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5LRS

The Transcriptional Regulator PrfA from Listeria Monocytogenes in complex with glutathione and a 30-bp operator PrfA-box motif

Experimental procedure
Experimental methodSINGLE WAVELENGTH
Source typeSYNCHROTRON
Source detailsESRF BEAMLINE ID29
Synchrotron siteESRF
BeamlineID29
Temperature [K]100
Detector technologyPIXEL
Collection date2016-07-06
DetectorDECTRIS PILATUS3 6M
Wavelength(s)1.073
Spacegroup nameP 43 21 2
Unit cell lengths78.961, 78.961, 265.224
Unit cell angles90.00, 90.00, 90.00
Refinement procedure
Resolution54.636 - 2.900
R-factor0.2495
Rwork0.248
R-free0.27920
Structure solution methodMOLECULAR REPLACEMENT
Starting model (for MR)2bgc
RMSD bond length0.003
RMSD bond angle0.530
Data reduction softwareXDS
Data scaling softwareAimless
Phasing softwarePHASER
Refinement softwarePHENIX ((1.10.1_2155: ???))
Data quality characteristics
 OverallOuter shell
Low resolution limit [Å]58.9003.080
High resolution limit [Å]2.9002.900
Rmerge0.1761.218
Number of reflections19427
<I/σ(I)>163.1
Completeness [%]99.599.8
Redundancy25.626.2
Crystallization Conditions
crystal IDmethodpHtemperaturedetails
1VAPOR DIFFUSION, SITTING DROP4.6291Prior to the crystallization setup GSH and DTT were added to the protein solution to final concentrations of 5 mM and 1 mM, respectively. Protein and duplex DNA were incubated together at a ratio of 1:1.3 (PrfA dimer:hly DNA) at final concentrations of 50 microM and 70 microM respectively in 20 mM Tris-HCl pH 8.0, 150 mM NaCl, 1 mM DTT for 60 min at room temperature, before being used for crystal setups. Crystals were obtained after 24 h by mixing 4 microL protein-DNA solution with 2 microL reservoir solution consisting of 8% PEG 8000, 100 mM sodium acetate pH 4.6, 100 mM magnesium acetate, 20% glycerol. Prior to vitrification the soaking of PrfAWT-DNA crystals were soaked in a reservoir solution containing 30% glycerol and 100 mM GSH for 24 h.

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