Dear all,
Hi I am new to gromacs. I want to calculate the Van der waals
interaction between two capped CNT facing each other using the pairwise LJ
potential.I haven't used gromacs already. Any know-how/procedures to do the
requiste would be very helpful.Whether Any tutorials are available
Hi Valeria,
> Dear all,
> I am making some tests to start using replica exchange molecular dynamics
> on my system in water. The setup is ok (i.e. one replica alone runs
> correctly), but I am not able to parallelize the REMD. Details follow:
>
> - the test is on 8 temperatures, so 8 replicas
> -
Hi Valeria,
> Dear all,
> I am making some tests to start using replica exchange molecular dynamics
> on my system in water. The setup is ok (i.e. one replica alone runs
> correctly), but I am not able to parallelize the REMD. Details follow:
>
> - the test is on 8 temperatures, so 8 replicas
> -
On 02/23/11, Valeria Losasso wrote:
>
> Dear all,
> I am making some tests to start using replica exchange molecular dynamics on
> my system in water. The setup is ok (i.e. one replica alone runs correctly),
> but I am not able to parallelize the REMD. Details follow:
>
> - the test is on 8
Dear all,
I am making some tests to start using replica exchange molecular dynamics
on my system in water. The setup is ok (i.e. one replica alone runs
correctly), but I am not able to parallelize the REMD. Details follow:
- the test is on 8 temperatures, so 8 replicas
- Gromacs version 4.5.3
Hi,
I have obtained the chromophore parameters of the GFP for charmm force field
but I am not able to find it out how to add it to the charmm FF file.. I
have two files one is the topology file , which looks like this :-
*
221
MASS13 CP2c 12.01100 C ! his CE1 carbon
MASS14 NR2c
On 23/02/2011 3:35 PM, Justin Kat wrote:
Im not quite sure if this is the right place to analyze, but a bit before the part in the
config.log where it states the error of "cannot compuete sizeof (off_t)", there
is this:
configure:25048: checking size of off_t
configure:25053: /usr/local/bin/
Im not quite sure if this is the right place to analyze, but a bit
before the part in the config.log where it states the error of "cannot
compuete sizeof (off_t)", there is this:
configure:25048: checking size of off_t
configure:25053: /usr/local/bin/mpicc -o conftest -O3 -fomit-frame-pointer -f
Sorry, why do you think the PMF should be asymmetric?
I pulled my peptide from d=9nm (above the membrane) to d=-3nm (below the
membrane) and I did windowed umbrella sampling in the range of d=-1.05nm to
d=9nm. At least the PMF should be symmetric with respect of the bilayer center
in the r
Hi all,
If anyone have a script that amb2gmx_dihe.pl provide by Guillem
Portella,could you send me a copy?
Thanks very much!--
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bharat gupta wrote:
Since the paper that I am following says that for that protein (GFP) 1ns
simulation is enough as other people carried out 10ns for the same
protein and rmsd follows the same pattern which is being shown by that
1ns simulation ..
When were those studies published? With m
Since the paper that I am following says that for that protein (GFP) 1ns
simulation is enough as other people carried out 10ns for the same protein
and rmsd follows the same pattern which is being shown by that 1ns
simulation ..
So I decided to do a 3ns simulation the RMSD that I got was same
bharat gupta wrote:
Hi
I did a simulation of 3 ns with OPLS AA 2001 Force Field for a protein
of 230 aa and also I carried out a simulation of 10ns for the same
protein but with different force field (Amber 2006) . I obtained the
rmsd of the trajectories of both simulation , which I found t
Hi
I did a simulation of 3 ns with OPLS AA 2001 Force Field for a protein of
230 aa and also I carried out a simulation of 10ns for the same protein but
with different force field (Amber 2006) . I obtained the rmsd of the
trajectories of both simulation , which I found to be different ?? i.e. 3ns
Jianguo Li wrote:
Thank you, Justin.
Actually I did windowed umbrella simulations from d=-1.05nm to d=9nm.
Since I think there is no problem in the region out of the membrane, so
I only show the configurations within the membrane. My objective is to
access the free energy barrier of the pept
Thank you for the the useful information, XAvier.
My peptide is highly positively charged, 18 AA with +12 charges. Other of my
group members told me their NMR experiment in water indicates the peptide
conformation is very dynamics. Actually I also did peptide refolding using REMD
in water, and
Thank you, Justin.
