lammps/tools/ch2lmp
Axel Kohlmeyer 9fd1e47968 ignore generated/copied files 2018-01-28 06:24:03 -05:00
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example recreate 1ac7 input deck with up to date tools and LAMMPS binary. 2018-01-28 06:23:09 -05:00
example-cmap recreate 1gb1 input deck with CMAP included. 2018-01-28 06:22:03 -05:00
other permission update for ch2lmp tool folder 2016-10-03 07:03:42 -04:00
.gitignore ignore generated/copied files 2018-01-28 06:24:03 -05:00
README some more updates to the README file to reflect the inclusion of the CMAP example and renamed file names 2016-10-05 18:41:45 -04:00
charmm2lammps.pl make formatting comment consistent 2017-01-11 07:46:07 -05:00
lammps2pdb.pl remove trailing whitespace 2016-10-03 07:07:28 -04:00

README

These tools were created by Pieter J. in 't Veld (pjintve@sandia.gov)
and Paul Crozier (pscrozi@sandia.gov), Sandia National Laboratories,
2005. They are intended to make it easy to use CHARMM as a builder and
as a post-processor for LAMMPS. Using charmm2lammps.pl, you can
convert an ensemble built in CHARMM into its LAMMPS equivalent.  Using
lammps2pdb.pl you can convert LAMMPS atom dumps into pdb files.

In this directory, you should find:
1) A perl script called "charmm2lammps.pl"
2) A perl script called "lammps2pdb.pl"
3) Two folders containing examples of how to use these tools.
4) An "other" folder containing other potentially useful tools.

In addition, you will need to provide the following input for
charmm2lammps.pl:

1) a CHARMM parameter file (par_<forcefield>.prm)
2) a CHARMM topology file (top_<forcefield>.rtf)
3) a CHARMM coordinates file or pdb file (<project>.crd or <project>.pdb)
   (NOTE: a .pdb file is required if the -cmap option is used)
4) a CHARMM psf file (<project>.psf)

To use the charmm2lammps.pl script, type: "perl charmm2lammps.pl
<forcefield> <project> [-option=value ...]" where <forcefield> is the
name of the CHARMM FF you are using, (i.e. all22_prot), and <project>
is the common name of your *.crd and *.psf files.  Possible options
are listed below.  If the option requires a parameter, the syntax
must be like this: -option=value (e.g. -border=5).

-help        display available options
-nohints     do not add charmm types and style hints to LAMMPS data file
-water       add TIP3P water [default: 1 g/cc]
-ions        add (counter)ions using Na+ and Cl- [default: 0 mol/l]
-center      recenter atoms
-quiet       do not print info
-pdb_ctrl    output project_ctrl.pdb
-l           set x-, y-, and z-dimensions simultaneously
-lx          x-dimension of simulation box
-ly          y-dimension of simulation box
-lz          z-dimension of simulation box
-border      add border to all sides of simulation box [default: 0 A]
-ax          rotation around x-axis
-ay          rotation around y-axis
-az          rotation around z-axis
-cmap        add CMAP section to data file and fix cmap command lines in
             input script" (NOTE: requires use of *.pdb file)

In the "example" folder, you will find example files that were created
by following the steps below. These steps describe how to take a
biomolecule and convert it into LAMMPS input, and then create a *.pdb
trajectory from the LAMMPS output.

1) Get the pdb file you want to model. http://www.rcsb.org/pdb/ For
this examples, we will use either 1ac7.pdb or 1gb1.pdb

2) If there are multiple models in the pdb file, choose the one you
want and delete the others. Save the pared-down file as 1ac7_pared.pdb

3) Download the charmm FF files and choose the one you want from the
tarball.  We will use all27_na for 1AC7 and all36_prot for 1GB1. The
required files for the example are included in their folders. You can
download complete CHARMM force field packages from:
http://mackerell.umaryland.edu/charmm_ff.shtml

