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3RSK

STRUCTURE OF THE K7A/R10A/K66A VARIANT OF RIBONUCLEASE A

Experimental procedure
Source typeROTATING ANODE
Source detailsRIGAKU RUH2R
Temperature [K]273
Detector technologyAREA DETECTOR
Collection date1997-09-11
DetectorSIEMENS
Spacegroup nameP 32 2 1
Unit cell lengths68.150, 68.150, 65.510
Unit cell angles90.00, 90.00, 120.00
Refinement procedure
Resolution30.000 - 2.000
Structure solution methodMOLECULAR REPLACEMENT
Starting model (for MR)1rph
RMSD bond length0.010
RMSD bond angle17.868

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Data reduction softwareXCALIBRE
Data scaling softwareXDS
Phasing softwareAMoRE
Refinement softwareTNT (5E)
Data quality characteristics
 OverallOuter shell
Low resolution limit [Å]30.0002.100
High resolution limit [Å]2.0002.000
Rmerge0.029

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0.171

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Total number of observations33804

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Number of reflections14929

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<I/σ(I)>20
Completeness [%]91.084
Redundancy2.3
Crystallization Conditions
crystal IDmethodpHtemperaturedetails
1VAPOR DIFFUSION, HANGING DROP4.520

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CRYSTALS WERE PREPARED USING THE HANGING DROP METHOD. LYOPHILIZED K7A/R10A/K66A RNASE A WAS DISSOLVED IN UNBUFFERED WATER TO A CONCENTRATION OF 60MG/ML. DROPS CONSISTING OF PROTEIN SOLUTION (1.5UL), WATER (1.5UL), AND RESERVOIR SOLUTION (3.0UL) WERE SUSPENDED OVER 0.5 ML OF RESERVOIR SOLUTION [0.1M SODIUM ACETATE BUFFER, PH 4.5, CONTAINING 36% PEG 4000., vapor diffusion - hanging drop
Crystallization Reagents in Literatures
IDcrystal IDsolutionreagent nameconcentration (unit)details
11dropprotein60 (mg/ml)
21dropwater0.0015mM
31reservoirsodium acetate0.1 (M)
41reservoirPEG400036 (%(w/v))

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