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6MV9

X-ray crystal structure of Bacillus subtilis ribonucleotide reductase NrdE alpha subunit with TTP and ADP

Experimental procedure
Experimental methodSINGLE WAVELENGTH
Source typeSYNCHROTRON
Source detailsCHESS BEAMLINE F1
Synchrotron siteCHESS
BeamlineF1
Temperature [K]100
Detector technologyPIXEL
Collection date2018-05-06
DetectorDECTRIS PILATUS 6M
Wavelength(s)0.9775
Spacegroup nameP 21 21 21
Unit cell lengths120.260, 126.400, 128.310
Unit cell angles90.00, 90.00, 90.00
Refinement procedure
Resolution19.975 - 2.950
R-factor0.2078
Rwork0.207
R-free0.23860
Structure solution methodMOLECULAR REPLACEMENT
Starting model (for MR)6cgm
RMSD bond length0.003
RMSD bond angle0.619
Data reduction softwareMOSFLM
Data scaling softwareAimless
Phasing softwarePHASER
Refinement softwarePHENIX ((1.13_2998: ???))
Data quality characteristics
 OverallOuter shell
Low resolution limit [Å]19.9803.070
High resolution limit [Å]2.9502.950
Rmerge0.1800.763
Rpim0.1080.452
Number of reflections414644649
<I/σ(I)>5.41.6
Completeness [%]99.299.8
Redundancy3.63.7
CC(1/2)0.9780.441
Crystallization Conditions
crystal IDmethodpHtemperaturedetails
1VAPOR DIFFUSION, SITTING DROP7.6293The crystal was grown by vapor diffusion from 4.5 mg/ml holo-NrdE in 50 mM HEPES (pH 7.6), 50 mM NaCl, 5 mM MgCl2, 2 mM TCEP, and 1% glycerol, supplemented with 5 mM ATP, 0.5 mM TTP, and 5 mM CDP. The protein solution was incubated for 10 minutes with freshly added nucleotides prior to being mixed in a 1:1 hanging drop with a precipitating solution of 6% PEG 3350, 1% w/v tryptone, and 50 mM HEPES at pH 6.9. Crystals were cryoprotected by soaking for 5-10 seconds in well solution mixed with 8% w/v sucrose, 2% w/v glucose, 8% v/v glycerol, 8% v/v ethylene glycol and supplemented with nucleotides, TCEP, and MgCl2 adjusted to the same concentrations used in the original protein solutions.

218500

數據於2024-04-17公開中

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