Against the odds? De novo structure determination of a pilin with two cysteine residues by sulfur SAD

Exploiting the anomalous signal of the intrinsic S atoms to phase a protein structure is advantageous, as ideally only a single well diffracting native crystal is required. However, sulfur is a weak anomalous scatterer at the typical wavelengths used for X‐ray diffraction experiments, and therefore...

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Veröffentlicht in:Acta crystallographica. Section D, Biological crystallography. Biological crystallography., 2015-05, Vol.71 (5), p.1095-1101
Hauptverfasser: Gorgel, Manuela, Bøggild, Andreas, Ulstrup, Jakob Jensen, Weiss, Manfred S., Müller, Uwe, Nissen, Poul, Boesen, Thomas
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Sprache:eng
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Zusammenfassung:Exploiting the anomalous signal of the intrinsic S atoms to phase a protein structure is advantageous, as ideally only a single well diffracting native crystal is required. However, sulfur is a weak anomalous scatterer at the typical wavelengths used for X‐ray diffraction experiments, and therefore sulfur SAD data sets need to be recorded with a high multiplicity. In this study, the structure of a small pilin protein was determined by sulfur SAD despite several obstacles such as a low anomalous signal (a theoretical Bijvoet ratio of 0.9% at a wavelength of 1.8 Å), radiation damage‐induced reduction of the cysteines and a multiplicity of only 5.5. The anomalous signal was improved by merging three data sets from different volumes of a single crystal, yielding a multiplicity of 17.5, and a sodium ion was added to the substructure of anomalous scatterers. In general, all data sets were balanced around the threshold values for a successful phasing strategy. In addition, a collection of statistics on structures from the PDB that were solved by sulfur SAD are presented and compared with the data. Looking at the quality indicator Ranom/Rp.i.m., an inconsistency in the documentation of the anomalous R factor is noted and reported.
ISSN:1399-0047
0907-4449
1399-0047
DOI:10.1107/S1399004715003272