I have been trying to find in the documentation if there is a way to do this but I have the following problem: In a recent structure we are currently refining we identified a spermine molecule sitting right on a crystallographic two-fold axis. Spermine has internal two-fold symmetry and it is part of extensive crystal contacts. I just wonder how to refine this with Phenix. In Refmac it is easy, I put the occupancies to 0.5 and the program ignores the clashes of the symmetry related molecule, but that doesn't seem to be the way that Phenix works. Can anyone give me advise on this? Thanks __________________________________________________________________________ | Marjolein Thunnissen Phone +46-(0)46-22 24584| | Associate Professor Fax +46-(0)46-22 24692| | Dept of Molecular Biophysics, Lund University http://www.mbfys.lu.se | | PO-Box 124 S-221 00 Lund, Sweden | | | |Scientific Coordinator I911 (Max-lab): MAD and fixed-wavelength stations | | for macromolecular crystallography | |__________________________________________________________________________|