[Chimera-users] MD trajectory analysis
meng at cgl.ucsf.edu
Mon Oct 10 15:19:02 PDT 2016
Any command you can execute at the command line, you can execute in MD Movie at each frame by defining a per-frame script (MD Movie menu: Per-Frame… Define script).
For example, at each frame you could report the frame number, select residues near ligand, and write list of the residues to the Reply Log with a per-frame command script:
sel ligand z<3.5
writesel - naming simple
…. or you could use “findclash” (find clashes or contacts command) instead of zone selection, e.g.
findclash ligand overlap -1 hb 0 make false log true naming simple
… which would give atoms instead of residues like the first example. If you wanted residues instead,
findclash ligand overlap -1 hb 0 make false select true
writesel - naming simple
Of course, these will give you a lot of results: a list of residues (or even the atoms) for each frame of your trajectory. See the command manual pages for the options of all these commands.
Guess I don’t understand why you were calculating occupancy. Each time you do that, it will calculate a separate “density” (occupancy) map. Looks like you did it at least 3 times, which is why you have 3 histograms in volume viewer. Then when you chose mesh, it only changes the “current” map (name highlighted in blue) map to mesh. The other two are still shown as solid surfaces. You can delete any of those 3 occupancy maps by clicking the “minus sign” button near the upper right corner of its histogram.
I hope this helps,
Elaine C. Meng, Ph.D.
UCSF Computer Graphics Lab (Chimera team) and Babbitt Lab
Department of Pharmaceutical Chemistry
University of California, San Francisco
> On Oct 10, 2016, at 1:54 PM, George Tzotzos <gtzotzos at me.com> wrote:
> My task is to identify ligand interactions with protein residues throughout an MD trajectory. I thought of something along the lines
> sel ligand z<3.5 #for vdW interactions, etc.
> I don’t think this can be done using the MD movie interface but I may be wrong.
> I then tried the following:
> 1. sel protein/hold selection steady
> 2. sel ligand
> 3. calculate occupancy (MD Movie/Analysis)
> 4. Chimera/select/clear selection
> 5. turned the Volume Viewer to mesh/level2.
> What I obtained is a mesh grid enclosing solid surfaces (see attached snapshot). I’m not able to get rid of these surfaces?
> I think that the problem ma be in step 2 above (sel :ligand). My ligand is N,N-Diethyl-meta-toluamide. Should I select the aromatic ring part separately of the amide part, run the above process and then repeat selecting the amide part?
> I also tried MD movie/Analysis/Residue interaction network, first selecting the ligand.
> The results I obtained are not satisfactory.
> Is there a better way of dealing with my problem?
> Thanks in advance for your kind help
> <PastedGraphic-1.tiff> <PastedGraphic-2.tiff>
> Chimera-users mailing list: Chimera-users at cgl.ucsf.edu
> Manage subscription: http://plato.cgl.ucsf.edu/mailman/listinfo/chimera-users
More information about the Chimera-users