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6EXL

The Transcriptional Regulator PrfA from Listeria Monocytogenes in complex with a ring-fused 2-pyridone (MK206) - folded HTH motif

Experimental procedure
Experimental methodSINGLE WAVELENGTH
Source typeSYNCHROTRON
Source detailsESRF BEAMLINE ID23-1
Synchrotron siteESRF
BeamlineID23-1
Temperature [K]100
Detector technologyPIXEL
Collection date2015-12-15
DetectorDECTRIS PILATUS 6M-F
Wavelength(s)0.975
Spacegroup nameP 21 21 21
Unit cell lengths47.749, 87.795, 116.183
Unit cell angles90.00, 90.00, 90.00
Refinement procedure
Resolution43.900 - 1.900
R-factor0.175
Rwork0.173
R-free0.22500
Structure solution methodMOLECULAR REPLACEMENT
Starting model (for MR)5f1r
RMSD bond length0.021
RMSD bond angle1.154
Data reduction softwareXDS
Data scaling softwareAimless
Phasing softwarePHASER
Refinement softwarePHENIX ((1.10.1_2155: ???))
Data quality characteristics
 OverallOuter shell
Low resolution limit [Å]43.8971.970
High resolution limit [Å]1.9001.900
Rmerge0.0890.783
Number of reflections38994
<I/σ(I)>13.42.5
Completeness [%]99.497.9
Redundancy7.26.9
Crystallization Conditions
crystal IDmethodpHtemperaturedetails
1VAPOR DIFFUSION, HANGING DROP5.5291Following cell lysis, the protein was extracted by Ni-NTA Superflow FF, followed by TEV protease cleavage in buffer (200 mM NaCl, 1 mM BME, 20 mM NaP (NaH2PO4+Na2HPO4, pH 7.1). Further purification included Ni-NTA, MonoS and Gelfiltration (in 200 mM NaCl and 20 mM NaP buffer pH 6.5). Purified PrfA was co-crystallized with complex (5 mol excess) using the hanging-drop vapor-diffusion technique. Crystals grew in 5 days after 2 microL of the protein solution (3.2-3.5 mg per ml PrfA, 200 mM NaCl, 20 mM NaP buffer, pH 6.5) was mixed with an equal volume of precipitant solution containing 20-24% PEG-4000, 17% isopropanol, 100 mM Na citrate pH 5.5 and allowed to equilibrate over a 1 ml solution of the precipitant in a Linbro plate (Hampton Research).

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