Actually I did windowed umbrella simulations from d=-1.05nm to d=9nm. Since I
think there is no problem in the region out of the membrane, so I only show the
configurations within the membrane. My objective is to access the free energy
barrier of the peptide translocate the ne
Nick wrote:
One last question!
1- So what are the 12 energy terms I get by passing index file onto step
2 below? I ignored rerun! what does rerun does?
I don't know what 12 terms you're referring to. You'll get A-A, A-B, and B-B
short-range nonbonded terms, the exact enumeration of wh
One last question!
1- So what are the 12 energy terms I get by passing index file onto step 2
below? I ignored rerun! what does rerun does?
2- So I dont have to include index file in mdrun initially..In brief what I
need is:
step 1 grompp .(no index)
step 2 mdrun -s old.tpr
Nick wrote:
Dear Justin,
Thanks for your reply and Sorry for asking naive questions...
1- I am looking at all possible interaction energies between components
A and B. that is A-A AB and BB. So interaction between single chains is
not what I want. With this I think my initial approach was
Dear Justin,
Thanks for your reply and Sorry for asking naive questions...
1- I am looking at all possible interaction energies between components A
and B. that is A-A AB and BB. So interaction between single chains is not
what I want. With this I think my initial approach was right. That is
putt
Nick wrote:
Dear experts,
1- I am trying to get interaction energies between solute (3 chains A)
and solvent 50 molecules B. In the index file I created two groups: one
for all atoms of [A] and and [B] for all solvent molecules. and by
setting A and B as energy groups in mdp file I am getti
Dear experts,
1- I am trying to get interaction energies between solute (3 chains A) and
solvent 50 molecules B. In the index file I created two groups: one for all
atoms of [A] and and [B] for all solvent molecules. and by setting A and B
as energy groups in mdp file I am getting break down as A-
ok, problem solved...
used same .tpr file all the time
should stop working for today :)
greetings
thomas
On 02/22/2011 08:49 PM, Thomas Schlesier wrote:
hi all,
i'm trying out GROMACS 4.5.3
i'm simulating (sd-integrator) a small rna hairpin in vacuum, without
pbc for 100ps. System has about 380
hi all,
i'm trying out GROMACS 4.5.3
i'm simulating (sd-integrator) a small rna hairpin in vacuum, without
pbc for 100ps. System has about 380 atoms.
If i do the simulation a second time (grompp + mdrun) i get identical
results.
first i had only *gen_seed = -1* but latter i set also *ld_seed = -
Hi all.
I've noticed an unexpected behaviour using g_density. I have a
trajectory (with time step 2) and it is split into two subsets (using
trjconv) with, lets say, even and odd steps respectively. According
the the algorithm I expected that the density obtained with the
original traject
Dear Gromacs users,
I really hope someone could give me some advise on my following
problem. I am simulating liquid bulk hexane using a shell (or Drude
oscillator) model that incorporates the electronic polarization in
GROMACS 4.5.3. To do this, I use the force field parameters from the
CHARMM d
A few notes:
- the original method (Kumar-JCC-1992) that inspired wham was actually
developed to mix different temperature simulations. It is however not
clear
for the type of system you are simulating how much a 500K simulation
would be useful to improve the sampling at 300 K or so. The reaso
Jianguo Li wrote:
Thanks Justin and Chris and sorry for confusing interpretation.
Let me make it more clear. My peptide is flexible Martini beads, and
highly positively charged. My membrane is a mixture of negatively
charged lipids (25%) and zitterionic lipids(75%). So there is strong
electr
Hello all
I obtained a top file after running the "amb2gmx.pl" script,but I feel some
errors in this top file.
The functype of the [dihedral] is 3 in this top file,but the [pairs] part aslo
presence in it. And the
manual is point that "with the Ryckaert-Bellemans potential the 1-4
interactions
leila karami wrote:
Dear Justin
My simulation system contains protein, dna and water.
I used your script already for obtaining %exist hydrogen bonds between
protein and dna:
#!/usr/bin/perl
#
# plot_hbmap.pl - plot the probability of finding a particular hydrogen bond
# based on several inpu
Sorry I forgot to attach my mdp files.
Here is the mdp file for pulling simulaition:
-
title= Martini
cpp = /usr/bin/cpp
define = -DPOSRES_LIP
integrator = md
; start t
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