitor (the fragment of interest or a known positive control, unlabelled) is added to the reaction. This should sequester the TF and hence make the retardation band disappear, proving that the binding is indeed specific - Experimental technique details Hydroxyl-radical footprinting (ECO:0005643) Hydroxyl-radical footprinting - ECO:0005643 Hydroxyl radical footprinting is almost identical to DNase footprinting, except that it uses hydroxyl radicals to digest non-protected DNA. While hydroxyl radicals yield much better resolution than DNases due to the considerable difference in their sizes, they are also harder and more time consuming to use, and thus this method is seen somewhat infrequently. -	activator	not specified