Quality Control

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This is an attempt of putting together a number of datasets with different characteristics (high and low resolution, good and bad crystals, untwinned and twinned), their evaluation with different versions of XDS up to the structure solution (as far as that can be done automatically), and the determination of the quality of the resulting data using experimental phasing and refinement.

The goal of this is to find generally optimal parameters for XDS data reduction, to compare new versions of XDS with older ones, and to discover bugs or regressions. At the same time, it serves to display standard procedures for solving crystal structures, which may be used for teaching or learning crystallography.

The metrics I would like to look at is

  • anomalous signal: SHELXC anomalous correlations (internally or between wavelengths); SHELXD (fixed version) success rates and CCall/CCweak maximum values. Clemens Vonrhein additionally suggested anomalous difference fourier peak heights.
  • refinement of a given (known) set of heavy atom positions in (e.g.) SHARP (fixed version): r.m.s. or absolute phase difference, or map correlation w.r.t. phases from good model
  • refinement with (e.g.) refmac5 (fixed version) of a given model, finding LL and R/Rfree

For each project mentioned below, both the raw data and the XDS data reduction is available - links are on the project pages, which are named according to their PDB ids.

The raw data (images) for the different datasets are either available from this site by FTP, or from the (publicly accessible!) JCSG dataset archive, or - for 1RQW - from [1] or [2].

There's currently data available for

  • 2-wl MAD: PDB id 1T92 (PulG, 116 residues, 2 copies/ASU, spacegroup P6522, resolution 2.8 Å)
  • 3-wl MAD: PDB id 1ZTV (JCSG target name TB1631F, resolution 3.1 Å) - evaluated with Qingping Xu; it's one of the JCSG datasets.
  • native data: PDB id 2GIF (AcrB, spacegroup C2, resolution 2.9 Å - a large membrane protein structure)
  • native data for MR: PDB id 1YCE (ATPase C-ring, spacegroup P21, resolution 2.4 Å - a large membrane protein structure, 44-fold NCS, strong diffuse scattering)
  • 2-wl Bromide MAD: PDB id 1RQW (Thaumatin, a sweet-tasting protein of 207 resides, spacegroup P41212, resolution 1.8 Å, collected at the DGK Workshop 2007; could also treat either peak or inflection as SAD. These datasets have been made available by Manfred S. Weiss and Annette Faust (see Xray Tutorial).
  • S-SAD: PDB id 2QVO (AF1382, a 95-residue protein used by James Tucker Swindell II to establish optimized procedures for data reduction. The data available to solve the structure are two runs of 360° collected at 1.9Å wavelength.
  • 3-wl SeMet-MAD data PDB id 3CSL (3CSL, a complex of a 22 stranded beta-barrel outer membrane protein (the ordered residues 112-865 harbour 9 SeMet), its 173-residue hemophore (1 SeMet), and heme. Datasets are at [3]. 2 complexes per ASU, useful data to 3.2Å, useful anomalous data to about 5Å. Challenging for humans, and too difficult for automatic methods of structure solution and model building.
  • hen egg-white lysozyme @ 0.65Å resolution, PDB id 2VB1. Data (sweeps a to h, each comprising 60 to 360 frames of 72MB) were collected by Zbigniew Dauter at APS 19-ID and are available from here. Details of data collection, processing and refinement are published.

Recently I've written SIM_MX which should make parts of testing and development of XDS independant from real data.