Subject: protein domain separate
Date: Mon, 19 Oct 2009 08:56:36 +0430
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Hi Tsjerk
Hi again
I use -pbc mol -ur compact but the problem still exist.
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Hi
I have done md simulation of a 2-domain protein in water, in 50 K but every
time I did it these domains are separated from each other, and dont correct
when I do trjconv -pbc nojump,
previous time when I did em or pr by doing trjconv -pbc nojump, it
corrected.
The 50.mdp file is:
title
Hi
As I told in my perevious mail, My system consist of a 2-domain protein
(Domain A and B), even when I did EM minimization this 2 damain separated.
my em.mpf is:
title = n.pdb
cpp = /lib/cpp
define = -DFLEXIBLE
constraints = none
integra
Hi
I want to do MD on a two-domain protein (Protein A, Protein B). After doning
position restranit for 20 ps, the final structure separated. How could I
keep these 2 domain close to each other during whole MD run.
Thank you in advance.
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Hi
I have a question about do_dssp program.is it posible to define the amount
of residus (the percentage) which have specific secondry structure, apart
from the graphic file? if yes what is the the command?
Thanks
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Hi
I am doing md with protein-LYS-PLP (pyridoxal phosphate) which attach
covalently. I could generate the DRG.itp, DRGPH.pdb files using PRODRG
server. then merge DRG.itp in to the topol.top and DRGPH.pdb into the
protein pdb file. When I use the grompp step before the energy minimization
I en
Hi
I want to do MD with a protien with prydoxal phosphate(PLP) which attache
covalently to one lysine.
For this I extract the Toplogy of lysine-PLP from PRODRG server.(DRGGMX.ITP
and DRGPOH.PDB).I Changed the name DRGGMX.ITP to DRG.itp.
after donig
pdb2gmx -f m.pdb -o m1.pdb -water spce with th
Hi Justin and all
Thak you very much my problem solve.
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Hi
my ligand is Arginine (so it is not neccessary to use PRODRG )and the OPLS
forcefield of gromacs make the itp file of it. I check and all the atoms
present in the ligand itp file.There is no missing atom in the file.
atoms ]
; nr type resnr residue atom cgnr charge mas
Hi
I want to analyze md. This md took 10 ns(1 ps) for a protein with 206
residue and 2 Mn plus about 17000 molecule solvent as water.
then I construct extra group containig Protein+2 Mn with make_ndx comand.
I did g_rmsf for extracting the average structure of the new group rmsd
equilibrated
Hi
I have 3 computer and I want to do mdrun_mpi.
I define this system in hostfile, lambhost-def, lam-hostmap.txt
after lamboot and lamnodes It defines me that I have 3 nodes:
h...@dma210:~/etc> lamnodes
n0 dma210.dma:2:origin,this_node
n1 dma211.dma:2:
n2 dma212.dma:2:
then I do:
hi
when I run mdrun command every thing is Ok and the mdrun go ahead.
but when I use mpimdrun -np 4 mdrungromacs_mpi (parallel mode) for that
system this error ocurres:
Step 0, time 0 (ps) LINCS WARNING
relative constraint deviation after LINCS:
max inf (between atoms 10 and 13) rms nan
bonds t
hi
I want to use mdrun, when i use It as one job it goes on.
but when i use as parallel job
> grompp -np 4 -f md300.mdp -c pr.pdb -p topol.top -o md300.tpr
>
then
> mpirun -np 4 mdrungromacs_mpi -nice 0 -v -s md300.tpr -o md300.trr -c
md300.pdb -e md300.edr -g md300.log
Hi gromacs users
I have done Position restrain for 50 ps.
after it had finished, I checked the rmsd for confident that rms reached to
it's equilibrate mode. When I check it by g_rms command and select system
subgroup, I find that it had not reached to equilibria, but after I check
It by p
hi
how could we test that the protein + solvent come to equilibration after
position restrain job.
my protein have 322 residue and I don't konw how much time the equilibtarion
peiods should be?
thank's.
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Tehran University of Medical Sciences
www.tums.ac.ir
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hi
How could we test that the protein + solvent come to equilibration after
position restrain job.
my protein have 322 residue and I don't konw how much time the equilibtarion
peiods should be?
thank's.
--
Tehran University of Medical Sciences
www.tums.ac.ir
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