4I8D
Crystal Structure of Beta-D-glucoside glucohydrolase from Trichoderma reesei
Experimental procedure
| Experimental method | SINGLE WAVELENGTH |
| Source type | SYNCHROTRON |
| Source details | APS BEAMLINE 23-ID-D |
| Synchrotron site | APS |
| Beamline | 23-ID-D |
| Temperature [K] | 100 |
| Detector technology | CCD |
| Collection date | 2011-01-01 |
| Detector | MARMOSAIC 300 mm CCD |
| Wavelength(s) | 0.9793 |
| Spacegroup name | C 1 2 1 |
| Unit cell lengths | 130.410, 107.860, 125.860 |
| Unit cell angles | 90.00, 115.59, 90.00 |
Refinement procedure
| Resolution | 44.890 - 2.480 |
| R-factor | 0.2038 |
| Rwork | 0.201 |
| R-free | 0.27020 |
| Structure solution method | MOLECULAR REPLACEMENT |
| Starting model (for MR) | 2x40 |
| Data reduction software | DENZO |
| Data scaling software | SCALEPACK |
| Phasing software | PHASER |
| Refinement software | PHENIX |
Data quality characteristics
| Overall | Inner shell | Outer shell | |
| Low resolution limit [Å] | 50.000 | 50.000 | 2.540 |
| High resolution limit [Å] | 2.480 | 6.780 | 2.480 |
| Rmerge | 0.147 | 0.045 | 0.849 |
| Number of reflections | 54914 | ||
| <I/σ(I)> | 6.4 | ||
| Completeness [%] | 99.8 | 99.5 | 99.9 |
| Redundancy | 4.2 | 4.1 | 4.2 |
Crystallization Conditions
| crystal ID | method | pH | temperature | details |
| 1 | VAPOR DIFFUSION, SITTING DROP | 9 | 277 | Protein solution (25mM sodium acetate, pH5.0) mixed in a 1:1 ratio with the well solution (4% 2-propanol, 0.1M BTP pH9.0, 20% MEPEG 5K) Cryoprotected with 4%2-propanol, 25% MEPEG 5K, 0.1M BTP pH9.0, 10% ethylene glycol, Vapor diffusion, sitting drop, temperature 277K |
