Provided by: gromacs-data_4.6.5-1build1_all
NAME
g_membed - embeds a protein into a lipid bilayer VERSION 4.6.5
SYNOPSIS
g_membed -f into_mem.tpr -n index.ndx -p topol.top -o traj.trr -x traj.xtc -c membedded.gro -e ener.edr -dat membed.dat -[no]h -[no]version -nice int -xyinit real -xyend real -zinit real -zend real -nxy int -nz int -rad real -pieces int -[no]asymmetry -ndiff int -maxwarn int -[no]start -[no]v -mdrun_path string
DESCRIPTION
g_membed embeds a membrane protein into an equilibrated lipid bilayer at the position and orientation specified by the user. SHORT MANUAL ------------ The user should merge the structure files of the protein and membrane (+solvent), creating a single structure file with the protein overlapping the membrane at the desired position and orientation. The box size is taken from the membrane structure file. The corresponding topology files should also be merged. Consecutively, create a .tpr file (input for g_membed) from these files,with the following options included in the .mdp file. - integrator = md - energygrps = Protein (or other group that you want to insert) - freezegrps = Protein - freezedim = Y Y Y - energygrp_excl = Protein Protein The output is a structure file containing the protein embedded in the membrane. If a topology file is provided, the number of lipid and solvent molecules will be updated to match the new structure file. For a more extensive manual see Wolf et al, J Comp Chem 31 (2010) 2169-2174, Appendix. SHORT METHOD DESCRIPTION ------------------------ 1. The protein is resized around its center of mass by a factor -xy in the xy-plane (the membrane plane) and a factor -z in the z-direction (if the size of the protein in the z-direction is the same or smaller than the width of the membrane, a -z value larger than 1 can prevent that the protein will be enveloped by the lipids). 2. All lipid and solvent molecules overlapping with the resized protein are removed. All intraprotein interactions are turned off to prevent numerical issues for small values of -xy or -z 3. One md step is performed. 4. The resize factor ( -xy or -z) is incremented by a small amount ((1-xy)/nxy or (1-z)/nz) and the protein is resized again around its center of mass. The resize factor for the xy-plane is incremented first. The resize factor for the z-direction is not changed until the -xy factor is 1 (thus after -nxy iterations). 5. Repeat step 3 and 4 until the protein reaches its original size ( -nxy + -nz iterations). For a more extensive method description see Wolf et al, J Comp Chem, 31 (2010) 2169-2174. NOTE ---- - Protein can be any molecule you want to insert in the membrane. - It is recommended to perform a short equilibration run after the embedding (see Wolf et al, J Comp Chem 31 (2010) 2169-2174), to re-equilibrate the membrane. Clearly protein equilibration might require longer.
FILES
-f into_mem.tpr Input Run input file: tpr tpb tpa -n index.ndx Input, Opt. Index file -p topol.top In/Out, Opt. Topology file -o traj.trr Output Full precision trajectory: trr trj cpt -x traj.xtc Output, Opt. Compressed trajectory (portable xdr format) -c membedded.gro Output Structure file: gro g96 pdb etc. -e ener.edr Output Energy file -dat membed.dat Output Generic data file
OTHER OPTIONS
-[no]hno Print help info and quit -[no]versionno Print version info and quit -nice int 0 Set the nicelevel -xyinit real 0.5 Resize factor for the protein in the xy dimension before starting embedding -xyend real 1 Final resize factor in the xy dimension -zinit real 1 Resize factor for the protein in the z dimension before starting embedding -zend real 1 Final resize faction in the z dimension -nxy int 1000 Number of iteration for the xy dimension -nz int 0 Number of iterations for the z dimension -rad real 0.22 Probe radius to check for overlap between the group to embed and the membrane -pieces int 1 Perform piecewise resize. Select parts of the group to insert and resize these with respect to their own geometrical center. -[no]asymmetryno Allow asymmetric insertion, i.e. the number of lipids removed from the upper and lower leaflet will not be checked. -ndiff int 0 Number of lipids that will additionally be removed from the lower (negative number) or upper (positive number) membrane leaflet. -maxwarn int 0 Maximum number of warning allowed -[no]startno Call mdrun with membed options -[no]vno Be loud and noisy -mdrun_path string Path to the mdrun executable compiled with this g_membed version
SEE ALSO
gromacs(7) More information about GROMACS is available at <http://www.gromacs.org/>. Mon 2 Dec 2013 g_membed(1)