Hi Ralf,
The coordinates of the ligand in the file I use for refinement are
similar to those I posted. I uploaded an overlay of the original
ligand and the ligand in my model. Green is model, blue is original...
You can see the picture on this site:
http://gallery.me.com/ruben.vandermeeren/100216
The cryst1 card of the pdb is the next:
CRYST1 98.500 104.050 415.200 90.00 90.00 90.00 P 21 21 21
The structure has 4 monomers in which I modeled a ligand monomer A and
B. I also checked the .geo file. In most cases (for bonds and Angles)
the model is almost equal to the ideal. For dihedrals there is much
more disagreement. E.g. for one dihedral the model is 168° whereas the
ideal is -60°. For non-bound interactions the distance is sometimes
less than the VDW-radius. Could this be the problem? But this is in
fact the thing I want to refine.
The log file can be downloaded here:
files.me.com/ruben.vandermeeren/9tuifv
Ruben
Citeren "Ralf W. Grosse-Kunstleve"
Hi Ruben,
I'm using phenix for the refinement of my protein (phenix.refine). But there is a problem...
Your pdb and cif file seem OK after a quick check (phenix.pdbtools --geometry-regularization tre.pdb tre.cif). My best guess is that the ligand conincides with a symmetry operation. Are the coordinates in the pdb file you posted similar to the coordinates in the file you used for refinement? Could you send me the CRYST1 card? The phenix.refine log would also be helpful. Note that all geometry restraints are listed in the .geo file written by phenix.refine. Look for nonbonded interactions involving your ligand.
Ralf _______________________________________________ phenixbb mailing list [email protected] http://www.phenix-online.org/mailman/listinfo/phenixbb