Rigid-body motion is the main source of diffuse scattering in protein crystallography

de Klijn, T.; Schreurs, A.M.M.; Kroon-Batenburg, L.M.J.

doi:10.1107/S2052252519000927

Figure 1
Experimental diffraction detector images for (a) CypA and (d) lysozyme after mode filtering and radial subtraction. The reconstructed hk0 reciprocal-space slice for CypA (b) after intensity merging with Friedel symmetry (−1) and (c) after merging with Laue symmetry (mmm). The hk0 reciprocal-space slice of lysozyme (e) after intensity merging with Friedel symmetry (−1) and (f) after merging with Laue symmetry (4/mmm). The slices comprise voxels between l = −1/5 and 1/5 and l = −1/10 and 1/10 for CypA and lysozyme, respectively. The slices range from h = −22 to 22, k = −27 to 27 for CypA and h = −40 to 40, k = −40 to 40 for lysozyme.

IUCrJ

Volume 6| Part 2| March 2019| Pages 277-289

ISSN: 2052-2525

https://doi.org/10.1107/S2052252519000927

BIOLOGY | MEDICINE

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