4) Create a *.pgn file for use with psfgen (you will need to have VMD
installed, http://www.ks.uiuc.edu/Research/vmd/ ). This is the hardest
step because you have to change the residue names from what the *.pdb
file has to the corresponding names in the charmm FF files. You'll
need to add a "pdbalias residue x xnew" line for each change that
needs to be made.  The *.pgn should contain something like this:

package require psfgen
topology top_all27_na.rtf
pdbalias residue A ADE
pdbalias residue T THY
pdbalias residue G GUA
pdbalias residue C CYT
.
.
.
segment A {pdb 1ac7_pared.pdb}
coordpdb 1ac7_pared.pdb A
guesscoord
writepdb 1ac7.pdb
writepsf charmm 1ac7.psf
exit

For 1GB1 the corresponding 1gb1.psf file has been created with CHARMM-GUI,
http://www.charmm-gui.org

5) Type "vmd -dispdev none -e 1ac7.pgn" to build the 1ac7.psf file, and the new
   1ac7.pdb file.

6) Run charmm2lammps.pl by typing:
"perl charmm2lammps.pl all27_na 1ac7 -border=2.0 -pdb_ctrl -water -ions"
or
"perl charmm2lammps.pl all36_prot 1gb1 -border=2.0 -cmap=36 -water -ions"

7) Run lammps by typing: "lmp_mpi -in 1ac7.in" or "lmp_mpi -in 1gb1.in"

8) Run lammps2pdb.pl by typing: "perl lammps2pdb.pl 1ac7"

** Additional notes:

The charmm2lammps.pl script takes the pdb and psf files for the 1ac7
or 1gb1 molecules and converts them into LAMMPS format. The -water option
embeds the molecule in water on a crystal lattice. The -border option
includes a layer of water surrounding the minimum dimensions of the
molecule. The -pdb_ctrl option produces the 1ac7_ctrl.pdb file that
can be visualized in a standard visualization package such as VMD. By
default, comments are added into the LAMMPS data file (everything
after the # sign is a comment) for user convenience in tracking atom
types etc. according to CHARMM nomenclature. If this is not desired,
the -nohints option can be used to turn off this function.

The provided 1ac7 example molecule is a DNA fragment. For peptides
longer than 2 amino acid residues or a protein is to be modeled,
e.g. the 1gb1 binding domain of a protein, the '-cmap' option should
be used. This will add CMAP section at the end of the data file that
will contain cmap crossterm corrections for the phi-psi dihedrals for
the amino acid residues. You will then need to also copy the
appropriate file for the cmap crossterms into your directory and be
sure that you are using the appropriate cmap crossterms that go with
the respective version of the charmm force field that is being used
(e.g, charmm22.cmap or charmm36.cmap). This is necessary to account
for the fact that the CHARMM group has provided updated cmap correction
terms for use with the c36 and more recent version of the charmm
protein force field.  Copies of charmm22.cmap and charmm36.cmap are
provided in the potentials directory.

The default timestep in the LAMMPS *.in file is set to 1.0 fs, which
can typically be increased to 2 fs after equilibration if the bonds
involving H are constrained via shake. Also, after equilibration, the
delay on neigh_modify can probably increased to 5 or so to improve
speed.

The -ions option allows the user to neutralize the simulation cell
with Na+ or Cl- counterions if the molecule has a net charge
Additional salt can be added by increasing the default concentration
(i.e., -ions=0.5).

** In the "other" file folder, you will find:

1) A FORTRAN 90 code called "mkpdb.f". Requires "in_mkpdb".  This is a
   fortran code that is an alternative way to convert LAMMPS dump
   files into pdb format.

2) A FORTRAN 90 code called "mkdcd.f" (and a FORTRAN 77 version called
   mkdcd_f77.f).  Requires "in_mkdcd". Creates CHARMM format
   trajectories from LAMMPS dump files.

3) A 3rd party perl script called "crd2pdb.pl"

4) A 3rd party fortran code called "pdb_to_crd.f"