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SummaryStructural detailsExperimental detailsFunctional detailsSequence NeighborHistoryDownloads

4AHS

Parallel screening of a low molecular weight compound library: do differences in methodology affect hit identification

Experimental procedure
Experimental methodSINGLE WAVELENGTH
Source typeSYNCHROTRON
Source detailsAUSTRALIAN SYNCHROTRON BEAMLINE MX1
Synchrotron siteAustralian Synchrotron
BeamlineMX1
Temperature [K]100
Detector technologyCCD
Collection date2008-03-13
DetectorADSC QUANTUM 210r
Spacegroup nameP 31
Unit cell lengths71.183, 71.183, 66.653
Unit cell angles90.00, 90.00, 120.00
Refinement procedure
Resolution61.660 - 1.750
R-factor0.20763
Rwork0.206
R-free0.24787
Structure solution methodMOLECULAR REPLACEMENT
Starting model (for MR)1bi4
RMSD bond length0.022
RMSD bond angle2.242
Data reduction softwareMOSFLM
Data scaling softwareSCALA
Phasing softwarePHASER
Refinement softwareREFMAC (5.6.0117)
Data quality characteristics
 OverallOuter shell
Low resolution limit [Å]61.7001.840
High resolution limit [Å]1.7501.750
Rmerge0.0700.450
Number of reflections36824
<I/σ(I)>16.21.9
Completeness [%]96.580.9
Redundancy4.92.6
Crystallization Conditions
crystal IDmethodpHtemperaturedetails
1VAPOR DIFFUSION, SITTING DROP5.5293PROTEIN: 5.5MG/ML IN 40MM TRIS BUFFER AT PH 8.0, 250MM NACL, 30MM MGCL2, 5MM DTT. CRYSTALLANT: 100MM SODIUM ACETATE PH 5.0 TO 5.5, 1.2 TO 1.5M AMMONIUM SULFATE AT 20C IN SITTING DROP PLATES. FRAGMENTS WERE SOAKED INTO PREFORMED CRYSTALS 24-48 HOURS PRIOR TO DATA COLLECTION.

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